DE20321115U1 - Carrier for growing cells comprises microbial cellulose, useful for culturing e.g. multipotent, mesenchymal stem cells or keratinocytes - Google Patents

Abstract

Carrier (A) for growing cell cultures consists of microbial cellulose.

Description

The The invention relates to a carrier for cell cultures.

animal Cell cultures usually grow in monolayer layers on the surface of carrier materials, where the cells are fixed by adsorptive processes. such Surface culture techniques come for the culture of animal or human cells is used, wherein the strength of the physical bond through specific properties the vehicles To be defined. This strength is often due to external factors, e.g. pH value shifts, changes in the inner thickness the media used, clearly influenced. Especially for the area of tissue engineering, where special emphasis is placed on structured three-dimensional expression the cultures are placed, play characteristics of the used carrier a special role.

The for the Tissue engineering materials are mostly natural ones Sources. You need to therefore in purity meet the requirements of "Medical Grade". Frequently they are chemically modified for better adsorption of the cells. she allowed to but not toxic or cytotoxic and should ideally be biological be degradable. These conditions must be at least partially met, so that with the materials good to excellent cellular interactions possible are. Depending on the tissue to be examined or harvested, these must Materials also meet certain requirements.

Examples for now used such carrier materials are on the one hand as polymer the collagens of type I with heterotrimeric helical structure. As the most common Polymer of mammals (Tendons, skin, bones) it is relatively easy to access but very thoroughly be cleaned to avoid any contamination with BSE agents or avoid other problem substances. The material is relatively light chemically crosslinked or modifiable by partial degradation. It is excellent for cell cultivation, but in general too quickly degradable. It is also used in medicine and surgery, for example, as a tamponade or in splenic ruptures, in orthodontics.

To the Others use glycosaminoglycans as natural polymers. They consist of repeating disaccharide units, predominantly uronsäurehaltig are. For example, chodroitin sulfate and dermatan sulfate used. This class of substance is also easy to esterify chemically modifiable. It has a high water binding. Indeed requires use in tissue engineering and as a cell culture support a very high cleaning effort. The uronic acid groups are easy with Calcium complexable, so that, for example, gels, membranes, hoses, sleeves and particles accessible are. In contrast to the collagens have the glycosaminoglycans only low antigenic and inflammatory properties, but lower adhesive Properties.

When third natural Group are called chitosans, the group partially or completely deacetylated Chitins. It is extracted from crustacean skeletons. Due to the It is adsorptively active and chemically charged modifiable.

At Synthetic polymers are given analogous conditions as on the natural substances. The base are mostly natural hydroxy acids, like Glycolic, lactic, and caproic acids, the high variability of the achieve mechanical properties in the polymers. These For example, products form the basis for the production of films hoses or fleeces. They are easily extrudable. Furthermore, it is a mixture between the basic mixtures possible.

(Minuth, W.W., Strehl, R., Schumacher, K .: Future Technology Tissue Engineering - From Cell Biology to the artificial Tissue. 1. Ed. - 2003, XII, 348 p., ISBN 3-527-30793-1, Wiley-VCH, Weinheim) All these materials need a cleaning effort, as they are in the process in which they are not obtained as pure de-product or not occur solely in the sources from which they are made available become. Furthermore, especially with the chemical-synthetic materials or in the chemically partially modified polymers a high Cleaning effort necessary to separate any interfering impurities and to exclude antigenic and inflammatory properties.

Out the document WO 0161026 A1 and its patent family is known that formed biomaterials based biosynthetically formed bacterial cellulose in cylindrical form as blood vessel replacement, for covering nerve tracts or as partial replacement of hollow organs can be used and that this material has been proven in animal experiments. It is described that attach to the inside endothelial cells can. However, the dimensions of these molded cellulose tablets are only with inner diameters of 1-3 mm or smaller. Furthermore, the colonization ability only for Endothelial cells from animal experiments described.

The object of the present invention is to provide a carrier for cell cultures, which the avoids the aforementioned disadvantages of the known carrier and allows a universal application of the carrier overgrown with cell cultures.

Surprisingly imagine a carrier consisting from microbial cellulose, as a very suitable one support material for cell cultures and for universal application of this dar.

The Biopolymer microbial cellulose is highly hydrated through those in the molecule existing hydroxyl groups very good attachment possibilities for training stable, mostly physical binding sites for both the cells as well as for needed Media components and is opposite Degradation stable. Due to the high hydration by the storage of watery Systems between the polymer chains is an ideal basis for cell cultures given.

Surprisingly could be further found that these are biosynthetically formed, according to Desired specially shaped, homogeneously structured and high-purity cellulose because of this high degree of hydration as an ideal carrier for most Cells of human and / or animal origin to be cultured suitable is.

The after DE 100 22 751 C2 . DE 101 16 602 A1 and WO 02/081725 A1 cellulose obtained is sterilized after washing in an autoclave, made into required shapes and sizes and added as needed with sterile nutrient medium. These nutrient media penetrate into the aqueous phase of the bacterial cellulose and allow a homogeneous distribution of nutrients over the entire surface. Less diffusible media due to unfavorable viscosities or physical bonds can be introduced by shaking, mixing, or other laboratory technologies.

The cell cultures are inoculated in the usual way on the cellulose supports and incubated at temperatures between 25 and 40 ° C, preferably between 32 and 38 ° C, in the incubator at 75-95%, preferably 85-92% moisture. In principle, every incubator is suitable. Incubators with controlled CO ₂ content, at best in the range of 5%, have proven to be particularly favorable. After just a few days, growth began and after 9 to 14 days, the monolayers were formed, depending on the cell type. With a somewhat longer growth, multilayer coatings also formed under the optimized conditions.

microbial Cellulose is a carrier material for all types of cell cultures. Particularly suitable are cultures of epithelial cells Skin, Human Keratinocytes, HaCaT Cells, Human Osteoblasts, SAOS-2, human osteoblasts, osteoblasts from horse, chondrocytes from the horse and multipotent mesenchymal stem cells (MSC), e.g. from the horse.

The invention will be based on three embodiments of the use of Glucoacetobacter xylinum after DE 100 22 751 A1 formed cellulose as a carrier of cell cultures.

1st embodiment

There are prepared at right angles prepared, 1-1.5 mm thick cellulose layers with an area of about 150 × 75 mm and with a culture solution Ham's F 12 containing 10% FCS, 50 ug ascorbic acid / ml, 30 ug ketoglutaric / ml, 100 U Penicillin / ml and 100 μg streptomycin / ml. 4 10 ⁵ multipotent mesenchymal stem cells / cm ^{2 are} transferred to these cellulose carriers and then this coated cellulose carrier is incubated in the incubator at 90% moisture and 5% CO ₂ at 37 ° C. After 10 days, cellular monolayer layers are formed which evolve to bilayer layers as they grow further.

2nd embodiment

It are epidermal cells, taken from healthy horses, among the in Example 1 conditions until a stable multilayer epidermis cell layer on the cellulose carrier (skin structure) has formed. This skin structure is subsequently poorly healing Transfer wounds to the leg of a horse. The transferred layer grows quickly and covers the wound.

3rd embodiment

• • Zellzahl-Bestimmung nach 24 und 48
• • ATP-Bestimmung
• • NMP-41-Bestimmung
• • Morphologische Bestimmungen

Human keratinocytes, so-called HaCaT cells, are applied to carriers of bacterial cellulose and cultured as described in Example 1. These cells are grown to determine the biocompatibility of test substances. The cells thus obtained are excellent and very sensitive marker cells for determining the biocompatibility. Due to the high sensitivity of the cells cultivated in vitro, the influence of metabolic activities on the added test substances is determined on the basis of marker activities of the cells. Marker activities are for example

• • Cell number determination after 24 and 48
• • ATP determination
• • NMP-41 determination
• • Morphological determinations

By adapting the forms of the cellulose support to the conditions of the test, the Such biocompatibility studies are made more economical and time-effective.

All in the description and the following claims Features can both individually and in any combination with each other invention essential be.

Claims (6)

carrier for growing in vitro cell cultures consisting of microbial Cellulose. carrier according to claim 1 with grown in vitro cell cultures, characterized characterized in that cell cultures by multipotent mesenchymal stem cells are formed. carrier according to claim 1 with grown in vitro cell cultures, characterized characterized in that the cell cultures are formed by keratinocytes are. carrier according to claim 1 with grown in vitro cell cultures, characterized characterized in that the cell cultures are formed by epidermal cells are. carrier according to claim 1 with grown in vitro cell cultures, characterized characterized in that the cell cultures are formed by osteoblasts are. carrier according to claim 1 with grown in vitro cell cultures, characterized characterized in that the cell cultures are formed by chondrocytes are.