HK1154400B

HK1154400B - Pluripotent cells

Info

Publication number: HK1154400B
Application number: HK11108494.1A
Authority: HK
Inventors: Alireza Rezania
Original assignee: Janssen Biotech, Inc.
Priority date: 2008-04-24
Filing date: 2009-04-22
Publication date: 2018-05-04

Description

FIELD OF THE INVENTION

The present invention is directed to pluripotent stem cells that can be readily expanded in culture on tissue culture polystyrene and do not require a feeder cell line. The present invention also provides methods to derive the pluripotent stem cell line from human embryonic stem cells.

BACKGROUND

Advances in cell-replacement therapy for Type I diabetes mellitus and a shortage of transplantable islets of Langerhans have focused interest on developing sources of insulin-producing cells, or β cells, appropriate for engraftment. One approach is the generation of functional β cells from pluripotent stem cells, such as, for example, embryonic stem cells.

In vertebrate embryonic development, a pluripotent cell gives rise to a group of cells comprising three germ layers (ectoderm, mesoderm, and endoderm) in a process known as gastrulation. Tissues such as, for example, thyroid, thymus, pancreas, gut, and liver, will develop from the endoderm, via an intermediate stage. The intermediate stage in this process is the formation of definitive endoderm. Definitive endoderm cells express a number of markers, such as, HNF-3 beta, GATA-4, Mixl1, CXCR4 and SOX-17.

Formation of the pancreas arises from the differentiation of definitive endoderm into pancreatic endoderm. Cells of the pancreatic endoderm express the pancreatic-duodenal homeobox gene, PDX-1. In the absence of PDX-1, the pancreas fails to develop beyond the formation of ventral and dorsal buds. Thus, PDX-1 expression marks a critical step in pancreatic organogenesis. The mature pancreas contains, among other cell types, exocrine tissue and endocrine tissue. Exocrine and endocrine tissues arise from the differentiation of pancreatic endoderm.

Cells bearing the features of islet cells have reportedly been derived from embryonic cells of the mouse. For example, Lumelsky et al. (Science 292:1389, 2001) report differentiation of mouse embryonic stem cells to insulin-secreting structures similar to pancreatic islets. Soria et al. (Diabetes 49:157, 2000) report that insulin-secreting cells derived from mouse embryonic stem cells normalize glycemia in streptozotocin-induced diabetic mice.

In one example, Hori et al. (PNAS 99: 16105, 2002) disclose that treatment of mouse embryonic stem cells with inhibitors of phosphoinositide 3-kinase (LY294002) produced cells that resembled β cells.

In another example, Blyszczuk et al. (PNAS 100:998, 2003) reports the generation of insulin-producing cells from mouse embryonic stem cells constitutively expressing Pax4.

Micallef et al. reports that retinoic acid can regulate the commitment of embryonic stem cells to form PDX-1 positive pancreatic endoderm. Retinoic acid is most effective at inducing PDX-1 expression when added to cultures at day 4 of embryonic stem cell differentiation during a period corresponding to the end of gastrulation in the embryo (Diabetes 54:301, 2005).

Miyazaki et al. reports a mouse embryonic stem cell line over-expressing PDX-1. Their results show that exogenous PDX-1 expression clearly enhanced the expression of insulin, somatostatin, glucokinase, neurogenin3, P48, Pax6, and HNF6 genes in the resulting differentiated cells (Diabetes 53: 1030, 2004).

Skoudy et al. reports that activin-A (a member of the TGFβ superfamily) upregulates the expression of exocrine pancreatic genes (p48 and amylase) and endocrine genes (PDX-1, insulin, and glucagon) in mouse embryonic stem cells. The maximal effect was observed using 1nM activin-A. They also observed that the expression level of insulin and PDX-1 mRNA was not affected by retinoic acid; however, 3nM FGF-7 treatment resulted in an increased level of the transcript for PDX-1 (Biochem. J. 379: 749, 2004).

Shiraki et al. studied the effects of growth factors that specifically enhance differentiation of embryonic stem cells into PDX-1 positive cells. They observed that TGFβ2 reproducibly yielded a higher proportion of PDX-1 positive cells (Genes Cells. 2005 Jun; 10(6): 503-16.).

Gordon et al. demonstrated the induction of brachyury+/HNF-3 beta+ endoderm cells from mouse embryonic stem cells in the absence of serum and in the presence of activin along with an inhibitor of Wnt signaling ( US2006/0003446A1 ).

Gordon et al. (PNAS, Vol 103, page 16806, 2006) states "Wnt and TGF-beta/noda1/ activin signaling simultaneously were required for the generation of the anterior primitive streak".

However, the mouse model of embryonic stem cell development may not exactly mimic the developmental program in higher mammals, such as, for example, humans.

Thomson et al. isolated embryonic stem cells from human blastocysts (Science 282:114, 1998). Concurrently, Gearhart and coworkers derived human embryonic germ (hEG) cell lines from fetal gonadal tissue (Shamblott et al., Proc. Natl. Acad. Sci. USA 95:13726, 1998). Unlike mouse embryonic stem cells, which can be prevented from differentiating simply by culturing with Leukemia Inhibitory Factor (LIF), human embryonic stem cells must be maintained under very special conditions ( U.S. Pat. No. 6,200,806 ; WO 99/20741 ; WO 01/51616 ).

D'Amour et al. describes the production of enriched cultures of human embryonic stem cell-derived definitive endoderm in the presence of a high concentration of activin and low serum (D'Amour KA et al. 2005). Transplanting these cells under the kidney capsule of mice resulted in differentiation into more mature cells with characteristics of some endodermal organs. Human embryonic stem cell-derived definitive endoderm cells can be further differentiated into PDX-1 positive cells after addition of FGF-10 ( US 2005/0266554A1 ).

D'Amour et al. (Nature Biotechnology - 24, 1392 - 1401 (2006)) states "We have developed a differentiation process that converts human embryonic stem (hES) cells to endocrine cells capable of synthesizing the pancreatic hormones insulin, glucagon, somatostatin, pancreatic polypeptide and ghrelin. This process mimics in vivo pancreatic organogenesis by directing cells through stages resembling definitive endoderm, gut-tube endoderm, pancreatic endoderm and endocrine precursor en route to cells that express endocrine hormones".

In another example, Fisk et al. reports a system for producing pancreatic islet cells from human embryonic stem cells ( US2006/0040387A1 ). In this case, the differentiation pathway was divided into three stages. Human embryonic stem cells were first differentiated to endoderm using a combination of n-butyrate and activin-A. The cells were then cultured with TGFB antagonists such as Noggin in combination with EGF or betacellulin to generate PDX-1 positive cells. The terminal differentiation was induced by nicotinamide.

In one example, Benvenistry et al. states: "We conclude that over-expression of PDX-1 enhanced expression of pancreatic enriched genes, induction of insulin expression may require additional signals that are only present in vivo" (Benvenistry et al, Stem Cells 2006; 24:1923-1930).

Current methods to culture human embryonic stem cells requires the use of either extracellular matrix proteins or a fibroblast feeder layer, or the addition of exogenous growth factors, such as, for example, bFGF.

In one example, Cheon et al (BioReprod DOI: 10.1095/biolreprod.105.046870, October 19, 2005) disclose a feeder-free, serum-free culture system in which embryonic stem cells are maintained in unconditioned serum replacement (SR) medium supplemented with different growth factors capable of triggering embryonic stem cell self-renewal.

In another example, Levenstein et al (Stem Cells 24: 568-574, 2006) disclose methods for the long-term culture of human embryonic stem cells in the absence of fibroblasts or conditioned medium, using media supplemented with bFGF.

In another example, US20050148070 discloses a method of culturing human embryonic stem cells in defined media without serum and without fibroblast feeder cells, the method comprising: culturing the stem cells in a culture medium containing albumin, amino acids, vitamins, minerals, at least one transferrin or transferrin substitute, at least one insulin or insulin substitute, the culture medium essentially free of mammalian fetal serum and containing at least about 100 ng/ml of a fibroblast growth factor capable of activating a fibroblast growth factor signaling receptor, wherein the growth factor is supplied from a source other than just a fibroblast feeder layer, the medium supported the proliferation of stem cells in an undifferentiated state without feeder cells or conditioned medium.

In another example, US20050233446 discloses a defined media useful in culturing stem cells, including undifferentiated primate primordial stem cells. In solution, the media is substantially isotonic as compared to the stem cells being cultured. In a given culture, the particular medium comprises a base medium and an amount of each of bFGF, insulin, and ascorbic acid necessary to support substantially undifferentiated growth of the primordial stem cells.

In another example, US6800480 states "In one embodiment, a cell culture medium for growing primate-derived primordial stem cells in a substantially undifferentiated state is provided which includes a low osmotic pressure, low endotoxin basic medium that is effective to support the growth of primate-derived primordial stem cells. The basic medium is combined with a nutrient serum effective to support the growth of primate-derived primordial stem cells and a substrate selected from the group consisting of feeder cells and an extracellular matrix component derived from feeder cells. The medium further includes nonessential amino acids, an anti-oxidant, and a first growth factor selected from the group consisting of nucleosides and a pyruvate salt."

In another example, US20050244962 states: "In one aspect the invention provides a method of culturing primate embryonic stem cells. One cultures the stem cells in a culture essentially free of mammalian fetal serum (preferably also essentially free of any animal serum) and in the presence of fibroblast growth factor that is supplied from a source other than just a fibroblast feeder layer. In a preferred form, the fibroblast feeder layer, previously required to sustain a stem cell culture, is rendered unnecessary by the addition of sufficient fibroblast growth factor."

In a further example, WO2005065354 discloses a defined, isotonic culture medium that is essentially feeder-free and serum-free, comprising: a. a basal medium; b. an amount of bFGF sufficient to support growth of substantially undifferentiated mammalian stem cells; c. an amount of insulin sufficient to support growth of substantially undifferentiated mammalian stem cells; and d. an amount of ascorbic acid sufficient to support growth of substantially undifferentiated mammalian stem cells.

In another example, WO2005086845 discloses a method for maintenance of an undifferentiated stem cell, said method comprising exposing a stem cell to a member of the transforming growth factor-beta (TGFβ) family of proteins, a member of the fibroblast growth factor (FGF) family of proteins, or nicotinamide (NIC) in an amount sufficient to maintain the cell in an undifferentiated state for a sufficient amount of time to achieve a desired result.

Additionally, formation of pancreatic endocrine cells, pancreatic hormone expressing cells, or pancreatic hormone secreting cells from human embryonic cells may require genetic manipulation of the human embryonic stem cells. Transfection of human embryonic stem cells using traditional techniques, such as, for example, lipofectamine or electroporation is inefficient.

WO2007027157 discloses a method comprising: (a) providing an embryonic stem (ES) cell; and (b) establishing a progenitor cell line from the embryonic stem cell; in which the progenitor cell line is selected based on its ability to self-renew. Preferably, the method selects against somatic cells based on their inability to self renew. Preferably, the progenitor cell line is derived or established in the absence of co-culture, preferably in the absence of feeder cells, which preferably selects against embryonic stem cells. Optionally, the method comprises (d) deriving a differentiated cell from the progenitor cell line.

Therefore, there still remains a significant need to develop conditions for establishing pluripotent stem cell lines that can be expanded to address the current clinical needs, while retaining the potential to differentiate into pancreatic endocrine cells, pancreatic hormone expressing cells, or pancreatic hormone secreting cells.

SUMMARY OF THE INVENTION

The invention provides a method for deriving a population of cells comprising cells expressing pluripotency markers comprising the steps of:

a. obtaining a population of cells expressing markers characteristic of the definitive endoderm lineage by differentiation of human embryonic stem cells, and
b. culturing the cells from (a) under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in a medium containing serum, activin-A and a Wnt ligand,

wherein the cells expressing pluripotency markers express at least one of the pluripotency markers selected from the group consisting of ABCG2, cripto, FoxD3, Connexin43, Connexin45, Oct4, SOX-2, Nanog, hTERT, UTF-1, ZFP42, SSEA-3, SSEA-4, Tra1-60, and Tra1-81. SUMMARY OF THE DISCLOSURE

The present disclosure provides a cell population with characteristics of human embryonic stem cells, that can be readily expanded in culture, in low serum, that requires no feeder cell line or a coating of complex matrix proteins, can be passaged in single cell suspension, can be transfected with a very high efficiency, and cultured under hypoxic conditions. This combination of unique attributes separates the cells described in the present disclosure from the prior art.

In one embodiment, the present disclosure provides a method for deriving a population of cells comprising cells expressing pluripotency markers, comprising the steps of:

a. Obtaining cells, and
b. Culturing the cells under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix prior to culturing the cells.

The cells may be human embryonic stem cells, or they may be cells expressing markers characteristic of the definitive endoderm lineage. The human embryonic stem cells may be cultured in normoxic conditions prior to culturing the cells on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix. Alternatively, the human embryonic stem cells may be cultured in hypoxic conditions.

The human embryonic stem cells may be cultured in normoxic conditions prior to culturing the cells on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, and treated with a Rho kinase inhibitor. Alternatively, the human embryonic stem cells may be cultured in hypoxic conditions, and treated with a Rho kinase inhibitor.

The cells expressing markers characteristic of the definitive endoderm lineage may be cultured in normoxic conditions prior to culturing the cells on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix. Alternatively, the cells expressing markers characteristic of the definitive endoderm lineage may be cultured in hypoxic conditions.

a. Culturing human embryonic stem cells,
b. Differentiating the human embryonic stem cells into cells expressing markers characteristic of definitive endoderm cells, and
c. Removing the cells, and subsequently culturing them under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix prior to culturing the cells.

The cells may be cultured under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in medium containing serum, activin-A, and a Wnt ligand. Alternatively, the cells may be cultured under hypoxic conditions, on a tissue culture substrate that is not pretreated with a protein or an extracellular matrix, in medium containing serum, activin-A, a Wnt ligand, and IGF-1.

The cells may be cultured under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in medium containing serum, a Rho kinase inhibitor, activin-A, and a Wnt ligand. Alternatively, the cells may be cultured under hypoxic conditions, on a tissue culture substrate that is not pretreated with a protein or an extracellular matrix, in medium containing serum, a Rho kinase inhibitor, activin-A, a Wnt ligand, and IGF-1.

a. Culturing human embryonic stem cells, and
b. Removing the cells, and subsequently culturing them under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix.

The cells expressing pluripotency markers derived by the methods of the present disclosure are capable of expansion in culture under hypoxic conditions, on tissue culture substrate that is not pre-treated with a protein or an extracellular matrix.

In one embodiment, the present disclosure provides a method to expand cells expressing markers characteristic of the definitive endoderm lineage, comprising the steps of culturing the cells under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix. In one embodiment, the cells expressing markers characteristic of the definitive endoderm lineage are derived from pluripotent cells formed by the methods of the present disclosure.

The cells may be cultured under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in medium containing serum, activin-A, a Wnt ligand, and a GSK-3B inhibitor.

BRIEF DESCRIPTION OF THE FIGURES

Figure 1 shows the expression of CXCR4 (CD 184, Y-axis) and CD9 (X-axis) in cells from the human embryonic stem cell line H9 at passage 54 that have been differentiated into definitive endoderm following treatment with low serum +Activin-A + WNT-3A for 4 days.
Figure 2 shows the real-time PCR analysis of cells from the human embryonic stem cell line H9 at passage 54 at day 4 and 6 of the definitive endoderm differentiation protocol outlined in Example 5. Panel a) depicts expression of AFP, Bry, CXCR4, GSC, and SOX-7. Panel b) depicts the expression of SOX-17, GATA-4, and HNF-3 beta.
Figure 3 shows the isolation protocol used to derive EXPRES cells from embryonic stem cells according to the methods of the present invention.
Figure 4 shows the morphology of expanded EXPRES cells at P0, at day 11, that were cultured in 2% FBS + DMEM-F12 + 100 ng/ml of Activin-A (Panel a) or 2% FBS + DMEM-F12 + 100 ng/ml of Activin-A + 20 ng/ml of WNT-3A (Panel b). Panel c shows the morphology of the EXPRES cells at passage 3.
Figure 5 shows the real-time PCR analysis of expanded EXPRES cells cultured in 2-5% FBS + DMEM-F12 + 100 ng/ml of Activin-A + 20 ng/ml of WNT-3A for three passages. Panel a) depicts expression of AFP, Bry, CXCR4, GSC, and SOX-7. Panel b) depicts the expression of SOX-17, GATA-4, and HNF-3 beta.
Figure 6 shows the effect of the addition of Wnt-3A on gene expression in EXPRES cells. Panel a) depicts real-time PCR expression of SOX-17, GATA-4, and HNF-3 beta. Panel b) depicts real-time PCR expression of AFP, Bry, CXCR4, GSC, and SOX-7.
Figure 7 shows the effect of IGF-1, Wnt-3A and activin-A on gene expression in EXPRES cells. Panel a) depicts real-time PCR expression of SOX-17, GATA-4, HNF-3 beta, Bry, CXCR4, and GSC. Panel b) depicts real-time PCR expression of and SOX-7 and AFP. Panel c) depicts real-time PCR expression of OCT-4.
Figure 8 shows the morphology of expanded EXPRES cells derived from the human embryonic stem cell line H9 at passage 54, cultured in a) 2% FBS +DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A, b) 2% FBS + DMEMF12 + 100 ng/ml of AA, c) 2% FBS + DMEM-F12 + 50 ng/ml of IGF-I.
Figure 9 shows the expansion potential of EXPRES 01 and 02 cells cultured on tissue culture polystyrene under hypoxic conditions. EXPRES 01 was cultured in 2% FBS + DM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A + 50 ng/ml of IGF-I and EXPRES 02 cells were cultured in 2% FBS + DM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A.
Figure 10 shows the morphology of EXPRES cells derived from single cell suspension of undifferentiated ES cells on TCPS (tissue culture polystyrene) in DM-F12 + 2% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 50 ng/ml of IGF-I.
Figure 11 shows the protein expression as determined by FACS in EXPRES 01 cells at passage 24 cells. Panel a) shows the expression levels of E-cadherin, panel b) shows the expression levels of CXCR4, panel c) shows the expression levels of CD9, panel d) shows the expression levels of CD117, panel e) shows the expression levels of CD30, panel f) shows the expression levels of LIF receptor, panel g) shows the expression levels of TRA 1-60, panel h) shows the expression levels of TRA 1-81, panel i) shows the expression levels of SSEA-1, panel j) shows the expression levels of SSEA-3, panel k) shows the expression levels of SSEA-4, and Panel 1) shows the expression levels of CD56.
Figure 12 shows the protein expression as determined by FACS in EXPRES 02 at passage 21 cells.
Panel a) shows the expression levels of E-cadherin, panel b) shows the expression levels of CXCR4, panel c) shows the expression levels of CD9, panel d) shows the expression levels of CD117, panel e) shows the expression levels of CD30, panel f) shows the expression levels of LIF receptor, panel g) shows the expression levels of TRA 1-60, panel h) shows the expression levels of TRA 1-81, panel i) shows the expression levels of SSEA-1, panel j) shows the expression levels of SSEA-3, panel k) shows the expression levels of SSEA-4, and panel 1) shows the expression levels of CD56.
Figure 13 shows immuno fluorescent images of EXPRES 01 at passage 10 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A + 50 ng/ml of IGF-I. Panel a) DAPI image for panel b, panel b) Nanog, panel c) DAPI (blue) and Oct-4 (green) co-staining, panel d) DAPI image for panel e, panel e) SOX-2, and panel f) DAPI (blue) and HNF-3 beta (green) co-staining.
Figure 14 shows immuno fluorescent images of EXPRES 02 at passage 9 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A. Panel a) DAPI image for panel b, panel b) HNf3B, panel c) DAPI image for panel d, panel d) OCT-4, panel e) DAPI image for panel f, panel f) SOX-2, panel g) DAPI image for panel h, panel h) NANOG.
Figure 15 shows gene expression as determined by real-time PCR for EXPRES 01 cells, EXPRES 02 cells, EB derived from H9 cells, SA002 cultured on MATRIGEL in MEF-CM, and undifferentiated H9 cells cultured on MATRIGEL in MEFCM. All the expression levels are normalized to undifferentiated H9 cells. Panel a) shows SOX-1 expression, panel b) shows FOXD3, MYOD1, POU5F1, and ZFP42 expression, panel c) shows ABCG2, Connexin 43, Connexin 45, and cytokeratin 15 expression, panel d) shows nestin, SOX-2, UTF1, and vimentin, panel e) shows GATA-2, Brachyury, TERT, and tubulin-beta III expression, panel f) shows CFC1, and GATA-4 expression, Panel g) shows AFP and FOXA2 expression, and Panel h) shows IPF1A and MSX1 expression.
Figure 16 shows the expression, as determined by FACS of CXCR4 (Y-axis) and CD9 (x-axis) in a) EXPRES 01 cells passage 5 cells cultured on tissue culture polystyrene in growth media and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A and 20 ng/ml of WNT3A for 2 days followed by additional 2 days in DMEM-F12 + 2% FBS + 100 ng/ml of activin-A, b) EXPRES 02 cells passage 4 cells cultured on tissue culture polystyrene in growth media and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A and 20 ng/ml of WNT3A for 2 days followed by additional 2 days in DMEM-F12 + 2% FBS + 100 ng/ml of activin-A.
Figure 17 shows gene expression as determined by real-time PCR in a) EXPRES 01 cells and b) EXPRES 02 cells treated with low serum plus AA + WNT3a.
Figure 18 shows immuno fluorescent images of EXPRES 01 cells at passage 5 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A + 50 ng/ml of IGF-I and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A and 20 ng/ml of WNT3A for 2 days, followed by additional 2 days in DMEM-F12 + 2% FBS + 100 ng/ml of activin-A. Panel a) DAPI image for panel b, panel b) GATA-4, panel c) DAPI image for panel d, panel d) SOX-17, panel e) DAPI image for panel f, panel f) HNF-3 beta, panel g) DAPI image for panel h, and panel h) OCT-4.
Figure 19 shows immuno fluorescent images of EXPRES 02 cells at passage 4 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A and 20 ng/ml of WNT3A for 2 days followed by additional 2 days in DMEM-F12 + 2% FBS + 100 ng/ml of activin-A. Panel a) DAPI image for panel b, panel b) GATA-4, panel c) DAPI image for panel d, panel d) SOX-17, panel e) DAPI image for panel f, panel f) HNF-3 beta, panel g) DAPI image for panel h, and panel h) OCT-4.
Figure 20 shows protein expression as determined by FACS of CXCR4 (Y-axis) and CD9 (x-axis) for a) EXPRES 01 cells at passage 19 cells and b) EXPRES 02 cells at passage 14 cells cultured on tissue culture polystyrene in growth media and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A + 100 nM GSK-3B inhibitor IX, and 20 ng/ml of WNT3A for 4days.
Figure 21 shows immuno fluorescent images of EXPRES 01 cells at passage 19 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A + 50 ng/ml of IGF-I and EXPRES 02 cells at passage 14 cultured in 2% FBS + DMEM-F12 + 100 ng/ml of AA + 20 ng/ml of WNT-3A and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml of activin-A + 100 nM GSK-3B inhibitor IX, and 20 ng/ml of WNT3A for 5days. Panel a) DAPI image for panel b, panel b) HNF-3 beta, panel c) DAPI image for panel d, panel d) GATA-4, panel e) DAPI image for panel f, panel f) SOX-17, panel g)DAPI image for panel h, panel h) HNF-3 beta, Panel i) DAPI image for panel j, panel j) GATA-4, panel k)DAPI image for panel 1, panel 1) SOX-17.
Figure 22 shows gene expression as determined by real-time PCR data for a) EXPRES 01 and EXPRES 02 cells treated with low serum plus AA + WNT3a + GSK-3B IX inhibitor for 5 days. Panel a depicts expression of AFP, Brachyury, CDX2, Mox1, OCT3/4, SOX-7, and ZIC1 and panel b shows expression levels of CXCR4, GATA-4, Goosecoid, HNf3B, and SOX-17.
Figure 23 shows gene expression as determined by real-time PCR for EXPRES 01 cells seeded at 5000-40000 cells/cm2 on tissue culture polystyrene in growth media and then switched to DMEM-F12 + 0.5% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 100 nM GSK-3B inhibitor IX for four days under hypoxic conditions. Panel a depicts expression levels of AFP, Brachyury, SOX-7, and OTX2. Panel b depicts expression levels of CXCR4, HNF-3 beta, GATA-4, SOX-17, Cerb, and GSC.
Figure 24 shows the results of a telomere length assay in low telomere control cells (lane 1), EXPRES 01 cells at passage 24 (lane 2), EXPRES 02 cells at passage 17 (lane 3), undifferentiated cells from the human embryonic stem cell line H1 at passage 40 (lane 4), and high telomere length control cells (lane 5).
Figure 25 shows gene expression as determined by real-time PCR data for EXPRES 01 cells at passage 21 that have been differentiated to foregut endoderm cells (S3), pancreatic endoderm cells (S4), and pancreatic endocrine cells (S5).
Figure 26 shows immuno fluorescent images of EXPRES 01 at passage 35 cultured according to Example 18. Panel a) DAPI image for panel b, panel b) Anti-1 trypsin, panel c) HNF-3 beta in green Albumin in Red, panel d) Albumin in red and DAPI (blue), panel e) DAPI image for panel f, panel f) PDX-1, panel g) DAPI image for panel h, panel h) SOX-17, panel i) DAPI image for panel j, panel j) CDX-2.
Figure 27 shows scatter plots of microarray data comparing, panel a) EXPRES 01 cells (y-axis) to undifferentiated cells from the human embryonic stem cell line H9 (x-axis), panel b) EXPRES 02 cells (y-axis) to undifferentiated cells from the human embryonic stem cell line H9 (x-axis), panel c) EXPRES 01 cells (y-axis) to EXPRES 02 cells (x-axis), panel d) EXPRES 01 cells (y-axis) to cells from the human embryonic stem cell line H9 that have been differentiated into definitive endoderm (x-axis), panel e) EXPRES 02 cells (y-axis) to cells from the human embryonic stem cell line H9 that have been differentiated into definitive endoderm (x-axis), panel f) undifferentiated cells from the human embryonic stem cell line H9 (y-axis) to cells from the human embryonic stem cell line H9 that have been differentiated into definitive endoderm (x-axis).
Figure 28 shows the morphology of EB bodies formed by EXPRES 01 cells.
Figure 29 shows gene expression as determined by real-time PCR for cells of the EXPRES 01 cell line, cells of the EXPRES 02 cell line, and cells from the human embryonic stem cell line H9 at passage 43, following five weeks of transplantation beneath the kidney capsule of NOD-SCID mice. Panels a-e, show mesoderm markers. Panels f & g show ectoderm markers. Panels h & i show endoderm markers. Panel j shows extra embryonic endoderm markers. Panels k-m show pluripotency markers.
Figure 30 shows the proliferation and cell cycle status of EXPRES 03 cells, as determined by BRDU incorporation. EXPRES 03 cells were cultured in 2% FBS/DMEM/F12, supplemented with, panel a) activin-A (100 ng/ml) and wnt3a (20ng/ml), panel b) Activin-A (100 ng/ml) and wnt3a (20ng/ml) and IGF (50nh/ml). Other cells shown include, panel c) hES cells (H9p43), panel d) Amniotic Fluid Cells (AFDX002) and panel e) mitomycin treated MEF cells. Panel f) shows the frequency of cells in S-phase, G1 and G2/M-phases of cell cycle for different cell populations studied.
Figure 31 shows the transfection efficiency and expression of EGFP in EXPRES 01 cells and human embryonic stem cells plated either as single cell dispersions or cell clusters. Cells were analyzed 24 hrs later by fluorescence microscopy and flow cytometry. Panel A) shows data obtained from EXPRES 01 cells. Panel B) shows data obtained from single cell dispersions of human embryonic stem cells and Panel C) shows data obtained from cell clusters of human embryonic stem cells.
Figure 32 shows average OD readings representing dehydrogenase enzyme activity versus cell number as measured by MTS assay for a) EXPRES 01 cells cultured in atmospheric oxygen (approximately 21%), b) EXPRES 01 cells cultured in 3% 02, c) EXPRES 02 cells cultured in atmospheric oxygen (approximately 21%), d) EXPRES 02 cells cultured in 3% 02 conditions.
Figure 33 shows gene expression as determined by real-time PCR for EXPRES 01 P27 cells seeded at 10000 cells/cm2 on tissue culture polystyrene in DMEMF12 + 0.5% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 100 nM GSK-3B inhibitor IX.. Panel a depicts expression levels of AFP, Brachyury, SOX-7, and OTX2. Panel b depicts expression levels of CXCR4, HNF-3 beta, GATA-4, SOX-17, Cer1, and GSC.
Figure 34 shows protein expression of CXCR4 (Y-axis) and CD9 (x-axis), as determined by FACS for EXPRES 01 P27 cells cultured on tissue culture polystyrene in DMEM-F12 + 0.5% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 100 nM GSK-3B inhibitor IX for three passages.
Figure 35 shows the effects of siRNA transfection on the expression of GSK-3B and beta-catenin. EXPRES cells were analyzed by fluorescence microscopy and quantitative RT-PCR methods. A) Fluorescence microscopy of cells transfected with i) CY3 labeled siRNA and ii) Fluorescein labeled siRNA. B) Target gene knockdown expressed as % remaining activity in cells transfected with i) GSK3b and ii) Beta-catenin siRNA oligo sequences.
Figure 36 shows the karyotype of two cell lines derived by methods of the present invention. Panel a: EXPRES 01 cell line. Panel b: EXPRES 02 cell line.
Figure 37 shows the morphology of EXPRES 15 cells at passage 0 after 24h culture in a) 2% FBS + DM-F12 + 100 ng/ml of activin-A+ 20 ng/ml of WNT-3A + 50 ng/ml IGF or b) 2% FBS + DM-F12 + 100 ng/ml of Activin-A+ 20 ng/ml of WNT-3A + 50 ng/ml IGF + 10 µM of the Rho kinase inhibitor Y-27632.
Figure 38 shows the karyotype of EXPRES 15 cells cultured in 2% FBS + DM-F12 + 100 ng/ml of Activin-A+ 20 ng/ml of WNT-3A + 50 ng/ml IGF + 10 µM of the Rho kinase inhibitor Y-27632 for 12 passages.
Figure 39 shows the proliferation as determined by A490 of EXPRES 11 cells cultured in basal media supplemented with IGF, activin-A, Wnt3A, and GSK inhibitor IX at the concentrations indicated at 24 h (panel a), 48 h (panel b), and 96 h (panel c).

DETAILED DESCRIPTION

For clarity of disclosure, and not by way of limitation, the detailed description of the invention is divided into the following subsections that describe or illustrate certain features, embodiments, or applications of the present invention.

Definitions

Stem cells are undifferentiated cells defined by their ability at the single cell level to both self-renew and differentiate to produce progeny cells, including self renewing progenitors, non-renewing progenitors, and terminally differentiated cells. Stem cells are also characterized by their ability to differentiate in vitro into functional cells of various cell lineages from multiple germ layers (endoderm, mesoderm and ectoderm), as well as to give rise to tissues of multiple germ layers following transplantation and to contribute substantially to most, if not all, tissues following injection into blastocysts.

Stem cells are classified by their developmental potential as: (1) totipotent, meaning able to give rise to all embryonic and extraembryonic cell types; (2) pluripotent, meaning able to give rise to all embryonic cell types; (3) multipotent, meaning able to give rise to a subset of cell lineages, but all within a particular tissue, organ, or physiological system (for example, hematopoietic stem cells (HSC) can produce progeny that include HSC (self- renewal), blood cell restricted oligopotent progenitors and all cell types and elements (e.g., platelets) that are normal components of the blood); (4) oligopotent, meaning able to give rise to a more restricted subset of cell lineages than multipotent stem cells; and (5) unipotent, meaning able to give rise to a single cell lineage (e.g. , spermatogenic stem cells).

Differentiation is the process by which an unspecialized ("uncommitted") or less specialized cell acquires the features of a specialized cell such as, for example, a nerve cell or a muscle cell. A differentiated or differentiation-induced cell is one that has taken on a more specialized ("committed") position within the lineage of a cell. The term "committed", when applied to the process of differentiation, refers to a cell that has proceeded in the differentiation pathway to a point where, under normal circumstances, it will continue to differentiate into a specific cell type or subset of cell types, and cannot, under normal circumstances, differentiate into a different cell type or revert to a less differentiated cell type. De-differentiation refers to the process by which a cell reverts to a less specialized (or committed) position within the lineage of a cell. As used herein, the lineage of a cell defines the heredity of the cell, i.e., which cells it came from and what cells it can give rise to. The lineage of a cell places the cell within a hereditary scheme of development and differentiation. A lineage-specific marker refers to a characteristic specifically associated with the phenotype of cells of a lineage of interest and can be used to assess the differentiation of an uncommitted cell to the lineage of interest.

"AFP" or "alpha-fetoprotein protein" as used herein, refers to an antigen produced at the onset of liver development. AFP may also be expressed in extraembryonic cells.

"Albumin" is a soluble monomeric protein that makes up about half of all serum proteins in adults.

"β-cell lineage" refer to cells with positive gene expression for the transcription factor PDX-1 and at least one of the following transcription factors: NGN-3, Nkx2.2, Nkx6.1, NeuroD, Isl-1, HNF-3 beta, MAFA, Pax4, and Pax6. Cells expressing markers characteristic of the β cell lineage include β cells.

"Brachyury", as used herein, is a T-box gene family member. It is the marker for primitive streak and mesoderm cells.

"Cells expressing markers characteristic of the definitive endoderm lineage" as used herein refer to cells expressing at least one of the following markers: SOX-17, GATA-4, HNF-3 beta, GSC, Cer1, Nodal, FGF8, Brachyury, Mix-like homeobox protein, FGF4 CD48, eomesodermin (EOMES), DKK4, FGF17, GATA-6, CXCR4, C-Kit, CD99, or OTX2. Cells expressing markers characteristic of the definitive endoderm lineage include primitive streak precursor cells, primitive streak cells, mesendoderm cells and definitive endoderm cells.

"c-Kit" and "CD117" both refer to a cell surface receptor tyrosine kinase having a sequence disclosed in Genbank Accession No. X06182, or a naturally occurring variant sequence thereof (e.g., allelic variant).

"CD99" as used herein refers to the protein encoded by the gene wit the accession number NM_002414.

"Cells expressing markers characteristic of the pancreatic endoderm lineage" as used herein refer to cells expressing at least one of the following markers: PDX-1, HNF-1beta, PTF-1 alpha, HNF-6, or HB9. Cells expressing markers characteristic of the pancreatic endoderm lineage include pancreatic endoderm cells.

"Cells expressing markers characteristic of the pancreatic endocrine lineage" as used herein refer to cells expressing at least one of the following markers: NGN-3, NeuroD, Islet-1, PDX-1, NKX6.1, Pax-4, Ngn-3, or PTF-1 alpha. Cells expressing markers characteristic of the pancreatic endocrine lineage include pancreatic endocrine cells, pancreatic hormone expressing cells, and pancreatic hormone secreting cells, and cells of the β-cell lineage.

"Cer1" or "Cerebrus" as used herein is a member of the cysteine knot superfamily of proteins.

"CXCR4" as used herein refers to the stromal cell-derived factor 1 (SDF-1) receptor, also known as "LESTR" or "fusin". In the gastrulating mouse embryo, CXCR4 is expressed in the definitive endoderm and mesoderm but not in extraembryonic endoderm.

"Definitive endoderm" as used herein refers to cells which bear the characteristics of cells arising from the epiblast during gastrulation and which form the gastrointestinal tract and its derivatives. Definitive endoderm cells express the following markers: HNF-3 beta, GATA-4, SOX-17, Cerberus, OTX2, goosecoid, C-Kit, CD99, and Mixl1.

"Extraembryonic endoderm" as used herein refers to a population of cells expressing at least one of the following markers: SOX-7, AFP, and SPARC.

"FGF-2", "FGF-4" "FGF-8" "FGF-10", and "FGF-17" as used herein, are members of the fibroblast growth factor family.

"GATA-4" and "GATA-6" are members of the GATA transcription factor family. This family of transcription factors is induced by TGF-β signaling, and contribute to the maintenance of early endoderm markers.

"GLUT-2", as used herein, refers to the glucose transporter molecule that is expressed in numerous fetal and adult tissues, including pancreas, liver, intestine, brain, and kidney.

"Goosecoid" or "GSC" as used herein, refers to a homeodomain transcription factor expressed in the dorsal lip of the blastopore.

"HB9" as used herein, refers to the homeobox gene 9.

"HNF-1 alpha", "HNF-1 beta", "HNF-3 beta", and "HNF-6" belong to the hepatic nuclear factor family of transcription factors, which is characterized by a highly conserved DNA binding domain and two short carboxy-terminal domains.

"Islet-1" or "Isl-1" as used herein is a member of the LIM/homeodomain family of transcription factors, and is expressed in the developing pancreas.

"MafA" as used herein is a transcription factor expressed in the pancreas, and controls the expression of genes involved in insulin biosynthesis and secretion.

"Markers" as used herein, are nucleic acid or polypeptide molecules that are differentially expressed in a cell of interest. In this context, differential expression means an increased level for a positive marker and a decreased level for a negative marker. The detectable level of the marker nucleic acid or polypeptide is sufficiently higher or lower in the cells of interest compared to other cells, such that the cell of interest can be identified and distinguished from other cells using any of a variety of methods known in the art.

"Mesendoderm cell" as used herein refers to a cell expressing at least one of the following markers: CD48, eomesodermin (EOMES), SOX-17, DKK4, HNF-3 beta, GSC, FGF17, GATA-6.

"Mixl1" as used herein refers to a homeobox gene, which is marker for the cells in the primitive streak, mesoderm, and endoderm.

"NeuroD" as used herein is basic helix-loop-helix (bHLH) transcription factor implicated in neurogenesis.

"NGN-3" as used herein, is a member of the neurogenin family of basic loophelix-loop transcription factors.

"Nkx-2.2" and "Nkx-6.1" as used herein are members of the Nkx transcription factor family.

"Nodal" as used herein, is a member of the TGF beta superfamily of proteins.

"Oct-4" is a member of the POU-domain transcription factor and is widely regarded as a hallmark of pluripotent stem cells. The relationship of Oct-4 to pluripotent stem cells is indicated by its tightly restricted expression to undifferentiated pluripotent stem cells. Upon differentiation to somatic lineages, the expression of Oct-4 disappears rapidly.

"Pancreatic endocrine cell", or "pancreatic hormone expressing cell" as used herein refers to a cell capable of expressing at least one of the following hormones: insulin, glucagon, somatostatin, and pancreatic polypeptide.

"Pancreatic hormone secreting cell" as used herein refers to a cell capable of secreting at least one of the following hormones: insulin, glucagon, somatostatin, and pancreatic polypeptide.

"Pax-4" and "Pax-6" as used herein are pancreatic β cell specific transcription factors that are implicated in islet development.

"PDX-1" as used herein refers to a homeodomain transcription factor implicated in pancreas development.

"Pre-primitive streak cell" as used herein refers to a cell expressing at least one of the following markers: Nodal, or FGF8

"Primitive streak cell" as used herein refers to a cell expressing at least one of the following markers: Brachyury, Mix-like homeobox protein, or FGF4.

"PTF-1 alpha" as used herein refers to a basic helix-loop-helix protein of 48 kD that is a sequence-specific DNA-binding subunit of the trimeric pancreas transcription factor-1(PTF1).

"SOX-1", "SOX-2", "SOX-7", and "SOX-17"as used herein, are a members of the SOX transcription factor family, and are implicated in embryogenesis.

"SPARC" as used herein is also known as "secreted protein acidic and rich in cysteine".

"SSEA-1" (Stage Specific Embryonic Antigen-1) is a glycolipid surface antigen present on the surface of murine teratocarcinoma stem cells (EC), murine and human embryonic germ cells (EG), and murine embryonic stem cells (ES).

"SSEA-3" (Stage Specific Embryonic Antigen-3) is a glycolipid surface antigen present on the surface of human teratocarcinoma stem cells (EC), human embryonic germ cells (EG), and human embryonic stem cells (ES).

"SSEA-4" (Stage Specific Embryonic Antigen-4) is a glycolipid surface antigen present on the surface of human teratocarcinoma stem cells (EC), human embryonic germ cells (EG), and human embryonic stem cells (ES).

"RA1-60" is a keratin sulfate related antigen that is expressed on the surface of human teratocarcinoma stem cells (EC), human embryonic germ cells (EG), and human embryonic stem cells (ES).

"RA1-81" is a keratin sulfate related antigen that is expressed on the surface of human teratocarcinoma stem cells (EC), human embryonic germ cells (EG), and human embryonic stem cells (ES).

"TRA2-49" is an alkaline phosphatase isozyme expressed on the surface of human teratocarcinoma stem cells (EC) and human embryonic stem cells (ES).

"UTF-1" as used herein, refers a transcriptional co-activator expressed in pluripotent embryonic stem cells and extra-embryonic cells.

"Zic1" as used herein is a member of the Zic transcription factor family. Zic1 regulates the expression of neural and neural crest-specific genes and is expressed in the cells of the dorsal neural tube and the premigratory neural crest.

Method to derive cells expressing pluripotency markers

Obtaining cells, and
Culturing the cells under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix prior to culturing the cells.

Culturing human embryonic stem cells,
Differentiating the human embryonic stem cells into cells expressing markers characteristic of definitive endoderm cells, and
Removing the cells, and subsequently culturing them under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix prior to culturing the cells.

Culturing human embryonic stem cells, and
Removing the cells, and subsequently culturing them under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix.

Cell culture under hypoxic conditions on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix

In one embodiment, the cells are cultured under hypoxic conditions, on a tissue culture substrate that is not coated with an extracellular matrix for about 1 to about 20 days. In an alternate embodiment, the cells are cultured under hypoxic conditions, on a tissue culture substrate that is not coated with an extracellular matrix for about 5 to about 20 days. In an alternate embodiment, the cells are cultured under hypoxic conditions, on a tissue culture substrate that is not coated with an extracellular matrix for about 15 days.

In one embodiment, the hypoxic condition is about 1% O₂ to about 20% O₂. In an alternate embodiment, the hypoxic condition is about 2% O₂ to about 10% O₂. In an alternate embodiment, the hypoxic condition is about 3% O₂.

The cells may be cultured, under hypoxic conditions on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in medium containing serum, activin-A, and a Wnt ligand. Alternatively, the medium may also contain IGF-1.

The culture medium may have a serum concentration in the range of about 2% to about 5%. In an alternate embodiment, the serum concentration may be about 2%.

Activin-A may be used at a concentration from about 1pg/ml to about 100µg/ml. In an alternate embodiment, the concentration may be about 1pg/ml to about 1µg/ml. In another alternate embodiment, the concentration may be about 1pg/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 50ng/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 100ng/ml.

The Wnt ligand may be selected from the group consisting of Wnt-1, Wnt-3a, Wnt-5a and Wnt-7a. In one embodiment, the Wnt ligand is Wnt-1. In an alternate embodiment, the Wnt ligand is Wnt-3a.

The Wnt ligand may be used at a concentration of about 1ng/ml to about 1000ng/ml. In an alternate embodiment, the Wnt ligand may be used at a concentration of about 10ng/ml to about 100ng/ml. In one embodiment, the concentration of the Wnt ligand is about 20ng/ml.

IGF-1 may be used at a concentration of about 1ng/ml to about 100ng/ml. In an alternate embodiment, the IGF-1may be used at a concentration of about 10ng/ml to about 100ng/ml. In one embodiment, the concentration of IGF-1 is about 50ng/ml.

The cells expressing pluripotency markers derived by the methods of the present invention are capable of expansion in culture under hypoxic conditions, on tissue culture substrate that is not pre-treated with a protein or an extracellular matrix.

The cells expressing pluripotency markers derived by the methods of the present invention express at least one of the following pluripotency markers selected from the group consisting of: ABCG2, cripto, FoxD3, Connexin43, Connexin45, Oct4, SOX-2, Nanog, hTERT, UTF-1, ZFP42, SSEA-3, SSEA-4, Tra1-60, and Tra1-81.

In one embodiment, the cells expressing pluripotency markers derived by the methods of the present invention are capable of expressing markers characteristic of pre-primitive streak cells.

In one embodiment, the cells expressing pluripotency markers derived by the methods of the present invention are capable of expressing markers characteristic of primitive streak cells.

In one embodiment, the cells expressing pluripotency markers derived by the methods of the present invention are capable of expressing markers characteristic of mesendoderm cells.

In one embodiment, the cells expressing pluripotency markers derived by the methods of the present invention are capable of expressing markers characteristic of definitive endoderm cells.

Further differentiation of cells expressing pluripotency markers derived by the methods of the present invention

Cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage by any method in the art.

For example, cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in D'Amour et al, Nature Biotechnology 23, 1534 - 1541 (2005).

For example, cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in Shinozaki et al, Development 131, 1651 - 1662 (2004).

For example, cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in McLean et al, Stem Cells 25, 29 - 38 (2007).

For example, cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in D'Amour et al, Nature Biotechnology 24, 1392 - 1401 (2006).

For example, cells expressing pluripotency markers derived by the methods of the present invention may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage by culturing the pluripotent stem cells in medium containing activin-A in the absence of serum, then culturing the cells with activin-A and serum, and then culturing the cells with activin-A and serum of a different concentration. An example of this method is disclosed in D'Amour et al, Nature Biotechnology, 23, 1534-1541, 2005.

Further differentiation of cells expressing markers characteristic of the definitive endoderm lineage

Cells expressing markers characteristic of the definitive endoderm lineage may be differentiated into cells expressing markers characteristic of the pancreatic endoderm lineage by any method in the art.

For example, cells expressing markers characteristic of the definitive endoderm lineage may be differentiated into cells expressing markers characteristic of the pancreatic endoderm lineage according to the methods disclosed in D'Amour et al, Nature Biotechnology 24, 1392 - 1401 (2006).

For example, cells expressing markers characteristic of the definitive endoderm lineage are further differentiated into cells expressing markers characteristic of the pancreatic endoderm lineage, by treating the cells expressing markers characteristic of the definitive endoderm lineage with a fibroblast growth factor and KAAD-cyclopamine, then removing the medium containing the fibroblast growth factor and KAAD-cyclopamine and subsequently culturing the cells in medium containing retinoic acid, a fibroblast growth factor and KAAD-cyclopamine. An example of this method is disclosed in D' Amour et al, Nature Biotechnology, 24: 1392-1401, (2006).

Further differentiation of cells expressing markers characteristic of the pancreatic endoderm lineage

Cells expressing markers characteristic of the pancreatic endoderm lineage may be differentiated into cells expressing markers characteristic of the pancreatic endocrine lineage by any method in the art.

For example, cells expressing markers characteristic of the pancreatic endoderm lineage may be differentiated into cells expressing markers characteristic of the pancreatic endocrine lineage according to the methods disclosed in D'Amour et al, Nature Biotechnology 24, 1392 - 1401 (2006).

Without being subject to limitation, the following sections contain examples of methods to obtain cells that are suitable starting materials for forming cells expressing pluripotency markers and markers characteristic of the definitive endoderm lineage according to the methods of the present invention.

Isolation, expansion and culture of human embryonic stem cells

Characterization of human embryonic stem cells: Human embryonic stem cells may express one or more of the stage-specific embryonic antigens (SSEA) 3 and 4, and markers detectable using antibodies designated Tra-1-60 and Tra-1-81 (Thomson et al., Science 282:1145, 1998). Differentiation of human embryonic stem cells in nitro results in the loss of SSEA-4, Tra- 1-60, and Tra-1-81 expression (if present) and increased expression of SSEA-1. Undifferentiated human embryonic stem cells typically have alkaline phosphatase activity, which can be detected by fixing the cells with 4% paraformaldehyde, and then developing with Vector Red as a substrate, as described by the manufacturer (Vector Laboratories, Burlingame Calif.). Undifferentiated pluripotent stem cells also typically express Oct-4 and TERT, as detected by RT-PCR.

Another desirable phenotype of propagated human embryonic stem cells is a potential to differentiate into cells of all three germinal layers: endoderm, mesoderm, and ectoderm tissues. Pluripotency of human embryonic stem cells can be confirmed, for example, by injecting cells into SCID mice, fixing the teratomas that form using 4% paraformaldehyde, and then examining them histologically for evidence of cell types from the three germ layers. Alternatively, pluripotency may be determined by the creation of embryoid bodies and assessing the embryoid bodies for the presence of markers associated with the three germinal layers.

Propagated human embryonic stem cell lines may be karyotyped using a standard G-banding technique and compared to published karyotypes of the corresponding primate species. It is desirable to obtain cells that have a "normal karyotype", which means that the cells are euploid, wherein all human chromosomes are present and not noticeably altered.

Sources of human Embryonic stem cells: Types of human embryonic stem cells include established lines of human embryonic cells derived from tissue formed after gestation, including pre-embryonic tissue (such as, for example, a blastocyst), embryonic tissue, or fetal tissue taken any time during gestation, typically but not necessarily before approximately 10-12 weeks gestation. Non-limiting examples relevant to the disclosure are established lines of human embryonic stem cells or human embryonic germ cells, such as, for example the human embryonic stem cell lines H1, H7, and H9 (WiCell). Also disclosed is use of the compositions of this disclosure during the initial establishment or stabilization of such cells, in which case the source cells would be primary pluripotent cells taken directly from the source tissues. Also relevant to the disclosure are cells taken from a pluripotent stem cell population already cultured in the absence of feeder cells. Also relevant to the disclosure are mutant human embryonic stem cell lines, such as, for example, BGOlv (BresaGen, Athens, GA).

In one part of the disclosure, Human embryonic stem cells are prepared as described by Thomson et al. (U.S. Pat. No. 5,843,780 ; Science 282:1145, 1998; Curr. Top. Dev. Biol. 38:133 ff., 1998; Proc. Natl. Acad. Sci. U.S.A. 92:7844, 1995).

Culture of human embryonic stem cells: In one embodiment, human embryonic stem cells are cultured in a culture system that is essentially free of feeder cells, but nonetheless supports proliferation of human embryonic stem cells without undergoing substantial differentiation. The growth of human embryonic stem cells in feeder-free culture without differentiation is supported using a medium conditioned by culturing previously with another cell type. Alternatively, the growth of human embryonic stem cells in feeder-free culture without differentiation is supported using a chemically defined medium.

In an alternate embodiment, human embryonic stem cells are initially cultured layer of feeder cells that support the human embryonic stem cells in various ways. The human embryonic are then transferred to a culture system that is essentially free of feeder cells, but nonetheless supports proliferation of human embryonic stem cells without undergoing substantial differentiation.

Examples of conditioned media suitable for use in the present disclosure are disclosed in US20020072117 , US6642048 , WO2005014799 , and Xu et al (Stem Cells 22: 972-980, 2004).

An example of a chemically defined medium suitable for use in the present disclosure may be found in US20070010011 .

Suitable culture media may be made from the following components, such as, for example, Dulbecco's modified Eagle's medium (DMEM), Gibco # 11965-092; Knockout Dulbecco's modified Eagle's medium (KO DMEM), Gibco # 10829-018; Ham's F12/50% DMEM basal medium; 200 mM L-glutamine, Gibco #15039-027; non-essential amino acid solution, Gibco 11140-050; β- mercaptoethanol, Sigma # M7522; human recombinant basic fibroblast growth factor (bFGF), Gibco # 13256-029.

In one embodiment, the human embryonic stem cells are plated onto a suitable culture substrate that is treated prior to treatment according to the methods of the present disclosure. In one embodiment, the treatment is an extracellular matrix component, such as, for example, those derived from basement membrane or that may form part of adhesion molecule receptor-ligand couplings. In one embodiment, the suitable culture substrate is MATRIGEL (Becton Dickenson). MATRIGEL is a soluble preparation from Engelbreth-Holm-Swarm tumor cells that gels at room temperature to form a reconstituted basement membrane.

Other extracellular matrix components and component mixtures are suitable as an alternative. This may include laminin, fibronectin, proteoglycan, entactin, heparan sulfate, and the like, alone or in various combinations.

The human embryonic stem cells are plated onto the substrate in a suitable distribution and in the presence of a medium that promotes cell survival, propagation, and retention of the desirable characteristics. All these characteristics benefit from careful attention to the seeding distribution and can readily be determined by one of skill in the art.

The human embryonic stem cells are then removed from the treated tissue culture substrate and plated onto a non-treated tissue culture substrate, prior to treatment according to the methods of the present invention to form cells expressing pluripotency markers and markers characteristic of the definitive endoderm lineage.

Differentiation of human embryonic stem cells into cells expressing markers characteristic of the definitive endoderm lineage

Human embryonic stem cells may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage by any method in the art. The cells expressing markers characteristic of the definitive endoderm lineage are suitable for treating according to the methods of the present disclosure.

For example, human embryonic stem cells may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in D'Amour et al, Nature Biotechnology 23, 1534 - 1541 (2005).

For example, human embryonic stem cells may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in Shinozaki et al, Development 131, 1651 - 1662 (2004).

For example, human embryonic stem cells may be differentiated into cells expressing markers characteristic of the definitive endoderm lineage according to the methods disclosed in McLean et al, Stem Cells 25, 29 - 38 (2007).

Differentiation of human embryonic stem cells cultured on an extracellular matrix into cells expressing markers characteristic of the definitive endoderm lineage

In one embodiment, the present disclosure provides a method for differentiating human embryonic stem cells expressing markers characteristic of the definitive endoderm lineage, comprising the steps of:

Plating the human embryonic stem cells on a tissue culture substrate coated with an extracellular matrix, and
Culturing the human embryonic stem cells with activin-A and a Wnt ligand.

The cells expressing markers characteristic of the definitive endoderm lineage are then subsequently treated by the methods of the present disclosure to form cells expressing pluripotency markers and markers characteristic of the definitive endoderm lineage.

Culturing the human embryonic stem cells with activin-A and a Wnt ligand may be performed in a single culture medium. Alternatively, culturing the human embryonic stem cells with activin-A and a Wnt ligand may be performed in more than one culture media. In one embodiment, culturing the human embryonic stem cells with activin-A and a Wnt ligand is performed in two culture media.

Extracellular Matrix: In one aspect of the present disclosure, the human embryonic stem cells are cultured and differentiated on a tissue culture substrate coated with an extracellular matrix. The extracellular matrix may be a solubilized basement membrane preparation extracted from mouse sarcoma cells (which is sold by BD Biosciences under the trade name MATRIGEL). Alternatively, the extracellular matrix may be growth factor-reduced MATRIGEL. Alternatively, the extracellular matrix may fibronectin. In an alternate embodiment, the human embryonic stem cells are cultured and differentiated on tissue culture substrate coated with human serum.

The extracellular matrix may be diluted prior to coating the tissue culture substrate. Examples of suitable methods for diluting the extracellular matrix and for coating the tissue culture substrate may be found in Kleinman, H.K., et al., Biochemistry 25:312 (1986), and Hadley, M.A., et al., J.Cell.Biol. 101:1511 (1985).

In one embodiment, the extracellular matrix is MATRIGEL. In one embodiment, the tissue culture substrate is coated with MATRIGEL at a 1:10 dilution. In an alternate embodiment, the tissue culture substrate is coated with MATRIGEL at a 1:15 dilution. In an alternate embodiment, the tissue culture substrate is coated with MATRIGEL at a 1:30 dilution. In an alternate embodiment, the tissue culture substrate is coated with MATRIGEL at a 1:60 dilution.

In one embodiment, the extracellular matrix is growth factor-reduced MATRIGEL. In one embodiment, the tissue culture substrate is coated with growth factor-reduced MATRIGEL at a 1:10 dilution. In an alternate embodiment, the tissue culture substrate is coated with growth factor-reduced MATRIGEL at a 1:15 dilution. In an alternate embodiment, the tissue culture substrate is coated with growth factor-reduced MATRIGEL at a 1:30 dilution. In an alternate embodiment, the tissue culture substrate is coated with growth factor reduced MATRIGEL at a 1:60 dilution.

Differentiation of human embryonic stem cells into cells expressing markers characteristic of the definitive endoderm lineage on an extracellular matrix, using a single culture medium: In one embodiment, the present disclosure provides a method for differentiating human embryonic stem cells expressing markers characteristic of the definitive endoderm lineage, comprising the steps of:

The culture medium should contain sufficiently low concentrations of certain factors to allow the differentiation of human embryonic stem cells to definitive endoderm, such as, for example insulin and IGF (as disclosed in WO2006020919 ). This may be achieved by lowering the serum concentration, or alternatively, by using chemically defined media that lacks insulin and IGF. Examples of chemically defined media are disclosed in Wiles et al (Exp Cell Res. 1999 Feb 25; 247(1): 241-8.).

The culture medium may have a serum concentration in the range of about 0% to about 10%. In an alternate embodiment, the concentration may be in the range of about 0% to about 5%. In an alternate embodiment, the concentration may be in the range of about 0% to about 2%. In an alternate embodiment, the concentration may be about 2%.

The time of culturing with activin-A and a Wnt ligand may range from about 1 day to about 7 days. In an alternate embodiment, the time of culturing may range from about 1 day to about 3 days. In an alternate embodiment, the time of culturing may be about 3 days.

Activin-A may be used at any concentration suitable to cause differentiation of the human embryonic stem cells. The concentration maybe from about 1pg/ml to about 100µg/ml. In an alternate embodiment, the concentration may be about 1pg/ml to about 1µg/ml. In another alternate embodiment, the concentration may be about 1pg/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 50ng/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 100ng/ml.

The choice of the Wnt ligand may be optimized to improve the efficiency of the differentiation process. The Wnt ligand may be selected from the group consisting of Wnt-1, Wnt-3a, Wnt-5a and Wnt-7a. In one embodiment, the Wnt ligand is Wnt-1. In an alternate embodiment, the Wnt ligand is Wnt-3a.

The Wnt ligand may be at a concentration of about 1ng/ml to about 1000ng/ml. In an alternate embodiment, the concentration may be about 10ng/ml to about 100ng/ml.

The single culture medium may also contain a GSK-3B inhibitor. The GSK-3B inhibitor may be selected from the group consisting of GSK-3B inhibitor IX and GSK-3B inhibitor XI. In one embodiment, the GSK-3B inhibitor is GSK-3B inhibitor IX.

When culturing human embryonic stem cells with a GSK-3B inhibitor, the concentration of the GSK-3B inhibitor may be from about 1nM to about 1000nM. In an alternate embodiment, the human embryonic stem cells are cultured with the GSK-3B inhibitor at a concentration of about 10nM to about 100nM.

The single culture medium may also contain at least one other additional factor that may enhance the formation of cells expressing markers characteristic of the definitive endoderm lineage from human embryonic stem cells. Alternatively, the at least one other additional factor may enhance the proliferation of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present invention. Further, the at least one other additional factor may enhance the ability of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present invention to form other cell types, or improve the efficiency of any other additional differentiation steps.

The at least one additional factor may be, for example, nicotinamide, members of TGF-β family, including TGF-β1, 2, and 3, serum albumin, members of the fibroblast growth factor family, platelet-derived growth factor-AA, and -BB, platelet rich plasma, insulin growth factor (IGF-I, II), growth differentiation factor (GDF-5, -6, -8, -10, 11), glucagon like peptide-I and II (GLP-I and II), GLP-1 and GLP-2 mimetobody, Exendin-4, retinoic acid, parathyroid hormone, insulin, progesterone, aprotinin, hydrocortisone, ethanolamine, beta mercaptoethanol, epidermal growth factor (EGF), gastrin I and II, copper chelators such as, for example, triethylene pentamine, forskolin, Na-Butyrate, activin, betacellulin, ITS, noggin, neurite growth factor, nodal, valporic acid, trichostatin A, sodium butyrate, hepatocyte growth factor (HGF), sphingosine 1, VEGF, MG132 (EMD, CA), N2 and B27 supplements (Gibco, CA), steroid alkaloid such as, for example, cyclopamine (EMD, CA), keratinocyte growth factor (KGF), Dickkopf protein family, bovine pituitary extract, islet neogenesis-associated protein (INGAP), Indian hedgehog, sonic hedgehog, proteasome inhibitors, notch pathway inhibitors, sonic hedgehog inhibitors, or combinations thereof.

The at least one other additional factor may be supplied by conditioned media obtained from pancreatic cells lines such as, for example, PANC-1 (ATCC No: CRL-1469), CAPAN-1 (ATCC No: HTB-79), BxPC-3 (ATCC No: CRL-1687), HPAF-II (ATCC No: CRL-1997), hepatic cell lines such as, for example, HepG2 (ATCC No: HTB-8065), and intestinal cell lines such as, for example, FHs 74 (ATCC No: CCL-241).

Differentiation of human embryonic stem cells into cells expressing markers characteristic of the definitive endoderm lineage on an extracellular matrix, using two culture media: Differentiation of human embryonic stem cells into cells of a definitive endoderm lineage may be accomplished by culturing the human embryonic stem cells with activin-A and a Wnt ligand using two culture media. Thus, the differentiation of the human embryonic stem cells may be accomplished as follows:

Plating the human embryonic stem cells on a tissue culture substrate coated with an extracellular matrix,
Culturing the human embryonic stem cells with activin-A and a Wnt ligand in a first culture medium, and
Culturing the human embryonic stem cells with activin-A in a second culture medium.

The first culture medium may contain serum at a low concentration, and the second culture medium may contain serum at a higher concentration than the first culture medium.

The second culture medium may contain a Wnt ligand.

First Culture Medium: The first culture medium should contain sufficiently low concentrations of certain factors to allow the differentiation of human embryonic stem cells into cells expressing markers characteristic of the definitive endoderm lineage, such as, for example insulin and IGF (as disclosed in WO2006020919 ). This may be achieved by lowing the serum concentration, or alternatively, by using chemically defined media that lacks insulin and IGF. Examples of chemically defined media are disclosed in Wiles et al (Exp Cell Res. 1999 Feb 25; 247(1):241-8.).

In the first culture medium there may be a lower concentration of serum, relative to the second culture medium. Increasing the serum concentration in the second culture medium increases the survival of the cells, or, alternatively, may enhance the proliferation of the cells. The serum concentration of the first medium may be in the range of about 0% to about 10%. Alternatively, the serum concentration of the first medium may be in the range of about 0% to about 2%. Alternatively, the serum concentration of the first medium may be in the range of about 0% to about 1%. Alternatively, the serum concentration of the first medium may be about 0.5%.

When culturing the human embryonic stem cells with activin-A and a Wnt ligand using at least two culture media, the time of culturing in the first culture medium may range from about 1 day to about 3 days.

The first culture medium may also contain a GSK-3B inhibitor. The GSK-3B inhibitor may be added to the first culture medium, to the second culture medium, or to both the first and second culture media.

The GSK-3B inhibitor may be selected from the group consisting of GSK-3B inhibitor IX and GSK-3B inhibitor XI. In one embodiment, the GSK-3B inhibitor is GSK-3B inhibitor IX.

The first culture medium may also contain at least one other additional factor that may enhance the formation of cells expressing markers characteristic of the definitive endoderm lineage from human embryonic stem cells. Alternatively, the at least one other additional factor may enhance the proliferation of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present disclosure. Further, the at least one other additional factor may enhance the ability of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present disclosure to form other cell types, or improve the efficiency of any other additional differentiation steps.

The at least one additional factor may be, for example, nicotinamide, members of the TGF-β family, including TGF-β1, 2, and 3, serum albumin, members of the fibroblast growth factor family, platelet-derived growth factor-AA, and -BB, platelet rich plasma, insulin growth factor (IGF-I, II), growth differentiation factor (GDF-5, -6, -8, -10, 11), glucagon like peptide-I and II (GLP-I and II), GLP-1 and GLP-2 mimetobody, Exendin-4, retinoic acid, parathyroid hormone, insulin, progesterone, aprotinin, hydrocortisone, ethanolamine, beta mercaptoethanol, epidermal growth factor (EGF), gastrin I and II, copper chelators such as, for example, triethylene pentamine, forskolin, Na-Butyrate, activin, betacellulin, ITS, noggin, neurite growth factor, nodal, valporic acid, trichostatin A, sodium butyrate, hepatocyte growth factor (HGF), sphingosine-1, VEGF, MG132 (EMD, CA), N2 and B27 supplements (Gibco, CA), steroid alkaloid such as, for example, cyclopamine (EMD, CA), keratinocyte growth factor (KGF), Dickkopf protein family, bovine pituitary extract, islet neogenesis-associated protein (INGAP), Indian hedgehog, sonic hedgehog, proteasome inhibitors, notch pathway inhibitors, sonic hedgehog inhibitors, or combinations thereof.

Second Culture Medium: The second culture medium should contain certain factors, such as, for example, insulin and IGF (as disclosed in WO2006020919 ), at a sufficient concentration to promote the survival of the cultured cells. This may be achieved by increasing the serum concentration, or, alternatively, by using chemically defined media where the concentrations of insulin and IGF are increased relative to the first culture medium. Examples of chemically defined media are disclosed in Wiles et al (Exp Cell Res. 1999 Feb 25; 247(1): 241-8.).

In a second culture medium having higher concentrations of serum, the serum concentration of the second culture medium may be in the range about 0.5% to about 10%. Alternatively, the serum concentration of the second culture medium may be in the range of about 0.5% to about 5%. Alternatively, the serum concentration of the second culture medium may be in the range of about 0.5% to about 2%. Alternatively, the serum concentration of the second culture medium may be about 2%. When culturing human embryonic stem cells with the second culture medium, the time of culturing may range from about 1 day to about 4 days.

Similar to the first culture medium, Activin-A may be used at any concentration suitable to cause differentiation of the human embryonic stem cells. The concentration maybe from about 1pg/ml to about 100µg/ml. In an alternate embodiment, the concentration may be about 1pg/ml to about 1µg/ml. In another alternate embodiment, the concentration may be about 1pg/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 50ng/ml to about 100ng/ml. In another alternate embodiment, the concentration may be about 100ng/ml.

The second culture medium may also contain a GSK-3B inhibitor. The GSK-3B inhibitor may be added to the first culture medium, to the second culture medium, or to both the first and second culture media.

Similar to the first culture medium, the second culture medium may also contain at least one other additional factor that may enhance the formation of cells expressing markers characteristic of the definitive endoderm lineage from human embryonic stem cells. Alternatively, the at least one other additional factor may enhance the proliferation of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present invention. Further, the at least one other additional factor may enhance the ability of the cells expressing markers characteristic of the definitive endoderm lineage formed by the methods of the present invention to form other cell types, or improve the efficiency of any other additional differentiation steps.

The at least one additional factor may be, for example, nicotinamide, members of the EGF-β family, including TGF-β1, 2, and 3, serum albumin, members of the fibroblast growth factor family, platelet-derived growth factor-AA, and -BB, platelet rich plasma, insulin growth factor (IGF-I, II), growth differentiation factor (GDF-5, -6, -8, -10, 11), glucagon like peptide-I and II (GLP-I and II), GLP-1 and GLP-2 mimetobody, Exendin-4, retinoic acid, parathyroid hormone, insulin, progesterone, aprotinin, hydrocortisone, ethanolamine, beta mercaptoethanol, epidermal growth factor (EGF), gastrin I and II, copper chelators such as, for example, triethylene pentamine, forskolin, Na-Butyrate, activin, betacellulin, ITS, noggin, neurite growth factor, nodal, valporic acid, trichostatin A, sodium butyrate, hepatocyte growth factor (HGF), sphingosine-1, VEGF, MG132 (EMD, CA), N2 and B27 supplements (Gibco, CA), steroid alkaloid such as, for example, cyclopamine (EMD, CA), keratinocyte growth factor (KGF), Dickkopf protein family, bovine pituitary extract, islet neogenesis-associated protein (INGAP), Indian hedgehog, sonic hedgehog, proteasome inhibitors, notch pathway inhibitors, sonic hedgehog inhibitors, or combinations thereof.

The present invention is further illustrated, but not limited by, the following examples.

Reference Example 1 Human Embryonic Stem Cell Culture

The human embryonic stem cell lines H1, H7 and H9 were obtained from WiCell Research Institute, Inc., (Madison, WI) and cultured according to instructions provided by the source institute. Briefly, cells were cultured on mouse embryonic fibroblast (MEF) feeder cells in ES cell medium consisting of DMEM/F12 (Invitrogen/GIBCO) supplemented with 20% knockout serum replacement, 100 nM MEM nonessential amino acids, 0.5 mM beta-mercaptoethanol, 2mM L-glutamine with 4ng/ml human basic fibroblast growth factor (bFGF) (all from Invitrogen/GIBCO). MEF cells, derived from E13 to 13.5 mouse embryos, were purchased from Charles River. MEF cells were expanded in DMEM medium supplemented with 10% FBS (Hyclone), 2mM glutamine, and 100 mM MEM nonessential amino acids. Sub-confluent MEF cell cultures were treated with 10µg/ml mitomycin C (Sigma, St. Louis, MO) for 3h to arrest cell division, then trypsinized and plated at 2x104/cm2 on 0.1% bovine gelatin-coated dishes. MEF cells from passage two through four were used as feeder layers. Human embryonic stem cells plated on MEF cell feeder layers were cultured at 37°C in an atmosphere of 5% CO₂ within a humidified tissue culture incubator. When confluent (approximately 5-7 days after plating), human embryonic stem cells were treated with 1mg/ml collagenase type IV (Invitrogen/GIBCO) for 5-10 min and then gently scraped off the surface using a 5-ml pipette. Cells were centrifuged at 900 rpm for 5 min, and the pellet was resuspended and re-plated at a 1:3 to 1:4 ratio of cells in fresh culture medium.

In parallel, H1, H7, and H9 human embryonic stem cells were also seeded on plates coated with a 1:30 dilution of growth factor reduced MATRIGEL (BD Biosciences) and cultured in MEF-conditioned media supplemented with 8 ng/ml bFGF. The cells cultured on MATRIGEL were routinely passaged with collagenase IV (Invitrogen/GIBCO), Dispase (BD Biosciences) or LIBERASE enzyme. Some of the human embryonic stem cell cultures were incubated under hypoxic conditions (approximately 3% O₂).

Reference Example 2 Fluorescence-Activated Cell Sorting (FACS) Analysis

Adhered human embryonic stem cells were removed from culture plates by a five-minute incubation with TrypLE™ Express solution (Invitrogen, CA). Released cells were resuspended in human embryonic stem cell culture medium and recovered by centrifugation, followed by washing and resuspending the cells in a staining buffer consisting of 2% BSA, 0.05% sodium azide in PBS (Sigma, MO). As appropriate, the cells were Fc-receptor blocked for 15 minutes using a 0.1% γ-globulin (Sigma) solution. Aliquots (approximately 1x10⁵ cells) were incubated with either phycoerythirin (PE) or allophycocyanin (APC) conjugated monoclonal antibodies (5 µl antibody per 1x10⁶ cells), as indicated in Table IA, or with an unconjugated primary antibody. Controls included appropriate isotype matched antibodies, unstained cells, and cells stained only with secondary conjugated antibody. All incubations with antibodies were performed for 30 mins at 4°C, after which the cells were washed with the staining buffer. Samples that were stained with unconjugated primary antibodies were incubated for an additional 30 mins at 4°C with secondary conjugated PE or -APC labeled antibodies. See Table IB for a list of secondary antibodies used. Washed cells were pelleted and resuspended in the staining buffer, and the cell surface molecules were identified using a FACS Array (BD Biosciences) instrument, collecting at least 10,000 events.

Reference Example 3 Immunocytochemistry

Adhered cells were fixed with 4% paraformaldheyde for 20 min at room temperature. Fixed cells were blocked for 1 h at room temperature with PBS/0.1%BSA/10% normal chick serum /0.5% Triton X-100 and then incubated overnight with primary antibodies in PBS/0.1%BSA/10% normal chick serum at 4°C. The list of primary antibodies and their working dilutions are shown in Table IA. After three washes in PBS/0.1% BSA, fluorescent secondary antibodies (Table IB) at a 1:100 dilution in PBS were incubated with cells for 1 h at room temperature to allow binding. Control samples included reactions where the primary antibody was omitted or where the primary antibody was replaced with corresponding matched negative control immunoglobulins at the same concentration as the primary antibodies. Stained samples were rinsed; a drop of PROLONG® (Invitrogen, CA) containing diamidino-2-phenylindole, dihydrochloride (DAPI) was added to each sample to counter-stain the nucleus and to function as an anti-fade reagent. Images were acquired using a Nikon Confocal Eclipse C-1 inverted microscope (Nikon, Japan) and a 10-60X objective.

Example 4 PCR Analysis of ES Derived-Cells

RNA extraction, purification, and cDNA synthesis: RNA samples were purified by binding to a silica-gel membrane (Rneasy Mini Kit, Qiagen, CA) in the presence of an ethanol-containing, high-salt buffer followed by washing to remove contaminants. The RNA was further purified using a TURBO DNA-free kit (Ambion, INC), and high-quality RNA was then eluted in water. Yield and purity were assessed by A260 and A280 readings on a spectrophotometer. CDNA copies were made from purified RNA using an ABI (ABI, CA) high capacity cDNA archive kit.

Real-time PCR amplification and quantitative analysis: Unless otherwise stated, all reagents were purchased from Applied Biosystems. Real-time PCR reactions were performed using the ABI PRISM® 7900 Sequence Detection System. TAQMAN® UNIVERSAL PCR MASTER MIX® (ABI, CA) was used with 20 ng of reverse transcribed RNA in a total reaction volume of 20 µl. Each cDNA sample was run in duplicate to correct for pipetting errors. Primers and FAM-labeled TAQMAN®probes were used at concentrations of 200 nM. The level of expression for each target gene was normalized using a human glyceraldehyde-3-phosphate dehydrogenase (GAPDH) endogenous control previously developed by Applied Biosystems. Primer and probe sets are listed in Table II. SOX-17 primers were designed using the PRIMERS program (ABI, CA) and were the following sequences: SOX-17: TGGCGCAGCAGATACCA, AGCGCCTTCCACGACTTG, and CCAGCATCTTGCTCAACTCGGCG. After an initial incubation at 50°C for 2 min followed by 95°C for 10 min, samples were cycled 40 times in two stages - a denaturation step at 95°C for 15 sec followed by an annealing/extension step at 60°C for 1 min. Data analysis was carried out using GENEAMP®7000 Sequence Detection System software. For each primer/probe set, a Ct value was determined as the cycle number at which the fluorescence intensity reached a specific value in the middle of the exponential region of amplification. Relative gene expression levels were calculated using the comparative Ct method. Briefly, for each cDNA sample, the endogenous control Ct value was subtracted from the gene of interest Ct to give the delta Ct value (ΔCt). The normalized amount of target was calculated as 2-ΔCt, assuming amplification to be 100% efficiency. Final data were expressed relative to a calibrator sample.

Reference Example 5 Differentiation of Human Embryonic Stem Cells Cultured on Tissue Culture Substrate Coated with MATRIGEL to Definitive Endoderm (DE)

Cells from the human embryonic stem cell line H9 at passage 54 were cultured under hypoxic conditions (approximately 3% O₂) and plated on MATRIGEL (1:30 dilution) coated dishes were exposed to DMEM/F12 medium supplemented with 0.5% FBS, 20 ng/ml WNT-3a (Catalog# 1324-WN-002, R&D Systems, MN), and 100 ng/ml Activin-A (R&D Systems, MN) for two days followed by treatment with DMEM/F12 media supplemented with 2% FBS and 100 ng/ml Activin-A (AA) for an additional 3-4 days. Figure 1 depicts the expression of CXCR4 by FACS at day 4. Figure 2 displays the real-time PCR data for cultures of cells from the human embryonic stem cell line H9 treated with low serum + AA + WNT3A at days 4 and 6. This protocol resulted in significant upregulation of definitive endoderm markers. This procedure will be further referred to as the DE (Definite Endoderm) protocol.

Reference Example 6 Isolation and Expansion of Human Embryonic Stem Cell Derived Cells Differentiated to the Definitive Endoderm Stage

Cells from the human embryonic stem cell lines H1 and H9 various passages (Passage 30-54) were cultured under hypoxic conditions (approximately 3% O₂) for at least three passages. The cells were cultured in MEF-CM supplemented with 8 ng/ml of bFGF and plated on MATRIGEL coated plates according to Example 1. The cells were exposed to the DE protocol outlined in Example 5. At days 3-6, the cultures were exposed to TrypLE™ Express solution (Invitrogen, CA) for 5 mins. Released cells were resuspended in DMEM-F12 + 2% FBS medium, recovered by centrifugation, and counted using a hemocytometer. The released cells were seeded at 1000-10,000 cells/cm² on tissue culture polystyrene (TCPS) treated flasks and cultured in DMEM-F12 + 2% FBS + 100 ng/ml activin-A + 20 ng/ml WNT-3A under hypoxic conditions (approximately 3% O₂) at 37 °C in standard tissue culture incubator. The TCPS flaks were not coated with MATRIGEL or other extracellular matrix proteins. The media was changed daily. In some cultures, the media was further supplemented with 10-50 ng/ml of IGF-I (insulin growth factor-I from R&D Systems, MN) or 1X ITS (Insulin, transferrin, and selenium from Invitrogen, Ca). In some of the culture conditions the basal media (DM-F12 + 2% FBS) was further supplemented with 0.1 mM mercaptoethanol (Invitrogen, CA) and non-essential amino acids (1X, NEAA from Invitrogen, CA). The first passage cells are referred to as P1. In parallel, similar cultures were established under normoxic conditions (approximately 21% O₂). The outline of this isolation procedure is depicted in Figure 3 .

Following 5-15 days of culturing, distinct cell colonies appeared surrounded by a large number of enlarged cells that appear to be in senescence ( Figure 4a-b ). At approximately 50-60% confluency, the cultures were passaged by exposure to TrypLE™ Express solution for 5 mins at room temperature. The released cells were resuspended in DMEM-F12 + 2% FBS medium, recovered by centrifugation, and seeded at 10,000 cells/cm² on tissue culture polystyrene (TCPS) treated flasks in DMEM-F12 + 2%FBS + 100 ng/ml activin-A + 20 ng/ml WNT-3A +/- 50 ng/ml of IGF-I. This media will be further referred to as the "growth media". Figure 4 c depicts the morphology of cells at passage 3 seeded at 10,000 cells/cm². At passage 3 (panel c) following the initial isolation, the cells appeared to have a uniform epithelial-like morphology with a large nucleus to cytoplasm ratio.

In some cultures the growth media was further supplemented with 1X NEAA plus 0.1 mM mercaptoethanol. Following three to four passages, the attached cells appeared to have a uniform morphology with a large nucleus to cytoplasm ratio. Parallel cultures established under normoxic conditions failed to show robust colony formation by attached cells. Following 2-3 passages, the cultures established under normoxic conditions were abandoned due to poor growth rate.

Reference Example 7 Role of activin-A, WNT3A, and IGF-I in Expansion and Maintenance of DE Markers Following Multiple Passages

Cultures derived from the parental human embryonic stem cell line H9 according to the methods described in Example 6 were passaged every 4-7 days. Figure 5 depicts real-time PCR results for the expanded cells cultured in 2% FBS + DMEM-F12 + 100 ng/ml of activin-A + 20 of WNT3A for three passages. This data is for a line isolated at day6 of the DE protocol outlined in Example 5. There is a clear decrease in DE markers, such as SOX-17 and HNF-3 beta following each passage. As shown in Figure 6 , addition of WNT3A to the growth media containing activin-A led to a significant boost in the expression of DE markers. However, addition of 50 ng/ml of IGF-I and withdrawal of Activin-A and WNT-3A ( Figure 7 a-c ) led to a precipitous drop in the expression of DE markers along with OCT-4 and an increase in expression of visceral endoderm markers, such as SOX-7 and AFP. Figure 8 a-c depicts the morphology of expanded cells derived from H9p54 at passage 5 cultured in a) 2% FBS + DMF12 + 100 ng/ml of activin-A + 20 ng/ml of WNT-3A, b) 2% FBS + DM-F12 + 100 ng/ml of activin-A, c) 2% FBS + DM-F12 + 50 ng/ml of IGF-I. Morphology of cells cultured in the presence of activin-A or activin-A + WNT3A were very similar and distinct from morphology of cells cultured in 2% FBS + IGF-I.

Reference Example 8 Expansion Potential of Human Embryonic Stem Cell Derived Cells Differentiated to the Definitive Endoderm stage

Cultures established from the parental human embryonic stem cell line H9 according to the methods described in Example 6 were passaged every 4-5 days when the growth media contained 50 ng/ml of IGF-I or ITS. However, cultures fed with growth media lacking the IGF or ITS supplements showed slower growth rate and were passaged every 5-7 days. The population doubling time of cells fed with growth media + 50 ng/ml of IGF-I was approximately 55 hrs where as the population doubling time of cultures fed only with the growth media was approximately 75 hrs. The cell population expanded according to Example 6 will be referred to as EXPRES cells (Expandable PRE-primitive Streak cells). Table III lists various EXPRES cells established according to methods outlined in Example 6. The expansion potential of two cell lines (EXPRES 01 and 02) is depicted in Figure 9 .

Reference Example 9 Derivation of EXPRES Cells from Suspensions of Single Human Embryonic Stem Cells

Cells from the human embryonic stem cell lines H1 P33 and H9 P45 were cultured under hypoxic conditions (approximately 3% O₂) for at least three passages. The cells were cultured in MEF-CM supplemented with 8 ng/ml of bFGF and plated on MATRIGEL coated plates according to Example 1. At approximately 60% confluency, the cultures were exposed to TrypLE™ Express solution (Invitrogen, CA) for 5 mins. Released cells were resuspended in DMEM-F12 + 2% FBS medium, recovered by centrifugation, and counted using a hemocytometer. The released cells were seeded at 1000 to 10,000 cells/cm² on tissue culture polystyrene (TCPS) treated flasks and cultured in DM-F12 + 2% FBS + 100 ng/ml activin-A + 20 ng/ml WNT-3A + 50 ng/ml of IGF-I + 0.1 mM mercaptoethanol (Invitrogen, CA) and non-essential amino acids (1X, NEAA from Invitrogen, CA) under hypoxic conditions (approximately 3% O₂) at 37 °C in a standard tissue culture incubator. The TCPS flasks were not coated with MATRIGEL or other extarcellular matrix proteins. The media was changed daily. The first passage cells are referred to as P1. In parallel, similar cultures were established under normoxic conditions (approximately 21% O₂). Cultures established under atmospheric conditions did not result in colony formation and there was poor cell proliferation. However, cultures established under hypoxic conditions resulted in formation of many colonies ( Figure 10 ) resembling embryonic stem cell colonies cultured on MATRIGEL or on MEF feeders. These cultures closely resemble the properties of EXPRES cells isolated during ES to DE differentiation.

Reference Example 10 Expression of Cell Surface Proteins by EXPRES Cells

The cell lines EXPRES 01 and EXPRES 02 were evaluated for expression of various cell-surface markers including markers associated with pluripotency. Cells from EXPRES 01 were evaluated at passages 9 to 24. Cells from EXPRES 02 were evaluated at passages 7 to 20. Both lines exhibited strong expression of pluripotency markers typically assigned to undifferentiated human embryonic stem cells. However, the EXPRES 02 line showed a higher percentage of expression of differentiation markers, such as CXCR4, LIF receptor, and NCAM as compared to the EXPRES 01 line. Representative FACS plots are depicted in Figure 11 for EXPRES 01 P24 and in Figure 12 for EXPRES 02 P21 line. Table IV lists the mean expression levels along with the ranges (in brackets) of the evaluated cell surface markers from three different experiments.

Reference Example 11 Expression of Pluripotency Associated Markers by EXPRES Cells- Immuno fluorescent (IF) Staining

EXPRES 01 and 02 cells maintained in their respective growth media were stained for pluripotency-associated markers using methods outlined in Example 3. Figure 13 depicts IF images for OCT-4, Nanog, SOX-2, and HNF-3 beta for EXPRES 01 P10 cells cultured in 2% FBS + DM-F12 + 100 ng/ml activin-A + 20 ng/ml WNT3A + 50 ng/ml IGF-I. Figure 14 depicts IF images for OCT-4, Nanog, SOX-2, and HNF-3 beta for EXPRES 02 passage 9 cells cultured in 2% FBS + DM-F12 + 100 ng/ml activin-A + 20 ng/ml WNT3A. EXPRES 01 cells strongly stain positive for OCT-4, Nanog, and SOX-2 and weakly for HNF-3 beta. However, EXPRES 02 cells show stronger expression for HNF-3 beta and weaker expression of OCT-4, NANOG, and SOX-2.

Reference Example 12 Expression of Definitive Endoderm and Undifferentiated Embryonic Stem Cell Markers by Real Time PCR

Real-time PCR analysis of embryonic markers (POU5F1, SOX-2, UTF1, ZFP42, Connexin43, Connexin45, FOXD3), extraembryonic markers (AFP, KRT15), ectoderm markers (SOX-1, TUBB3, NESTIN), endoderm markers (FOXA2, IPF1, KRT15, GATA-4), and mesoderm markers (GATA-4, GATA-2, MYOD, MSX1, CFC1, ABCG2) expressed by EXPRES 01 passage 11 and EXPRES 02passage 7 lines cultured in their respective growth media is depicted in Figure 15 a-h. All of the data is normalized to fold change with respect to undifferentiated cells from the human embryonic stem cell line H9, cultured in MEF-CM on MATRIGEL coated plates. As a control, EB bodies were formed from H9 cells using standard methods of collagenase digestion and seeding on non-treated surfaces in DMEM-F12 + 20 % FBS for approximately 10 days. Gene expression of various germ layers was upregulated by EB bodies as compared to undifferentiated ES cells. Another reference RNA was collected from undifferentiated SA002 line (Cellartis, Sweden) cultured on MATRIGEL in MEF-CM. As expected gene expression of various germ layers was strongly upregulated by EB bodies as compared to EXPRES 01, EXPRES 02, SA002, and H9 lines. Both EXPRES 01 and 02 lines showed expression of FOXA2 as compared to undifferentiated SA002 and H9 lines. Neither of the EXPRES lines exhibited strong expression of extra embryonic, mesoderm or ectoderm markers. Furthermore, expression of embryonic markers by EXPRES cells was similar to the SA002 and H9 reference cell lines.

Reference Example 13 Various Growth Media Useful for Expansion of EXPRES Cells

EXPRES cells have been successfully cultured in the following media compositions for at least 2-30 passages:

DM-F12 + 2% FBS + 100 ng/ml AA + 20 ng/ml WNT-3A
DM-F12 + 2% FBS + 100 ng/ml AA + 20 ng/ml WNT-3A + 50 ng/ml IGF-I
DM-F12 + 2% FBS + 100 ng/ml AA + 20 ng/ml WNT-3A + 10 ng/ml IGF-I
DM-F12 + 2% FBS + 50 ng/ml AA + 20 ng/ml WNT-3A + 50 ng/ml IGF-I
DM-F12 + 2% FBS + 50 ng/ml AA + 10 ng/ml WNT-3A + 50 ng/ml IGF-I
DM-F12 + 2% FBS + 50 ng/ml AA + 20 ng/ml WNT-3A + 10 ng/ml IGF-I
DM-F12 + 2% FBS + 100 ng/ml AA + 10 ng/ml WNT-3A + 10 ng/ml IGF-I

HEScGRO defined media (Chemicon, CA)

The basal component of the above listed media may be replaced with similar media such as, RPMI, DMEM, CRML, Knockout™DMEM, and F12.

Reference Example 14 Differentiation of EXPRES Cells Cultured on Tissue Culture Substrate to Definitive Endoderm (DE) cells

EXPRES 01 cells at passage 5 and EXPRES 02 cells at passage 4, cultured on TCPS in their respective media were exposed to DMEM/F12 medium supplemented with 0.5% FBS, 20 ng/ml WNT-3a, and 100 ng/ml activin-A (R&D Systems, MN) for two days followed by treatment with DMEM/F12 media supplemented with 2% FBS and 100 ng/ml activin-A (AA) for an additional 3-5 days. Figure 16 depicts the expression of CXCR4 by FACS at days 4 for EXPRES 01 cells ( Figure 16 a , approximately 17% CXCR4 positive) and EXPRES 02 cells ( Figure 16b , approximately 40% CXCR4 positive). Figure 17 displays the real-time PCR data for EXPRES 01 cell ( Figure 17a ) and EXPRES 02 cell ( Figure 17b ) cultures treated with low serum + AA + WNT3A at days 2-5. Figures 18 and 19 depict immunofluoresence images of EXPRES 01 and 02 cells, respectively, treated with the same treatment mentioned above for 4 days. Overall EXPRES 02 cells appear to show a stronger expression of DE markers as compared to EXPRES 01 cells. As evident by FACS, immuno staining, and PCR data, lowering of serum concentration and removal of IGF did enhance the expression of DE markers. However, the overall expression level of DE markers such as CXCR4 and HNF-3 beta was lower than what we have routinely observed in undifferentiated human ES cultures differentiated to the DE stage.

In order to enhance expression of DE markers, the DE differentiation protocol was changed to the following: EXPRES 01 cells at passage 19 and EXPRES 02 cells at passage 14 cultured on TCPS in their respective media were exposed to DMEM/F12 medium supplemented with 0.5% FBS, 20 ng/ml WNT-3a, 100 ng/ml activin-A, and 100 nM GSK-3B inhibitor IX (Catalog# 361550, Calbiochem, CA) for 4 to 5 days. Figure 20 depicts the expression of CXCR4 by FACS at days 4 for EXPRES 01 ( Figure 20 a , approximately 57% CXCR4 positive) and EXPRES 02 ( Figure 20b , approximately 86% CXCR4 positive). Figure 21 depicts the corresponding immuno fluorescent images at day 5 for EXPRES 01 cells (panels a-f) and EXPRES 02 cells (panels g-l) cells differentiated to the DE stage. Figure 22 displays the real-time PCR data for EXPRES 01 ( Figure 22a ) and EXPRES 02 ( Figure 22b ).

Reference Example 15 Effect of Seeding Density on the Differentiation of EXPRES 01 Cells to DE

EXPRES 01 P31 cells were seeded at 5000, 10000, 20000, or 40000 cells/cm² on TCPS plates in DM-F12 + 2% FBS + 0.1 mM mercaptoethanol + 1X, NEAA + 100 ng/ml activin-A + 20 ng/ml WNT3A under hypoxic conditions (approximately 3% O₂) at 37 °C in standard tissue culture incubator. Following two days post seeding, the media was switched to DMEM-F12 + 0.5% FBS + 100 ng/ml activin-A + 20 ng/ml WNT3A + 100 nM GSK-3B inhibitor IX for four days under hypoxic conditions (approximately 3% O₂) at 37 °C in standard tissue culture incubator. Figure 23 depicts the real-time PCR analysis of definitive endoderm markers at day 4 of differentiation. It appears that a seeding density of at least 10000-20000 cells/cm² is required for the robust formation of definitive endoderm.

Reference Example 16 Telomere Length of EXPRES Cells

The telomere length of two EXPRES lines isolated according to Example 5 along with undifferentiated cells from the human embryonic stem cell line H1 was analyzed by using the Telo TAGGG Telomere Length Assay (Roche, IN) and following the manufacturer's instruction. Figure 24 depicts the telomere length for EXPRES 01 cells at P24, EXPRES 02 cells at P17, H1 cells at P40, high and low telomere controls provided by the kit, along with the scale marker. Both lines appear to have shorter telomere length than undifferentiated ES cells.

Reference Example 17 Further Differentiation of EXPRES Cells Cultured on Tissue Culture Substrate to Pancreatic Endoderm

EXPRES 01 cells at passage 21 underwent a 5 day differentiation by treatment with 100ng/ml activin-A, 10ng/ml of Wnt3a, and 100 nM GSK3beta inhibitor IX in 0.5% FBS, DMEM:F12 media. Cells were analyzed by FACS and showed 80% of the cells were positive for CXCR4. The cells were then treated for 3 days in each of the following steps: 2%FBS DMEM:F12 containing 50ng/ml FGF-10, and 0.25µM KAAD-Cyclopamine (Calbiochem, CA); followed by, 1%B27 DMEM, low glucose containing 50 ng/ml FGF-10, 0.25µM KAAD-Cyclopamine and 1µM Retinoic Acid (Sigma, MO); followed by, 1%B27 DMEM, low glucose containing 1µM DAPT (Calbiochem, CA) plus 50 ng/ml Exendin4 (Sigma, MO); and lastly followed by, 1% B27 DMEM CMRL containing 50ng/ml each of IGF, HGF and Exendin4. Samples were taken at the end of each step, and RNA was extracted for the cells. Q-RT PCR was conducted for the markers shown. As depicted in Figure 25 , Insulin levels were increased 100 fold over untreated cells and PDX-1 levels were also increased over 1000 fold.

Reference Example 18 Further Differentiation of EXPRES Cells Cultured on Tissue Culture Substrate to Foregut Endoderm

EXPRES01 cells at passage 35 underwent a 5 day differentiation by treatment with 100ng/ml activin-A, 20ng/ml of Wnt3a, and 100 nM GSK3beta inhibitor IX in 0.5% FBS, DMEM:F12 media. Cells were analyzed by FACS and showed approximately 70% of the cells were positive for CXCR4. The cells were then treated for in each of the following steps: 2%FBS DMEM:F12 containing 50ng/ml FGF-10, and 0.25µM KAAD-Cyclopamine (Calbiochem, CA) for 3 days; Step3, 1%B27 DMEM, low glucose containing 50 ng/ml FGF-10, 0.25µM KAAD-Cyclopamine and 1µM Retinoic Acid (Sigma, MO) for 4 days; and Step 4, 1%B27 DMEM, low glucose containing 1µM DAPT (Calbiochem, CA) plus 50 ng/ml Exendin4 (Sigma, MO) for 4 days.. This protocol is based on a prior publication by D'Amour et al (Nature Biotech, 24, 1392, 2006). Cells were fixed at end of stage 4 and stained for PDX-1, HNF-3 beta, SOX-17, Albumin, anti-trypsin, and CDX-2. As depicted in Figure 26 , EXPRES cells can be readily differentiated to foregut endoderm as measured by expression of PDX-1 (approximately 20% of culture stained positive), HNF-3 beta (approximately 90% positive), albumin (approximately 5% positive), anti-1-Trypsin (approximately 70% positive), SOX-17 (approximately 70%), and CDX-2 (approximately 5% positive).

Reference Example 19 Microarray Analysis of EXPRES Cells Versus Undifferentiated Human Embryonic Stem Cells

Total RNA was isolated from cultures of the human embryonic stem cell line H9,at passage 44, EXPRES 01 P11 and EXPRES 02 P7 using an RNeasy mini kit (Qiagen): All groups contained three biological replicates and each biological replicate was repeated on two separate gene chips. Sample preparation, hybridization, and image analysis were performed according to the Affymetrix Human Genome U133 Plus 2.0 Array. Following normalization and a log transformation, data analysis was performed using OmniViz® software (MA) and GENESIFTER (VizXLabs, WA). Significant differences in gene expression between the samples were evaluated using analysis of variance and an F-test with adjusted P-value (Benjamini and Hochberg correction) of less than or equal to 0.05. Only genes with a present call in at least one group were included in the analysis. Table V lists the mean normalized log-transformed signal intensity of genes showing at least 5-fold difference between groups (undifferentiated ES, EXPRES 01 and EXPRES 02 cells) along with the adjusted P-value for each gene. Genes representing primitive streak or definite endoderm are highlighted in bold. Only the top 200 genes that are upregulated or down regulated are shown in Table V.

Reference Example 20 Microarray Analysis of EXPRES Cells Differentiated to the DE Stage Versus Human Embryonic Stem Cells Differentiated to the DE Stage

Total RNA was isolated from the following cultures using an RNeasy mini kit (Qiagen): A) H9P33 cells cultured on MATRIGEL-coated plates (1:30 dilution) and exposed to DMEM/F12 medium supplemented with 0.5% FBS and 100 ng/ml Activin-A and 20 ng/ml of wnt3A for two days followed by treatment with DMEM/F12 medium supplemented with 2% FBS and 100 ng/ml Activin-A (AA) for an additional three days; B) EXPRES 01 P24 cells cultured on TCPS and exposed to DMEM/F12 medium supplemented with 0.5% FBS, 100 ng/ml Activin-A, 20 ng/ml of WNT3A, and 100 nm GSK-3B IX inhibitor (Catalog# 361550, Calbiochem, CA) for five days C) EXPRES02 P17 cells cultured on TCPS and exposed to DMEM/F12 medium supplemented with 0.5% FBS, 100 ng/ml Activin-A, 20 ng/ml of WNT3A, and 100 nm GSK-3B IX inhibitor (Catalog# 361550, Calbiochem, CA) for five days, D) H9P39 cells cultured on MATRIGEL-coated plates (1:30 dilution) and exposed to DMEM/F12 medium supplemented with 0.5% FBS and 100 ng/ml Activin-A and 20 ng/ml of wnt3A for two days followed by treatment with DMEM/F12 medium supplemented with 2% FBS and 100 ng/ml Activin-A (AA) for an additional two days RNA samples were collected from group D at 2hrs, 6hrs, 24 hrs, 30 hrs, 48 hrs, 72 hrs, and 96 hrs. EXPRES 01 and 02 cultured in their respective growth media were also included as controls. All groups contained three biological replicates and each biological replicate was repeated on two separate gene chips.

Sample preparation, hybridization, and image analysis were performed according to the Affymetrix Human Genome U133 Plus 2.0 Array. Following normalization and a log transformation, data analysis was performed using OmniViz® software (MA) and GENESIFTER (VizXLabs, WA). Significant differences in gene expression between the samples were evaluated using analysis of variance and an F-test with adjusted P-value (Benjamini and Hochberg correction) of less than or equal to 0.05. Only genes with a present call in at least one group were included in the analysis. Table VI lists the mean normalized log-transformed signal intensity of genes showing at least 5-fold between group A, group B, group C, and group D at various time points along with the adjusted P-value for each gene. Only the top 200 genes that are upregulated or down regulated are shown in Table VI. Genes representing primitive streak or definite endoderm are highlighted in bold. Table VII lists the correlation coefficient for each comparison group. Scatter plots corresponding to the correlation coefficients are depicted in Figure 27 . The global expression profile of EXPRES 01 cells appear to resemble the expression profile of samples at 30 hrs or less of the DE stage, whereas the EXPRES 02 cells appear to resemble the expression profile of samples at greater than 48 hrs of the DE stage.

Reference Example 21 Formation of Embryoid Bodies and Differentiation to Various Lineages

EXPRES 01 passage 27 cultures were removed as single cells using TrypLE™ Express solution, spun at 200g for 4 mins, and resuspended in DMEM-F12 + 20% FBS. The cell suspension was seeded on low adhesion Petri dishes. 3-4 days post seeding, embryoid body (EB) like structures were formed ( Figure 28 ). Treatment of the cultures with DMEM-F12 + 2% FBS + 1 micro molar retinoic acid induced expression of ectoderm markers, such as NeuroD.

Reference Example 22 Formation of Teratomas in the Kidney Capsules of NOD-SCID Mice

Undifferentiated cells from the human embryonic stem cell line H9 at passage 42, EXSPRES 01 Passage 30, and EXPRES 02 P22 cells were released from cultures using TRYPLE, washed in basal media, and then suspended in DMEM-F12 basal media. Approximately 1x10⁶ undifferentiated H9 P42, 1.5 million EXPRES 01 and 02 cells were injected into the kidney capsule of six week old NOD-SCID mice. Five weeks following transplantation, the animals were sacrificed; kidneys were excised and fixed in formalin or placed in lysis buffer to collect RNA for subsequent PCR analysis. Figure 29 depicts expression of markers characteristic of mesoderm, ectoderm, endoderm, extraembryonic visceral endoderm, and pluripotency markers for collected samples. Similar to H9 line, both EXPRES lines show strong expression of all germ layers along with extra embryonic endoderm.

Reference Example 23 Proliferation And Cell Cycle Analysis of EXPRES 03 cells

Human embryonic stem cells have a unique cell cycle status that is distinguishable from other somatic cells, characterized by high proportion of cells in S-Phase, and shortened or truncated Gap phases (G1 and G2). The cell cycle control mechanisms in hES cells may be functionally linked to their self-renewal and pluripotency capacity of these cells, and may be different from control mechanism in their differentiated/committed counterparts. These experiments were designed to determine the cells cycle nature of EXPRES cells that have been shown to express many of the markers of pluripotency hES cells.

Methods: Cells were seeded at 5,000-10,000 cells /cm² in Cell Bind tissue culture flasks (Corning) and cultured for 2-4 days. EXPRES 03 cells were cultured either in growth medium containing 2% FBS inDMEM/F12 and Activin-A (100 ng/ml), wnt3a (10-20 ng/ml) and IGF (50 ng/ml). For comparative proliferation analysis, IGF was sometimes omitted from the growth factor cocktail. Cell proliferation was analyzed using the APC BRDU Flow kit according to the Manufacturer's recommendations (BD Biosciences, San Diego, CA). Briefly, cells were pulsed with BRDU for 1-2 hrs at the end of culture period, released using Tryple E Express and counted. Cells were fixed in BD Cytofix/Cytosperm Buffer, incubated for 30 min, followed by incubation with BD Cytoperm buffer for 10 minutes on ice. Cells were then treated with DNAse for 1 hr at 37° C to expose incorporated BRDU, followed by staining with APC conjugated anti-BRDU antibody. For cell cycle analysis, cells were stained with 7AAD, and analyzed on FACS Array.

Results: Similar to the highly hES cells, EXPRES 03 cells retained a highly proliferation rate, as shown by the high percentage of cells that in S-phase determined by their capacity to incorporate BRDU in culture. The frequency of cells in S-Phase was typically greater than 45% (range 40-60%), similar to hES cells ( Figure 30 a-c ). Although the number of EXPRES 03 cells grown in the presence of IGF were 2-3 times the number of cells grown in absence of IGF after 3-4 days, there was only marginal differences in frequency of cells in S-phase when cell were exposed to BRDU for 1 hour or more ( Figure 30 f). This high frequency of cell in S-phase and cell cycle structure is unlike that observed in somatic cells, as shown here for human amniotic fluid cells (AFDX002) ( Figure 30 d). Furthermore, mitomycin treated cells Mouse Embryo Fibroblast (MEF, Figure 30 e) do not proceed into S-phase but show apparent accumulation in the G2/M phase (64%), which may be related to the inability of mitomycin treated cells to separate the DNA strands at mitosis.

Reference Example 24 Transfection Efficiency of ES cells vs EXPRES cells

A major limitation of genetic manipulation of hES is their relative resistance to conventional methods of transfection and viral transduction. In addition to their highly proliferative rates, EXPRES cells are easy to transfect in vitro. To compare transfection efficiency, in EXPRES and hES cells were transfected in culture with EGFP and analyzed by fluorescence microscopy and flow cytometric methods.

Methods: EXPRES 01 cells were seeded on human fibronectin coated (10ug/ml) 6 well tissue culture plates in growth medium comprising 2% FBS in DMEM/F12, Activin-A (100 ng/ml), wnt3a (10-20 ng/ml) and IGF (50 ng/ml). For cell clusters hES cell were passaged by routine methods using collagenase into MATRIGEL coated 6 well culture plates, and grown in MEF conditioned hES medium. For single cells, hES cells were passaged by exposing cells to TRYPLE for 3 minutes at 37° C, followed by plating onto MATRIGEL coated 6 well culture plates. When cells achieved desired confluency (70-80%), cells were transfected with Lipofectamine 2000 according to the manufacturer's recommendations (Invitrogen, Carlsbad, CA). Briefly, 4 µg of DNA was diluted into 250 µl Opti-MEM I Reduced serum medium. Five microliters of Lipofectamine 200 was mixed into total of 250 µl Opti-MEM I medium for 5 minutes and gently mixed with diluted DNA. The DNA/Lipofectamine complexes were allowed to form at room temperature for 20 minutes, and then added to the respective wells with gentle swirling motions of the plates for gentle mixing. Cells were incubated in presence of complexes for another 24 hrs followed by complete change of medium. Cells were analyzed by fluorescence microscopy and flow cytometry 48 hrs following transfection.

Results: The uptake and expression of eGFP was compared by transfection of EXPRES 01 cells and hES cells plated as single cell dispersion or cell clusters, and analyzed 48 hrs later. EXPRES 01 cell showed the highest level of eGFP protein expression, with 75% of cell expressing eGFP by flow cytometric analysis ( Figure 31 ). In contrast, hES were more resistant to transfection, with only 3% of cell expressing eGFP protein by FACS when cell clusters were used. Preparing a single cell dispersion of hES enhanced the level of DNA uptake and eGFP expression to about 20 %, but which is still by about three fold less the expression in EXPRES 01 cells.

Reference Example 25 EXPRES Cells as a Versatile Tool for Screening

EXPRES cells were grown in DMEM:F12 medium containing 2% FBS, 100ng/ml recombinant human Activin-A (R&D Systems), and 20ng/ml recombinant mouse Wnt3a (R&D Systems). Growth medium for EXPRES 01 cells also contained 50ng/ml recombinant human IGF-1 (R&D Systems). Both cell lines were routinely grown at 37°C in an atmosphere of low oxygen (3%) and 5% CO₂. EXPRES 01 and EXPRES 02 cells were released from culture as a single cell suspension using TrypLE enzymatic digestion (Invitrogen, CA) then washed and counted to determine accurate cell numbers and viability (>95%). Aliquots ranging from 1,250 to 80,000 cells were distributed into human fibronectin-coated wells of a 96-well plate (Corning-Costar) in a final volume of 100 µl culture medium. Control wells were also fibronectin-coated and contained an equivalent volume of culture medium without cells. Plates were allowed to equilibrate overnight in a humidified chamber incubated under standard low oxygen, 5% CO₂ at 37°C. During this time, the cells attached as monolayer cultures with varying degrees of confluency dependent upon the initial seeding density. After overnight culture, 20µl of MTS reagent (CellTiter 96 Aqueous Assay; Promega) was added to each well. MTS is reduced to formazan and can be used as a measure of dehydrogenase enzyme activity directly proportional to the number of live cells. One plate was returned to low oxygen culture while an identical parallel plate was incubated in normal oxygen (20%). After 4 hours, absorbance was read at 490nm on a spectrophormetric plate reader (Molecular Devices). Statistical calculations for mean OD, standard deviation, and percent coefficient of variation (CV) were determined for replicate sample sets within each plate and then compared to similar wells between both plates.

Standard deviation and percent coefficient of variation values demonstrate that EXPRES cells can be evenly distributed between wells for high plating efficiency and good well-to-well reproducibility (Table VIII a-f). As seen with average OD₄₉₀ readings for equivalent numbers of cells, the EXPRES 01 line has a higher metabolic activity than the EXPRES 02 line. For each EXPRES line, percent CV values between the two plates suggest there are no differences in metabolic activity for parallel conditions regardless of atmospheric oxygen levels in this short-term assay. Optimal cell numbers per well within the linear range for this assay were determined by graphing average OD readings ( Figure 32 ): less than 20,000 cells/well for EXPRES 01 and less than 40,000 cells/well for EXPRES 02. Again, atmospheric differences in oxygen levels did not affect optimal cell number results in this short-term assay. These results suggest that EXPRES cells are amenable to screening protocols that can measure toxicological effects of various agents on cell proliferation and/or metabolic rate.

Reference Example 26 Expansion of DE-like Cells Derived from EXPRES Cells

Previous examples establish that EXPRES cells can be derived from embryonic stem cells and can be readily expanded on TCPS in various growth media. Most of these media formulation contain IGF as a supplement or insulin/IGF in 2% FBS used in the growth media. These factors have been shown to inhibit DE related genes through the PI-3 kinase pathway (Stem cells, 25:29-38, 2007). An alternative media was formulated based on DM-F12 + 0.5% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 100 nM GSK-3B inhibitor IX (further referred to as "growth media for DE cells"). EXPRES 01 at passage 27 cells cultured in the above media were able to propagate at the same rate as cells cultured in DM-F12 + 2% FBS + 100 ng/ml AA + 20 ng/ml WNT3A + 50 ng/ml IGF-I. Furthermore, cells cultured in the growth media for DE cells expressed strong DE markers by real-time PCR ( Figure 33 ) through three passages. Approximately 72% of cells expressed CXCR4 ( Figure 34 ).

Reference Example 27 siRNA Knockdown of Target Genes in EXPRES cells

Efficient knockdown of target genes in human embryonic stem cells using siRNA is severely limited by the ability to achieve high levels of transfection in human embryonic stem cells grown as cluster colonies. EXPRES cells are easily transfected with siRNA using conventional methods, and thus offer a valuable system to screen siRNA oligo sequences, as well as evaluate the role played by targeted genes.

Methods: EXPRES 03 cells were seeded on fibronectin coated (10µg/ml) 6 well tissue culture plates in growth medium comprising 2% FBS in DMEM/F12, Activin-A (100 ng/ml), wnt3a (10-20 ng/ml) and IGF (50 ng/ml). For 6 well plates, 200,000 cells were seeded 24 hrs prior to transfection with the siRNA oligo sequences.

To evaluate target gene knockdown, cells at 70-80% confluency cells were transfected using Lipofectamine 2000 according to the manufacturer's recommendations (Ambion (Applied Biosystems), Foster City, CA). Briefly, the appropriate amount of siRNA was diluted into 250 µl Opti-MEM I Reduced serum medium to achieve a final concentration of 100 nmol. Five microlitres of Lipofectamine 2000 was diluted in 250 µl Opti-MEM I medium and incubated for 5 minutes. The complexes were incubated for 15-20 min at room temperature, and then added to the cells with gentle swirling motions of the plates for gentle mixing. Cells were incubated in presence of siRNA for another 24 hrs followed by complete change of medium. Cells were visualized with fluorescence microscopy 24-48 hrs following transfection, and RNA harvested for analysis of target gene knockdown by quantitative RT-PCR methods. The following pre-validated siRNA oligo sequences, purchased from Ambion were tested: Beta-catenin (Id. No. 42816) and GSK3b (Id. No. 42839).

Results: Fluorescence microscopy revealed a very high level of siRNA uptake by EXPRES cells (>80%) when using fluorescently labeled siRNA ( Figure 35 ). RNA harvested from the cells was analyzed by PCR for target gene knockdown, and compared with control siRNA oligo transfected cells. Beta-catenin and GSK3b siRNA oligos achieved very high levels of gene knockdown in EXPRES cells, with greater than 93% gene knockdown. Other non-validated oligo sequences to other gene targets eg Hes-1, Oct-4 achieved lower and variable levels of target gene knockdown.. Specificity of oligo sequences was verified by analysis of other gene transcripts, which did not show any appreciable knockdown.

Reference Example 28 Cytokine Antibody Array analysis for EXPRES 01 and 02 lines

EXPRES 01 and 02 lines at passage 22 and 23, respectively, were grown to approximately 70% confluency in their respective media and then cell lystaes was collected using mammalian cell lysis kit (Sigma-Aldrich, MO). Cytokine array analysis was completed using Cytokine Array panels provided by RayBiotech, GA (http://www.raybiotech.com/). Table IX a-c lists cytokine, cytokine and growth factor receptor expression following normalization of the data and background subtraction. For each panel, positive and negative controls are also included. The panels were run for two different samples per cell type.

Reference Example 29 Karyotype Analysis

The karyotype of EXPRES 01 cells at passage 20 and EXPRES 02 cells at passage 15 was determined by G-band analysis. Cytogenetic analysis was performed on twenty-one G-banded cells from EXPRES 01 and on twenty G-banded cells from EXPRES 02. Half of the G-banded EXPRES 01 cells showed a normal 46XX karyotype while the rest showed abnormal karyotype such as trisomy 17. The EXPRES 02 line also showed a chromosome rearrangement with a duplication of almost all of the chromosome 1 short-arm.

Reference Example 30 Derivation of EXPRES Cells from a Suspension of Single Human Embryonic Stem Cells in the Presence of a Rho-Kinase (ROCK) Inhibitor

Cells from the human embryonic stem cell line H9 at passage 35 lines were cultured under hypoxic conditions (approximately 3% O₂) for at least three passages. The cells were cultured in MEF-CM supplemented with 8 ng/ml of bFGF and plated on MATRIGEL coated plates according to Example 1. At approximately 60% confluency, the cultures were exposed to TrypLE™ Express solution (Invitrogen, CA) for 5 mins. Released cells were resuspended in DM-F12 + 2% FBS medium, recovered by centrifugation, and counted using a hemocytometer. The released cells were seeded at 1000-10,000 cells/cm² on tissue culture polystyrene (TCPS) flasks and cultured in DM-F12 + 2% FBS + 100 ng/ml activin-A + 20 ng/ml WNT-3A + 50 ng/ml of IGF-I + 0.1 mM mercaptoethanol (Invitrogen, CA), non-essential amino acids (1X, NEAA from Invitrogen, CA) +/-10 µm ROCK inhibitor (Y-27632, Calbiochem, CA) under hypoxic conditions (approximately 3% O₂) at 37 °C in a standard tissue culture incubator. The TCPS flaks were not coated with MATRIGEL or other extracellular matrix proteins. The media was changed daily. The first passage cells are referred to as P1. As shown in Figure 37 , 24 hrs after seeding, addition of the ROCK inhibitor resulted in a significantly larger number of attached cells as compared to cultures derived in the absence of the ROCK inhibitor. EXPRES cells derived using the ROCK inhibitor, Y27632 were designated as EXPRES 15.

Reference Example 31 Karyotype Analysis

The karyotype of EXPRES 15 cells at passage 5 and 12 were determined by G-band analysis. Cytogenetic analysis was performed on twenty-one G-banded cells from EXPRES 15 all of the cells showed a normal 46XX karyotype ( Figure 38 ). FISH analysis of chromosomes 12 and 17 also showed that all cells demonstrated a normal signal pattern for the ETV6 BAP (TEL) gene located on chromosome 12 and all cells demonstrated a normal signal pattern for the Her2/neu gene and 17 centromere on chromosome 17.

Reference Example 32 EXPRES Cells can be Maintained in Media Containing a Range of Concentrations of IGF, WNT3A, activin-A, and GSK-3B inhibitors

EXPRES 11 cells were grown in DMEM/F12 (Invitrogen) containing 2% FBS, 100ng/ml activin-A, 20ng/ml Wnt3a and 50ng/ml IGF. At 80% confluency, cells were passed using TrypLE Express (Invitrogen) into 96-well plates at a density of 4000 cells/well in DMEM/F12 containing 2% FBS. Cells were allowed to adhere to the substrate for 1 hour in a humidified incubator held at 37°C with 5% CO2, prior to the addition of activin-A ranging from 50 to 100ng/ml, Wnt3a ranging from 10 to 20ng/ml, IGF ranging from 10 to 50ng/ml, and 50 to 100 nM GSK-3B inhibitor (IX). At 24, 48 and 96 hours, cell viability was determined using the CellTiter® 96 AQueous One Solution Cell Proliferation Assay (Promega). Briefly, MTS reagent was added to the 96-well plates and allowed to incubate with the cells for 1-4 hours and then reading the absorbance at 490nm on a plate reader. The absorbance reading was directly proportional to the number of living cells. Figure 39 a-c shows the absorbance readings at a) 24 hrs, b) 48 hrs, and c) 96 hrs post seeding.

Table IA: List of primary antibodies used for FACS and immuno staining analysis.


SSEA-1	Chemicon (CA)	Mouse IgM	MAB4301
SSEA-3	Chemicon (CA)	Mouse IgG3	MAB4303
SSEA-4	Chemicon (CA)	Rat IgM	MAB1435
TRA 1-60	Chemicon (CA)	Mouse IgM	MAB4360
TRA 1-81	Chemicon (CA)	Mouse IgM	MAB4381
TRA 1-85	Chemicon (CA)	Mouse IgG1	MAB4385
AP	R&D Systems (MN)	Mouse IgG1	FAB1448A
HNF3β	R&D Systems	Goat IgG	AF2400
PDX1	Santa Cruz Biotechnology, INC (CA)	Goat IgG	sc-14664
GATA4	R&D Systems	Goat IgG	AF2606
Sox 17	R&D Systems	Goat IgG	AF1924
CD 9	BD Bioscience (CA)	Mouse IgG1	341647
CXCR4	R&D Systems	Mouse IgG2A	FAB170A
SOX2	R&D Systems	Goat IgG	AF2018
Nanog	R&D Systems	Goat IgG	AF 1997
OCT4	R&D Systems	Goat IgG	AF1759
Gata6	R&D Systems	Goat IgG	AF1700
Ecad	R&D Systems	Mouse IgG	MAB1838
Ncam	R&D Systems	Mouse IgG	MAB777
HNF1b	R&D Systems	Goat IgG	AF3330
b-catenin	R&D Systems	Mouse IgG	MAB13291
HNF1a	BD Bioscience	Mouse IgG	610902
CD99	Invitrogen (CA)	Mouse IgG	18-0235
Cerebus	Santa Cruz Biotechnology, INC	Goat IgG	SC15131
Hex	Santa Cruz Biotechnology, INC	Goat IgG	SC15129
AFP	R&D Systems	Mouse IgG	MAB1269
Antitrypsin	DAKO (CA)	Rabbit	A0012
islet 1	R&D Systems	Goat IgG	AF1837

Table IB: List of secondary conjugated antibodies used for FACS and immuno staining analysis.


Goat Anti-Mouse IgG APC conjugated	Jackson ImmunoResearch (PA)	1:200
Goat Anti-Mouse IgG PE conjugated	Jackson ImmunoResearch (PA)	1:200
Donkey anti-rabbit PE or - APC conjugated	Jackson ImmunoResearch (PA)	1:200
Donkey anti-goat PE or - APC conjugated	Jackson ImmunoResearch (PA)	1:200
Goat anti-mouse IgM PE	SouthernBiotech (AL)	1:200
Goat anti-Rat IgM PE	SouthernBiotech (AL)	1:200
Goat anti-mouse IgG3 PE	SouthernBiotech (AL)	1:200

Table II List of primers used for real-time PCR analysis using TAQMAN®probes


18s	4310893E
ABCG2	Hs00184979_m1
AchE	Hs00241307_m1
AFP	Hs00173490_m1
ALB	Hs00609411_m1
alpha-antitrypsin	Hs02384981_m1
Amylase	Hs00420710_g1
AP	Hs00240993_m1
Atoh1	Hs00944192_s1
4310886E
B3Tubulin	Hs00964962_g1
B-Catenin	Hs99999168_m1
Barx1	Hs00222053_m1
Brachyury (T)	Hs00610080_m1
CCK	Hs00174937_m1
Cdx1	Hs00156451_m1
Cdx2	Hs00230919_m1
CEBPa	Hs00269972_s1
CEBPb	Hs00942496_s1
Cerberus	Hs00193796_m1
CFC1 (Cripto)	Hs00414425_m1
CGA	Hs00174938_m1
CK19 (KRT19)	Hs00761767_s1
CLDN4 (claudin4)	Hs00533616_s1
C-Myc Binding Protein	Hs00429315_g1
Connexin32 (GJB-1)	Hs00939759_s1
Connexin45	Hs00271416_s1
CTNNβ1	Hs00170025_m1
CXCR4	Hs00237052_m1
Cylcin-D1	Hs00277039_m1
Dapper1 (DACT-1)	Hs00420410_m1
DKK1	Hs00183740_m1
DKK4	Hs00205290_m1
Endoglin	Hs00164438_m1
Exo1	Hs00243513_m1
F3	Hs00175225_m1
FAH	Hs00164611_m1
FGF4	Hs00173564_m1
FGF10	Hs00610298_m1
FGFR1	Hs00241111_m1
FGFR3	Hs00179839_m1
FGFR4	Hs00242558_m1
Flk1	Hs00911705_g1
FOXA1	Hs00270129_m1
FOXA3	Hs00270130_m1
FOXD3	Hs00255287_s1
FOXF1	Hs00230962_m1
GAPDH (human)	4310884E
Gastrin	Hs00174945_m1
GATA1	Hs00231112_m1
GATA4	Hs00171403_m1
GATA5	Hs00388359_m1
GATA6	Hs00232018_m1
GCK	Hs00175951_m1
GFAP	Hs00157674_m1
GIP	Hs00175030_m1
Gli	Hs01110766_m1
Glucagon	Hs00174967_m1
Glut-2	Hs00165775_m1
Goosecoid	Hs00418279_m1
GS	Hs00374213 m1
Handy1	Hs00231848_m1
HB9	Hs00232128_m1
Hes1	Hs00172878_m1
Hex1	Hs00172696_m1
HEYL	Hs00232718_m1
HHIP (hedgehog interacting protein)	Hs01011009_m1
hHIF1a	Hs00153153_m1
HNF1	Hs00167041_m1
HNF1α	Hs00167041_m1
HNF1β	Hs00172123_m1
HNF3β	Hs00232764_m1
HNF4α	Hs00230853_m1
HNF6 (onecut)	Hs00413554 m1
HoxB1	Hs00157973_m1
IBSP	Hs00173720_m1
Insulin II	Hs00355773_m1
Islet-1	Hs00158126_m1
Jagged-1 (JAG1)	Hs00164982_m1
KDR	Hs00176676_m1
KRT15	Hs00267035_m1
MafA	Hs00999118_m1
MAML1	Hs00207373_m1
Map2	Hs00159041_m1
MapK14	Hs00176247 m1
MapK8	Hs00177083_m1
MBP (myelin basic protein)	Hs00921945_m1
MixI1	Hs00430824_g1
MMP1 (matrix metalloprotease1)	Hs00233958_m1
MOX1	Hs00793059_m1
MSX1	Hs00427183_m1
Mucin1	Hs00904328_m1
Mucin2	Hs00159374_m1
Myf5	Hs00271574_m1
MyoD1	Hs00159528_m1
N-Cadherin (CDH2)	Hs00169953_m1
N-Cam1	Hs00169851_m1
NEFH	Hs00606024_m1
NEFL	Hs00196245_m1
Nestin	Hs00707120_s1
NeuroD1	Hs00159598_m1
Ngn3	Hs00360700_q1
Nkx2.1	Hs00163037_m1
Nkx2.2	Hs00159616_m1
Nkx6.1	Hs00232355_m1
Notch1	Hs01062014_m1
NTS	Hs00175048_m1
Hs00377820_m1
Oct3/4	Hs00742896_s1
OTX2	Hs00222238_m1
Pax3	Hs00240950_m1
Pax4	Hs00173014_m1
Pax6	Hs00240871_m1
Pax8	Hs00247586_m1
Pax9	Hs00196354_m1
PDX-1 (IPF1)	Hs00236830_m1
Ptch (Patched)	Hs00970985_m1
PTF1a	Hs00603586_q1
PYY	Hs01062281_m1
RA receptor alpha	Hs00230907_m1
RALDH	Hs01125173_m1
RBPSUH	Hs00794653_m1
Rex1 (ZFP42)	Hs00399279_m1
SCGB1	Hs00171092_m1
Secretin	Hs00360814_q1
sFRP	Hs00610060_m1
sFRP5	Hs00169366_m1
SHH	Hs00179843_m1
SLC5A8	Hs01068911_m1
Snai1	Hs00195591_m1
Snai2	Hs00161904_m1
Somatostatin	Hs00174949_m1
Sox1	Hs00534426_s1
Sox10	Hs00366918_m1
Sox17	see "Sox17" tab
Sox2	Hs00602736_s1
Sox3	Hs00271627_s1
Sox7	Hs00846731_s1
Sox9	Hs00165814_m1
Sparc	Hs00234160_m1
SP-C	Hs00161628_m1
TBX6	Hs00365539_m1
Tert	Hs00162669_m1
THBD	Hs00264920_s1
Twist1	Hs00361186_m1
UtF1	Hs00747497_q1
Vim	Hs00185584_m1
Wnt3a (human)	Hs01055707_m1
Wnt3a (mouse)	Mm00437337_m1
WT1	Hs01103754_m1
Zic1	Hs00604749_m1
Zic2	Hs00600845_m1

Table III List of EXPRES lines generated from H1 & H9 parent lines

ID#	ES Parent line, Passage number	Day of derivation during DE differentiation	Media used to propagate cells
EXPRES 01	H9P54	Day 4	Growth media + 50 ng/ml IGF-I
EXPRES 02	H9P54	Day 6	DM-F12-+ 2% FBS +100 ng/ml AA +20 ng/ml WNT-3A (growth media)
EXPRES 03	H9P39	Day 3	Growth media + 50 ng/ml IGF-I
EXPRES 04	H9P39	Day 4	Growth media + 50 ng/ml IGF-I
EXPRES 05	H9P39	Day 5	Growth media + 50 ng/ml IGF-I
EXPRES 06	H9P49	Day 5	Growth media
EXPRES 07	H1P50	Day 5	Growth media
EXPRES 08	H1P39	Day 4	Growth media + 50 ng/ml IGF-I + 0.1mM mercaptoethanol
EXPRES 09	H1P39	Day 6	Growth media + 50 ng/ml IGF-I + 0.1mM mercaptoethanol
EXPRES 10	H1P49	Day 4	Growth media
EXPRES 11	H9P30	Day 4	Growth media + 50 ng/ml IGF-I + 0.1mM mercaptoethanol
EXPRES 12	H9P30	Day 6	Growth media + 50 ng/ml IGF-I + 0.1mM mercaptoethanol

Table IV Expression of cell surface markers by EXPRES 01 and 02 lines

Marker	EXPRES 01- % Expression	EXPRES 02- % Expression
TRA 1-60	100	100
TRA1-81	100	100
SSEA-3	100	86 (85-88)
SSEA-4	100	87 (83-88)
CD56 (NCAM)	<1	38 (35-40)
CXCR4	<1	20 (10-25)
SSEA-1	<1	26 (9-32)
E-cadherin	90 (85-95)	75 (72-79)
CD9	99	66 (62-68)
CD30	97 (96-98)	43 (40-46)
LIF-receptor	<1	20 (15-21)
CD117	92 (90-95)	73 (67-75)

Table V DIFFERENTIAL EXPRESSION OF GENES BETWEEN UNDIFFERENTIATED EMBRYONIC STEM CELLS CULTURED ON MATRIGEL™ AND EXPRES 01 (A) AND 02 (B) CELLS CULTURED ON TCPS


ES	EXPRES 01	Ratio	Direction	adj. p-value	Gene Identifier	Gene Name
-5.03662	3.037629	269.52	Up	8.34E-05	BG099432	ESTs
-2.82645	3.094183	60.57	Up	3.88E-03	NM_013445	Homo sapiens glutamate decarboxylase 1 (brain, 67kD) (GAD1), transcript variant GAD25, mRNA. /PROD=glutamate decarboxylase 1, isoform GAD25 /FL=gb:NM_013445.1 gb:AF178853.1 gb:BC002815.1
-4.71714	0.961816	51.23	Up	6.59E-05	AI796169	GATA-binding protein 3 /FL=gb:NM_002051.1 gb:M69106.1 gb:BC003070.1
-1.57973	4.092731	51	Up	6.13E-03	AL513917	solute carrier family 16 (monocarboxylic acid transporters), member 3 /FL=gb:U81800.1 gb:NM_004207.1
-2.24566	3.409815	50.4	Up	1.19E-03	NM_016588	Homo sapiens neuritin (LOC51299), mRNA. /PROD=neuritin /FL=gb:NM_016588.1 gb:BC002683.1 gb:AF136631.1
-0.66473	4.897427	47.25	Up	1.97E-04	R06655	ESTs, Moderately similar to AF078844 1 hqp0376 protein (H.sapiens)
-2.96204	2.589425	46.9	Up	1.79E-03	NM_001311	Homo sapiens cysteinerich protein 1 (intestinal) (CRIP1), mRNA. /PROD=cysteine-rich protein 1 (intestinal) /FL=gb:U58630.1 gb:BC002738.1 gb:NM_001311.1 gb:U09770.1
-0.08298	5.388254	44.36	Up	2.48E-04	NM_004207	Homo sapiens solute carrier family 16 (monocarboxylic acid transporters), member 3 (SLC16A3), mRNA. /PROD=solute carrier family 16 (monocarboxylic acidtransporters), member 3/FL=gb:U81800.1 gb:NM_004207.1
-4.21525	1.240929	43.9	Up	4.36E-04	NM_006119	Homo sapiens fibroblast growth factor 8 (androgen-induced) (FGF8), mRNA. /PROD=fibroblast growth factor 8 (androgen-induced) /FL=gb:U36223.1 gb:U46212.1 gb:NM_006119.1
-3.11273	2.306225	42.78	Up	5.07E-03	AW444761	ESTs
-4.05111	1.075159	34.93	Up	1.19E-03	J03580	Human, parathyroid-like protein (associated with humoral hypercalcemia of malignancy) mRNA, complete cds. /FL=gb:J03580.1
-1.81534	3.025351	28.65	Up	7.00E-04	AW590925	ESTs
-2.36335	2.448218	28.08	Up	1.62E-02	AI189359	mevalonate (diphospho) decarboxylase /FL=gb:NM_002461.1 gb:BC000011.1 gb:U49260.1
-3.00328	1.794842	27.82	Up	7.77E-03	AI571798	Rho GDP dissociation inhibitor (GDI) alpha
-4.17258	0.510307	25.69	Up	2.29E-04	AI040887	ESTs
-0.11332	4.420733	23.17	Up	8.78E-05	NM_003670	Homo sapiens basic helix-loop-helix domain containing, class B, 2 (BHLHB2), mRNA. /PROD=differentiated embryo chondrocyte expressed gene1 /FL=gb:AB004066.1 gb:NM_003670.1
-1.94	2.590871	23.12	Up	3.90E-03	NM_016569	Homo sapiens TBX3-iso protein (TBX3-iso), mRNA. /PROD=TBX3-iso protein /FL=gb:NM_016569.1 gb:AF216750.1
-2.18113	2.33099	22.82	Up	1.12E-02	NM_004041	Homo sapiens arrestin, beta 1 (ARRB1), transcript variant 1, mRNA. /PROD=arrestin beta 1, isoform A /FL=gb:BC003636.1 gb:AF084040.1 gb:NM_004041.2
-2.85963	1.609384	22.15	Up	6.37E-03	BC005961	Homo sapiens, parathyroid hormone-like hormone, clone MGC:14611, mRNA, complete cds. /PROD=parathyroid hormone-like hormone /FL=gb:BC005961.1
0.044298	4.505436	22.03	Up	4.17E-05	W57613	ESTs
-3.65051	0.757197	21.23	Up	7.11E-04	AF213459	Homo sapiens ephrin receptor EPHA3 complete form (EPHA3) mRNA, complete cds. /PROD=ephrin receptor EPHA3 complete form /FL=gb:NM_005233.1 gb:M83941.1 gb:AF213459.1
-1.25226	2.990178	18.93	Up	2.70E-04	NM_013445	Homo sapiens glutamate decarboxylase 1 (brain, 67kD) (GAD1), transcript variant GAD25, mRNA. /PROD=glutamate decarboxylase 1, isoform GAD25 /FL=gb:NM_013445.1 gb:AF178853.1 gb:BC002815.1
-0.63516	3.41866	16.61	Up	1.05E-03	AA149250	ESTs, Weakly similar to WDNM RAT WDNM1 PROTEIN PRECURSOR (R.norvegicus)
-0.14916	3.880272	16.33	Up	8.45E-04	NM_002521	Homo sapiens natriuretic peptide precursor B (NPPB), mRNA. /PROD=natriuretic peptide precursor B /FL=gb:NM_002521.1 gb:M25296.1
-2.88485	1.143234	16.31	Up	2.83E-03	BF437711	ESTs
-2.7136	1.194285	15.01	Up	2.14E-02	NM_001898	Homo sapiens cystatin SN (CST1), mRNA. /PROD=cystatin SN /FL=gb:J03870.1 gb:NM_001898.1
-0.07353	3.816817	14.83	Up	1.62E-02	AF116616	Homo sapiens PRO0998 mRNA, complete cds. /PROD=PR00998 /FL=gb:AF116616.1
-1.44577	2.422113	14.6	Up	1.34E-02	AL544576	ESTs
2.301255	6.091008	13.83	Up	6.50E-05	BC020935	Homo sapiens, Similar to otoconin 90, clone IMAGE:4277593, mRNA.
3.006559	6.79047	13.77	Up	8.80E-05	AI263909	ras homolog gene family, member B /FL=gb:NM_004040.1
-0.512	3.268087	13.74	Up	2.96E-03	AF345910	Homo sapiens NYD-SP14 mRNA, complete cds. /PROD=NYD-SP14 /FL=gb:AF345910.1
3.484047	7.24746	13.58	Up	4.12E-04	NM_003564	Homo sapiens transgelin 2 (TAGLN2), mRNA. /PROD=transgelin 2 /FL=gb:D21261.1 gb:NM_003564.1
2.623145	6.382732	13.54	Up	7.32E-05	AI050866	nodal, mouse, homolog
2.91184	6.66195	13.46	Up	1.44E-04	BC002616	Homo sapiens, transgelin
				2, clone MGC:2989, mRNA, complete cds. /PROD=transgelin 2 /FL=gb:BC002616.1
-1.18027	2.546953	13.24	Up	1.42E-02	AI123555	ESTs
-0.92213	2.770179	12.93	Up	1.08E-04	AK000345	Homo sapiens cDNA FLJ20338 fis, clone HEP12179.
-1.85154	1.840613	12.93	Up	6.40E-03	AI949760	ESTs, Weakly similar to unnamed protein product (H.sapiens)
0.899321	4.507212	12.19	Up	1.08E-04	AW 196940	ESTs
1.651788	5.252439	12.13	Up	5.58E-05	NM_001553	Homo sapiens insulin-like growth factor binding protein 7 (IGFBP7), mRNA. /PROD=insulin-like growth factor binding protein 7 /FL=gb:NM_001553.1 gb:L19182.1
-1.20347	2.387268	12.05	Up	2.76E-02	BF063186	ESTs
3.669215	7.251816	11.98	Up	2.01E-05	NM_000700	Homo sapiens annexin A1 (ANXA1), mRNA. /PROD=annexin I /FL=gb:BC001275.1 gb:NM_000700.1
-3.52039	0.041471	11.81	Up	1.58E-02	AW 162210	Homo sapiens cDNA FLJ11490 fis, clone HEMBA1001918
3.006317	6.564471	11.78	Up	2.04E-04	NM_006183	Homo sapiens neurotensin (NTS), mRNA. /PROD=neurotensin precursor /FL=gb:NM_006183.2 gb:U91618.1
3.227575	6.777916	11.72	Up	2.01E-05	U15174	Homo sapiens BCL2adenovirus E1B 19kD-interacting protein 3 (BNIP3) mRNA, complete cds. /PROD=BCL2adenovirus E1B 19kD-interacting protein 3 /FL=gb:AF002697.1 gb:NM_004052.2 gb:U15174.1
1.869893	5.411751	11.65	Up	2.01E-05	NM_001854	Homo sapiens collagen, type XI, alpha 1 (COL11A1), mRNA. /PROD=collagen, type XI, alpha 1/FL=gb:J04177.1 gb:NM_001854.1
2.851479	6.371229	11.47	Up	3.61E-05	AI950472	ESTs
-0.1081	3.393761	11.33	Up	1.39E-03	BG028597	ESTs
0.41954	3.911282	11.25	Up	1.42E-04	AI670948	ESTs
-1.71451	1.771584	11.21	Up	7.77E-03	B1254089	Homo sapiens full length
	insert cDNA clone ZD50E03
-1.66293	1.80547	11.07	Up	2.68E-02	NM_000817	Homo sapiens glutamate decarboxylase 1 (brain, 67kD) (GAD1), transcript variant GAD67, mRNA. /PROD=glutamate decarboxylase 1, isoform GAD67 /FL=gb:NM_000817.1 gb:M81883.1 gb:L16888.1
0.451086	3.904705	10.96	Up	5.45E-04	NM_007038	Homo sapiens a disintegrin-like and metalloprotease (reprolysin type) with thrombospondin type 1 motif, 5 (aggrecanase-2) (ADAMTS5), mRNA. /PROD=a disintegrin and metalloprotease withthrombospondin motifs-5 preproprotein /FL=gb:NM_007038.1 gb:AF14209
-1.44798	1.988376	10.83	Up	1.07E-02	AW376860	ESTs
1.19822	4.633038	10.81	Up	1.22E-04	NM_016931	Homo sapiens NADPH oxidase 4 (NOX4), mRNA. /PROD=NADPH oxidase 4 /FL=gb:AF261943.1 gb:NM_016931.1 gb:AF254621.1 gb:AB041035.1
1.552808	4.981033	10.76	Up	3.24E-04	NM_000602	Homo sapiens serine (or cysteine) proteinase inhibitor, clade E (nexin, plasminogen activator inhibitor type 1), member 1 (SERPINE1), mRNA. /PROD=serine (or cysteine) proteinase inhibitor, cladeE (nexin, plasminogen activator inhibitor type 1), membe
-0.62725	2.792215	10.7	Up	3.24E-04	BC017942	Homo sapiens, Similar to otoconin 90, clone IMAGE:4285317, mRNA.
-1.22834	2.18828	10.68	Up	2.50E-02	BG402859	ESTs
-0.85366	2.55067	10.59	Up	3.53E-04	N36408	hypothetical protein FLJ23306 /FL=gb:NM_024530.1
1.55625	4.952105	10.53	Up	1.52E-03	BG164365	microtubule-associated protein 1 B /FL=gb:NM_005909.1
0.93094	4.285883	10.23	Up	4.17E-05	AL038787	6-phosphofructo-2-kinasefructose-2,6-biphosphatase 4
-3.33551	0.008356	10.15	Up	9.88E-03	BF221850	ESTs
-1.97569	1.35098	10.03	Up	2.12E-02	NM_002149	Homo sapiens hippocalcin-like 1 (HPCAL1), mRNA. /PROD=hippocalcin-like 1 /FL=gb:NM_002149.1 gb:D16227.1
0.624024	3.934756	9.92	Up	2.01E-05	AF154054	Homo sapiens DRM (DRM) mRNA, complete cds. /PROD=DRM /FL=gb:NM_013372.1 gb:AF110137.2 gb:AF045800.1 gb:AF154054.1
-2.37515	0.931587	9.9	Up	2.83E-02	NM_025136	Homo sapiens hypothetical protein FLJ22187 (FLJ22187), mRNA. /PROD=hypothetical protein FLJ22187 /FL=gb:BC005059.1 gb:NM_025136.1
0.906004	4.154799	9.51	Up	1.45E-04	NM_013372	Homo sapiens cysteine knot superfamily 1, BMP antagonist 1 (CKTSF1B1), mRNA. /PROD=cysteine knot superfamily 1, BMP antagonist 1 /FL=gb:NM_013372.1 gb:AF110137.2 gb:AF045800.1 gb:AF154054.1
1.423659	4.64236	9.31	Up	2.01E-05	AB019695	Homo sapiens mRNA for thioredoxin reductase II beta, complete cds. /PROD=thioredoxin reductase II beta /FL=gb:AB019695.1
0.620478	3.822765	9.2	Up	6.53E-05	AL567376	G protein-coupled receptor 39
2.317589	5.509474	9.14	Up	1.02E-05	J04177	Cluster Incl. J04177:Human alpha-1 type XI collagen (COL11A1) mRNA, complete cds /cds=(161,5581) /gb=J04177 /gi=179729 /ug=Hs.82772 /len=6158
-0.01596	3.175621	9.14	Up	9.88E-03	L37033	Cluster Incl. L37033:Human FK-506 binding protein homologue (FKBP38) mRNA, complete cds /cds=(140,1207) /gb=L37033 /gi=965469 /ug=Hs.173464 /len=1613
3.119777	6.302535	9.08	Up	5.07E-03	AI954041	F-box only protein 9 /FL=gb:NM_012347.1
0.891337	4.058968	8.99	Up	1.66E-04	NM_000325	Homo sapiens paired-like homeodomain
				transcription factor 2 (PITX2), mRNA. /PROD=paired-like homeodomain transcription factor 2 /FL=gb:NM_000325.1 gb:U69961.1 gb:AF048720.1
2.106895	5.247359	8.82	Up	2.13E-04	NM_001458	Homo sapiens filamin C, gamma (actin-binding protein-280) (FLNC), mRNA. /PROD=gamma filamin /FL=gb:AF089841.1 gb:NM_001458.1
-1.42687	1.693258	8.69	Up	2.43E-02	AF243424	Homo sapiens SG2NA beta isoform mRNA, partial cds. /PROD=SG2NA beta isoform
0.657996	3.771559	8.66	Up	2.06E-02	AU158380	Homo sapiens cDNA FLJ13698 fis, clone PLACE2000176
0.23287	3.334996	8.59	Up	2.01E-05	R40917	phosphodiesterase 4D, cAMP-specific (dunce (Drosophila)-homolog phosphodiesterase E3) /FL=gb:L20969.1 gb:NM_006203.1 gb:U02882.1
-0.06159	3.027095	8.51	Up	3.60E-04	U16797	Human LERK-5 (EPLG5) mRNA, complete cds. /PROD=LERK-5 /FL=gb:U16797.1 gb:NM_004093.1 gb:L38734.1 gb:U81262.1
4.07051	7.149479	8.45	Up	4.86E-05	M10943	Human metallothionein-If gene (hMT-If)
-0.35204	2.705807	8.33	Up	1.09E-03	BC004490	Homo sapiens, v-fos FBJ murine osteosarcoma viral oncogene homolog, clone MGC:11074, mRNA, complete cds. /PROD=v-fos FBJ murine osteosarcoma viral oncogenehomolog /FL=gb:NM_005252.2 gb:BC004490.1
-2.0132	1.043139	8.32	Up	3.61E-02	BE328496	hypothetical protein PRO2032 /FL=gb:AF116683.1 gb:NM_018615.1
-0.68954	2.36447	8.31	Up	8.94E-04	NM_005181	Homo sapiens carbonic anhydrase III, muscle specific (CA3), mRNA. /PROD=carbonic anhydrase III /FL=gb:BC004897.1 gb:NM_005181.2
-0.00953	3.031935	8.23	Up	9.88E-03	AA831438	Mad4 homolog
3.079271	6.1137	8.19	Up	4.17E-05	NM_001553	Homo sapiens insulin-like growth factor binding protein 7 (IGFBP7), mRNA. /PROD=insulin-like growth factor binding protein 7 /FL=gb:NM_001553.1 gb:L19182.1
0.788995	3.806044	8.1	Up	6.41E-05	AV734646	DNA segment on chromosome X (unique) 9928 expressed sequence
0.9926	4.004698	8.07	Up	8.48E-05	AI202327	ESTs
0.051719	3.059444	8.04	Up	6.98E-04	NM_007350	Homo sapiens pleckstrin homology-like domain, family A, member 1 (PHLDA1), mRNA. /PROD=pleckstrin homology-like domain, family A,member 1 /FL=gb:NM_007350.1
-1.69103	1.312148	8.02	Up	1.82E-03	U32500	Human type 2 neuropeptide Y receptor mRNA, complete cds. /PROD=type 2 neuropeptide Y receptor /FL=gb:U42766.1 gb:U36269.1 gb:U32500.1
-0.93931	2.060071	8	Up	6.51E-03	AA004300	hypothetical protein DKFZp566I133
1.164666	4.161028	7.98	Up	2.51E-03	BC005807	Homo sapiens, clone MGC:10264, mRNA, complete cds. /PROD=Unknown (protein for MGC:10264) /FL=gb:BC005807.1
2.462987	5.441963	7.88	Up	1.45E-04	NM_016651	Homo sapiens heptacellular carcinoma novel gene-3 protein (LOC51339), mRNA. /PROD=heptacellular carcinoma novel gene-3 protein /FL=gb:NM_016651.2 gb:AF251079.2
0.581498	3.560033	7.88	Up	1.07E-04	U38945	Human hypothetical 18.1 kDa protein (CDKN2A) mRNA, complete cds. /FL=gb:U38945.1 gb:U26727.1
0.470814	3.417829	7.71	Up	8.26E-03	AF176039	Homo sapiens high mobility group protein-R mRNA, complete cds. /PROD=high mobility group protein-R /FL=gb:AF176039.1
-1.50663	1.438639	7.7	Up	7.38E-04	BF223214	ESTs
-2.43082	0.495104	7.6	Up	1.71E-02	BF508288	ESTs
1.084464	4.009912	7.6	Up	1.16E-03	BC004865	Homo sapiens, cleft lip
				and palate associated transmembrane protein 1, clone MGC:10593, mRNA, complete cds. /PROD=cleft lip and palate associated transmembraneprotein 1 /FL=gb:BC004865.1
4.232374	7.152167	7.57	Up	1.54E-03	BF971587	tubulin, beta polypeptide /FL=gb:BC001352.1
0.129315	3.042634	7.53	Up	2.17E-04	NM_005442	Homo sapiens eomesodermin (Xenopus laevis) homolog (EOMES), mRNA. /PROD=eomesodermin (Xenopus laevis) homolog /FL=gb:AB031038.1 gb:NM_005442.1
-0.20075	2.710846	7.52	Up	2.58E-02	NM_003377	Homo sapiens vascular endothelial growth factor B (VEGFB), mRNA. /PROD=vascular endothelial growth factor B/FL=gb:NM_003377.1 gb:U43368.1 gb:U52819.1
-0.45681	2.439084	7.44	Up	7.82E-03	AI417362	ESTs, Moderately similar to ALU 1_HUMAN ALU SUBFAMILY J SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.155309	3.037724	7.37	Up	8.78E-04	NM_007061	Homo sapiens serum constituent protein (MSE55), mRNA. /PROD=serum constituent protein /FL=gb:M88338.1 gb:NM_007061.1
1.506057	4.362244	7.24	Up	7.30E-05	NM_001425	Homo sapiens epithelial membrane protein 3 (EMP3), mRNA. /PROD=epithelial membrane protein 3 /FL=gb:U52101.1 gb:NM_001425.1 gb:U87947.1
-1.75194	1.091177	7.18	Up	3.15E-02	NM_021570	Homo sapiens BarH-like homeobox 1 (BARX1), mRNA. /PROD=BarH-like homeobox 1 /FL=gb:NM_021570.2 gb:AF213356.1
2.455614	5.294065	7.15	Up	9.88E-03	AF279899	Homo sapiens PNAS-145 mRNA, complete cds. /PROD=PNAS-145 /FL=gb:U03105.1 gb:NM_006813.1
				gb:AF279899.1
1.422626	4.257559	7.14	Up	2.01E-05	NM_006365	Homo sapiens transcriptional activator of the c-fos promoter (CROC4), mRNA. /PROD=transcriptional activator of the c-fos promoter /FL=gb:NM_006365.1 gb:U49857.1
-2.40588	0.424388	7.11	Up	1.64E-02	NM_002433	Homo sapiens myelin oligodendrocyte glycoprotein (MOG), mRNA. /PROD=myelin oligodendrocyte glycoprotein /FL=gb:U18798.1 gb:U64564.1 gb:NM_002433.1
-1.86904	0.959227	7.1	Up	4.35E-02	AB033831	Homo sapiens hSCDGF mRNA for spinal cord-derived growth factor, complete cds. /PROD=spinal cord-derived growth factor /FL=gb:NM_016205.1 gb:AB033831.1 gb:AF091434.1 gb:AF244813.1
1.811736	4.639749	7.1	Up	1.09E-03	M27830	Human 28S ribosomal RNA gene, complete cds.
-0.54131	2.28595	7.1	Up	3.63E-03	BE504838	ESTs
4.065536	6.887587	7.07	Up	4.08E-04	NM_005796	Homo sapiens nuclear transport factor 2 (placental protein 15) (PP15), mRNA. /PROD=nuclear transport factor 2 (placental protein15) /FL=gb:BC002348.1 gb:NM_005796.1 gb:U43939.1
-0.4348	2.379408	7.03	Up	4.24E-03	BF686824	death-associated protein kinase 3 /FL=gb:AB007144.1 gb:AB022341.1 gb:NM_001348.1
1.448288	4.255531	7	Up	2.01E-05	AF096296	Homo sapiens thymic stroma chemokine-1 precursor, mRNA, complete cds. /PROD=thymic stroma chemokine-1 precursor /FL=gb:AF142434.1 gb:AF096296.1 gb:AF124601.1 gb:AB010447.1 gb:NM_006072.1
3.504052	6.307554	6.98	Up	4.05E-05	NM_006622	Homo sapiens serum-inducible kinase (SNK), mRNA. /PROD=serum-inducible kinase /FL=gb:AF059617.1 gb:NM_006622.1 gb:AF223574.1
2.124541	4.927935	6.98	Up	8.80E-05	J05008	Homo sapiens endothelin-1 (EDN1) gene, complete cds /FL=gb:NM_001955.1
1.872394	4.674078	6.97	Up	1.02E-05	AK022852	Homo sapiens cDNA FLJ12790 fis, clone NT2RP2001985, weakly similar to Homo sapiens high-risk human papilloma viruses E6 oncoproteins targeted protein E6TP1 alpha mRNA.
1.764338	4.563535	6.96	Up	1.43E-04	AA909044	tryptase, alpha
1.401293	4.178686	6.86	Up	1.66E-04	NM_003256	Homo sapiens tissue inhibitor of metalloproteinase 4 (TIMP4), mRNA. /PROD=tissue inhibitor of metalloproteinase 4precursor /FL=gb:NM_003256.1 gb:U76456.1
0.767075	3.54446	6.86	Up	1.88E-03	AY029208	Homo sapiens type VI collagen alpha 2 chain precursor (COL6A2) mRNA, complete cds, alternatively spliced. /PROD=type VI collagen alpha 2 chain precursor /FL=gb:AY029208.1
-1.94468	0.831091	6.85	Up	1.92E-02	NM_153036	Homo sapiens hypothetical protein FLJ32239 (FLJ32239), mRNA. /FL=gb:NM_153036.1
0.586923	3.359675	6.83	Up	4.17E-05	NM_000047	Homo sapiens arylsulfatase E (chondrodysplasia punctata 1) (ARSE), mRNA. /PROD=arylsulfatase E precursor /FL=gb:X83573.1 gb:NM_000047.1
1.064878	3.834572	6.82	Up	2.41E-04	NM_002610	Homo sapiens pyruvate dehydrogenase kinase, isoenzyme 1 (PDK1), nuclear gene encoding mitochondrial protein, mRNA. /PROD=pyruvate dehydrogenase kinase, isoenzyme 1 /FL=gb:NM_002610.2 gb:L42450.1
-0.11882	2.64743	6.8	Up	6.88E-04	AI702438	ESTs
-0.34208	2.418198	6.78	Up	2.31E-04	AI860150	ESTs, Weakly similar to A49134 Ig kappa chain V-I region (H.sapiens)
4.156522	6.9125	6.76	Up	6.48E-05	NM_003240	Homo sapiens endometrial bleeding associated factor (left-right determination, factor A; transforming growth factor beta superfamily) (EBAF), mRNA. /PROD=transforming growth factor, beta 4 /FL=gb:U81523.1 gb:NM_003240.1 gb:AF081513.1
-1.8911	0.860193	6.73	Up	2.83E-03	NM_001191	Homo sapiens BCL2-like 1 (BCL2L1), mRNA. /PROD=BCL2-like 1 /FL=gb:NM_001191.1
-0.53771	2.208449	6.71	Up	1.41E-02	AI806338	T-box 3 (ulnar mammary syndrome) /FL=gb:AF170708.2 gb:NM_005996.1
3.824397	6.568635	6.7	Up	1.66E-04	AL031602	Human DNA sequence from clone RP5-1174N9 on chromosome 1p34.1-35.3. Contains the gene for a novel protein with IBR domain, a (pseudo?) gene for a novel protein similar to MT1 E (metallothionein 1E (functional)), ESTs, STSs, GSSs and two putative Cp...
0.001822	2.741586	6.68	Up	4.44E-05	NM_004904	Homo sapiens cAMP response element-binding protein CRE-BPa (H_GS165L15.1), mRNA. /PROD=cAMP response element-binding protein CRE-BPa /FL=gb:NM_004904.1 gb:L05911.1
0.301216	3.030236	6.63	Up	4.76E-04	AA812232	upregulated by 1,25-dihydroxyvitamin D-3 /FL=gb:NM_006472.1 gb:S73591.1
4.63387	7.360687	6.62	Up	4.17E-05	BF217861	metallothionein 1E (functional)
0.413191	3.124723	6.55	Up	5.00E-02	AL136925	Homo sapiens mRNA; cDNA DKFZp586H1320 (from clone DKFZp586H1320); complete cds. /PROD=hypothetical protein /FL=gb:AL136925.1
-0.28056	2.427947	6.54	Up	1.39E-03	AW090187	dihydropyrimidinase-like 4 /FL=gb:NM_006426.1 gb:AB006713.1
1.095892	3.804014	6.53	Up	2.43E-04	NM_001146	Homo sapiens angiopoietin 1 (ANGPT1), mRNA. /PROD=angiopoietin 1 /FL=gb:NM_001146.1 gb:D13628.1 gb:U83508.1
-0.0845	2.62025	6.52	Up	2.59E-04	AA625683	ESTs
2.13274	4.835771	6.51	Up	2.01E-04	AL574210	serine (or cysteine) proteinase inhibitor, clade E (nexin, plasminogen activator inhibitor type 1), member 1 /FL=gb:NM_000602.1 gb:M16006.1
-0.64252	2.055951	6.49	Up	2.10E-04	NM_001035	Homo sapiens ryanodine receptor 2 (cardiac) (RYR2), mRNA. /PROD=ryanodine receptor 2 (cardiac) /FL=gb:NM_001035.1
4.450364	7.144308	6.47	Up	3.61E-05	BF246115	RNA helicase-related protein
0.405368	3.094055	6.45	Up	6.25E-05	AW 188198	tumor necrosis factor, alpha-induced protein 6 /FL=gb:NM_007115.1
-0.34351	2.332751	6.39	Up	5.54E-05	NM_000077	Homo sapiens cyclin-dependent kinase inhibitor 2A (melanoma, p16, inhibits CDK4) (CDKN2A), mRNA. /PROD=cyclin-dependent kinase inhibitor 2A (melanoma,p16, inhibits CDK4) /FL=gb:NM_000077.1 gb:L27211.1
-0.88122	1.790331	6.37	Up	1.37E-03	AA775681	hypothetical protein FLJ23091
3.508565	6.179917	6.37	Up	8.80E-05	NM_000158	Homo sapiens glucan (1,4-alpha-), branching enzyme 1 (glycogen branching enzyme, Andersen disease, glycogen storage disease type IV) (GBE1), RNA. /PROD=glucan (1,4-alpha-), branching enzyme 1(glycogen branching enzyme) /FL=gb:L07956.1 gb:NM_000158.1
-1.84589	0.82486	6.37	Up	3.13E-03	AV705309	ESTs
-0.18263	2.487276	6.36	Up	1.49E-02	AC006942	Homo sapiens chromosome 19, cosmid R31181
3.759854	6.426778	6.35	Up	2.01E-05	AF313413	Homo sapiens putative small membrane protein NID67 mRNA, complete
				cds. /PROD=putative small membrane protein NID67 /FL=gb:AF313413.1
2.4094	5.066795	6.31	Up	3.61E-05	AI809870	HSKM-B protein
-2.08089	0.570296	6.28	Up	7.70E-03	BC016043	Homo sapiens, hypothetical protein MGC2865, clone MGC:20246 IMAGE:4635389, mRNA, complete cds. /FL=gb:BC016043.1
1.37641	4.004952	6.18	Up	1.20E-04	AU148611	Human pTR7 mRNA for repetitive sequence
1.384716	4.012773	6.18	Up	4.52E-04	NM_006275	Homo sapiens splicing factor, arginineserine-rich 6 (SFRS6), mRNA. /PROD=splicing factor, arginineserine-rich 6 /FL=gb:U30883.1 gb:NM_006275.1
2.979212	5.604053	6.17	Up	1.52E-04	M27830	Human 28S ribosomal RNA gene, complete cds.
0.310893	2.921559	6.11	Up	3.42E-04	NM_007279	Homo sapiens U2 small nuclear ribonucleoprotein auxiliary factor (65kD) (U2AF65), mRNA. /PROD=U2 small nuclear ribonucleoprotein auxiliaryfactor (65kD) /FL=gb:NM_007279.1
0.65284	3.256353	6.08	Up	2.49E-04	AI819043	ESTs
1.609773	4.213168	6.08	Up	1.35E-04	M29277	Human isolate JuSo MUC18 glycoprotein mRNA (3 variant), complete cds. /PROD=MUC18 glycoprotein /FL=gb:M29277.1
-0.62167	1.968272	6.02	Up	4.11E-04	AI963304	ESTs
4.459837	7.047717	6.01	Up	1.02E-04	NM_004052	Homo sapiens BCL2adenovirus E1B 19kD-interacting protein 3 (BNIP3), nuclear gene encoding mitochondrial protein, mRNA. /PROD=BCL2adenovirus E1B 19kD-interacting protein 3 /FL=gb:AF002697.1 gb:NM_004052.2 gb:U15174.1
3.178404	5.762898	6	Up	1.27E-04	AB037810	Homo sapiens mRNA for KIAA1389 protein, partial cds. /PROD=KIAA1389 protein
-1.08931	1.494664	6	Up	2.35E-03	AB020683	Homo sapiens mRNA for KIAA0876 protein, partial cds. /PROD=KIAA0876
				protein
1.9194	4.501184	5.99	Up	3.61E-05	AK000162	Homo sapiens cDNA FLJ20155 fis, clone COL08754, highly similar to ACSA_ECOLI ACETYL-COENZYME A SYNTHETASE.
0.671205	3.243641	5.95	Up	2.48E-04	AA46362E	ESTs
0.091029	2.660133	5.93	Up	9.55E-04	AF277174	Homo sapiens PNAS-137 mRNA, complete cds. /PROD=PNAS-137 /FL=gb:AF277174.1
1.479222	4.042679	5.91	Up	6.34E-05	NM_005454	Homo sapiens cerberus 1 (Xenopus laevis) homolog (cysteine knot superfamily) (CER1), mRNA. /PROD=cerberus 1 /FL=gb:NM_005454.1
-0.29455	2.259676	5.87	Up	2.79E-03	AF312393	Homo sapiens leucine-zipper protein FKSG13 (FKSG13) mRNA, complete cds. /PROD=leucine-zipper protein FKSG13 /FL=gb:AF312393.1
-0.81321	1.740607	5.87	Up	3.72E-02	NM_002160	Homo sapiens hexabrachion (tenascin C, cytotactin) (HXB), mRNA. /PROD=hexabrachion (tenascin C, cytotactin) /FL=gb:M55618.1 gb:NM_002160.1
0.167058	2.720179	5.87	Up	1.02E-04	NM_021223	Homo sapiens myosin light chain 2a (LOC58498), mRNA. /PROD=myosin light chain 2a /FL=gb:NM_021223.1
0.901323	3.451092	5.86	Up	3.05E-05	NM_005767	Homo sapiens purinergic receptor (family A group 5) (P2Y5), mRNA. /PROD=purinergic receptor (family A group 5) /FL=gb:AF000546.1 gb:NM_005767.1
1.007578	3.543738	5.8	Up	2.13E-04	NM_001955	Homo sapiens endothelin 1 (EDN1), mRNA. /PROD=endothelin 1 /FL=gb:NM_001955.1
1.327779	3.862686	5.8	Up	1.51E-04	NM_007115	Homo sapiens tumor necrosis factor, alpha-induced protein 6 (TNFAIP6), mRNA. /PROD=tumor necrosis factor, alpha-induced protein 6 /FL=gb:NM_007115.1
-0.2077	2.32716	5.8	Up	1.52E-04	AA211909	ESTs
1.304257	3.835269	5.78	Up	3.02E-04	NM_005451	Homo sapiens enigma (LIM domain protein)
				(ENIGMA), mRNA. /PROD=enigma protein /FL=gb:BC001093.1 gb:NM_005451.2 gb:AF265209.1
-0.30113	2.227329	5.77	Up	4.58E-03	BE968750	Homo sapiens ryanodine receptor 2 (cardiac) (RYR2), mRNA
1.678635	4.204607	5.76	Up	9.75E-05	AA086229	enigma (LIM domain protein)
1.411335	3.932627	5.74	Up	1.58E-02	NM_003370	Homo sapiens vasodilator-stimulated phosphoprotein (VASP), mRNA. /PROD=vasodilator-stimulated phosphoprotein /FL=gb:NM_003370.1
-1.32153	1.183922	5.68	Up	2.72E-02	AF217536	Homo sapiens truncated mevalonate kinase mRNA, partial cds, alternatively spliced. /PROD=truncated mevalonate kinase
1.058988	3.560886	5.66	Up	3.56E-03	H05812	insulin-like growth factor 1 receptor /FL=gb:NM_000875.2
4.435207	6.93459	5.65	Up	3.61E-05	AF078844	Homo sapiens hqp0376 protein mRNA, complete cds. /PROD=hqp0376 protein /FL=gb:AF078844.1
2.418835	4.908301	5.62	Up	3.47E-03	NM_012268	Homo sapiens similar to vaccinia virus HindIII K4L ORF (HU-K4), mRNA. /PROD=similar to vaccinia virus HindIII K4L ORF /FL=gb:U60644.1 gb:BC000553.1 gb:NM_012268.1
-0.56112	1.927121	5.61	Up	6.37E-03	AL041124	hypothetical protein PP1665
-1.63462	0.844727	5.58	Up	4.98E-03	AI831874	ESTs
-0.34446	2.130828	5.56	Up	3.75E-05	NM_006379	Homo sapiens sema domain, immunoglobulin domain (Ig), short basic domain, secreted, (semaphorin) 3C (SEMA3C), mRNA. /PROD=sema domain, immunoglobulin domain (Ig), shortbasic domain, secreted, (semaphorin) 3C /FL=gb:NM_006379.1 gb:AB000220.1
4.143258	6.618477	5.56	Up	1.18E-05	AU146532	pyruvate dehydrogenase kinase, isoenzyme 1
-0.52233	1.950739	5.55	Up	1.54E-03	AI091047	solute carrier family 2 (facilitated glucose transporter), member 1 /FL=gb:K03195.1 gb:NM_006516.1
0.690529	3.155168	5.52	Up	9.91E-04	BC033088	Homo sapiens, Similar to lamin AC, clone MGC:45654 IMAGE:3623265, mRNA, complete cds. /PROD=Similar to lamin AC /FL=gb:BC033088.1
-0.00098	2.454314	5.48	Up	2.48E-04	NM_013281	Homo sapiens fibronectin leucine rich transmembrane protein 3 (FLRT3), mRNA. /PROD=fibronectin leucine rich transmembrane protein3 /FL=gb:AF169677.1 gb:NM_013281.1
-0.87622	1.577138	5.48	Up	1.84E-02	M15329	Human interleukin 1-alpha (IL 1A) mRNA, complete cds. /PROD=interleukin 1-alpha IFL=gb:M15329.1
5.117294	7.564809	5.45	Up	6.25E-05	M83248	Human nephropontin mRNA, complete cds. /PROD=nephropontin /FL=gb:M83248.1
2.352834	4.796495	5.44	Up	4.17E-05	AI653107	ESTs
3.27933	5.719116	5.43	Up	3.24E-04	NM_016639	Homo sapiens type I transmembrane protein Fn14 (FN14), mRNA. /PROD=type I transmembrane protein Fn14 /FL=gb:NM_016639.1 gb:BC002718.1 gb:AB035480.1 gb:AF191148.1
-2.06232	0.368788	5.39	Up	6.40E-03	AA148534	pregnancy-associated plasma protein A /FL=gb:NM_002581.1 gb:U28727.1
3.982825	6.413408	5.39	Up	7.48E-05	AA678241	stearoyl-CoA desaturase (delta-9-desaturase) /FL=gb:AB032261.1 gb:AF097514.1 gb:NM_005063.1
0.399566	2.809822	5.32	Up	7.81E-04	AF144103	Homo sapiens NJAC protein (NJAC) mRNA, complete cds. /PROD=NJAC protein /FL=gb:AF144103.1 gb:AF106911.1 gb:AF073957.1 gb:BC003513.1 gb:NM_004887.1
4.15299	6.560926	5.31	Up	6.59E-05	NM_0009 35	Homo sapiens procollagen-lysine, 2-oxoglutarate 5-dioxygenase (lysine hydroxylase) 2 (PLOD2), mRNA.
				/PROD=procollagen-lysine, 2-oxoglutarate 5-dioxygenase(lysine hydroxylase) 2 /FL=gb:NM_000935.1 gb:U84573.1
0.319769	2.724257	5.29	Up	8.94E-04	AL552534	Human mRNA for CD44 antigen, 5UTR (sequence from the 5cap to the start codon).
3.347359	5.750515	5.29	Up	5.27E-03	AF047002	Homo sapiens transcriptional coactivator ALY mRNA, partial cds. /PROD=transcriptional coactivator ALY
4.571448	6.973787	5.29	Up	3.53E-04	AI631159	solute carrier family 2 (facilitated glucose transporter), member 3 /FL=gb:NM_006931.1 gb:M20681.1
1.93843	4.333496	5.26	Up	1.21E-04	NM_019886	Homo sapiens carbohydrate (N-acetylglucosamine 6-O) sulfotransferase 7 (CHST7), mRNA. /PROD=carbohydrate (N-acetylglucosamine 6-O)sulfotransferase 7 /FL=gb:NM_019886.1 gb:AB037187.1 gb:AB040711.1
-0.3185	2.064012	5.21	Up	1.55E-03	U83508	Human angiopoietin-1 mRNA, complete cds. /PROD=angiopoietin-1 /FL=gb:NM_001146.1 gb:D13628.1 gb:U83508.1
1.484424	3.866551	5.21	Up	3.49E-04	BC000076	Homo sapiens, cyclin D1 (PRAD1: parathyroid adenomatosis 1), clone MGC:2316, mRNA, complete cds. /PROD=cyclin D1 (PRAD1: parathyroid adenomatosis 1) /FL=gb:M73554.1 gb:BC000076.1
4.465458	6.844763	5.2	Up	1.52E-04	AF003114	Homo sapiens CYR61 mRNA, complete cds. /FL=gb:AF003114.1
-1.33756	1.041706	5.2	Up	8.51E-03	BF196010	ESTs
3.747557	6.125638	5.2	Up	4.52E-04	AA554833	neuroendocrine secretory protein 55
-0.24196	2.129273	5.17	Up	2.80E-04	AV734646	DNA segment on chromosome X (unique) 9928 expressed sequence
2.657439	5.023981	5.16	Up	1.66E-04	NM_006472	Homo sapiens upregulated by 1,25-dihydroxyvitamin D-3 (VDUP1), mRNA.
	/PROD=upregulated by 1,25-dihydroxyvitamin D-3 /FL=gb:NM_006472.1 gb:S73591.1
1.275689	3.642133	5.16	Up	1.65E-04	BF982289	ESTs, Weakly similar to elastin like protein (D.melanogaster)
2.11271	4.458591	5.08	Up	1.97E-04	H15920	ESTs, Weakly similar to RTA RAT PROBABLE G PROTEIN-COUPLED RECEPTOR RTA (R.norvegicus)
2.624088	4.968498	5.08	Up	1.45E-04	M28882	Human MUC18 glycoprotein mRNA, complete cds. /PROD=MUC18 glycoprotein /FL=gb:M28882.1
4.046173	6.388326	5.07	Up	6.34E-05	NM_015641	Homo sapiens testin (DKFZP586B2022), mRNA. /PROD=testin /FL=gb:BC001451.1 gb:AF245357.1 gb:AF245356.1 gb:NM_015641.1
0.946455	3.284436	5.06	Up	5.46E-04	BM976939	Homo sapiens cDNA FLJ31611 fis, clone NT2RI2002923.
1.389207	3.725552	5.05	Up	1.08E-04	AL136805	Homo sapiens mRNA; cDNA DKFZp434J1521 (from clone DKFZp434J1521); complete cds. /PROD=hypothetical protein /FL=gb:AL136805.1
0.710433	3.041407	5.03	Up	1.08E-03	NM_004472	Homo sapiens forkhead box D1 (FOXD1 MRNA /PROD=forkhead box D1 /FL=gb:U59832.1 gb:NM_004472.1
2.800881	5.127991	5.02	Up	6.53E-05	NM_017817	Homo sapiens hypothetical protein FLJ20429 (FLJ20429), mRNA. /PROD=hypothetical protein FLJ20429 /FL=gb:NM_017817.1
0.432778	2.759117	5.02	Up	2.50E-03	A1692523	ESTs
-0.94056	1.385676	5.01	Up	4.17E-03	AI927458	Homo sapiens mRNA; cDNA DKFZp434A196 (from clone DKFZp434A196); complete cds
0.224112	2.550074	5.01	Up	4.11E-04	BF060767	ESTs
-0.47823	1.845598	5.01	Up	2.75E-03	AA489100	ESTs
4.590104	-3.36994	249.01	Down	2.26E-04	AA167449	nuclear receptor subfamily 1, group I, member 3
6.024741	-1.32044	162.6	Down	1.79E-03	AF017987	Homo sapiens secreted
				apoptosis related protein 2 (SARP2) mRNA, complete cds. /PROD=secreted apoptosis related protein 2 /FL=gb:AF056087.1 gb:NM_003012.2 gb:AF017987.1 gb:AF001900.1
1.940449	-5.04898	127.07	Down	3.05E-05	BE644917	nuclear receptor subfamily 1, group I, member 3
2.68759	-3.61621	79	Down	1.25E-03	AL569326	Homo sapiens cAMP-dependent protein kinase inhibitor beta mRNA, complete cds
5.005827	-1.03397	65.79	Down	1.30E-04	NM_003020	Homo sapiens secretory granule, neuroendocrine protein 1 (7B2 protein) (SGNE1), mRNA. /PROD=secretory granule, neuroendocrine protein 1 (7B2protein) /FL=gb:BC005349.1 gb:NM_003020.1
0.357833	-5.67924	65.67	Down	2.26E-03	BG38978 9	Human mRNA upregulated during camptothecin-induced apoptosis of U937 cells.
6.500961	0.756526	53.61	Down	4.17E-05	NM_003012	Homo sapiens secreted frizzled-related protein 1 (SFRP1), mRNA. /PROD=secreted frizzled-related protein 1 /FL=gb:AF056087.1 gb:NM_003012.2 gb:AF017987.1 gb:AF001900.1
2.077151	-3.59883	51.13	Down	3.75E-03	BF223193	nuclear receptor subfamily 1, group I, member 3
3.29779	-2.3376	49.71	Down	3.05E-05	U17496	Human proteasome subunit LMP7 (allele LMP7B) mRNA, complete cds. /PROD=proteasome subunit LMP7 /FL=gb:U17497.1 gb:U17496.1
4.803291	-0.78667	48.17	Down	3.75E-05	AA628440	nuclear receptor subfamily 1, group I, member 3
4.124115	-1.42293	46.75	Down	7.16E-04	AW262311	ESTs
2.437935	-3.10907	46.75	Down	2.41E-04	BE672557	ESTs
4.276201	-1.19736	44.43	Down	9.47E-04	AV699347	nuclear receptor subfamily 1, group I, member 3
1.710253	-3.7619	44.39	Down	8.66E-05	NM_016179	Homo sapiens transient receptor potential channel 4 (TRPC4), mRNA. /PROD=transient receptor potential 4 /FL=gb:NM_016179.1 gb:AF175406.1
2.313549	-3.12747	43.44	Down	5.45E-04	AV726956	ESTs, Weakly similar to C35826 hypothetical 13K protein A (H.sapiens)
2.835599	-2.26295	34.26	Down	2.50E-03	AI735586	ESTs
0.588183	-4.50758	34.2	Down	2.89E-04	AU118882	endothelin receptor type A /FL=gb:NM_001957.1 gb:L06622.1
0.349102	-4.73558	33.93	Down	2.50E-02	BM682352	Homo sapiens cDNA FLJ37204 fis, clone BRALZ2006976.
-0.10303	-5.00884	29.98	Down	1.97E-04	NM_022168	Homo sapiens melanoma differentiation associated protein-5 (MDA5), mRNA. /PROD=melanoma differentiation associated protein-5 /FL=gb:AY017378.1 gb:NM_022168.1 gb:AF095844.1
2.325274	-2.506	28.47	Down	1.35E-04	AW193693	DKFZP566K1924 protein
0.252976	-4.55112	27.94	Down	2.54E-02	NM_018043	Homo sapiens hypothetical protein FLJ10261 (FLJ10261), mRNA. /PROD=hypothetical protein FLJ10261 /FL=gb:NM_018043.1
2.719388	-2.08299	27.9	Down	1.72E-02	NM_002048	Homo sapiens growth arrest-specific 1 (GAS1), mRNA. /PROD=growth arrest-specific 1 /FL=gb:NM_002048.1 gb:L13698.1
3.257726	-1.54343	27.88	Down	6.25E-05	NM_004335	Homo sapiens bone marrow stromal cell antigen 2 (BST2), mRNA. /PROD=bone marrow stromal cell antigen 2 /FL=gb:NM_004335.2 gb:D28137.1
4.353788	-0.41404	27.24	Down	4.72E-04	AI332407	secreted frizzled-related protein 1 /FL=gb:AF056087.1 gb:NM_003012.2 gb:AF017987.1 gb:AF001900.1
4.387855	-0.27888	25.4	Down	6.82E-05	AF225513	Homo sapiens cAMP-dependent protein kinase inhibitor beta mRNA, complete cds. /PROD=cAMP-dependent protein kinase inhibitor beta /FL=gb:AF225513.1
0.027478	-4.62508	25.15	Down	9.89E-03	NM_152647	Homo sapiens hypothetical protein FLJ32800 (FLJ32800), mRNA. /FL=gb:NM_152647.1
1.767203	-2.80617	23.81	Down	4.44E-04	AI742043	ESTs
1.665643	-2.69521	20.55	Down	1.08E-04	AF282250	Homo sapiens calneuron 1 (CALN1) mRNA, complete cds. /PROD=calneuron 1 /FL=gb:AF282250.1
0.414323	-3.84422	19.14	Down	3.42E-04	AF283777	Homo sapiens clone TCBAP0702 mRNA sequence.
3.779853	-0.4664	18.98	Down	4.72E-04	AV646597	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
1.995324	-2.233	18.74	Down	1.01E-03	NM_014862	Homo sapiens KIAA0307 gene product (KIAA0307), mRNA. /PROD=KIAA0307 gene product /FL=gb:AB002305.1 gb:NM_014862.1
1.946332	-2.24096	18.22	Down	2.40E-03	BG166705	small inducible cytokine subfamily B (Cys-X-Cys), member 5 (epithelial-derived neutrophil-activating peptide 78)
1.179963	-2.9904	18.01	Down	2.13E-04	U96136	Homo sapiens delta-catenin mRNA, complete cds. /PROD=delta-catenin /FL=gb:NM_001332.1 gb:U72665.1 gb:AB013805.1 gb:U96136.1 gb:AF035302.1
2.060687	-2.07873	17.62	Down	1.01E-03	AI269290	solute carrier family 18 (vesicular monoamine), member 2 /FL=gb:L14269.1 gb:L23205.1 gb:L09118.1 gb:NM_003054.1
2.480221	-1.64839	17.49	Down	1.22E-03	NM_004900	Homo sapiens phorbolin (similar to apolipoprotein B mRNA editing protein) (DJ742C19.2), mRNA. /PROD=phorbolin (similar to apolipoprotein B mRNAediting protein) /FL=gb:NM_004900.1 gb:U61083.1
0.971941	-3.12304	17.09	Down	1.07E-02	NM_018018	Homo sapiens hypothetical protein FLJ10191 (FLJ10191), mRNA. /PROD=hypothetical protein FLJ10191 /FL=gb:NM_018018.1
2.263194	-1.81469	16.89	Down	2.69E-03	AF052108	Homo sapiens clone 23687 mRNA sequence.
2.115848	-1.84267	15.55	Down	3.89E-02	AF213678	Homo sapiens HAI-2 related small protein (HAI-2) mRNA, complete cds. /PROD=HAI-2 related small protein /FL=gb:AB038317.1 gb:AF213678.1
2.348373	-1.56046	15.02	Down	7.77E-03	NM_016354	Homo sapiens solute carrier family 21 (organic anion transporter), member 12 (SLC21A12), mRNA. /PROD=organic anion transporter OATP-E /FL=gb:AB031051.1 gb:NM_016354.1 gb:AF205072.1 gb:AF187817.1
1.910263	-1.99418	14.97	Down	3.77E-04	NM_006994	Homo sapiens butyrophilin, subfamily 3, member A3 (BTN3A3), mRNA. /PROD=butyrophilin, subfamily 3, member A3 /FL=gb:U90548.1 gb:NM_006994.2
2.699795	-1.16113	14.53	Down	5.07E-03	NM_012281	Homo sapiens potassium voltage-gated channel, Shal-related subfamily, member 2 (KCND2), mRNA. /PROD=potassium voltage-gated channel, Shal-relatedsubfamily, member 2 /FL=gb:NM_012281.1 gb:AB028967.1 gb:AF121104.1
2.172559	-1.66608	14.31	Down	7.83E-03	BE673445	Homo sapiens chromosome 19, cosmid R28379
0.265765	-3.53873	13.97	Down	2.21E-03	AI675836	Human DNA sequence from clone RP11-446H13 on chromosome 10. Contains the 3 end of the gene for a novel protein similar to KIAA1059 (ortholog of mouse VPS10 domain receptor protein SORCS), an RPL23A (60S ribosmal protein 23A) pseudogene, ESTs, STSs an
5.440506	1.644236	13.89	Down	6.34E-05	M34455	Human interferon-gamma-inducible indoleamine 2,3-dioxygenase (IDO) mRNA, complete cds. /FL=gb:NM_002164.1 gb:M34455.1
0.330556	-3.45471	13.79	Down	5.46E-04	BE972639	ESTs
0.437404	-3.31877	13.51	Down	4.52E-04	H05254	ESTs
1.32524	-2.42314	13.44	Down	1.57E-02	H29627	ESTs
1.673028	-2.06656	13.36	Down	5.30E-03	AF141339	Homo sapiens LYST-interacting protein LIP3 mRNA, partial cds. /PROD=LYST-interacting protein LIP3
1.319614	-2.39234	13.1	Down	1.43E-02	NM_004389	Homo sapiens catenin (cadherin-associated protein), alpha 2 (CTNNA2), mRNA. /PROD=catenin (cadherin-associated protein), alpha 2/FL=gb:NM_004389.1 gb:M94151.2
1.708627	-1.98647	12.95	Down	1.75E-02	NM_017596	Homo sapiens KIAA0449 protein (KIAA0449), mRNA. /PROD=hypothetical protein DKFZp434J212 /FL=gb:NM_017596.1
2.777148	-0.8902	12.71	Down	4.36E-04	NM_022034	Homo sapiens estrogen regulated gene 1 (ERG-1), mRNA. /PROD=estrogen regulated gene 1 /FL=gb:AF305835.1 gb:NM_022034.1
1.982765	-1.67669	12.64	Down	6.88E-04	BE672659	ESTs
0.457009	-3.18081	12.45	Down	3.30E-04	AW449813	KIAA0918 protein
0.510314	-3.12055	12.39	Down	1.71E-02	AW780006	ESTs
0.536704	-3.05382	12.05	Down	1.92E-02	AL049250	Homo sapiens mRNA; cDNA DKFZp564D113 (from clone DKFZp564D113).
2.294336	-1.27392	11.86	Down	1.66E-02	U11058	Homo sapiens large conductance calcium- and voltage-dependent potassium channel alpha subunit (MaxiK) mRNA, complete cds. /PROD=large conductance calcium- and voltage-dependentpotassium channel alpha subunit /FL=gb:U23767.1 gb:NM_002247.1 gb:AF025999
2.177763	-1.38062	11.78	Down	8.80E-05	NM_002590	Homo sapiens protocadherin 8 (PCDH8), mRNA. /PROD=protocadherin 8 /FL=gb:NM_002590.2 gb:AF061573.2
-0.48821	-4.01809	11.55	Down	2.29E-02	AB040812	Homo sapiens mRNA for protein kinase PAK5, complete cds. /PROD=protein kinase
1.785431	-1.74236	11.53	Down	2.18E-03	R15072	PAK5 /FL=gb:AB040812.1 ESTs
1.459269	-2.00069	11	Down	3.74E-04	NM_000277	Homo sapiens phenylalanine hydroxylase (PAH), mRNA. /PROD=phenylalanine hydroxylase /FL=gb:U49897.1 gb:NM_000277.1
1.995493	-1.44407	10.85	Down	7.11E-03	U91903	Human Fritz mRNA, complete cds. /PROD=Fritz /FL=gb:U24163.1 gb:U68057.1 gb:NM_001463.1 gb:U91903.1
0.679665	-2.7484	10.76	Down	5.57E-03	BC000568	Homo sapiens, clone MGC:3040, mRNA, complete cds. /PROD=Unknown (protein for MGC:3040) /FL=gb:BC000568.1
1.841888	-1.57619	10.69	Down	1.16E-03	AW072790	contactin 1
-0.42571	-3.8118	10.45	Down	1.58E-02	AK023699	Homo sapiens cDNA FLJ13637 fis, clone PLACE1011165.
1.923237	-1.4606	10.44	Down	4.11E-04	AW072102	Homo sapiens mRNA; cDNA DKFZp434H205 (from clone DKFZp434H205)
0.931661	-2.45074	10.43	Down	1.07E-02	AW 149405	neurexin 1 /FL=gb:AB035356.1
0.781816	-2.56699	10.19	Down	2.50E-02	NM_000698	Homo sapiens arachidonate 5-lipoxygenase (ALOX5), mRNA. /PROD=arachidonate 5-lipoxygenase /FL=gb:NM_000698.1 gb:J03600.1 gb:J03571.1
1.939598	-1.40726	10.17	Down	2.29E-03	AB014737	Homo sapiens mRNA for SMAP-2b, complete cds. /PROD=SMAP-2b /FL=gb:AB014737.1
0.874376	-2.46854	10.15	Down	1.59E-02	U82671	Homo sapiens chromosome Xq28 melanoma antigen family A2a (MAGEA2A), melanoma antigen family A12 (MAGEA12), melanoma antigen family A2b (MAGEA2B), melanoma antigen family A3 (MAGEA3), caltractin (CALT), NAD(P)H dehydrogenase-like protein (NSDHL), a...
3.315768	0.011663	9.88	Down	7.33E-04	AK098525	Homo sapiens cDNA
				FLJ25659 fis, clone TST00427, highly similar to Mus musculus hedgehog-interacting protein (Hip) mRNA.
0.121165	-3.1782	9.84	Down	4.65E-03	AI985987	ESTs, Moderately similar to ALU 1_HUMAN ALU SUBFAMILY J SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.686587	-2.59339	9.71	Down	2.72E-02	NM_000439	Homo sapiens proprotein convertase subtilisinkexin type 1 (PCSK1), mRNA. /PROD=proprotein convertase subtilisinkexin type 1 /FL=gb:NM_000439.2 gb:M90753.1
3.113317	-0.0881	9.2	Down	7.30E-05	AL565745	ESTs, Weakly similar to 2108402A carnitine palmitoyltransferase I (H.sapiens)
2.890305	-0.29832	9.12	Down	3.24E-04	NM_015474	Homo sapiens DKFZP564A032 protein (DKFZP564A032), mRNA. /PROD=DKFZP564A032 protein /FL=gb:AF228421.1 gb:AL050267.1 gb:AB013847.1 gb:NM_015474.1
0.447048	-2.73882	9.1	Down	4.19E-02	BE645435	ESTs
3.142124	-0.03564	9.05	Down	3.76E-03	AL832535	Homo sapiens mRNA; cDNA DKFZp547J1816 (from clone DKFZp547 J1816).
0.767101	-2.38787	8.91	Down	1.92E-02	BC003517	Homo sapiens, clone IMAGE:3542589, mRNA, partial cds. /PROD=Unknown (protein for IMAGE:3542589)
4.315048	1.168713	8.85	Down	7.92E-04	NM_016139	Homo sapiens 16.7Kd protein (LOC51142), mRNA. /PROD=16.7Kd protein /FL=gb:NM_016139.1 gb:AF078845.1 gb:BC003079.1
-0.47937	-3.61302	8.78	Down	2.49E-02	BE968773	Homo sapiens mRNA; cDNA DKFZp564O1262 (from clone DKFZp564O1262)
3.26376	0.151239	8.65	Down	1.74E-04	BE644809	ESTs
0.384182	-2.72567	8.63	Down	3.02E-02	NM_005825	Homo sapiens RAS guanyl releasing protein 2 (calcium and DAG-regulated) (RASGRP2),
	mRNA. /PROD=RAS guanyl releasing protein 2 (calcium andDAG-regulated) /FL=gb:AF043723.1 gb:NM_005825.1
2.363587	-0.72928	8.53	Down	7.38E-04	NM_024645	Homo sapiens hypothetical protein FLJ13842(FLJ13842), mRNA. /PROD=hypothetical protein FLJ 13842 /FL=gb:NM_024645.1
4.756657	1.668488	8.5	Down	1.30E-04	AV715309	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.995551	-2.07915	8.43	Down	3.01E-02	NM_005386	Homo sapiens neuronatin (NNAT), mRNA. /PROD=neuronatin /FL=gb:NM_005386.1 gb:BC001768.1 gb:AB002392.1 gb:U25033.1
2.380226	-0.68921	8.39	Down	8.34E-05	NM_016546	Homo sapiens complement C1 r-like proteinase precursor, (LOC51279), mRNA. /PROD=complement C1r-like proteinase precursor, /FL=gb:AF178985.1 gb:NM_016546.1
2.598916	-0.46577	8.37	Down	6.59E-05	AW051591	ESTs, Moderately similar to unnamed protein product (H.sapiens)
1.045717	-2.01579	8.35	Down	1.44E-02	AI937060	KIAA1151 protein
3.009579	-0.04543	8.31	Down	7.08E-04	AB037730	Homo sapiens mRNA for KIAA1309 protein, partial cds. /PROD=KIAA1309 protein
1.440541	-1.60998	8.29	Down	1.58E-02	BE503640	ESTs
0.4785	-2.56291	8.23	Down	2.46E-02	BG532690	integrin, alpha 4 (antigen CD49D, alpha 4 subunit of VLA-4 receptor)
5.84374	2.812887	8.17	Down	6.34E-05	BC000069	Homo sapiens, retinoic acid receptor responder (tazarotene induced) 2, clone MGC:1544, mRNA, complete cds. /PROD=retinoic acid receptor responder (tazaroteneinduced) 2 /FL=gb:BC000069.1 gb:NM_002889.2 gb:AB015632.1 gb:U77594.1
1.110683	-1.89628	8.04	Down	8.48E-04	AA557324	ESTs, Weakly similar to fatty acid omega-hydroxylase (H.sapiens)
1.386384	-1.61585	8.01	Down	3.53E-04	AF196571	Homo sapiens Delta-like-1 protein (DLL1) mRNA, complete cds. /PROD=Delta-like-1 protein /FL=gb:NM_005618.2 gb:AF196571.1
5.363884	2.372618	7.95	Down	7.30E-05	NM_007015	Homo sapiens chondromodulin I precursor (CHM-I), mRNA. /PROD=chondromodulin I precursor /FL=gb:NM_007015.1 gb:AB006000.1
1.364581	-1.62447	7.94	Down	2.16E-02	NM_145280	Homo sapiens similar to hepatocellular carcinoma-associated antigen HCA557b (LOC151194), mRNA. /FL=gb:BC009462.1 gb:NM_145280.1
2.628136	-0.35867	7.93	Down	1.22E-04	NM_001957	Homo sapiens endothelin receptor type A (EDNRA), mRNA. /PROD=endothelin receptor type A /FL=gb:NM_001957.1 gb:L06622.1
1.712212	-1.25121	7.8	Down	8.48E-04	R62432	Cluster Incl. R62432:yg52e11.s1 Homo sapiens cDNA, 3 end /clone=IMAGE-36023 /clone_end=3 /gb=R62432 /gi=834311 /ug=Hs.12321 /Ien=487
1.443731	-1.51616	7.78	Down	4.37E-03	AJ272267	Homo sapiens partial mRNA for choline dehydrogenase (chdh gene). /PROD=choline dehydrogenase
3.106596	0.148375	7.77	Down	1.23E-02	NM_002305	Homo sapiens lectin, galactoside-binding, soluble, 1 (galectin 1) (LGALS1), mRNA. /PROD=beta-galactosidase binding lectin precursor /FL=gb:NM_002305.2 gb:BC001693.1 gb:J04456.1
1.961633	-0.98665	7.72	Down	8.93E-03	NM_001463	Homo sapiens frizzled-related protein (FRZB), mRNA. /PROD=frizzled-related protein /FL=gb:U24163.1 gb:U68057.1
				gb:NM_001463.1 gb:U91903.1
2.38092	-0.54428	7.6	Down	6.34E-04	AF053712	Homo sapiens osteoprotegerin ligand mRNA, complete cds. /PROD=osteoprotegerin ligand /FL=gb:AF053712.1 gb:AF019047.1
0.685413	-2.22507	7.52	Down	2.98E-02	NM_018383	Homo sapiens hypothetical protein FLJ11294 (FLJ11294), mRNA. /PROD=hypothetical protein FLJ 11294 /FL=gb:NM_018383.1
-0.24717	-3.14972	7.48	Down	3.67E-04	AF429305	Homo sapiens C23up NCRMS mRNA, partial sequence; alternatively spliced.
3.893148	0.997757	7.44	Down	1.29E-04	AU144892	Homo sapiens cDNA FLJ11569 fis, clone HEMBA1003304
0.82553	-2.06523	7.42	Down	4.10E-02	BC041933	Homo sapiens, clone IMAGE:5300703, mRNA.
0.728978	-2.13318	7.27	Down	1.25E-03	AL573058	complement component 1, r subcomponent
1.033324	-1.8148	7.2	Down	5.93E-03	N80918	Novel human gene mapping to chomosome 13
2.858719	0.013383	7.19	Down	4.37E-03	L10374	Human (clone CTG-A4) mRNA sequence.
2.260317	-0.57539	7.14	Down	1.02E-03	AI138603	ESTs
2.003902	-0.82254	7.09	Down	8.00E-03	BF109660	ESTs
3.85985	1.037668	7.07	Down	2.70E-04	R40892	ESTs
3.921983	1.12675	6.94	Down	3.53E-04	AA206141	ESTs
-0.17018	-2.96268	6.93	Down	2.08E-02	AV741130	ESTs, Moderately similar to ALU8_HUMAN ALU SUBFAMILY SX SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
1.610685	-1.16078	6.83	Down	9.82E-04	AA886335	Homo sapiens serologically defined breast cancer antigen NY-BR-20 mRNA, partial cds
2.859538	0.089114	6.82	Down	2.22E-03	AW014734	ESTs
3.212409	0.467551	6.7	Down	2.69E-04	BG434174	Homo sapiens cDNA FLJ13555 fis, clone PLACE1007677
2.116702	-0.60252	6.59	Down	3.35E-03	AF107846	Homo sapiens neuroendocrine-specific Golgi protein p55 (XLalphas) gene, exon XL2 and complete cds
3.179908	0.462842	6.58	Down	3.24E-04	U82811	Human homeodomain-containing protein (HANF) mRNA, complete cds.
	/PROD=HANF /FL=gb:U82811.1 gb:NM_003865.1
2.509452	-0.20066	6.54	Down	1.04E-03	NM_001609	Homo sapiens acyl-Coenzyme A dehydrogenase, shortbranched chain (ACADSB), nuclear gene encoding mitochondrial protein, mRNA. /PROD=acyl-Coenzyme A dehydrogenase, shortbranchedchain precursor /FL=gb:U12778.1 gb:NM_001609.1
2.596054	-0.10733	6.51	Down	1.39E-03	BC005107	Homo sapiens, clone IMAGE:3840937, mRNA, partial cds. /PROD=Unknown (protein for IMAGE:3840937)
0.559211	-2.13754	6.48	Down	2.20E-02	BF000203	ESTs
4.534853	1.872557	6.33	Down	9.75E-05	R38389	olfactomedin related ER localized protein
2.068166	-0.59258	6.32	Down	1.69E-03	BF698797	ESTs
2.168796	-0.49174	6.32	Down	2.44E-04	NM_002522	Homo sapiens neuronal pentraxin I (NPTX1), mRNA. /PROD=neuronal pentraxin I precursor /FL=gb:NM_002522.1 gb:U61849.1
-0.10024	-2.75761	6.31	Down	3.60E-02	BC033812	Homo sapiens, Similar to LOC155399, clone MGC:45477 IMAGE:5181460, mRNA, complete cds. /PROD=Similar to LOC155399 /FL=gb:BC033812.1
0.994947	-1.65385	6.27	Down	7.39E-03	NM_024034	Homo sapiens hypothetical protein MGC3129 similar to ganglioside-induced differentiation-associated protein (MGC3129), mRNA. /PROD=hypothetical protein MGC3129 similar toganglioside-induced differentiation-associated protein /FL=gb:NM_024034.1 gb:BC0
3.758058	1.109291	6.27	Down	4.39E-04	NM_005356	Homo sapiens lymphocyte-specific protein tyrosine kinase (LCK), mRNA. /PROD=lymphocyte-specific protein tyrosine
				kinase /FL=gb:U07236.1 gb:NM_005356.1 gb:M36881.1
1.553207	-1.09181	6.26	Down	2.54E-02	AI653050	ESTs, Weakly similar to HPPD_HUMAN 4-HYDROXYPHENYLPYRU VATE DIOXYGENASE (H.sapiens)
3.702164	1.060081	6.24	Down	4.08E-04	U26662	Human neuronal pentraxin II (NPTX2) mRNA, partial cds. /PROD=neuronal pentraxin II
4.260791	1.638346	6.16	Down	6.25E-05	AA603344	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
2.172331	-0.44991	6.16	Down	2.44E-04	NM_003839	Homo sapiens tumor necrosis factor receptor superfamily, member 11a, activator of NFKB (TNFRSF11A), mRNA. /PROD=tumor necrosis factor receptor superfamily,member 11a, activator of NFKB /FL=gb:NM_003839.1 gb:AF018253.1
4.981307	2.359848	6.15	Down	4.17E-05	NM_005103	Homo sapiens fasciculation and elongation protein zeta 1 (zygin I) (FEZ1), transcript variant 1, mRNA. /PROD=zygin 1, isoform 1 /FL=gb:U60060.1 gb:U69139.1 gb:NM_005103.2
3.826815	1.207679	6.14	Down	6.48E-05	BG401568	Homo sapiens mRNA; cDNA DKFZp434H 1235 (from clone DKFZp434H1235); partial cds
1.027188	-1.59055	6.14	Down	8.40E-03	BG169832	adenylate kinase 5 /FL=gb:NM_012093.1 gb:AF062595.1
2.054962	-0.54704	6.07	Down	2.86E-03	NM_002800	Homo sapiens proteasome (prosome, macropain) subunit, beta type, 9 (large multifunctional protease 2) (PSMB9), mRNA. /PROD=proteasome (prosome, macropain) subunit, betatype, 9 (large multifunctional protease 2) /FL=gb:U01025.1 gb:NM_002800.1
5.372736	2.7744	6.06	Down	8.80E-05	AA669799	Cluster Incl. AA669799:ag36c04.s1 Homo sapiens cDNA, 3 end /clone=IMAGE-1118886 /clone_end=3 /gb=AA669799 /gi=2631298 /ug=Hs.6315 /len=679
0.24636	-2.3444	6.02	Down	1.31E-03	AW057589	ESTs
1.145878	-1.44369	6.02	Down	9.46E-03	AI056877	Human DNA sequence from clone RP4-530115 on chromosome 20. Contains the 3 end of the PTPN1 gene for protein tyrosine phosphatase, non-receptor type 1 (EC 3.1.3.48), the gene for a novel protein similar to placental protein DIFF40, an RPL36 (60S Ribos
0.976009	-1.61054	6.01	Down	5.39E-03	AW264204	ESTs
0.497515	-2.08762	6	Down	2.83E-02	AF052117	Homo sapiens clone 23809 mRNA sequence.
0.381933	-2.20139	5.99	Down	8.66E-04	AI913749	ESTs
0.528494	-2.05438	5.99	Down	4.17E-02	BG290908	ESTs, Moderately similar to ALU8_HUMAN ALU SUBFAMILY SX SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
3.795925	1.232161	5.91	Down	2.20E-04	NM_004688	Homo sapiens N-myc (and STAT) interactor (NMI), mRNA. /PROD=N-myc and STAT interactor /FL=gb:BC001268.1 gb:NM_004688.1 gb:U32849.1
1.934415	-0.62283	5.89	Down	4.93E-04	NM_001351	Homo sapiens deleted in azoospermia-like (DAZL), mRNA. /PROD=deleted in azoospermia-like /FL=gb:U66726.2 gb:NM_001351.1 gb:U65918.1 gb:U66078.1
1.805448	-0.75007	5.88	Down	1.88E-03	AI681917	ESTs, Highly similar to IRX3 MOUSE IROQUOIS-CLASS HOMEODOMAIN PROTEIN IRX-3 (M.musculus)
2.788534	0.237692	5.86	Down	7.40E-03	AW450929	heterogeneous nuclear ribonucleoprotein A1
2.99034	0.457208	5.79	Down	5.23E-04	NM_002993	Homo sapiens small inducible cytokine subfamily B (Cys-X-Cys), member 6 (granulocyte chemotactic protein 2)
				(SCYB6), mRNA. /PROD=small inducible cytokine subfamily B(Cys-X-Cys), member 6 (granulocyte chemotactic protein 2) /FL=gb:U81234.1 gb:NM_00299
0.362564	-2.17012	5.79	Down	1.28E-02	AB018580	Homo sapiens mRNA for hluPGFS, complete cds. /PROD=hluPGFS /FL=gb:NM_003739.2 gb:AF149416.2 gb:AB018580.1 gb:D17793.1
1.673874	-0.85315	5.76	Down	8.93E-03	NM_005965	Homo sapiens myosin, light polypeptide kinase (MYLK), mRNA. /PROD=myosin, light polypeptide kinase /FL=gb:AB037663.1 gb:AF069601.2 gb:NM_005965.1
1.858219	-0.66565	5.75	Down	2.13E-04	NM_005084	Homo sapiens phospholipase A2, group VII (platelet-activating factor acetylhydrolase, plasma) (PLA2G7), mRNA. /PROD=phospholipase A2, group VII (platelet-activatingfactor acetylhydrolase, plasma) /FL=gb:U20157.1 gb:U24577.1 gb:NM_005084.1
3.016209	0.501482	5.71	Down	6.48E-05	AW026379	ESTs
3.692792	1.179422	5.71	Down	1.52E-04	N21096	ESTs
1.28245	-1.23083	5.71	Down	3.20E-04	AF063824	Homo sapiens trp-related protein 4 truncated variant delta mRNA, complete cds. /PROD=trp-related protein 4 truncated variant delta /FL=gb:AF063824.1
3.772564	1.260638	5.7	Down	3.53E-04	AA404269	ESTs
2.016986	-0.49385	5.7	Down	6.37E-03	AI741439	ESTs
2.453774	-0.04433	5.65	Down	1.01E-03	NM_007191	Homo sapiens Wnt inhibitory factor-1 (WIF-1), mRNA. /PROD=Wnt inhibitory factor-1 /FL=gb:AF122922.1 gb:NM_007191.1
5.545158	3.061783	5.59	Down	1.71E-04	BF057809	ESTs
5.219258	2.740374	5.57	Down	1.08E-04	AA974416	protein phosphatase 2 (formerly 2A), regulatory subunit B (PR 52), beta isoform
2.913327	0.434686	5.57	Down	2.99E-04	NM_012419	Homo sapiens regulator of G-protein signalling 17 (RGS17), mRNA. /PROD=regulator of G-protein signalling 17 /FL=gb:AF202257.2 gb:NM_012419.2
1.651332	-0.81962	5.54	Down	1.35E-02	NM_007181	Homo sapiens mitogen-activated protein kinase kinase kinase kinase 1 (MAP4K1 mRNA. /PROD=mitogen-activated protein kinase kinase kinasekinase 1 /FL=gb:U66464.1 gb:NM_007181.1
1.293775	-1.16956	5.51	Down	1.15E-02	BF593660	ESTs
1.417933	-1.04305	5.51	Down	4.93E-04	NM_002738	Homo sapiens protein kinase C, beta 1 (PRKCB1), mRNA. /PROD=protein kinase C, beta 1 /FL=gb:NM_002738.1
3.66812	1.207732	5.5	Down	1.97E-04	NM_133329	Homo sapiens potassium voltage-gated channel, subfamily G, member 3 (KCNG3), transcript variant 1, mRNA. /PROD=potassium voltage-gated channel, subfamily G,member 3 isoform 1 /FL=gb:AF454548.1 gb:AF348982.1 gb:AB070604.1 gb:NM_133329.4
3.002731	0.549124	5.48	Down	4.89E-04	R54042	ESTs
5.276628	2.824048	5.47	Down	6.48E-05	BC005127	Homo sapiens, adipose differentiation-related protein, clone MGC:10598, mRNA, complete cds. /PROD=adipose differentiation-related protein /FL=gb:BC005127.1 gb:NM_001122.1
3.380946	0.937118	5.44	Down	1.22E-04	AU151342	Homo sapiens cDNA FLJ12935 fis, clone NT2RP2004982
2.01577	-0.42783	5.44	Down	1.92E-03	BE220341	casein kinase 2, alpha 1 polypeptide
1.307387	-1.12824	5.41	Down	1.08E-04	AK021452	Homo sapiens cDNA FLJ11390 fis, clone HEMBA1000561, weakly similar to ZINC FINGER PROTEIN 91.
0.36507	-2.02151	5.23	Down	4.98E-03	BF062244	ESTs
0.756663	-1.62346	5.21	Down	1.69E-03	BG533580	ESTs
3.876819	1.518834	5.13	Down	4.76E-04	AI651212	ESTs
0.619594	-1.73795	5.12	Down	1.18E-03	BE467611	ESTs
0.482843	-1.87385	5.12	Down	1.04E-03	BG284890	ESTs
1.048359	-1.30538	5.11	Down	8.93E-03	AA464273	ESTs
3.527039	1.198446	5.02	Down	2.69E-03	BG283790	ESTs
2.522705	0.194248	5.02	Down	3.09E-03	U07236	Human mutant lymphocyte-specific protein tyrosine kinase (LCK) mRNA, complete cds. /PROD=lymphocyte-specific protein tyrosine kinase /FL=gb:U07236.1 gb:NM_005356.1 gb:M36881.1
2.356401	0.028606	5.02	Down	6.23E-04	NM_024893	Homo sapiens hypothetical protein FLJ14220 (FLJ14220), mRNA. /PROD=hypothetical protein FLJ14220 /FL=gb:NM_024893.1
4.587367	2.264046	5	Down	2.70E-04	AL049589	Human DNA sequence from clone 570L12 on chromosome Xq13.1-21.1. Contains the PGK1 gene for phosphoglycerate kinase 1, the gene for a novel protein similar to TAF2G (TATA box binding protein (TBP)-associated factor, RNA polymerase II, G, 32kD) (TAF...



ES	EXPRES 02	Ratio	Direction	adj. p-value	Gene Identifier	Gene Name
-2.7136	7.077563	886	Up	9.62E-04	NM_001898	Homo sapiens cystatin SN(CST1), mRNA. /PROD=cystatin SN /FL=gb:J03870.1 gb:NM_001898.1
-2.3713	6.959692	644.03	Up	6.55E-05	R72286	microfibrillar-associated protein 4
-3.78394	5.172093	496.63	Up	1.06E-04	AW157548	insulin-like growth factor binding protein 5 /FL=gb:M65062.1 gb:M62782.1 gb:NM_000599.1 gb:AF055033.1
-4.79257	3.432794	299.28	Up	1.81E-03A	A352113	ESTs
-5.16453	3.053666	297.8	Up	5.30E-03	NM_002345	Homo sapiens lumican (LUM), mRNA. /PROD=lumican /FL=gb:NM_002345.1
				gb:U18728.1 gb:U21128.1
-2.55753	5.625595	290.65	Up	1.79E-04	D87811	Homo sapiens mRNA for GATA-6, complete cds. /PROD=GATA-6 /FL=gb:U66075.1 gb:NM_005257.1 gb:D87811.1
-5.03662	3.030028	268.1	Up	7.79E-05	BG099432	ESTs
-2.97296	4.901727	234.7	Up	5.95E-05	AI821586	ESTs, Moderately similar to JE0284 Mm-1 cell derived transplantability-associated protein 1 b (H.sapiens)
-3.06613	4.772945	228.98	Up	2.57E-03	AI422986	ESTs
-4.37538	3.399327	218.99	Up	7.01E-05	AA552969	ESTs
-3.47045	4.200612	203.81	Up	4.26E-03	NM_025140	Homo sapiens hypothetical protein FLJ22471 (FLJ22471), mRNA. /PROD=hypothetical protein FLJ22471 /FL=gb:NM_025140.1
-4.82833	2.813842	199.77	Up	1.40E-04	BF064262	ESTs
-5.1127	2.479359	192.95	Up	1.06E-04	NM_002653	Homo sapiens paired-like homeodomain transcription factor 1 (PITX1), mRNA. /PROD=paired-like homeodomain transcription factor 1 /FL=gb:NM_002653.1
-3.4841	4.092799	190.93	Up	4.34E-04	BM128432	Homo sapiens full length insert cDNA clone YA81B05
-4.64254	2.721466	164.74	Up	2.38E-05	AY177407	Homo sapiens homeobox protein goosecoid mRNA, complete cds. /PROD=homeobox protein goosecoid /FL=gb:AY177407.1 gb:NM_173849.1
-3.40132	3.923976	160.37	Up	1.34E-02	BF589787	ESTs
-1.20324	6.071574	154.86	Up	2.23E-04	NM_001643	Homo sapiens apolipoprotein A-II (APOA2), mRNA. /PROD=apolipoprotein A-II precursor /FL=gb:M29882.1 gb:NM_001643.1 gb:BC005282.1
-3.4292	3.808106	150.89	Up	4.62E-04	AB028021	Cluster Incl. AB028021 :Homo sapiens HNF-3beta mRNA for hepatocyte
				nuclear factor-3 beta, complete cds /cds=(196,1569) /gb=AB028021 /gi=4958949 /ug=Hs.155651 /len=1944
-4.71714	2.374201	136.37	Up	6.98E-05	AI796169	GATA-binding protein 3 /FL=gb:NM_002051.1 gb:M69106.1 gb:BC003070.1
-2.26798	4.781861	132.5	Up	9.04E-05	NM_001322	Homo sapiens cystatin SA (CST2), mRNA. /PROD=cystatin SA /FL=gb:NM_001322.1
-0.81321	6.174771	126.94	Up	1.57E-03	NM_002160	Homo sapiens hexabrachion (tenascin C, cytotactin) (HXB), mRNA. /PROD=hexabrachion (tenascin C, cytotactin) /FL=gb:M55618.1 gb:NM_002160.1
-2.38522	4.594021	126.17	Up	6.89E-05	AA502609	Homo sapiens ankyrin-like with transmembrane domains 1 (ANKTM1), mRNA
-3.75387	3.204091	124.32	Up	2.13E-04	AI991459	ESTs
-4.21525	2.671776	118.36	Up	1.99E-04	NM_006119	Homo sapiens fibroblast growth factor 8 (androgen-induced) (FGF8), mRNA. /PROD=fibroblast growth factor 8 (androgen-induced) /FL=gb:U36223.1 gb:U46212.1 gb:NM_006119.1
-2.02474	4.768631	110.92	Up	7.31E-03	NM_021827	Homo sapiens hypothetical protein FLJ23514 (FLJ23514), mRNA. /PROD=hypothetical protein FLJ23514 /FL=gb:NM_021827.1
-2.38432	4.381798	108.84	Up	1.01 E-03	AL534095	hypothetical protein FLJ23091
-2.25187	4.311095	94.55	Up	7.26E-03	AL136944	Homo sapiens mRNA; cDNA DKFZp586J0624 (from clone DKFZp586J0624); complete cds. /PROD=hypothetical protein /FL=gb:AF215636.1
				gb:NM_014585.1 gb:AF231121.1 gb:AF226614.1 gb:AL136944.1
-1.92189	4.619888	93.17	Up	9.02E-04	AV700724	GATA-binding protein 4 /FL=gb:NM_002052.1 gb:L34357.1 gb:D78260.1
-3.42725	2.997778	85.93	Up	2.95E-03	NM_022469	Homo sapiens hypothetical protein FLJ21195 similar to protein related to DAC and cerberus (FLJ21195), mRNA. /PROD=hypothetical protein FLJ21195 similar to proteinrelated to DAC and cerberus /FL=gb:NM_022469.1
-3.14404	3.270152	85.28	Up	6.55E-05	AB028021	Homo sapiens HNF-3beta mRNA for hepatocyte nuclear factor-3 beta, complete cds. /PROD=hepatocyte nuclear factor-3 beta /FL=gb:AB028021.1 gb:NM_021784.1
-0.88122	5.526622	84.91	Up	1.25E-04	AA775681	hypothetical protein FLJ23091
-2.96204	3.439168	84.52	Up	1.08E-03	NM_001311	Homo sapiens cysteine-rich protein 1 (intestinal) (CRIP1), mRNA. /PROD=cysteine-rich protein 1 (intestinal) /FL=gb:U58630.1 gb:BC002738.1 gb:NM_001311.1 gb:U09770.1
-3.42819	2.876705	79.06	Up	2.31E-04	AL121722	Human DNA sequence from clone RP4-788L20 on chromosome 20 Contains the HNF3B (hepatocyte nuclear factor 3, beta) gene. a novel gene based on ESTs, ESTs, STSs, GSSs and CpG Islands
-1.01231	5.27686	78.2	Up	1.85E-04	NM_001643	Homo sapiens apolipoprotein A-II (APOA2), mRNA. /PROD=apolipoprotein A-II precursor /FL=gb:M29882.1
	gb:NM_001643.1 gb:BC005282.1
-2.13331	4.095704	75.01	Up	2.99E-04	NM_003867	Homo sapiens fibroblast growth factor 17 (FGF17), mRNA. /PROD=fibroblast growth factor 17 /FL=gb:NM_003867.1 gb:AB009249.1
-0.14916	6.052967	73.63	Up	2.30E-04	NM_002521	Homo sapiens natriuretic peptide precursor B (NPPB), mRNA. /PROD=natriuretic peptide precursor B /FL=gb:NM_002521.1 gb:M25296.1
-2.9139	3.274181	72.91	Up	9.48E-04	NM_005143	Homo sapiens haptoglobin (HP), mRNA. /PROD=haptoglobin /FL=gb:K00422.1 gb:L29394.1 gb:NM_005143.1
-2.33028	3.85605	72.82	Up	2.04E-04	X02162	Human mRNA for apolipoprotein Al (apo Al=. /PROD=preproapolipo protein Al
-4.75249	1.427636	72.51	Up	8.97E-04	AJ276395	Homo sapiens mRNA for MSF-FN70 (FN gene). /PROD=migration stimulation factor FN70
-1.50663	4.672617	72.47	Up	9.82E-05	BF223214	ESTs
-4.40099	1.778003	72.45	Up	8.87E-05	AI733179	ESTs
-2.56553	3.594638	71.51	Up	4.24E-04	D31771	Homo sapiens mRNA for MSX-2, complete cds. /PROD=MSX-2 /FL=gb:NM_002449.2 gb:D31771.1
-3.67415	2.447201	69.62	Up	1.97E-02	BC042378	Homo sapiens, clone IMAGE:5277693, mRNA.
-1.33141	4.770833	68.7	Up	2.36E-04	AI640307	protocadherin 10
-2.41293	3.673615	67.96	Up	8.00E-04	NM_000846	Homo sapiens glutathione S-transferase A2 (GSTA2), mRNA. /PROD=glutathione S-transferase A2 /FL=gb:BC002895.1 gb:M25627.1 gb:M16594.1 gb:M14777.1 gb:M15872.1 gb:M21758.1
gb:NM_000846.1
-2.95346	3.079949	65.5	Up	7.93E-05	NM_000420	Homo sapiens Kell blood group (KEL), mRNA. /PROD=Kell blood group antigen /FL=gb:BC003135.1 gb:NM_000420.1
-3.41755	2.612638	65.35	Up	1.03E-02	AI808090	ESTs
-4.08201	1.927438	64.42	Up	5.56E-04	AK000680	Homo sapiens cDNA FLJ20673 fis, clone KAIA4464. /FL=gb:AF240634.1 gb:NM_018440.1
-0.1416	5.830942	62.79	Up	6.89E-05	NM_022454	Homo sapiens hypothetical protein FLJ22252 similar to SRY-box containing gene 17 (FLJ22252), mRNA. /PROD=hypothetical protein FLJ22252 similar to SRY-boxcontaining gene 17 /FL=gb:NM_022454.1
-1.79329	4.15609	61.79	Up	7.58E-04	AL575177	noggin /FL=gb:NM_005450.1
-0.88683	5.039046	60.79	Up	8.36E-05	AI821669	ESTs
-3.76697	2.141612	60.07	Up	2.25E-04	NM_001147	Homo sapiens angiopoietin 2 (ANGPT2), mRNA. /PROD=angiopoietin 2 /FL=gb:AB009865.1 gb:AF004327.1 gb:NM_001147.1
0.720535	6.617979	59.61	Up	5.95E-05	AW007532	Human insulin-like growth factor binding protein 5 (IGFBP5) mRNA
-1.03589	4.784337	56.5	Up	2.23E-04	AI242583	Homo sapiens cDNA FLJ11550 fis, clone HEMBA1002970
-2.28856	3.531402	56.49	Up	4.54E-04	AF211891	Homo sapiens Mix-like homeobox protein 1 (MILD1) mRNA, complete cds. /PROD=Mix-like homeobox protein 1 /FL=gb:AF211891.1
-2.04403	3.759502	55.85	Up	2.17E-03	NM_000039	Homo sapiens apolipoprotein A-I (APOA1), mRNA. /PROD=apolipoprotein A-I precursor /FL=gb:M27875.1 gb:M11791.1 gb:NM_000039.1 gb:BC005380.1
0.129315	5.920102	55.36	Up	6.89E-05	NM_005442	Homo sapiens eomesodermin
				(Xenopus laevis) homolog (EOMES), mRNA. /PROD=eomesodermi n (Xenopus laevis) homolog /FL=gb:AB031038.1 gb:NM_005442.1
-1.57973	4.207564	55.23	Up	5.25E-03	AL513917	solute carrier family 16 (monocarboxylic acid transporters), member 3 /FL=gb:U81800.1 gb:NM_004207.1
-4.11172	1.670966	55.05	Up	4.57E-04	BG256677	interferon, gamma-inducible protein 16 /FL=gb:AF208043.1
-0.28789	5.482347	54.58	Up	6.89E-05	AW772192	Homo sapiens clone 23736 mRNA sequence
-1.44577	4.307421	53.94	Up	3.59E-03	AL544576	ESTs
-3.9513	1.76416	52.54	Up	7.33E-05	NM_016341	Homo sapiens pancreas-enriched phospholipase C (LOC51196), mRNA. /PROD=pancreas-enriched phospholipase C /FL=gb:AF117948.1 gb:NM_016341.1 gb:AF190642.2
0.05538	5.762108	52.23	Up	7.33E-05	AI817041	G protein-coupled receptor
-3.52376	2.14189	50.76	Up	8.23E-05	AW300217	ESTs, Moderately similar to C212_HUMAN 28.3 KD PROTEIN C21ORF2 (H.sapiens)
-3.18877	2.469472	50.5	Up	7.47E-03	AF260333	Homo sapiens AD036 mRNA, complete cds. /PROD=AD036 /FL=gb:AF260333.1
-1.973	3.674867	50.14	Up	1.91E-04	AA772920	ESTs
-2.30094	3.341814	49.96	Up	7.23E-03	AI806174	transcription factor 8 (represses interleukin 2 expression)
-2.25531	3.356433	48.9	Up	6.63E-03	AI380207	ESTs
-2.71676	2.892681	48.82	Up	5.25E-04	AU 144167	Homo sapiens cDNA FLJ11428 fis, clone HEMBA1001071, highly similar to PROCOLLAGEN ALPHA 1(III) CHAIN PRECURSOR
-0.16429	5.442379	48.73	Up	6.83E-04	L01639	Human (clone HSY3RR) neuropeptide Y receptor (NPYR) mRNA, complete cds. /PROD=neuropeptide
	Y receptor /FL=gb:L06797.1 gb:NM_003467.1 gb:AF025375.1 gb:AF147204.1 gb:M99293.1 gb:L01639.1
-4.03477	1.563749	48.45	Up	1.19E-02	U12170	Human zinc finger homeodomain protein mRNA, complete cds. /PROD=zinc finger homeodomain protein /FL=gb:U12170.1
-0.08298	5.493663	47.72	Up	2.19E-04	NM_004207	Homo sapiens solute carrier family 16 (monocarboxylic acid transporters), member 3 (SLC16A3), mRNA. /PROD=solute carrier family 16 (monocarboxylic acidtransporters), member 3 /FL=gb:U81800.1 gb:NM_004207.1
-2.99405	2.552238	46.73	Up	4.78E-04	AI767388	Human DNA sequence from clone RP5-1024N4 on chromosome 1p32.1-33. Contains the gene for a novel Sodium:solute symporter family member similar to SLC5A1 (SGLT1), a pseudogene similar to part of butyrophilin family members, a novel gene, ESTs, STSs, GS
-4.61432	0.925434	46.52	Up	2.53E-04	NM_005221	Homo sapiens distal-less homeo box 5 (DLX5), mRNA. /PROD=distal-less homeo box 5 /FL=gb:NM_005221.3
-3.22309	2.302183	46.05	Up	4.60E-03	AW207243	ESTs
-2.82645	2.655384	44.69	Up	4.60E-03	NM_013445	Homo sapiens glutamate decarboxylase 1 (brain, 67kD) (GAD1), transcript variant GAD25, mRNA. /PROD=glutamate decarboxylase 1, isoform GAD25 /FL=gb:NM_013445.1 gb:AF178853.1
	gb:BC002815.1
0.533443	5.958927	42.98	Up	6.55E-05	NM_001899	Homo sapiens cystatin S (CST4), mRNA. /PROD=cystatin S /FL=gb:NM_001899.1
0.116207	5.518477	42.29	Up	1.27E-04	NM_000599	Homo sapiens insulin-like growth factor binding protein 5 (IGFBP5), mRNA. /PROD=insulin-like growth factor binding protein 5 /FL=gb:M65062.1 gb:M62782.1 gb:NM_000599.1 gb:AF055033.1
-2.1675	3.230235	42.16	Up	1.53E-04	NM_021804	Homo sapiens angiotensin I converting enzyme (peptidyl-dipeptidase A) 2 (ACE2), mRNA. /PROD=angiotensin I converting enzyme(peptidyl-dipeptidase A) 2 /FL=gb:NM_021804.1 gb:AF241254.1 gb:AB046569.1 gb:AF291820.1
-0.61985	4.752547	41.42	Up	3.54E-04	NM_001963	Homo sapiens epidermal growth factor (beta-urogastrone) (EGF), mRNA. /PROD=epidermal growth factor (beta-urogastrone) /FL=gb:NM_001963.2
-1.73746	3.627971	41.22	Up	3.35E-04	NM_014391	Homo sapiens cardiac ankyrin repeat protein (CARP), mRNA. /PROD=cardiac ankyrin repeat protein /FL=gb:NM_014391.1
-3.68848	1.657514	40.67	Up	2.86E-03	NM_018557	Homo sapiens low density lipoprotein-related protein 1 B (deleted in tumors) (LRP1B), mRNA. /PROD=low density lipoprotein-related protein 1B(deleted in tumors) /FL=gb:AF176832.1 gb:NM_018557.1
-3.11273	2.220281	40.31	Up	5.02E-03	AW444761	ESTs
-2.78886	2.517881	39.58	Up	7.89E-03	NM_001115	Homo sapiens adenylate cyclase 8
				(brain) (ADCY8), mRNA. /PROD=adenylate cyclase 8 /FL=gb:NM_001115.1
-1.93668	3.348112	38.98	Up	7.23E-03	BE670361	G protein-coupled receptor 72 /FL=gb:NM_016540.1 gb:AF236081.1
-3.65051	1.595241	37.94	Up	3.80E-04	AF213459	Homo sapiens ephrin receptor EPHA3 complete form (EPHA3) mRNA, complete cds. /PROD=ephrin receptor EPHA3 complete form /FL=gb:NM_005233.1 gb:M83941.1 gb:AF213459.1
0.767075	5.998268	37.56	Up	2.55E-04	AY029208	Homo sapiens type VI collagen alpha 2 chain precursor (COL6A2) mRNA, complete cds, alternatively spliced. /PROD=type VI collagen alpha 2 chain precursor /FL=gb:AY029208.1
-2.34732	2.874499	37.32	Up	6.51E-03	AI240545	glycophorin B (includes Ss blood group)
-2.41622	2.773394	36.49	Up	6.29E-04	NM_001977	Homo sapiens glutamyl aminopeptidase (aminopeptidase A) (ENPEP), mRNA. /PROD=glutamyl aminopeptidase (aminopeptidase A) /FL=gb:L12468.1 gb:NM_001977.1 gb:L14721.1
-1.58875	3.588854	36.19	Up	2.45E-03	NM_152506	Homo sapiens hypothetical protein FLJ32835 (FLJ32835), mRNA. /FL=gb:NM_152506.1
-0.93849	4.238505	36.18	Up	1.38E-02	BE222344	splicing factor, arginineserine-rich 5
1.479222	6.611842	35.08	Up	5.95E-05	NM_005454	Homo sapiens cerberus 1 (Xenopus laevis) homolog (cysteine knot superfamily) (CER1), mRNA. /PROD=cerberus 1 /FL=gb:NM_005454.1
-0.46494	4.666106	35.04	Up	2.90E-04	AI141603	collagen, type VI,
	alpha 1
-2.23021	2.897749	34.97	Up	4.92E-04	NM_001785	Homo sapiens cytidine deaminase (CDA), mRNA. /PROD=cytidine deaminase /FL=gb:L27943.1 gb:NM_001785.1
-3.12836	1.991299	34.77	Up	8.63E-04	NM_002770	Homo sapiens protease, serine, 2 (trypsin 2) (PRSS2), mRNA. /PROD=protease, serine, 2 (trypsin 2) /FL=gb:M27602.1 gb:NM_002770.1
-0.98659	4.115782	34.35	Up	1.19E-04	M65062	Human insulin-like growth factor binding protein 5 (IGFBP-5) mRNA, complete cds. /PROD=insulin-like growth factor binding protein 5 /FL=gb:M65062.1 gb:M62782.1 gb:NM_000599.1 gb:AF055033.1
-2.50194	2.569744	33.63	Up	4.84E-03	AJ277914	Homo sapiens partial LHX9 gene for LIM-homeobox 9, 3UTR.
-1.27526	3.792158	33.53	Up	1.12E-03	AI688418	plexin A2
-3.34034	1.708137	33.09	Up	2.46E-03	AA781795	ESTs
1.339655	6.36612	32.59	Up	7.93E-05	AJ224869	Homo sapiens CXCR4 gene encoding receptor CXCR4
-0.6944	4.326307	32.46	Up	7.33E-05	R73554	Human insulin-like growth factor binding protein 5 (IGFBP5) mRNA
-0.67187	4.337831	32.22	Up	7.54E-05	AI692659	heat shock 90kD protein 1, alpha
-0.46298	4.533319	31.92	Up	3.96E-04	S69738	MCP-1=monocyte chemotactic protein (human, aortic endothelial cells, mRNA, 661 nt). /PROD=MCP-1
-2.56712	2.414446	31.59	Up	1.67E-03	AI813758	collagen, type III, alpha 1 (Ehlers-Danlos syndrome type IV, autosomal dominant) /FL=gb:NM_000090.1
-0.31684	4.651259	31.3	Up	7.83E-04	BF130943	ESTs
-2.78124	2.184054	31.24	Up	8.36E-05	NM_020995	Homo sapiens haptoglobin-related protein (HPR), mRNA. /PROD=haptoglobin-related protein
/FL=gb:NM_020995.1
-1.24179	3.719223	31.15	Up	4.92E-04	AL534095	hypothetical protein FLJ23091
-0.35003	4.606618	31.05	Up	6.88E-03	NM_001778	Homo sapiens CD48 antigen (B-cell membrane protein) (CD48), mRNA. /PROD=CD48 antigen (B-cell membrane protein) /FL=gb:NM_001778.1 gb:M37766.1 gb:M59904.1
-1.81534	3.141104	31.05	Up	5.86E-04	AW590925	ESTs
-1.93655	3.000448	30.63	Up	5.42E-03	NM_0133 69	Homo sapiens DNA (cytosine-5-)-methyltransferase 3-like (DNMT3L), mRNA. /PROD=DNA (cytosine-5-)-methyltransferase 3-like /FL=gb:BC002560.1 gb:NM_013369.1 gb:AF194032.1
1.122063	6.03378	30.1	Up	7.33E-05	X58851	Human MLC1emb gene for embryonic myosin alkaline light chain, promoter and exon 1
-0.4721	4.436335	30.03	Up	7.93E-05	D89377	Homo sapiens mRNA for MSX-2, complete cds. /PROD=MSX-2 /FL=gb:D89377.1
0.044298	4.952379	30.02	Up	6.89E-05	W57613	ESTs
-0.59928	4.305866	29.96	Up	1.03E-03	AF020769	Homo sapiens cardiac ventricular troponin C mRNA, complete cds. /PROD=cardiac ventricular troponin C /FL=gb:NM_003280.1 gb:AF020769.1
-1.04571	3.857701	29.93	Up	4.57E-03	NM_001362	Homo sapiens deiodinase, iodothyronine, type III (DIO3), mRNA. /PROD=thyroxine deiodinase type III /FL=gb:NM_001362.1 gb:S79854.1
-3.24802	1.648226	29.78	Up	1.47E-03	AI694325	ESTs
-2.50665	2.356234	29.1	Up	8.64E-03	BE222668	ESTs
-2.27119	2.568908	28.64	Up	2.53E-03	NM_002608	Homo sapiens platelet-derived growth factor beta polypeptide (simian sarcoma viral (v-sis) oncogene homolog) (PDGFB),
				mRNA. /PROD=platelet-derived growth factor beta polypeptide(simian sarcoma viral (v-sis) oncogene homolog) /FL=gb:M12783.1 gb:NM_002
-4.34018	0.485509	28.36	Up	7.34E-05	AU144247	Homo sapiens cDNA FLJ13443 fis, clone PLACE1002853
-1.02297	3.794799	28.2	Up	3.36E-03	AF208043	Homo sapiens IFI16b (IFI16b) mRNA, complete cds. /PROD=IFI16b /FL=gb:AF208043.1
-2.79469	2.013598	28.02	Up	9.94E-05	AI700341	ESTs
-2.73255	2.070789	27.92	Up	1.35E-03	X89271	H.sapiens mRNA for HG11 orphan receptor. /PROD=HG11 orphan receptor /FL=gb:NM_005161.1
-3.05797	1.724772	27.53	Up	3.48E-04	AI801626	ESTs, Moderately similar to ALU4_HUMAN ALU SUBFAMILY SB2 SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
-2.83953	1.922194	27.13	Up	5.16E-04	BG290193	hypothetical protein FLJ14299 /FL=gb:NM_025069.1
-4.60716	0.149736	27.04	Up	1.22E-02	NM_0046 96	Homo sapiens solute carrier family 16 (monocarboxylic acid transporters), member 4 (SLC16A4), mRNA. /PROD=solute carrier family 16 (monocarboxylic acidtransporters), member 4 /FL=gb:U59185.1 gb:NM_004696.1
-1.57919	3.174205	26.97	Up	5.94E-04	AL524520	G protein-coupled receptor 49
-1.36626	3.37132	26.68	Up	2.16E-03	AI824037	ESTs, Weakly similar to FCE2 MOUSE LOW AFFINITY IMMUNOGLOBULIN EPSILON FC RECEPTOR (M.musculus)
0.167058	4.895371	26.51	Up	6.90E-05	NM_021223	Homo sapiens myosin light chain 2a (LOC58498), mRNA. /PROD=myosin light
				chain 2a /FL=gb:NM_021223.1
-1.4009	3.316905	26.31	Up	6.35E-04	BC029835	Homo sapiens, clone IMAGE:5169759, mRNA.
-2.16518	2.549789	26.26	Up	1.77E-03	AI521166	ESTs, Moderately similar to MTR5_HUMAN MYOTUBULARIN-RELATED PROTEIN 5 (H.sapiens)
-3.32235	1.375121	25.95	Up	2.00E-04	BC039433	Homo sapiens, clone IMAGE:5303550, mRNA.
-5.7338	-1.05152	25.67	Up	8.80E-03	NM_020130	Homo sapiens chromosome 8 open reading frame 4 (C8ORF4), mRNA. /PROD=chromosome 8 open reading frame 4 /FL=gb:NM_020130.1 gb:AF268037.1
1.214325	5.878585	25.36	Up	7.93E-05	M36172	Human embryonic myosin alkali light chain (MLC1) mRNA, complete cds. /FL=gb:M36172.1 gb:M24121.1 gb:NM_002476.1
-2.20104	2.461597	25.33	Up	4.67E-03	NM_000939	Homo sapiens proopiomelanocortin (adrenocorticotropin beta-lipotropin alpha-melanocyte stimulating hormone beta-melanocyte stimulating hormone beta-endorphin) (POMC), mRNA. /PROD=proopiomelan ocortin (adrenocorticotropinbe ta-lipotropin alpha-melanocyt
-0.2674	4.336009	24.31	Up	9.18E-05	N48299	ESTs, Moderately similar to NFY-C (H.sapiens)
1.367677	5.968973	24.27	Up	1.00E-04	AF116676	Homo sapiens PRO1957 mRNA, complete cds. /PROD=PRO1957 /FL=gb:AF116676.1
-0.62697	3.974228	24.27	Up	4.69E-04	NM_005531	Homo sapiens interferon, gamma-inducible protein 16 (IFI16), mRNA. /PROD=interferon, gamma-inducible
	protein 16 /FL=gb:M63838.1 gb:NM_005531.1
-3.90861	0.686447	24.17	Up	3.72E-03	BC022531	Homo sapiens, olfactomedin 3, clone MGC:26675 IMAGE:4812035, mRNA, complete cds. /PROD=olfactomedin 3 /FL=gb:AF397394.1 gb:BC022531.1
-2.75089	1.840723	24.11	Up	2.60E-04	AL365343	Homo sapiens mRNA full length insert cDNA clone EUROIMAGE 32539.
-0.6097	3.975428	24	Up	1.05E-04	L12468	Homo sapiens aminopeptidase A mRNA, complete cds. /PROD=aminopeptidas e A/FL=gb:L12468.1 gb:NM_001977.1 gb:L14721.1
-3.18285	1.397334	23.92	Up	3.32E-04	BC041441	Homo sapiens, clone IMAGE:5167131, mRNA.
-1.92796	2.645248	23.81	Up	1.20E-02	BE551416	ESTS, Weakly similar to KIAA1330 protein (H.sapiens)
-4.05111	0.51291	23.65	Up	1.05E-03	J03580	Human, parathyroid-like protein (associated with humoral hypercalcemia of malignancy) mRNA, complete cds. /FL=gb:J03580.1
-2.79378	1.767388	23.61	Up	3.68E-02	AW291402	ESTs
-2.80173	1.752943	23.5	Up	7.26E-03	AW088232	ESTs
0.422022	4.975085	23.48	Up	1.38E-04	D49958	Homo sapiens mRNA for membrane glycoprotein M6, complete cds. /PROD=membrane glycoprotein M6 /FL=gb:D49958.1
-1.20314	3.343061	23.36	Up	3.63E-04	M60721	Human homeobox gene, complete cds. /FL=gb:M60721.1 gb:NM_021958.1
1.932439	6.477785	23.35	Up	7.33E-05	H92988	tyrosine 3-monooxygenasetrypto phan 5-monooxygenase activation protein, eta polypeptide
-3.00328	1.524799	23.07	Up	8.50E-03	AI571798	Rho GDP dissociation inhibitor (GDI) alpha
0.526605	5.052252	23.03	Up	7.01E-05	N71923	fibronectin leucine rich
	transmembrane protein 3 /FL=gb:AF169677.1 gb:NM_013281.1
-1.26047	3.239318	22.62	Up	5.12E-03	NM_007250	Homo sapiens Kruppel-like factor 8 (KLF8), mRNA. /PROD=Kruppel-like factor 8 /FL=gb:U28282.1 gb:NM_007250.1
-1.93118	2.556654	22.44	Up	2.34E-04	L33477	Human (clone 8B1) Br-cadherin mRNA, complete cds. /PROD=Br-cadherin /FL=gb:L34057.1 gb:L33477.1 gb:NM_004061.1
0.005876	4.456564	21.87	Up	6.89E-05	AK023621	Homo sapiens cDNA FLJ13559 fis, clone PLACE1007852, highly similar to Homo sapiens mRNA for KIAA0878 protein.
-1.94	2.509492	21.85	Up	4.29E-03	NM_016569	Homo sapiens TBX3-iso protein (TBX3-iso), mRNA. /PROD=TBX3-iso protein /FL=gb:NM_016569.1 gb:AF216750.1
-3.44347	1.001698	21.78	Up	1.61E-02	AF187858	Homo sapiens angiopoietin-2 isoform-1 mRNA, complete cds, alternatively spliced. /PROD=angiopoietin-2 isoform-1 /FL=gb:AF187858.1
0.586923	5.027737	21.72	Up	6.55E-05	NM_000047	Homo sapiens arylsulfatase E (chondrodysplasia punctata 1) (ARSE), mRNA. /PROD=arylsulfatase E precursor /FL=gb:X83573.1 gb:NM_000047.1
1.422626	5.860875	21.68	Up	5.95E-05	NM_006365	Homo sapiens transcriptional activator of the c-fos promoter (CROC4), mRNA. /PROD=transcriptional activator of the c-fos promoter /FL=gb:NM_006365.1 gb:U49857.1
-4.18575	0.241573	21.52	Up	7.54E-03	NM_001736	Homo sapiens complement
				component 5 receptor 1 (C5a ligand) (C5R1), mRNA. /PROD=complement component 5 receptor 1 (C5a ligand) /FL=gb:M62505.1 gb:NM_001736.1
2.301255	6.712959	21.28	Up	7.68E-05	BC020935	Homo sapiens, Similar to otoconin 90, clone IMAGE:4277593, mRNA.
-3.61192	0.788317	21.12	Up	1.71E-03	R37101	ESTs
-0.62474	3.768383	21.01	Up	6.55E-05	NM_000313	Homo sapiens protein S (alpha) (PROS1), mRNA. /PROD=protein S (alpha) /FL=gb:M15036.1 gb:NM_000313.1
-0.62725	3.760374	20.93	Up	1.52E-04	BC017942	Homo sapiens, Similar to otoconin 90, clone IMAGE:4285317, mRNA.
-1.52261	2.858274	20.83	Up	2.98E-03	NM_002614	Homo sapiens PDZ domain containing 1 (PDZK1), RNA. /PROD=PDZ domain containing 1 /FL=gb:NM_002614.1 gb:AF012281.1
-1.11347	3.25087	20.6	Up	4.26E-03	N69091	ESTs
-0.11332	4.231933	20.33	Up	1.05E-04	NM_003670	Homo sapiens basic helix-loop-helix domain containing, class B, 2 (BHLHB2), mRNA. /PROD=differentiated embryo chondrocyte expressed gene1 /FL=gb:AB004066.1 gb:NM_003670.1
-1.69238	2.643704	20.2	Up	3.73E-03	W05495	ESTs
-2.18113	2.138504	19.97	Up	1.23E-02	NM_004041	Homo sapiens arrestin, beta 1 (ARRB1), transcript variant 1, mRNA. /PROD=arrestin beta 1, isoform A /FL=gb:BC003636.1 gb:AF084040.1 gb:NM_004041.2
1.306329	5.625069	19.96	Up	6.90E-05	NM_001200	Homo sapiens bone morphogenetic protein 2 (BMP2), mRNA. /PROD=bone morphogenetic protein 2 precursor /FL=gb:NM_001200.1
-1.23777	3.066156	19.75	Up	6.27E-04	AI917371	ESTs
-0.00098	4.266076	19.25	Up	9.82E-05	NM_013281	Homo sapiens fibronectin leucine rich transmembrane protein 3 (FLRT3), mRNA. /PROD=fibronectin leucine rich transmembrane protein3 /FL=gb:AF169677.1 gb:NM_013281.1
-2.0132	2.250432	19.21	Up	1.37E-02	BE328496	hypothetical protein PRO2032 /FL=gb:AF116683.1 gb:NM_018615.1
1.758844	6.008618	19.02	Up	6.55E-05	N21138	KIAA0878 protein /FL=gb:NM_014899.1 gb:AB020685.1
0.095309	4.341668	18.98	Up	8.55E-04	AA524250	deleted in liver cancer 1
-0.96212	3.265791	18.74	Up	2.04E-04	AY113699	Homo sapiens presenilin stabilization factor b (PSF) mRNA, complete cds; alternatively spliced. /PROD=presenilin stabilization factor b /FL=gb:AY113699.1
0.502339	4.722511	18.64	Up	1.04E-04	AI676059	ESTs
-1.74369	2.474001	18.61	Up	7.33E-05	NM_001882	Homo sapiens corticotropin releasing hormone-binding protein (CRHBP), mRNA. /PROD=corticotropin releasing hormone-binding protein /FL=gb:NM_001882.2
0.70975	4.924051	18.56	Up	1.64E-04	BF939489	glycoprotein M6A /FL=gb:D49958.1
-2.40752	1.7892	18.34	Up	4.46E-03	AI738662	homeo box HB9 /FL=gb:NM_005515.1
-1.34609	2.844235	18.26	Up	7.33E-05	NM_018388	Homo sapiens hypothetical protein FLJ11316 (FLJ11316), mRNA. /PROD=hypothetical protein FLJ11316 /FL=gb:NM_018388.1
-0.74044	3.448679	18.24	Up	7.33E-05	N63706	ESTs
-1.55229	2.611591	17.92	Up	4.34E-04	AU158444	Homo sapiens cDNA FLJ14216 fis, clone NT2RP3003672, weakly similar to T-CELL SURFACE GLYCOPROTEIN E2 PRECURSOR
0.082922	4.230149	17.72	Up	1.63E-04	AI632223	hypothetical protein DKFZp434F2322
-1.66293	2.482886	17.7	Up	1.56E-02	NM_000817	Homo sapiens glutamate decarboxylase 1 (brain, 67kD) (GAD1), transcript variant GAD67, mRNA. /PROD=glutamate decarboxylase 1, isoform GAD67 /FL=gb:NM_000817.1 gb:M81883.1 gb:L16888.1
-1.82505	2.319685	17.69	Up	7.89E-03	T16257	G protein-coupled receptor 37 (endothelin receptor type B-like) /FL=gb:NM_005302.1 gb:AF017262.1
-3.11387	1.027176	17.64	Up	9.68E-03	U70370	Human hindlimb expressed homeobox protein backfoot (Bft) mRNA, complete cds. /PROD=hindlimb expressed homeobox protein backfoot /FL=gb:U70370.1 gb:BC003685.1
-0.98938	3.143558	17.54	Up	6.04E-03	AF190725	Homo sapiens beta-site APP cleaving enzyme (BACE) mRNA, complete cds. /PROD=beta-site APP cleaving enzyme /FL=gb:AF200343.1 gb:AF204943.1 gb:AF190725.1 gb:AF201468.1 gb:NM_012104.1
-0.74839	3.363245	17.29	Up	5.33E-03	M17955	Human MHC class II HLA-DQ-beta mRNA, complete cds. /FL=gb:M33907.1 gb:M17955.1 gb:M16996.1 gb:M17563.1 gb:M20432.1 gb:M26042.1
2.851479	6.958929	17.24	Up	5.95E-05	AI950472	ESTs
-2.85963	1.242896	17.18	Up	7.55E-03	BC005961	Homo sapiens, parathyroid hormone-like hormone, clone MGC:14611, mRNA, complete cds. /PROD=parathyroid hormone-like hormone /FL=gb:BC005961.1
-1.18027	2.905057	16.97	Up	1.03E-02	AI123555	ESTs
-1.53522	2.547506	16.94	Up	2.58E-03	NM_006456	Homo sapiens sialyltransferase
				(STHM), mRNA. /PROD=sialyltransfera se/FL=gb:U14550.1 gb:NM_006456.1
1.620279	5.700292	16.91	Up	1.08E-04	AI583173	major histocompatibility complex, class II, DQ beta 1
1.446234	5.516116	16.79	Up	6.55E-05	AF348491	Homo sapiens chemokine receptor CXCR4 mRNA, complete cds. /PROD=chemokine receptor CXCR4 /FL=gb:AF348491.1
0.880085	4.948285	16.77	Up	6.90E-05	NM_006096	Homo sapiens N-myc downstream regulated (NDRG1), mRNA. /PROD=N-myc downstream regulated /FL=gb:AF004162.1 gb:BC003175.1 gb:D87953.1 gb:NM_006096.1
-1.11823	2.945099	16.72	Up	1.28E-02	NM_002100	Homo sapiens glycophorin B (includes Ss blood group) (GYPB), mRNA. /PROD=glycophorin B precursor /FL=gb:J02982.1 gb:NM_002100.2
-1.68075	2.377232	16.66	Up	4.35E-03	NM_012431	Homo sapiens sema domain, immunoglobulin domain (Ig), short basic domain, secreted, (semaphorin) 3E (SEMA3E), mRNA. /PROD=sema domain, immunoglobulin domain (Ig), shortbasic domain, secreted, (semaphorin) 3E /FL=gb:NM_012431.1 gb:AB002329.1
0.70158	4.759011	16.65	Up	1.07E-04	U46768	Human stanniocalcin mRNA, complete cds. /PROD=stanniocalcin /FL=gb:U25997.1 gb:NM_003155.1 gb:U46768.1
2.429693	6.487025	16.65	Up	6.89E-05	AA284532	tyrosine 3-monooxygenasetrypto phan 5-monooxygenase activation protein, eta
	polypeptide
1.964573	6.018949	16.61	Up	1.18E-04	NM_030781	Homo sapiens scavenger receptor with C-type lectin (SRCL), mRNA. /PROD=scavenger receptor with C-type lectin /FL=gb:NM_030781.1
0.399566	4.451136	16.58	Up	1.57E-04	AF144103	Homo sapiens NJAC protein (NJAC) mRNA, complete cds. /PROD=NJAC protein /FL=gb:AF144103.1 gb:AF106911.1 gb:AF073957.1 gb:BC003513.1 gb:NM_004887.1
4.590104	-3.21322	223.38	Down	7.77E-05	AA167449	nuclear receptor subfamily 1, group I, member 3
1.940449	-5.370717	158.81	Down	8.36E-05	BE644917	nuclear receptor subfamily 1, group I, member 3
3.29779	-3.911445	147.98	Down	2.38E-05	U17496	Human proteasome subunit LMP7 (allele LMP7B) mRNA, complete cds. /PROD=proteasome subunit LMP7 /FL=gb:U17497.1 gb:U17496.1
4.124115	-2.85548	126.2	Down	2.99E-03	AW262311	ESTs
3.702164	-2.970402	102.01	Down	2.53E-03	U26662	Human neuronal pentraxin II (NPTX2) mRNA, partial cds. /PROD=neuronal pentraxin II
1.785431	-4.509786	78.53	Down	1.45E-03	R15072	ESTs
5.545158	-0.710745	76.42	Down	7.01E-05	BF057809	ESTs
1.946332	-3.865792	56.19	Down	7.43E-04	BG166705	small inducible cytokine subfamily B (Cys-X-Cys), member 5 (epithelial-derived neutrophil-activating peptide 78)
1.717184	-3.902593	49.17	Down	1.30E-04	AF237813	Homo sapiens NPD009 mRNA, complete cds. /PROD=NPD009 /FL=gb:NM_020686.1 gb:AF237813.1
3.179908	-2.381796	47.23	Down	9.96E-04	U82811	Human homeodomain-containing protein (HANF) mRNA, complete cds. /PROD=HANF /FL=gb:U82811.1
2.359289	-3.177031	46.41	Down	1.72E-04	NM_006334	gb:NM_003865.1 Homo sapiens neuroblastoma (nerve tissue) protein (AMY), mRNA. /PROD=neuroblastom a (nerve tissue) protein /FL=gb:NM_006334.1 gb:D82343.1
4.276201	-1.247561	46.01	Down	7.33E-05	AV699347	nuclear receptor subfamily 1, group I, member 3
2.435058	-2.963261	42.18	Down	1.36E-04	BF056204	Homo sapiens, clone IMAGE:3603836, mRNA, partial cds
2.348373	-2.98029	40.19	Down	7.34E-05	NM_016354	Homo sapiens solute carrier family 21 (organic anion transporter), member 12 (SLC21A12), mRNA. /PROD=organic anion transporter OATP-E /FL=gb:AB031051.1 gb:NM_016354.1 gb:AF205072.1 gb:AF187817.1
4.315048	-0.819678	35.13	Down	3.33E-03	NM_016139	Homo sapiens 16.7Kd protein (LOC51142), mRNA. /PROD=16.7Kd protein /FL=gb:NM_016139.1 gb:AF078845.1 gb:BC003079.1
2.348717	-2.72835	33.76	Down	9.42E-04	NM_001877	Homo sapiens complement component (3dEpstein Barr virus) receptor 2 (CR2), mRNA. /PROD=complement component (3dEpstein Barr virus)receptor 2 /FL=gb:NM_001877.1 gb:M26004.1
3.342331	-1.710595	33.2	Down	6.55E-05	AA876372	Homo sapiens mRNA; cDNA DKFZp667D095 (from clone DKFZp667D095)
1.995324	-3.045119	32.91	Down	4.60E-03	NM_014862	Homo sapiens KIAA0307 gene product (KIAA0307), mRNA. /PROD=KIAA0307 gene product /FL=gb:AB002305.1 gb:NM_014862.1
2.890305	-2.133881	32.54	Down	1.71E-03	NM_015474	Homo sapiens DKFZP564A032 protein
				(DKFZP564A032), mRNA. /PROD=DKFZP564A0 32 protein /FL=gb:AF228421.1 gb:AL050267.1 gb:AB013847.1 gb:NM_015474.1
2.443445	-2.518495	31.17	Down	7.43E-03	NM_152332	Homo sapiens chromosome 14 open reading frame 47 (C14orf47), mRNA. /FL=gb:NM_152332.1
3.692792	-1.250743	30.77	Down	8.80E-04	N21096	ESTs
2.266312	-2.653405	30.27	Down	7.22E-03	NM_003026	Homo sapiens SH3-domain GRB2-like 2 (SH3GL2), mRNA. /PROD=SH3-domain GRB2-like 2 /FL=gb:AF036268.1 gb:NM_003026.1
2.453774	-2.402069	28.96	Down	7.93E-05	NM_007191	Homo sapiens Wnt inhibitory factor-1 (WIF-1), mRNA. /PROD=Wnt inhibitory factor-1 /FL=gb:AF122922.1 gb:NM_007191.1
2.325274	-2.512615	28.6	Down	3.19E-05	AW 193693	DKFZP566K1924 protein
1.982765	-2.836916	28.24	Down	1.21E-04	BE672659	ESTs
0.997895	-3.793735	27.7	Down	3.97E-03	AW025928	ESTs, Weakly similar to 138588 reverse transcriptase homolog (H.sapiens)
4.756657	0.005012	26.94	Down	6.55E-05	AV715309	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
4.803291	0.085342	26.32	Down	7.34E-05	AA628440	nuclear receptor subfamily 1, group I, member 3
1.124153	-3.582082	26.1	Down	5.42E-03	W52934	ESTs, Weakly similar to similar to serinethreonine kinase (C.elegans)
0.874376	-3.810554	25.72	Down	2.24E-02	U82671	Homo sapiens chromosome Xq28 melanoma antigen family A2a (MAGEA2A), melanoma antigen family A12 (MAGEA12), melanoma antigen family A2b
	(MAGEA2B), melanoma antigen family A3 (MAGEA3), caltractin (CALT), NAD(P)H dehydrogenase-like protein (NSDHL), a...
0.621075	-4.029928	25.12	Down	5.18E-03	BC028721	Homo sapiens, Similar to solute carrier family 1 (high affinity aspartateglutamate transporter), member 6, clone MGC:33092 IMAGE:5269300, mRNA, complete cds. /PROD=Similar to solute carrier family 1 (highaffinity aspartateglutamate transporter), memb
1.49883	-3.130556	24.75	Down	7.87E-04	BF057784	ESTs
2.074855	-2.552806	24.72	Down	1.87E-03	AI420156	ESTs
3.2597	-1.357805	24.55	Down	1.05E-03	NM_017671	Homo sapiens hypothetical protein FLJ20116 (FLJ20116), mRNA. /PROD=hypothetical protein FLJ20116 /FL=gb:NM_017671.1
-0.10303	-4.717227	24.49	Down	7.33E-05	NM_022168	Homo sapiens melanoma differentiation associated protein-5 (MDA5), mRNA. /PROD=melanoma differentiation associated protein-5 /FL=gb:AY017378.1 gb:NM_022168.1 gb:AF095844.1
2.688175	-1.908993	24.2	Down	2.73E-04	NM_014178	Homo sapiens HSPC156 protein (HSPC156), mRNA. /PROD=HSPC156 protein /FL=gb:NM_014178.1 gb:AF161505.1
1.24677	-3.309288	23.52	Down	2.54E-02	BC028359	Homo sapiens, clone IMAGE:4828836, mRNA.
0.686587	-3.862863	23.42	Down	1.28E-03	NM_000439	Homo sapiens proprotein convertase subtilisinkexin type 1 (PCSK1), mRNA. /PROD=proprotein convertase subtilisinkexin type 1 /FL=gb:NM_000439.2 gb:M90753.1
5.363884	0.82261	23.28	Down	7.68E-05	NM_007015	Homo sapiens chondromodulin I precursor (CHM-I), mRNA. /PROD=chondromodul in I precursor /FL=gb:NM_007015.1 gb:AB006000.1
3.962328	-0.577927	23.27	Down	6.90E-05	AL533416	axonal transport of synaptic vesicles
2.086969	-2.410461	22.59	Down	9.65E-03	AL359055	Homo sapiens mRNA full length insert cDNA clone EUROIMAGE 2344436.
0.536704	-3.939442	22.26	Down	4.78E-03	AL049250	Homo sapiens mRNA; cDNA DKFZp564D113 (from clone DKFZp564D113).
4.260791	-0.214844	22.25	Down	6.89E-05	AA603344	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.121165	-4.34837	22.15	Down	1.36E-04	AI985987	ESTs, Moderately similar to ALU1_HUMAN ALU SUBFAMILY J SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.437404	-4.019211	21.96	Down	2.48E-02	H05254	ESTs
2.263194	-2.16575	21.54	Down	7.34E-04	AF052108	Homo sapiens clone 23687 mRNA sequence.
4.055226	-0.3701	21.49	Down	1.16E-04	NM_001307	Homo sapiens claudin 7 (CLDN7), mRNA. /PROD=claudin 7 /FL=gb:BC001055.1 gb:NM_001307.1
5.440506	1.023282	21.37	Down	1.02E-04	M34455	Human interferon-gamma-inducible indoleamine 2,3-dioxygenase (IDO) mRNA, complete cds. /FL=gb:NM_002164.1 gb:M34455.1
2.169025	-2.207268	20.77	Down	3.41E-03	NM_022467	Homo sapiens N-acetylgalactosamine-4-O-sulfotransferase (GALNAC-4-ST), mRNA. /PROD=N-acetylgalactosamine-4-O-sulfotransferase /FL=gb:NM_022467.1 gb:AF300612.1
0.252976	-4.116368	20.67	Down	3.36E-03	NM_018043	Homo sapiens hypothetical protein FLJ10261 (FLJ10261), mRNA. /PROD=hypothetical protein FLJ10261 /FL=gb:NM_018043.1
1.353776	-3.010836	20.6	Down	2.85E-02	AF147427	Homo sapiens full length insert cDNA clone YP80A10.
2.437935	-1.918781	20.49	Down	1.70E-03	BE672557	ESTs
2.46341	-1.870689	20.17	Down	4.16E-04	NM_003182	Homo sapiens tachykinin, precursor 1 (substance K, substance P, neurokinin 1, neurokinin 2, neuromedin L, neurokinin alpha, neuropeptide K,neuropeptide gamma) (TAC1), transcript variant beta, mRNA. /PROD=tachykinin 2 precursor, isoform beta/FL=gb:U3
2.294336	-2.028037	20.01	Down	7.10E-03	U11058	Homo sapiens large conductance calcium-and voltage-dependent potassium channel alpha subunit (MaxiK) mRNA, complete cds. /PROD=large conductance calcium-and voltage-dependentpotassium channel alpha subunit /FL=gb:U23767.1 gb:NM_002247.1 gb:AF025999
4.534853	0.221559	19.88	Down	7.68E-05	R38389	olfactomedin related ER localized protein
3.142124	-1.136699	19.41	Down	1.73E-02	AL832535	Homo sapiens mRNA; cDNA DKFZp547J1816 (from clone DKFZp547J1816).
3.85985	-0.410223	19.29	Down	7.34E-05	R40892	ESTs
4.557488	0.304559	19.07	Down	1.43E-04	AK026546	Homo sapiens cDNA: FLJ22893 fis, clone KAT04792.
5.966394	1.719122	18.99	Down	1.99E-04	AL117612	Homo sapiens mRNA; cDNA DKFZp564B1264 (from clone DKFZp564B1264).
1.212373	-3.013161	18.71	Down	5.22E-04	AI564075	ESTs
2.27629	-1.932316	18.49	Down	1.09E-04	BC044830	Homo sapiens, Similar to RIKEN cDNA
				1700011F14gene, clone MGC:35062 IMAGE:5166167, mRNA, complete cds. /PROD=Similar to RIKEN cDNA 1700011F14 gene /FL=gb:BC044830.1
3.18092	-1.007603	18.23	Down	1.29E-03	AJ011712	Homo sapiens TNNT1 gene, exons 1-11 (and joined CDS)
2.598916	-1.553059	17.78	Down	2.46E-03	AW051591	ESTs, Moderately similar to unnamed protein product (H.sapiens)
2.003902	-2.139208	17.67	Down	4.71E-03	BF109660	ESTs
1.905278	-2.229324	17.56	Down	5.05E-04	NM_0189 64	Homo sapiens solute carrier family 37 (glycerol-3-phosphate transporter), member 1 (SLC37A1), mRNA. /PROD=solute carrier family 37 (glycerol-3-phosphatetransporter), member 1 /FL=gb:NM_018964.1
0.330556	-3.792993	17.43	Down	3.26E-04	BE972639	ESTs
1.044277	-3.067425	17.29	Down	1.23E-02	AL529104	ESTs
0.733534	-3.349221	16.94	Down	4.39E-03	BF061389	ESTs, Weakly similar to JC1405 6-pyruvoyltetrahydropteri n synthase (H.sapiens)
2.684281	-1.394654	16.9	Down	2.91 E-04	BF449063	collagen, type XIV, alpha 1 (undulin)
4.572354	0.512428	16.68	Down	5.89E-04	BF437747	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
2.313549	-1.734907	16.55	Down	6.84E-03	AV726956	ESTs, Weakly similar to C35826 hypothetical 13K protein A (H.sapiens)
0.679665	-3.355919	16.4	Down	1.43E-03	BC000568	Homo sapiens, clone MGC:3040, mRNA, complete cds. /PROD=Unknown (protein for MGC:3040) /FL=gb:BC000568.1
4.099873	0.092088	16.09	Down	6.90E-05	AI057619	ESTs, Highly similar to T42654 hypothetical protein DKFZp434G 1115.1 (H.sapiens)
1.459269	-2.519	15.76	Down	6.26E-03	NM_000277	Homo sapiens phenylalanine
	hydroxylase (PAH), mRNA. /PROD=phenylalanine hydroxylase /FL=gb:U49897.1 gb:NM_000277.1
2.220936	-1.733714	15.5	Down	1.34E-04	AF237813	Homo sapiens NPD009 mRNA, complete cds. /PROD=NPD009 /FL=gb:NM_020686.1 gb:AF237813.1
2.81177	-1.140906	15.48	Down	6.89E-05	NM_002593	Homo sapiens procollagen C-endopeptidase enhancer (PCOLCE), mRNA. /PROD=procollagen C-endopeptidase enhancer /FL=gb:BC000574.1 gb:NM_002593.2 gb:AB008549.1 gb:L33799.1
1.529971	-2.399749	15.24	Down	2.29E-02	NM_024789	Homo sapiens hypothetical protein FLJ22529 (FLJ22529), mRNA. /PROD=hypothetical protein FLJ22529 /FL=gb:NM_024789.1
0.255558	-3.655262	15.04	Down	4.26E-03	BC039509	Homo sapiens, clone IMAGE:5578073, mRNA.
0.970967	-2.921559	14.85	Down	4.46E-03	AI144156	ESTs
2.38092	-1.504443	14.78	Down	4.36E-04	AF053712	Homo sapiens osteoprotegerin ligand mRNA, complete cds. /PROD=osteoprotegeri n ligand /FL=gb:AF053712.1 gb:AF019047.1
3.779853	-0.095194	14.67	Down	3.22E-04	AV646597	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
1.651332	-2.189895	14.33	Down	3.45E-03	NM_007181	Homo sapiens mitogen-activated protein kinase kinase kinase kinase 1 (MAP4K1), RNA. /PROD=mitogen-activated protein kinase kinase kinasekinase 1 /FL=gb:U66464.1
	gb:NM_007181.1
3.786136	-0.030985	14.1	Down	1.49E-04	BF057731	ESTs
3.257726	-0.553697	14.04	Down	4.48E-04	NM_004335	Homo sapiens bone marrow stromal cell antigen 2 (BST2), mRNA. /PROD=bone marrow stromal cell antigen 2 /FL=gb:NM_004335.2 gb:D28137.1
-0.33527	-4.146199	14.03	Down	4.21E-03	BE968806	ESTs, Weakly similar to ALU4_HUMAN ALU SUBFAMILY SB2 SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
0.349102	-3.450633	13.93	Down	1.30E-02	BM682352	Homo sapiens cDNA FLJ37204 fis, clone BRALZ2006976.
2.172559	-1.624126	13.9	Down	2.32E-03	BE673445	Homo sapiens chromosome 19, cosmid R28379
0.381933	-3.390833	13.67	Down	1.84E-02	AI913749	ESTs
1.120467	-2.648498	13.63	Down	1.85E-03	BE672607	ESTs
1.924097	-1.801676	13.23	Down	8.92E-03	AW242920	ESTs
1.491527	-2.224633	13.14	Down	7.01E-05	BG258131	ESTs
2.060687	-1.652733	13.12	Down	5.63E-03	AI269290	solute carrier family 18 (vesicular monoamine), member 2/FL=gb:L14269.1 gb:L23205.1 gb:L09118.1 gb:NM_003054.1
2.886142	-0.811762	12.98	Down	4.93E-04	U83115	Human non-lens beta gamma-crystallin like protein (AIM1) mRNA, partial cds. /PROD=non-lens beta gamma-crystallin like protein
0.626797	-3.063928	12.91	Down	4.51E-02	AF393369	Homo sapiens sigma 1C adaptin (AP1S3) mRNA, complete cds. /PROD=sigma 1C adaptin /FL=gb:AF393369.1
1.575227	-2.112834	12.89	Down	1.85E-03	BE856544	hypothetical protein FLJ22573
0.4785	-3.197824	12.78	Down	1.72E-04	BG532690	integrin, alpha 4 (antigen CD49D, alpha 4 subunit of VLA-4 receptor)
1.707178	-1.969084	12.78	Down	1.84E-02	AF043179	Homo sapiens T cell receptor beta chain (TCRBV13S1-TCRBJ2S1) mRNA,
				complete cds. /PROD=T cell receptor beta chain /FL=gb:AF043179.1
0.47298	-3.177323	12.56	Down	8.00E-03	AF311324	Homo sapiens ubiquitin-like fusion protein mRNA, complete cds. /PROD=ubiquitin-like fusion protein /FL=gb:AF311324.1
2.641731	-0.985721	12.36	Down	1.49E-04	AL133653	Homo sapiens mRNA; cDNA DKFZp434M2415 (from clone DKFZp434M2415).
2.913327	-0.707745	12.3	Down	3.70E-03	NM_012419	Homo sapiens regulator of G-protein signalling 17 (RGS17), mRNA. /PROD=regulator of G-protein signalling 17 /FL=gb:AF202257.2 gb:NM_012419.2
2.127724	-1.49095	12.28	Down	1.49E-03	NM_001275	Homo sapiens chromogranin A (parathyroid secretory protein 1) (CHGA), mRNA. /PROD=chromogranin A /FL=gb:BC001059.1 gb:NM_001275.2 gb:J03915.1 gb:J03483.1
0.80034	-2.81487	12.25	Down	4.62E-03	AW003107	ESTs
2.11511	-1.494168	12.2	Down	1.27E-03	NM_000593	Homo sapiens ATP-binding cassette, subfamily B (MDRTAP), member 2 (ABCB2), mRNA. /PROD=ATP-binding cassette, subfamily B, member 2 /FL=gb:NM_000593.2 gb:L21205.1 gb:L21206.1 gb:L21207.1 gb:L21204.1 gb:L21208.1
3.690675	0.086414	12.16	Down	1.85E-03	AW274018	ESTs
1.283746	-2.317044	12.13	Down	4.10E-03	NM_014031	Homo sapiens VLCS-H1 protein (VLCS-H1), mRNA. /PROD=very long-chain acyl-CoA synthetase homolog 1 /FL=gb:AF064254.1 gb:NM_014031.1
0.467003	-3.132847	12.12	Down	4.39E-02	AL117530	Homo sapiens mRNA;
				cDNA DKFZp434B172 (from clone DKFZp434B172); partial cds. /PROD=hypothetical protein
2.6402	-0.955567	12.09	Down	3.80E-02	NM_013267	Homo sapiens breast cell glutaminase (GA), mRNA. /PROD=breast cell glutaminase /FL=gb:AF110331.1 gb:AF110330.1 gb:AF223944.1 gb:NM_013267.1
1.858597	-1.724557	11.98	Down	5.91E-04	AA757457	ESTs
0.945333	-2.635993	11.97	Down	2.41E-03	BC040959	Homo sapiens, clone IMAGE:5242616, mRNA.
3.795925	0.223304	11.9	Down	1.71E-03	NM_004688	Homo sapiens N-myc (and STAT) interactor (NMI), mRNA. /PROD=N-myc and STAT interactor /FL=gb:BC001268.1 gb:NM_004688.1 gb:U32849.1
2.074972	-1.490898	11.84	Down	2.94E-03	NM_017933	Homo sapiens hypothetical protein FLJ20701 (FLJ20701), mRNA. /PROD=hypothetical protein FLJ20701 /FL=gb:NM_017933.1
-0.42571	-3.975429	11.71	Down	1.54E-03	AK023699	Homo sapiens cDNA FLJ13637 fis, clone PLACE1011165.
3.742964	0.195658	11.69	Down	1.19E-04	T62571	microtubule-associated protein 7 /FL=gb:NM_003980.1
1.621518	-1.924672	11.68	Down	2.63E-02	NM_003725	Homo sapiens oxidative 3 alpha hydroxysteroid dehydrogenase; retinol dehydrogenase; 3-hydroxysteroid epimerase (RODH), mRNA. /PROD=oxidative 3 alpha hydroxysteroid dehydrogenase;retinol dehydrogenase; 3-hydroxysteroid epimerase /FL=gb:AF016509.1 gb:A
6.076777	2.566425	11.4	Down	6.90E-05	AF229180	Homo sapiens alpha-aminoadipate semialdehyde synthase mRNA,
				complete cds. /PROD=alpha-aminoadipate semialdehyde synthase /FL=gb:AF229180.1
3.758058	0.25238	11.36	Down	1.89E-04	NM_005356	Homo sapiens lymphocyte-specific protein tyrosine kinase (LCK), mRNA. /PROD=lymphocyte-specific protein tyrosine kinase /FL=gb:U07236.1 gb:NM_005356.1 gb:M36881.1
3.797019	0.297284	11.31	Down	2.69E-04	AI871745	ESTs
2.469508	-1.020673	11.24	Down	9.14E-04	W63754	Homo sapiens mRNA for gycosyltransferase (ORF1)
1.048359	-2.438018	11.21	Down	1.39E-02	AA464273	ESTs
3.146674	-0.339455	11.21	Down	1.26E-04	BF435773	cortactin SH3 domain-binding protein
1.627801	-1.848139	11.13	Down	3.70E-03	L39833	Homo sapiens (clone hKvBeta3) K+ channel beta subunit mRNA, complete cds. /PROD=K+ channel beta-subunit /FL=gb:U16953.1 gb:L39833.1
1.594689	-1.879508	11.11	Down	4.03E-02	AJ236915	Homo sapiens mRNA for pak5 protein. /PROD=pak5 protein /FL=gb:NM_020168.1 gb:AF276893.1
2.806504	-0.6571	11.03	Down	1.21E-04	NM_003645	Homo sapiens fatty-acid-Coenzyme A ligase, very long-chain 1 (FACVL1), mRNA. /PROD=very long-chain fatty-acid-Coenzyme A ligase 1 /FL=gb:AF096290.1 gb:D88308.1 gb:NM_003645.1
3.826815	0.364324	11.02	Down	6.55E-05	BG401568	Homo sapiens mRNA; cDNA DKFZp434H1235 (from clone DKFZp434H1235); partial cds
2.99034	-0.471936	11.02	Down	7.16E-04	NM_002993	Homo sapiens small inducible cytokine subfamily B (Cys-X-Cys), member 6 (granulocyte chemotactic protein 2) (SCYB6), mRNA.
	/PROD=small inducible cytokine subfamily B(Cys-X-Cys), member 6 (granulocyte chemotactic protein 2) /FL=gb:U81234.1 gb:NM_00299
3.788599	0.329467	11	Down	8.58E-05	NM_002252	Homo sapiens potassium voltage-gated channel, delayed-rectifier, subfamily S, member 3 (KCNS3), mRNA. /PROD=potassium voltage-gated channel,delayed-rectifier, subfamily S, member 3 /FL=gb:AF043472.1 gb:NM_002252.1 gb:BC004987.1 gb:BC004148.1
4.397278	0.939176	10.99	Down	1.22E-04	NM_021614	Homo sapiens potassium intermediatesmall conductance calcium-activated channel, subfamily N, member 2 (KCNN2), mRNA. /PROD=potassium intermediatesmall conductancecalcium-activated channel, subfamily N, member 2 /FL=gb:NM_021614.1 gb:AF239613.1
1.027188	-2.423197	10.93	Down	1.22E-03	BG169832	adenylate kinase 5 /FL=gb:NM_012093.1 gb:AF062595.1
1.022495	-2.421211	10.88	Down	2.47E-02	BC002832	Homo sapiens, Similar to butyrophilin, subfamily 3, member A2, clone MGC:3790, mRNA, complete cds. /PROD=Similar to butyrophilin, subfamily 3, member A2 /FL=gb:U90144.1 gb:NM_007047.1 gb:U90546.1 gb:BC002832.1
0.311203	-3.122447	10.81	Down	1.70E-03	AI964053	ESTs
1.673874	-1.728682	10.57	Down	2.25E-03	NM_005965	Homo sapiens myosin, light polypeptide kinase (MYLK), mRNA. /PROD=myosin, light
				polypeptide kinase /FL=gb:AB037663.1 gb:AF069601.2 gb:NM_005965.1
1.443731	-1.955774	10.55	Down	1.43E-03	AJ272267	Homo sapiens partial mRNA for choline dehydrogenase (chdh gene). /PROD=choline dehydrogenase
0.383563	-3.004508	10.47	Down	2.48E-02	AI377688	ESTs
0.995551	-2.39165	10.46	Down	5.14E-03	NM_005386	Homo sapiens neuronatin (NNAT), mRNA. /PROD=neuronatin /FL=gb:NM_005386.1 gb:BC001768.1 gb:AB002392.1 gb:U25033.1
3.45531	0.070626	10.44	Down	1.94E-04	AV733308	integrin, alpha 6
3.527039	0.143408	10.44	Down	5.95E-05	BG283790	ESTs
2.950823	-0.418278	10.33	Down	1.38E-03	NM_003645	Homo sapiens fatty-acid-Coenzyme A ligase, very long-chain 1 (FACVL1), mRNA. /PROD=very long-chain fatty-acid-Coenzyme A ligase 1 /FL=gb:AF096290.1 gb:D88308.1 gb:NM_003645.1
1.55078	-1.80799	10.26	Down	3.70E-03	H28597	thymopoietin
5.005827	1.649812	10.24	Down	1.90E-04	NM_003020	Homo sapiens secretory granule, neuroendocrine protein 1 (7B2 protein) (SGNE1), mRNA. /PROD=secretory granule, neuroendocrine protein 1 (7B2protein) /FL=gb:BC005349.1 gb:NM_003020.1
0.760646	-2.590248	10.2	Down	2.29E-02	AW589793	ESTs
2.209313	-1.126222	10.09	Down	5.95E-05	AA747379	calcitonin-related polypeptide, beta /FL=gb:NM_000728.1
-0.10418	-3.43217	10.04	Down	4.66E-03	NM_017655	Homo sapiens hypothetical protein FLJ20075 (FLJ20075), mRNA. /PROD=hypothetical protein FLJ20075 /FL=gb:NM_017655.1
2.598488	-0.722855	10	Down	2.03E-03	L08599	Human uvomorulin (E-cadherin) (UVO) mRNA, complete cds. /PROD=uvomorulin
1.858219	-1.457169	9.95	Down	1.81E-03	NM_005084	/FL=gb:NM_004360.1 gb:L08599.1 Homo sapiens phospholipase A2, group VII (platelet-activating factor acetylhydrolase, plasma) (PLA2G7), mRNA. /PROD=phospholipase A2, group VII (platelet-activatingfactor acetylhydrolase, plasma) /FL=gb:U20157.1 gb:U24577.1 gb:NM_005084.1
1.910263	-1.3945	9.88	Down	1.27E-03	NM_006994	Homo sapiens butyrophilin, subfamily 3, member A3 (BTN3A3), mRNA. /PROD=butyrophilin, subfamily 3, member A3/FL=gb:U90548.1 gb:NM_006994.2
2.001097	-1.297629	9.84	Down	1.19E-03	BC028721	Homo sapiens, Similar to solute carrier family 1 (high affinity aspartateglutamate transporter), member 6, clone MGC:33092 IMAGE:5269300, mRNA, complete cds. /PROD=Similar to solute carrier family 1 (highaffinity aspartateglutamate transporter), memb
5.020283	1.723791	9.83	Down	1.63E-04	AK025084	Homo sapiens cDNA: FLJ21431 fis, clone COL04214, highly similar to HSU80736 Homo sapiens CAGF9 mRNA.
2.474373	-0.811562	9.75	Down	5.94E-03	NM_013272	Homo sapiens solute carrier family 21 (organic anion transporter), member 11 (SLC21A11), mRNA. /PROD=solute carrier family 21 (organic aniontransporter), member 11 /FL=gb:NM_013272.2 gb:AF205074.1 gb:AB031050.2 gb:AF187816.1
2.116702	-1.16308	9.71	Down	4.40E-02	AF107846	Homo sapiens
	neuroendocrine-specific Golgi protein p55 (XLalphas) gene, exon XL2 and complete cds
2.472358	-0.803312	9.68	Down	2.33E-03	NM_000363	Homo sapiens troponin I, cardiac (TNNI3), mRNA. /PROD=troponin I, cardiac /FL=gb: M64247.1 gb:NM_000363.1
0.384182	-2.880367	9.61	Down	4.26E-03	NM_005825	Homo sapiens RAS guanyl releasing protein 2 (calcium and DAG-regulated) (RASGRP2), mRNA. /PROD=RAS guanyl releasing protein 2 (calcium and DAG-regulated) /FL=gb:AF043723.1 gb:NM_005825.1
2.394742	-0.866876	9.59	Down	1.57E-04	AI733027	ESTs, Weakly similar to RET2_HUMAN RETINOL-BINDING PROTEIN II, CELLULAR (H.sapiens)
1.319792	-1.930717	9.52	Down	5.95E-05	M18767	Human complement subcomponent C1s, alpha- and beta-chains, complete cds. /FL=gb:J04080.1 gb:M18767.1 gb:NM_001734.1
3.859451	0.610002	9.51	Down	5.73E-04	AJ242502	Homo sapiens mRNA for E-MAP-115105 (MAP gene). /PROD=epithelial microtubule-associated protein
3.009579	-0.239729	9.51	Down	5.22E-04	AB037730	Homo sapiens mRNA for KIAA1309 protein, partial cds. /PROD=KIAA1309 protein
2.600702	-0.646217	9.49	Down	1.43E-02	AA740186	biliverdin reductase A /FL=gb:NM_000712.1 gb:U34877.1
0.971941	-2.274152	9.49	Down	7.72E-04	NM_018018	Homo sapiens hypothetical protein FLJ10191 (FLJ10191), mRNA. /PROD=hypothetical protein FLJ10191 /FL=gb:NM_018018.1
0.414323	-2.829854	9.48	Down	6.30E-03	AF283777	Homo sapiens clone TCBAP0702 mRNA sequence.
6.139688	2.900659	9.44	Down	4.48E-04	BC036488	Homo sapiens, clone MGC:43145 IMAGE:5261574, mRNA, complete cds. /PROD=Unknown (protein for MGC:43145) /FL=gb:BC036488.1
1.569503	-1.668679	9.44	Down	1.24E-03	BF195118	ESTs, Weakly similar to ALU7_HUMAN ALU SUBFAMILY SQ SEQUENCE CONTAMINATION WARNING ENTRY (H.sapiens)
1.665643	-1.567308	9.4	Down	8.63E-04	AF282250	Homo sapiens calneuron 1 (CALN1) mRNA, complete cds. /PROD=calneuron 1 /FL=gb:AF282250.1
4.319584	1.104655	9.29	Down	5.53E-04	AA618420	Homo sapiens cDNA: FLJ23597 fis, clone LNG15281
4.436354	1.227541	9.25	Down	2.94E-04	AI912275	B-cell CLLlymphoma 11A (zinc finger protein) /FL=gb:NM_022893.1 gb:NM_018014.1
1.923237	-1.283751	9.23	Down	3.70E-03	AW072102	Homo sapiens mRNA; cDNA DKFZp434H205 (from clone DKFZp434H205)
2.59299	-0.613677	9.23	Down	1.94E-04	NM_003887	Homo sapiens development and differentiation enhancing factor 2 (DDEF2), mRNA. /PROD=ADP-ribosylation factor(arf)-directed GTPaseactivating protein /FL=gb:AB007860.1 gb:NM_003887.1
3.20248	0.002668	9.19	Down	5.80E-04	AF220153	Homo sapiens four and a half LIM domains 1 protein isoform C (FHL1) mRNA, complete cds, alternatively spliced. /PROD=four and a half LIM domains 1 protein isoform C /FL=gb:AF220153.1
1.689335	-1.505873	9.16	Down	2.46E-03	NM_031272	Homo sapiens testis expressed sequence 14 (TEX14), mRNA. /PROD=testis
	expressed sequence 14 /FL=gb:NM_031272.1
3.026209	-0.167981	9.15	Down	6.90E-05	BC032302	Homo sapiens, similar to UDP-glucose ceramide glucosyltransferase-like 2, clone MGC:40268 IMAGE:5169731, mRNA, complete cds. /PROD=similar to UDP-glucose ceramideglucosyltransf erase-like 2 /FL=gb:BC032302.1
3.116245	-0.070826	9.11	Down	7.93E-05	NM_017947	Homo sapiens hypothetical protein FLJ20733(FLJ20733), mRNA. /PROD=hypothetical protein FLJ20733 /FL=gb:NM_017947.1
2.91664	-0.26326	9.06	Down	1.68E-03	AW003367	Homo sapiens clone 25237 mRNA sequence
4.453662	1.27718	9.04	Down	7.33E-05	AV681807	v-erb-b2 avian erythroblastic leukemia viral oncogene homolog 3
3.454075	0.278604	9.03	Down	1.86E-04	AV691491	Homo sapiens mRNA; cDNA DKFZp564D1462 (from clone DKFZp564D1462)
1.883578	-1.291525	9.03	Down	2.67E-02	BF970287	Human DNA sequence from clone RP1-310013 on chromosome 20q11.2. Contains (part of) four novel genes, ESTs, STSs, GSSs and four putative CpG islands
2.326737	-0.838174	8.97	Down	2.61E-03	NM_015982	Homo sapiens germ cell specific Y-box binding protein (LOC51087), mRNA. /PROD=germ cell specific Y-box binding protein /FL=gb:NM_015982.1 gb:AF096834.1
0.392456	-2.771428	8.96	Down	2.73E-02	NM_003007	Homo sapiens semenogelin I (SEMG1), mRNA. /PROD=semenogelin I /FL=gb:J04440.1 gb:NM_003007.1
3.116953	-0.041715	8.93	Down	3.90E-04	AA469071	Cluster Incl.
				AA469071:ne17f11.s1 Homo sapiens cDNA, 3 end /clone=IMAGE-881517 /clone_end=3 /gb=AA469071 /gi=2195605 /ug=Hs.180479 /len=758
3.113317	-0.040507	8.9	Down	2.36E-03	AL565745	ESTs, Weakly similar to 2108402A carnitine palmitoyltransferase I (H.sapiens)
5.010828	1.86984	8.82	Down	3.28E-04	AK027006	Homo sapiens cDNA: FLJ23353 fis, clone HEP14321, highly similar to HSU80736 Homo sapiens CAGF9 mRNA.
3.249727	0.113464	8.79	Down	2.14E-04	BC001745	Homo sapiens, clone MGC:3328, mRNA, complete cds. /PROD=Unknown (protein for MGC:3328) /FL=gb:BC001745.1 gb:NM_014392.1
1.532208	-1.601117	8.77	Down	3.19E-03	AI796813	advillin
5.063502	1.934512	8.75	Down	1.01E-04	AB018289	Homo sapiens mRNA for KIAA0746 protein, partial cds. /PROD=KIAA0746 protein
1.934415	-1.192238	8.73	Down	3.13E-03	NM_001351	Homo sapiens deleted in azoospermia-like (DAZL), mRNA. /PROD=deleted in azoospermia-like /FL=gb:U66726.2 gb:NM_001351.1 gb:U65918.1 gb:U66078.1
2.522705	-0.592752	8.67	Down	9.13E-03	U07236	Human mutant lymphocyte-specific protein tyrosine kinase (LCK) mRNA, complete cds. /PROD=lymphocyte-specific protein tyrosine kinase /FL=gb:U07236.1 gb:NM_005356.1 gb:M36881.1
3.995648	0.881994	8.66	Down	6.55E-05	AI961231	KIAA0808 gene product /FL=gb:AB018351.1 gb:NM_014729.1
2.077151	-1.020617	8.56	Down	7.33E-05	BF223193	nuclear receptor subfamily 1, group I, member 3
6.650173	3.554864	8.55	Down	8.55E-04	NM_004360	Homo sapiens cadherin 1, type 1, E-cadherin (epithelial) (CDH1), mRNA. /PROD=cadherin 1, type 1, E-cadherin (epithelial) /FL=gb:NM_004360.1 gb:L08599.1
1.440541	-1.650241	8.52	Down	1.11E-03	BE503640	ESTs
1.344522	-1.721548	8.37	Down	1.97E-02	AW071705	dipeptidylpeptidase VI
4.319671	1.253603	8.37	Down	1.05E-04	AF063002	Homo sapiens LIM protein SLIMMER mRNA, complete cds. /PROD=LIM protein SLIMMER /FL=gb:AF063002.1 gb:AF098518.1
2.575606	-0.489298	8.37	Down	1.24E-03	BC016785	Homo sapiens, Similar to hypothetical protein PRO1722, clone IMAGE:4096414, mRNA.
1.070412	-1.992167	8.35	Down	7.29E-04	AF070642	Homo sapiens clone 24488 mRNA sequence.
3.083054	0.021788	8.35	Down	2.33E-03	BC026969	Homo sapiens, clone IMAGE:5116073, mRNA, partial cds.
6.075972	3.015223	8.34	Down	1.35E-04	NM_001449	Homo sapiens four and a half LIM domains 1 (FHL1), mRNA. /PROD=four and a half LIM domains 1 /FL=gb:U60115.1 gb:NM_001449.1 gb:U29538.1
0.779095	-2.27952	8.33	Down	1.58E-02	AF497717	Homo sapiens tissue-type lung unknown mRNA.
4.227241	1.173625	8.3	Down	3.47E-04	AI193252	ESTs, Weakly similar to AF133270 1 SLIT2 (H.sapiens)
1.139113	-1.908335	8.27	Down	1.40E-02	AI741469	ESTs
3.120689	0.079671	8.23	Down	6.27E-04	U01874	Human me20m mRNA, complete cds. /PROD=me20m /FL=gb:NM_006928.1 gb:BC001414.1 gb:U01874.1
3.499377	0.460367	8.22	Down	2.16E-03	NM_024572	Homo sapiens hypothetical protein FLJ12691 (FLJ12691), mRNA. /PROD=hypothetical protein FLJ12691 /FL=gb:NM_024572.1
2.568736	-0.463022	8.18	Down	4.78E-03	AA531287	ESTs

Table VII- Correlation coefficient between differentiated ES cells, EXPRES 01, EXPRES 02 and various time points during differentiation to DE

	ES	EXPRES 02	EXPRES 01
EXPRES 02	0.882
EXPRES 01	0.906	0.912
2 hr DE	0.914	0.895	0.922
6 hr DE	0.904	0.887	0.915
24hr DE	0.912	0.898	0.924
30hr DE	0.91	0.902	0.926
48hr DE	0.906	0.913	0.921
72hr DE	0.896	0.918	0.91
96hr DE	0.895	0.919	0.912
5 days DE	0.883	0.925	0.904

Table IX Expression of cytokines, growth factors, and receptors as measured by protein arrays




54,220	54,220	54,220	54,220
0	0	0	0
1,049	957	2,098	1,494
461	383	165	219
173	182	0	206
0	0	0	29
0	0	0	114
0	0	0	0
751	870	745	654
38	88	118	137
0	43	0	30
0	0	36	44
0	0	0	0
0	0	0	0
122	12	55	62
74	39	33	6
468	376	457	341
327	209	31	11
0	0	0	0
885	847	655	716
0	8	0	0
792	830	702	841
199	142	62	99
1,262	1,408	846	867
0	0	56	98
1,437	1,368	1,880	1,597
111	125	95	48
470	426	348	445
758	633	631	553
87	0	0	0
1,274	1,022	1,053	1,055
219	53	0	0
66	103	0	0
934	946	815	829
825	930	819	904
212	230	213	304
959	939	851	849
930	891	994	975
1,214	1,013	1,005	1,074
0	0	0	0
0	0	0	0
1,611	1,632	6,146	4,338
225	203	212	257
463	445	364	248
228	170	244	149
267	342	307	282
218	299	140	252
898	863	789	976
107	236	145	281
386	518	472	495
92	159	91	67
0	0	0	0
90	77	69	230
2,623	1,755	467	583
0	0	127	102
0	0	0	0
532	493	168	290
0	0	0	0
716	788	806	840
73	111	0	16
748	825	760	908
269	316	247	307




43,203.88	39,506.01	36,640.81	42,748.84
0.00	0.00	0.00	0.00
1,044.38	797.16	429.05	408.73
926.38	812.41	1,132.59	1,111.92
164.38	193.08	183.69	149.23
62.38	39.17	65.41	67.20
203.88	165.35	203.92	235.90
420.38	390.43	330.99	529.97
551.38	581.78	449.28	504.69
144.38	126.52	114.65	144.58
317.88	278.12	254.92	294.20
769.88	610.44	824.79	738.91
453.88	383.50	352.10	276.14
175.88	145.47	158.63	204.43
325.38	272.11	290.98	421.63
165.88	105.73	97.51	244.15
8,897.88	9,437.80	8,026.40	5,317.62
92.38	2.66	28.91	131.69
156.88	65.05	65.41	242.09
362.88	140.39	82.12	312.77
334.88	267.49	415.86	535.13
161.38	97.87	152.47	127.04
0.88	0.00	30.23	0.00
0.00	2.20	19.24	0.00
0.00	0.00	0.00	0.00
452.38	433.42	399.15	458.26
446.88	302.62	397.83	297.81
340.38	342.83	454.55	325.67
364.88	310.01	295.82	382.42
1,194.38	1,087.42	3,883.43	4,764.05
272.38	200.47	179.29	286.46
326.38	89.09	74.64	180.18
83.38	55.35	29.79	97.12
60.38	0.00	21.00	0.00
12.88	36.86	23.63	62.55
158.38	25.30	54.85	144.58
504.38	450.98	282.19	257.05
0.00	16.99	50.46	30.57
30.38	43.79	29.35	6.84
442.38	454.68	436.52	356.62
507.38	459.76	124.33	187.40
278.88	228.21	254.92	207.01
483.38	379.34	413.66	465.48
199.38	148.25	157.75	181.21
312.88	218.04	184.13	182.25
472.88	353.92	454.11	483.02
1,047.88	765.73	382.44	469.09
0.00	0.00	0.00	0.00
113.88	123.29	50.90	55.33
68.38	50.73	14.84	53.27
291.38	218.96	165.22	198.24
57.88	53.50	119.49	94.02
166.88	143.16	109.38	180.70
432.38	329.89	1,175.24	208.04
510.88	367.33	437.40	801.34
41.38	38.25	20.12	0.00
23,824.38	23,824.38	23,824.38	23,824.38




55,531.00	63,702.50	55,954.13	76,525.06
0.00	0.00	0.00	0.00
140.00	100.45	119.63	179.61
221.50	239.23	261.80	443.17
0.00	0.00	58.85	104.61
0.00	0.00	0.00	0.00
210.00	351.20	368.94	523.07
64,959.00	75,788.69	57,182.11	65,024.38
0.00	0.00	0.00	0.00
0.00	0.00	0.00	0.00
455.50	399.01	258.71	415.13
57.00	48.55	70.18	12.09
0.00	0.00	0.00	0.00
83.50	92.28	30.52	33.82
726.00	842.78	781.52	939.43
374.00	460.83	352.97	450.17
232.50	130.77	110.36	218.17
271.00	520.31	295.28	460.69
688.00	895.85	223.68	973.77
0.00	0.00	0.00	0.00
242.00	109.19	140.75	167.00
1,380.00	1,572.29	929.87	1,270.97
962.00	1,043.39	920.08	1,080.31
162.50	108.03	194.83	217.46
0.00	0.00	0.00	0.00
752.00	848.62	571.88	614.89
0.00	0.00	0.00	0.00
169.00	439.25	190.20	372.37
314.50	285.89	245.31	368.17
236.00	314.46	133.54	237.09
226.00	354.11	283.43	373.77
0.00	32.80	0.00	92.70
187.50	178.59	135.60	299.47
174.00	130.19	91.82	227.28
163.00	198.41	140.23	245.50
120.00	114.44	72.24	164.89
434.50	488.24	422.50	553.21
163.00	114.44	327.73	144.57
741.00	782.72	694.47	1,053.68
721.50	763.48	551.28	754.38
177.00	68.37	93.88	135.46
2,703.00	2,577.05	2,491.12	3,008.58
251.00	257.89	236.56	341.53
15.50	0.00	14.55	56.95
242.50	233.99	184.02	279.15
376.50	303.38	250.98	408.12
37.00	101.03	108.81	253.21
380.50	390.27	432.29	696.90
466.50	394.35	361.21	504.15
180.50	198.41	195.86	220.27
18.00	36.30	203.08	209.05
0.00	0.00	0.00	0.00
11.50	0.00	694.47	267.93
0.00	0.00	0.00	0.00
175.00	123.19	172.17	223.77
1,718.50	2,953.76	487.41	502.74
256.50	231.65	227.80	256.02
0.00	0.00	127.36	94.10
239.00	273.64	277.25	370.27
104.50	84.12	103.66	319.10
311.00	289.97	305.06	523.77
0.00	0.00	0.00	0.00
18,664.17	18,664.17	18,664.17	18,664.17

SEQUENCE LISTING

<110> Rezania, Alireza
<120> PLURIPOTENT CELLS
<130> CEN5217USNP
<140> 12/108,872 <141> 2008-04-24
<160> 3
<170> PatentIn version 3.5
<210> 1 <211> 17 <212> DNA <213> Artificial Sequence
<220> <223> SYNTHETIC CONSTRUCT
<400> 1 tggcgcagca gatacca 17
<210> 2 <211> 18 <212> DNA <213> Artificial Sequence
<220> <223> SYNTHETIC CONSTRUCT
<400> 2 agcgccttcc acgacttg 18
<210> 3 <211> 23 <212> DNA <213> Artificial Sequence
<220> <223> SYNTHETIC CONSTRUCT
<400> 3 ccagcatctt gctcaactcg gcg 23

Claims

A method for deriving a population of cells comprising cells expressing pluripotency markers comprising the steps of:
a. obtaining a population of cells expressing markers characteristic of the definitive endoderm lineage by differentiation of human embryonic stem cells, and

b. culturing the cells from (a) under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in a medium containing serum, activin-A and a Wnt ligand,
wherein the cells expressing pluripotency markers express at least one of the pluripotency markers selected from the group consisting of ABCG2, cripto, FoxD3, Connexin43, Connexin45, Oct4, SOX-2, Nanog, hTERT, UTF-1, ZFP42, SSEA-3, SSEA-4, Tra1-60, and Tra1-81.
The method of claim 1, wherein cells expressing markers characteristic of the definitive endoderm lineage are cultured in:
a. normoxic conditions; or

b. hypoxic conditions
prior to culturing the cells under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix.
The method of claim 1, wherein the hypoxic conditions are an O₂ level:
a. from 1% to 20%; or

b. from 2% to 10%; or

c. of 3%.
The method of claim 1, wherein the cells are cultured under hypoxic conditions, on a tissue culture substrate that is not pre-treated with a protein or an extracellular matrix, in medium containing:
a. serum at a concentration from 2% to 5%; or

b. serum at a concentration of 2%; or

c. IGF-1 at a concentration from 25ng/ml to 50ng/ml; or

d. IGF-1 at a concentration of 50ng/ml; or

e. a GSK-3B inhibitor.
The method of claim 1, wherein said activin-A is at a concentration from 50ng/ml to 100ng/ml or of 100ng/ml.
The method of claim 1, wherein said Wnt ligand is at a concentration from 10ng/ml to 20ng/ml or of 200ng/ml.
The method of claim 1, wherein the cells expressing pluripotency markers express markers characteristic of:
a. pre-primitive streak cells; or

b. primitive streak cells; or

c. mesoendoderm cells.
The method of claim 1, wherein the Wnt ligand is Wnt-3a.