AU2004200026A1 - Purification of echinocandin cyclopeptide compounds - Google Patents
Purification of echinocandin cyclopeptide compounds Download PDFInfo
- Publication number
- AU2004200026A1 AU2004200026A1 AU2004200026A AU2004200026A AU2004200026A1 AU 2004200026 A1 AU2004200026 A1 AU 2004200026A1 AU 2004200026 A AU2004200026 A AU 2004200026A AU 2004200026 A AU2004200026 A AU 2004200026A AU 2004200026 A1 AU2004200026 A1 AU 2004200026A1
- Authority
- AU
- Australia
- Prior art keywords
- product
- acetic acid
- group
- echinocandin
- mixture
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
- 150000001875 compounds Chemical class 0.000 title claims description 33
- 238000000746 purification Methods 0.000 title description 16
- 108010049047 Echinocandins Proteins 0.000 title description 13
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- 238000000034 method Methods 0.000 claims description 55
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- OGNAOIGAPPSUMG-UHFFFAOYSA-N spiro[2.2]pentane Chemical compound C1CC11CC1 OGNAOIGAPPSUMG-UHFFFAOYSA-N 0.000 description 1
- 239000007858 starting material Substances 0.000 description 1
- 125000004079 stearyl group Chemical group [H]C([*])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])C([H])([H])[H] 0.000 description 1
- 238000003756 stirring Methods 0.000 description 1
- PXQLVRUNWNTZOS-UHFFFAOYSA-N sulfanyl Chemical class [SH] PXQLVRUNWNTZOS-UHFFFAOYSA-N 0.000 description 1
- 238000010189 synthetic method Methods 0.000 description 1
- 150000003512 tertiary amines Chemical class 0.000 description 1
- 229930192474 thiophene Natural products 0.000 description 1
- 239000010891 toxic waste Substances 0.000 description 1
- 238000003828 vacuum filtration Methods 0.000 description 1
- 239000003643 water by type Substances 0.000 description 1
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- Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
- Peptides Or Proteins (AREA)
Description
AUSTRALIA
Patents Act 1990 ELI LILLY AND COMPANY COMPLETE SPECIFICATION STANDARD PATENT Invention Title: Purification of echinocandin cyclopeptide compounds The following statement is a full description of this invention including the best method of performing it known to us: m:\specifications\500000\502000\5O2O58cmpmjc.doc PURIFICATION OF ECHINOCANDIN CYCLOPEPTIDE COMPOUNDS TECHNICAL FIELD The present invention relates to a process for purification of cyclopeptide compounds containing at least one protonatable amino group, in particular, the process relates to the purification of an Echinocandin-type compound by adsorption onto a hydrophobic, reversed phase chromatographic media and eluting with a continuous nearly linear gradient of increasing acetic acid. A purification process is also provided for selectively removing a tripeptide-aldehyde by-product of the Echinocandin fermentation process to yield a higher purity Echinocandin compound.
BACKGROUND ART Echinocandin cyclopeptides are natural products that have been shown to have antifungal activities. Included in the Echinocandin cyclopeptide family are natural products such as Echinocandin B (ECB), Echinocandin C, Aculeacin Ay, Mulundocandin, Sporiofungin A, Pneumocandin Ao, WF11 899A, and Pneumocandin
B
0 The natural products are typically produced by culturing various microorganisms.
For example, Echinocandin B is produced from the fermentation of the fungus, Aspergillus nidulans.
In the search for more active materials, the niatural products have been modified in a variety of ways. One of the most common modifications has been the replacement of the N-acyl side chain on the natural product to produce a semisynthetic derivative. For example, U.S. Patent Nos. 4,293,489; 4,320,052; 5,166,135; and 5,541,160; and EP 359529; 448353; 447186; 462531; and 561639 describe a variety of N-acyl derivatized Echinocandin compounds that provide varying degrees of antifungal activity.
The N-acyl derivatives are produced by deacylating the natural product followed by reacylation with a different acyl group. The deacylation is typically achieved by means of an enzyme deacylase enzyme). The deacylase enzyme may be obtained from the microorganism Actinoplanes utahensis or Pseudomonas species. See U.S Patent Nos. 4,293,482; and 4,304,716; and EP 460,882. The deacylated compound is typically referred to as the nucleus of the corresponding natural product the deacylated product of Echinocandin B is referred to as the Echinocandin B nucleus (ECBN)). Unfortunately, both the fermentation and deacylation processes produce several by-products that are difficult to remove and decrease the purity of the desired deacylated cyclic peptide nucleus.
U.S. Patent No. 4,874,843 describes a chromatographic process using nonfunctional resins in a reversed mode to purify Echinocandin-type products. Even though the process improved the purity of products derived from a fermentation process, further improvements are still needed to remove contaminants that are difficult to separate from both the intermediate deacylated nucleus and the final acylated pharmaceutically active compounds. Since the potency of the final pharmaceutical product is dependent upon the purity of the intermediates used to make the final product, improvements in purity at any stage of the manufacturing process are highly desirable. Ideally, the contaminants are removed at the earliest stage possible in the manufacturing process.
General discussions of non-functional resins and their applications in liquid chromatographic separations may be found in J. Chromatography, 201, 287-292 (1980) and Grieser, M.D. et al, Analytical Chemistry, 45, 1348-1353 (1973). The use of either step or continuous gradients are discussed; however, the eluents contain significant amounts of organic solvents. In a manufacturing process, the use of organic solvents raises several concerns such as environmental regulations air quality emission standards), special handling requirements flammability standards) and disposal limitations toxic waste regulations). Therefore, there is a need for an eluent system that minimizes the use of organic solvents yet effectively separates mixtures into their pure components.
DISCLOSURE OF THE INVENTION The present invention provides a method for separating and purifying a wide variety of fermentation cyclopeptide products containing at least one protonatable amino group (including the deacylated Echinocandin-type compounds) from their fermentation or mixed broths and partially purified process streams by adsorbing the mixture onto a hydrophobic, reversed phase, chromatographic media and eluting with a continuous nearly linear acetic acid gradient ranging from 0.1% acetic acid to 10.0% acetic acid by volume in water, preferably from 0.5% (pH=5.5) to 4.0% acetic acid.
In another embodiment of the present invention, a process for purifying Echinocandin-type compounds (including simple derivatives thereof) is provided where an aldehyde by-product (in particular, a tripeptide-aldehyde by-product) in the fermentation mixture or partially purified mixture is reacted with a derivatizing agent.
Preferably, the fermentation broth or mixed broth is reacted with the derivatizing agent prior to purification of the corresponding Echinocandin nucleus using.the.
method described above.
As used herein, the term "derivatizing agent" refers to a reagent capable of reacting with the aldehyde functionality of the tripeptide by-product to produce an intermediate that is sufficiently different in hydrophobicity to allow separation of the tripeptide intermediate from the desired Echinocandin-type compound.
The term "protonatable amino group" refers to an amino group that undergoes protonation when subjected to the eluting conditions of the present invention 0.1% acetic acid to 10% acetic acid by volume in water).
The term "Echinocandin-type compounds" refers to compounds having the following general structure including any simple derivatives thereof: HO RI 0
HO
R N O O R4.
OH
R6 wherein R is a hydrogen or where R' is an alkyl group, an alkenyl group, an alkynyl group, an aryl group, or heteroaryl group having attached thereon at least one protonatable amino group; RI is -H or -OH; R2 is -H or -CH 3 R3 is -CH 3
-CH
2
CONH
2 or -CH 2
CH
2
NH
2 R4 is -H or -OH; R5 is -OH, -OPO 3
H
2 or -OSO 3
H;
and R6 is -H or -OSO 3 H. "Echinocandin nucleus" refers to the deacylated Echinocandin compound where R is a hydrogen. "ECBN" refers to the Echinocandin B nucleus where RI, R4 and R5 are hydroxyl groups, R2, R3, and R7 are methyl groups; and RI and R6 are hydrogens.
The term "alkyl" refers to a hydrocarbon radical of the general formula CnH 2 n+i containing from 1 to 30 carbon atoms unless otherwise indicated. The alkane radical may be straight methyl, ethyl, propyl, butyl, etc.), branched isopropyl, isobutyl, tertiary butyl, neopentyl, etc.), cyclic cyclopropyl, cyclobutyl, cyclopentyl, methylcyclopentyl, cyclohexyl, etc.), or multi-cyclic bicyclo[2.2.1]heptane, spiro[2.2]pentane, etc.). The alkane radical may be substituted or unsubstituted. Similarly, the alkyl portion of an alkoxy group or alkanoate has the same definition as above.
The term "alkenyl" refers to an acyclic hydrocarbon containing at least one carbon-carbon double bond. The alkene radical may be straight, branched, cyclic, or multi-cyclic. The alkene radical may be substituted or unsubstituted.
The term "alkynyl" refers to an acyclic hydrocarbon containing at least one carbon-carbon triple bond. The alkyne radical may be straight, or branched. The alkyne radical may be substituted or unsubstituted.
The term "aryl" refers to aromatic moieties having single phenyl) or fused ring systems naphthalene, anthracene, phenanthrene, etc.). The aryl groups may be substituted or unsubstituted.
The term "heteroaryl" refers to aromatic moieties containing at least one heteratom within the aromatic ring system pyrrole, pyridine, indole, thiophene, furan, benzofuran, imidazole, pyrimidine, purine, benzimidazole, quinoline, etc.).
The aromatic moiety may consist of a single or fused ring system. The heteroaryl groups may be substituted or unsubstituted.
Within the field of organic chemistry and particularly within the field of organic biochemistry, it is widely understood that significant substitution of compounds is tolerated or even useful. In the present invention, for example, the term alkyl group allows for substitutents which is a classic alkyl, such as methyl, ethyl, propyl, hexyl, isooctyl, dodecyl, stearyl, etc. The term "group" specifically envisions and allows for substitutions on alkyls which are common in the art, such as hydroxy, halogen, alkoxy, carbonyl, keto, ester, carbamato, etc., as well as including the unsubstituted alkyl moiety. However, it is generally understood by those skilled in the art that the substituents should be selected so as to not adversely affect the pharmacological characteristics of the compound or adversely interfere with the use of the medicament. Suitable substituents for any of the groups defined above include alkyl, alkenyl, alkynyl, aryl, halo, hydroxy, alkoxy, aryloxy, mercapto, alkylthio, arylthio, mono- and di-alkyl amino, quaternary ammonium salts, aminoalkoxy, hydroxyalkylamino, aminoalkylthio, carbamyl, carbonyl, carboxy, glycolyl, glycyl, hydrazino, guanyl, and combinations thereof.
BEST MODE FOR CARRYING OUT THE INVENTION Fermentation and mixed broths contain a number of by-products that are very difficult to separate from the desired cyclopeptide product. "Mixed broth" refers to a conversion mixture where the fermentation broth is treated directly with a deacylating enzyme without purification to produce the deacylated product ECBN).
Reversed-phase, liquid chromatography has been used in the past with reasonable success; however, the need for higher purity compounds demands more improved methods of purification. Applicants have discovered that the separation of fermentation by-products from the desired fermentation product containing a protonatable amino group can be improved by using a reversed-phase chromatographic media in combination with a continuous, nearly linear acetic acid elution scheme.
Suitable hydrophobic chromatographic media include reversed phase silicas, and organic polymers such as copolymers of styrene and divinylbenzene, methacrylate polymer. A variety of reversed-phase silicas are commercially available from vendors such as BTR, E. Merck, Eka Nobel, Millipore, Phenomenex, Whatman, or YMC. The silicas are derivatized with straight chain alkyl hydrocarbons ranging in length from Ci to C 1 8 (Ci, C 4 C8 and C 1 8 being the most common) or other hydrophobic ligands such phenyl or cyano). A variety of styrene/divinylbenzene resins designed for reversed-phase, liquid chromatography are also available commercially such as DiaionT m HP and SP resins (available from Mitsubishi Chemical Industries Limited, Tokyo, Japan), and Amberlite XAD-2,4, and 16 resins (available from Rohm and Haas Chemical Co., Philadelphia, PA), and the CG-161, 300, and 1000 Amberchrom resins from Toso Haas (Montgomeryville, PA). Non- O O functional resins are generally characterized by their pore volume (0.5-4.5 ml/g), specific surface area (200-800 m 2 pore diameter (40-1300 pore size distribution and/or bead size distribution. Preferred non-functional resins include Diaion HP-20 having a surface area of 500 m 2 a pore size of 200-300 A and particle size of 200-800 pm; SP-825 having a surface area of 1,000 m 2 pore size of 50-60 A and particle size of 250-600 pm; SP-207 (brominated version of having a surface area of 630 m 2 pore size of 100-200 A and particle size of 200-800 pm; and CG-161CD having a surface area of 900 m 2 pore size of 110-175 A, and particle size of 80-160 pim. More preferred are the HP-20 and SP-825 resins.
Initially, a crude or partially purified solution is provided that contains the desired cyclic peptide compound having at least one protonatable amino group.
Generally, the amino group can be protonated during the course of the acetic acid gradient that spans the pH range from 5.5 to 2.5. Preferably the amino group is a primary amine; however, the amino group may be a secondary amine or tertiary amine so long as the additional substituents on the nitrogen atom are not sufficiently hydrophobic such that they overcome the polarity of the positively charged amine.
The solution may originate from a fermentation process or a synthetic process. For example, the cyclic peptide compounds may be prepared by the synthetic methods described in U.S. Patent No. 5,696,084; J. Am. Chem. Soc., 108, 6041 (1986); Evans, et al., J. Am. Chem. Soc., 109, 5151 (1987); J. Med. Chem., 35, 2843 (1992); and Kurokawa, et al., Tetrahedron, 49, 6195 (1993). The crude solution is usually a mixed broth. Alternatively, the process may be used to further purify (or polish) partially purified material.
Depending upon the particular fermentation process used, it may be desirable to prefilter the solution to remove particulates that may interfere with the chromatographic process. Filtration may be accomplished by any number of means known to those skilled in the art including gravity filtration, vacuum filtration through a ceramic filter which may or may not include a CeliteT
M
filter aid, etc. Solids in the fermentation broth may also be removed by centrifugation followed by decanting the liquid from the solids.
The fermentation solution may be concentrated if desired using a variety of means which are also well known to those skilled in the art such as evaporative concentration, lyophilization, etc. The concentrate may be filtered a second time to remove any precipitate that may have formed during the concentration process.
The crude or partially purified solution is loaded onto a chromatography column packed with one of the hydrophobic chromatographic media described above.
The desired cyclic peptide product is then eluted from the chromatographic media using a continuous nearly linear gradient ranging from about 0.1% acetic acid to about acetic acid, preferably from about 0.5% acetic acid (pH=5.5) to about 4% acetic acid The upper end of the range of acetic acid concentration selected is based upon the stability of the chromatographic media used and the stability of the compound being purified at that pH. The lower end of the range is selected based upon the pH where the amino group is protonated and concentration of acetic acid required to elute the product from the hydrophobic surface. Those skilled inthe ait will appreciate that the gradient does not have to be perfectly linear. Within the meaning of "nearly linear" includes a flat convex or concave gradient.
At the end of the gradient elution process step, an additional volume of the higher concentrated acetic solution is typically used to complete the elution. At the end of the process, the column may be regenerated so that the column may be re-used for additional purification cycles. The regeneration step typically involves washing the column with mixtures of an organic solvent and water at both a neutral and alkaline pH to remove any residual materials left on the column matrix. Suitable solvents include acetonitrile, methanol, isopropanol, and acetone. The linear acetic acid elution scheme not only provides good selectivity (see Example I below), but also limits the use of organic solvents to the regeneration step of the column operation. Thus, both the absolute quantity of organic solvent used and the volume of column effluent that must be treated prior to disposal is minimized.
The fermentation product may be recovered from the eluate using a variety of methods. Suitable recovery methods include crystallization, evaporative concentration, and lyophilization.
The fermentation broth for Echinocandin B contains varying levels of a tripeptide-aldehyde (Asn-Gln-Leu-H) by-product having the following chemical structure The tripeptide-aldehyde by-product under goes deacylation as well as Echinocandin B during the enzymatic deacylation process to form the corresponding deacylated tripeptide-aldehyde (Ib).
NH,
0. H 0
HN
0
(I)
where R is C(O)CH2CH(OH)CqHi9 (la fermentation by-product) or a hydrogen (Ib deacylation by-product from a mixed broth).
Surprisingly, the retention time of the deacylated tripeptide-aldehyde is very similar to ECBN in reversed phase, liquid chromatography, even under optimum elution conditions, thus making it very difficult to separate the deacylated tripeptidealdehyde (Ib) from the desired ECBN. If the tripeptide is not removed, then the free amino group of the tripeptide competes with the free amino group of the ECBN compound during the reacylation process. As a result, an excess of acylating compound must be added to insure complete acylation of the ECBN compound. The tripeptide contaminate not only consumes needed starting materials but also produces an acylated by-product that is difficult to remove in subsequent purification of the acylated ECB compound. Preferably, the tripeptide by-product is removed prior to the reacylation of the ECBN compound.
The tripeptide-aldehyde by-product may be removed from either the fermentation mixture or the mixed broth deacylation mixture) by reacting the aldehyde with a derivatizing agent prior to chromatographic purification. The derivatizing agent may be added to the aldehyde functionality to change the chromatographic retention time of the tripeptide-aldehyde in relation to the desired ECB compound. Suitable derivatizing agents include sodium bisulfite, hydroxyl amine and semicarbazide hydrochloride. Some advantages of using derivatizing agents as opposed to other means of modifying the chromatographic retention times are the selectivity of the derivatizing agents for the aldehyde functionality and the mild conditions under which the reaction occurs. If the reaction between the derivatizing agent and the tripeptide-aldehyde is reversible. then the aldehyde can be easily recovered by removing the derivatizing agent. The recovered tripeptide can then be used for other purposes.
EXAMPLES
The following abbreviations are used through out the examples to represent the respective listed materials: ACN acetonitrile TFA trifluoroacetic acid HP-20 styrene/divinylbenzene resin having a surface area of 500 m 2 a pore size of 200-300 A and particle size of 200-800 pim.
SP-825 styrene/divinylbenzene resin having a surface area of 1,000 m 2 /g, pore size of 50-60 A and particle size of 250-600 pmr SP-207 brominated styrene/divinylbenzene resin having a surface area of 630 m 2 pore size of 100-200 A and particle size of 200-800 pm CG-161CD styrene/divinylbenzene resin having a surface area of 900 m 2 /g, pore size of 110-175 A, and particle size of 80-160 pm.
0 0 Chromatographic preparation and ECBN purification procedures: Glass columns were used ranging in size from 0.2 to 5 liters. The chromatographic matrices studied included HP-20, SP-825 and SP-207 (all available form Mitsubishi) and CG-161cd (available from Toso Haas). The matrices were batch washed with 50/50 water/ACN, 0.1 M sodium hydroxide, and finally by pure acetonitrile (ACN) prior to column packing. The matrix of choice was packed into the appropriate size column using simple slurry settling techniques. Column sizes less than one liter were operated using conventional FPLC instrumentation (available from Pharmacia). The five liter column experiments were conducted using a Waters Delta Prep 3000 controller system.
ECBN mixtures were clarified by filtration using Cuno 30S filters prior to loading onto the respective columns. The HP-20 and SP-825 columns were preequilibrated in 0.5% acetic acid (HOAc), adjusted to a pH of 5.5 with sodium hydroxide (NaOH), and loaded with the clarified ECBN solution. The columns were loaded to approximately 5 to 5.5 g ECBN/liter of packed resin while the SP-825 columns were loaded at approximately 1.1 to 12 g/liter. After loading, the columns were washed with 5 column volumes (CV) of the equilibration buffer. The product was eluted using a continuous 5 CV, linear gradient ranging from HOAc (pH=5.5) to 4% HOAc At the end of the gradient, an additional 2 CV of the 4% HOAc solution was used to complete the elution. During elution of the product, 0.2 CV fractions were collected. The fractions were characterized by a variety of reversed-phase HPLC (RP-HPLC) methods, the appropriate fractions were combined to yield the mainstream pool. The columns were regenerated by washing with a 3 CV 60/40 mixture of ACN and water, followed by a 3 CV 60/40 mixture of ACN and 0.1 M NaOH. The flow rates used during the operation were 2 CV/hour (150 cm/hour) for load, wash, regeneration and re-equilibration and 1 CV/hour cm/hour) for elution. The mainstream pools were concentrated.
For comparison, the following mobile phase conditions (organic modifier and pH) and gradient elution profiles were studied in addition to the matrix type.
O O ACN modifier: Examples 1-3 used a 5 CV, linear ACN gradient (pH 5.5 with an acetate buffer).
Acetic Acid Elution: In addition to the conditions described earlier, the concentration of acetic acid was increased to 5% (Example 10). A step gradient and convex gradient were also compared to the continuous linear gradient described above on both the HP-20 and SP-825 columns (Examples 13-19).
Analytical characterization ofsamples: The quality and quantity of ECBN chromatographic samples were evaluated using the following analytical methods.
Phosphate system: A Zorbox SB C-18, 3.5 micron particle column (0.46 cm ID x 15 cm), was eluted with a 0.2% phosphoric acid/ACN mobile phase at a flow rate of 1.0 ml/min. The column was operated at 40 0 C and the effluent was monitored at 210 nm. The column is equilibrated in 1% ACN and after sample injection, a gradient ranging from I to 18.5% ACN over 9 minutes was used to elute ECBN.
After elution, the column was washed with 50% ACN to elute any highly retained components.
Phosphate/Octanesulfonic Acid (OSA) system: This system is similar to the phosphate system discussed above, with the exception that the mobile phase contains mM OSA. The column is equilibrated with 9% ACN. After the sample is injected, elution of ECBN is accomplished with a gradient ranging from 9 to 24% ACN over 9 minutes. The column was then washed with 50% ACN to elute highly retained components. Column flow rate and detector wavelength were as above, while the column temperature was 50'C. This system is particularly useful for quantitating the Asn-Gln-Leu-H tripeptide-aldehyde component.
TFA system: A Vydac C-18, 3.5 micron column (0.46 x 25 cm) was used for the assay. The mobile phase contained 0.1% TFA and elution was accomplished using a linear ACN gradient of 0 to 10% over 20 minutes, followed by a column wash of 50%. Column flow rate, temperature, and detector wavelength were the same as for the phosphate system described above.
Amino acid analysis (AAA) was also conducted on samples as an alternative method for determining the tripeptide content. Samples were acid hydrolyzed, and the moles of Asn, Gln, and Thr in the hydrolysate were determined by ion exchange chromatography and ninhydrin derivatization. The Thr recovery was used to determine the moles of ECBN in the sample, while the Gln content represented the tripeptide levels. The mole% of the Asn-Gln-Leu-H tripeptide versus ECBN was calculated using the following equation: M% Asn-Gln-Leu-H 2x[Gln]/[Thr] Optical density (OD) measurements were conducted on select samples at the specified wavelength to estimate relative sample turbidity (OD @550 runm) or total protein content (OD @280 nm).
The following examples are provided to illustrate but not limit the claimed invention.
Example 1 Example 1 compares RP-HPLC chromatographic processes using an acetonitrile elution scheme with an acetic acid elution scheme in combination with a variety of non-functional resins. Table 1 summarizes the results observed using the designated elution schemes and column media.
>0 Table 1 Ex. Matrix Column ECON RP- %Desmethyl Mainstream No. type Load' Elution Scheme Yield HPLC inipurityb Volume purity I' HP-20 3.8 0-10% ACN 84% 77.5% 2.09% 2.7 2' HP-20 7.7 0-10% ACN 66% 76% 1.2% 4.2 ~pH 5.5 3P HP-20 10.0 0-10% ACN 48% 52.3% 1.2% 4.2 pH 5.5 HP-20 6.0 HOAc 82% 70.5% 11.4% 1.8 gradient HP-20 6.0 0.5-4% HOAc 69% 89% 1.8% linear grad.
6 SP-207 12.0 0.54% HOAc 77% 83% 6.35% 3.9 linear 7 CG- 161 6.0 0.5.4% HOAc 59% 90.2% 1.3% 3.01 7 linear grad. 8 CG- 161 10.0 0.5-4% HOAc 75.2% 83% 2.5% 4.7 7 linear grad. 9' CG- 161 8.0 100 mM H P04 51% 80% 3.3% 4.4 SP-825 12.0 0.5-5% HOAc 72% 78.5% 5.5% 2.8 7 linear grad. I I SP-825 14.0 0.5-4% HOAc 70% 82% 3.57% linear grad. 12 SP-825 18.0 0.54% HOAc 83% 85% 4.0% 4.8.
linear 13 HP-20 6.0 0.5-4% HOAc 70.5% 85% 2.68% linear grad. 14' HP-20 6.0 0-5-4% HQAc 65% 81.6% 3.11% 1.44 I CV 1* HP-20 6.0 .5 H c3.5 04 2.93% 0.77 ~Step gradient 16 SP-825 9.1 0.54% HOAc 77% 92% 2.6% 2.9 ~5 linear 17' SP-825 9.1 0.54% HOAc 58% 91% 2.5% 2.7 Convex grad.
18' SP-825 9.1 0.5-4% HOAc 56.6% 89% 3.4% 2.3 gradient 19 SP-825 11.8 0.5-4% HOAC 59% 87% 2.8% 2.6 l inear HP-20 5.0 0.54% HOAc 81% 88% 2.2% 2.6 linear [L I HP-2 6.3 0.54% HOAc 81% 86% 3.3% linear grad. In Table 1, *Comparative examples; 'Measured in grams of ECBN per liter of resin; bDesmethyl impurity refers to a mixture of two ECBN compounds where the methyl group is missing on the threonine and the methyl proline peptide units, respectively.
The (ACN) modifier scheme provided good yield, overall purity and resolution of the desmethyl components; however, acetonitrile is an organic solvent.
Table I clearly shows that acetic ac id provides an alternative to the traditional organic solvent elution scheme. The data also shows that a continuous gradient of acetic acid significantly enhances resolution as compared to either a step gradient or convex gradient of acetic acid. Even though the product yield for Example 5 (linear gradient) is slightly lower and the mainstream volume larger as compared to Example 4 (step gradient), the overall ECBN purity is higher (83% vs. 71%) and the desmethyl content is lower vs. 11%).
The elution of ECBN from the hydrophobic matrix using the acetic acid elution process is believed to be accomplished in two ways: acetic acid acts as an organic modifier, thereby increasing the elution strength of the mobile phase; and (2) the lower pH of the B solvent (strong elution solvent, pH=2.5) serves to protonate the amine functionality of ECBN thus making it more polar and therefore less retained by the hydrophobic stationary phase. Both the organic modifier and pH that affects of the 4% acetic solution are apparent in comparing Examples 8 and 9. In Example 9, 1 00mM phosphoric acid (pH=2.5) was substituted for the 4% HOAc (pH=2.5) as the B solvent. If the elution of the ECBN was dependent only on the pH of the mobile phase, the elution position and recovery of ECBN should be similar to that observed in Example 8. In fact, the phosphate elution resulted in only about 50% recovery of ECBN and the product peak showed a significant degree-of tailing. Thus the 4% HOAc may bring about elution by both lowering the pH of the mobile phase and increasing the elution strength of the mobile phase by acting as an organic modifier.
Acetic acid also provides for greater selectivity than acetonitrile. When RP- HPLC chromatograms for mainstreams collected from HP-20 columns eluted with ACN versus HOAc (Examples 1 and 5, respectively) are compared, an absence of backside impurities in the mainstream eluted using HOAc was observed. In the HOAc elution scheme, these components are not eluted until the column is regenerated.
Example 2 Example 2 compares chromatographic processes using a single column/linear acetic acid elution scheme (described above) with a dual column/convex acetonitrile elution scheme. In addition, a comparison between untreated lots of ECBN (Examples 2-8 and 2-10) with ECBN lots treated with sodium metabisulfite prior to purification on the column (Examples 2-7 and 2-9) is described. The pretreatment with sodium metabisulfite was accomplished by simply adding 10 mM of sodium metabisulfite to the column charge and allowing the solution to stir for a period of 6- 18 hours. The single column process is the same as described above using a linear gradient acetic acid elution scheme.
The comparative dual column process uses two HP-20 columns that operate in a lead-trail configuration. A fermentation broth is loaded onto two HP-20 columns connected in series. Any ECBN which is not retained by the first column is concentrated on the second column. The ECBN is believed to be distributed in approximately equal proportions between the two columns. After loading, the lead column is disconnected and washed with 3.8 column volumes (CV) of water. Elution of the lead column is accomplished by washing with 3.3 CV of 5% HOAc. The mainstream from the first column is adjusted to a pH of 5.0 and charged onto the partially loaded second (trail) column. The column is washed with 6.3 CV of water prior to elution. A convex acetonitrile gradient over about 5 CV containing HOAc) is used to elute the column. The column effluent is fractionated and fractions having the desired purity (greater than 75% reversed-phase HPLC main peak purity and less than 10% desmethyl component) are pooled as the mainstream. The pooled solution is then concentrated.
Table 2 compares the results observed for the single column versus the dual column chromatographic process, and the treated versus untreated ECBN fermentation broths.
0 0 Table 2 ECBN Purity ECBN Purity Post Column Purification Crystal" Ex. Column type Column ECBN/O No. configuation Load %MP Des' %tripeptide D RO Potency b Purityd 2-1 HP-20 5.0 88.4 1.8 7.0 0.71 74.9 2-2 SP-825 12.0 88.2 1.9 6.2 0.59 73.1 2-3 HP-20/HP-20 84/7 2.2 7.1 -0.53 60.5 2-4 HP-20 5.3 83.0 2.0 11.8 0.69 76.4 SP-825 12.0 79.4 2.3 12.7 0.68 63.14 2-6 HP-20/HP-20 81.9 1.7 12.8 0.67 76.8 2-7 HP-20 4.8 87.7 1.8 1.5 0.65 74.3 2-8 HP-20/HP-20 84.6. 1.9 7.9 0.62 2-9 SP-825 10.5 88.2 3.2 3.3 0.56 2-10 HP-20/HP-20 79.6 2.8 13.6 0.68 In Table 2, aValues reported represent the average of two independent crystallizations and analytical determinations; b%Main peak versus total RP-HPLC peak area; c%Desmethyl impurites; dECBN/OD grams of ECBN (RP-HPLC)/Total OD grams; where OD grams OD@280 nm and assuming Eo.I% of 1.0; 'One of the two lots had high water content; therefore, average potency was reduced.
The analytical results reported above for ECBN purity were obtained after the mainstreams had been concentrated. Both the reversed-phase HPLC main peak purity and the desmethyl levels are similar for the single HP-20 and SP-825 column experiments. However, the single HP-20 operation consistently yields a slightly greater reduction in the desmethyl component. In general, the ECBN reversed-phase HPLC purity of the single column process is equivalent to or better than the ECBN purity from the two column process thus providing a more economical means of purification.
None of the column purification schemes were able to significantly reduce the level of the tripeptide; however, pretreatment with sodium bisulfite significantly reduced the amount of tripeptide impurites. The ECBN/OD purity of the product from the single column studies was equivalent to or greater than that obtained in the two column studies. Although the ECBN/OD value does not represent an absolute measure of purity, it does provide a good relative comparison of the ECBN purity resulting from the various column operations. All of the column operations gave a 18 10-15 fold increase in ECBN/OD purity when the values for the column charge solutions (data not shown) are compared to those concentrated mainstreams.
All references cited herein, are hereby incorporated herein. Although the foregoing invention has been described in some detail, by way of illustration and example for the purposes of clarity and understanding, it will be apparent to those skilled in the art that certain changes and modifications can be practiced. Therefore, the description and examples should not be construed as limiting the scope of the invention, which is delineated by the appended claims.
Any discussion of documents, acts, materials, devices, articles or the like which has been included in the present specification is solely for the purpose of providing a context for the present invention. It is not to be taken as an admission that any or all of these matters form part of the prior art base or were common general knowledge in the field relevant to the present invention as it existed before the priority date of each claim of this application.
Throughout this specification the word "comprise", or variations such as "comprises" or "comprising", will be understood to imply the inclusion of a stated element, integer or step, or group of elements, integers or steps, but not the exclusion of any other element, integer or step, or group of elements, integers or steps.
Claims (19)
1. A method for separating and purifying cyclopeptide products comprising the steps of: providing a mixture comprising a cyclopeptide compound having attached thereon at least one protonatable amino group; (ii) adsorbing said mixture onto a hydrophobic, reversed phase chromatographic media; and (iii) eluting with a continuous nearly linear acetic acid gradient ranging from 0.1% acetic acid to 10.0% acetic acid by volume in water.
2. The method of Claim 1 wherein said acetic acid gradient ranges from acetic acid to 4.0% acetic acid by volume in water.
3. The method of Claim 1 wherein said cyclopeptide compound is represented by the following structure: HO R1 0 HO R3 N 0 OH /N R3 OO "OH OH RS R6 wherein R is a hydrogen or where R' is an alkyl group, an alkenyl group, an alkynyl group, an aryl group, or heteroaryl group having attached thereon at least one protonatable amino group; RI is -H or -OH; R2 is -H or -CH 3 R3 is -CH 3 0 0 -CH 2 CONH 2 or -CH 2 CH 2 NH 2 R4 is -H or -OH; R5 is -OH, -OP0 3 H 2 or -OSO 3 H; and R6 is -H or -OSO 3 H.
4. The method of Claim 3 wherein R is hydrogen.
The method of Claim I wherein said hydrophobic, reversed-phase media is an organic polymer.
6. The method of Claim 5 wherein said organic polymer is a copolymer of styrene and divinylbenzene or a methacrylate polymer.
7. The method of Claim 5 wherein said organic polymer is a styrene/divinylbenzene resin having a surface area of 500 m2/g, a pore size of 200-300 A and particle size of 200-800 pm; or a styrene/divinylbenzene resin having a surface area of 1,000 m 2 pore size of 50-60 A and particle size of 250-600 pm.
8. The method of Claim I wherein said mixture is a product of a mixed broth.
9. The method of Claim 1 further comprising the step (iv)recovering said cyclopeptide compound.
A process for purifying Echinocandin-type compounds containing an aldehyde by-product comprising the steps of: providing a mixture of a Echinocandin-type compound and an aldehyde by product; (ii) adding a derivatizing agent to said mixture to produce a derivatized aldehyde product; and (iii) separating said Echinocandin-type compound from said derivatized aldehyde product. 0 7 O
11. The process of Claim 10 wherein said separating step (iii) comprises the method of Claim 1.
12. The process of Claim 10 wherein said Echinocandin-type compound is represented by the following structure: HO R1 0 N R3 N SOH RS R6 wherein R is a hydrogen or where R' is an alkyl group, an alkenyl group, an alkynyl group, an aryl group, or heteroaryl group having attached thereon at least one protonatable amino group; R1 is -H or -OH; R2 is -H or -CH 3 R3 is -CH 3 -CH 2 CONH 2 or -CH 2 CH 2 NH 2 R4 is -H or -OH; R5 is -OH, -OP0 3 H 2 or -OSO 3 H; and R6 is -H or -OSO 3 H.
13. The process of Claim 12 wherein R is a hydrogen.
14. The process of Claim 13 wherein said separating step (iii) comprises the method of Claim 1.
15. The process of Claim 10 wherein said aldehyde by-product is represented by the following structure: 0 NH, H H H N N R 0 H HN 0 wherein R is -C(O)CH 2 CH(OH)C 9 H 9 or a hydrogen.
16. The process of Claim 10 wherein said mixture is a product of a fermentation broth.
17. The process of Claim 10 wherein said mixture is a product of a mixed fermentation broth.
18. The process of Claim 10 wherein said derivatizing agent is selected from the group consisting of sodium bisulfite, hydroxyl amine and semicarbazide hydrochloride.
19. The process of Claim 15 wherein said derivatizing agent is sodium bisulfite. The process of Claim 15 wherein said separating step (iii) comprises the method of Claim 1.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| AU2004200026A AU2004200026A1 (en) | 1998-12-09 | 2004-01-06 | Purification of echinocandin cyclopeptide compounds |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US60/111524 | 1998-12-09 | ||
| AU31132/00A AU766091B2 (en) | 1998-12-09 | 1999-12-08 | Purification of echinocandin cyclopeptide compounds |
| AU2004200026A AU2004200026A1 (en) | 1998-12-09 | 2004-01-06 | Purification of echinocandin cyclopeptide compounds |
Related Parent Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU31132/00A Division AU766091B2 (en) | 1998-12-09 | 1999-12-08 | Purification of echinocandin cyclopeptide compounds |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| AU2004200026A1 true AU2004200026A1 (en) | 2004-01-29 |
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Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU2004200026A Abandoned AU2004200026A1 (en) | 1998-12-09 | 2004-01-06 | Purification of echinocandin cyclopeptide compounds |
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| Country | Link |
|---|---|
| AU (1) | AU2004200026A1 (en) |
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2004
- 2004-01-06 AU AU2004200026A patent/AU2004200026A1/en not_active Abandoned
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| Date | Code | Title | Description |
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| MK1 | Application lapsed section 142(2)(a) - no request for examination in relevant period |