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A novel method of encapsulating and cultivating adherent mammalian cells within collagen microcarriers

机译:在胶原微载体内封装和培养粘附哺乳动物细胞的新方法

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A novel method of preparing collagen micro-carriers was developed and used to entrap adherent cells for I cell culturing. This new technique involved seeding of cells in micro gel beads comprised of collagen fibrils dispersed in alginate. The gel beads were washed with phosphate buffered saline (PBS) to remove alginate and the resulting micro-spheres, about 300-500 mu m in diameter, contained evenly distributed collagen fibrils which provided a 3D biomimetic environment for cell growth. The applicability of this micro-encapsulating system was demonstrated by its ability to support the growth of C2C12 myoblast cells. When seeded and cultured within the 3D collagen microcarriers, the a population of C2C12 cells entrapped within the microcarriers increased by 1.5 folds in 7 days after inoculation. This encapsulation technique is potentially useful for culturing cells and especially useful for adherent cells that require a 3D fibrillar collagen environment.
机译:开发了一种制备胶原蛋白微载体的新方法,并将其用于捕获粘附细胞以进行I细胞培养。这项新技术涉及将细胞播种在微凝胶珠中,微珠由分散在藻酸盐中的胶原纤维组成。用磷酸盐缓冲盐水(PBS)洗涤凝胶珠以去除藻酸盐,并且所得的直径约300-500μm的微球包含均匀分布的胶原纤维,其为细胞生长提供了3D仿生环境。通过支持C2C12成肌细胞生长的能力证明了该微囊化系统的适用性。当在3D胶原蛋白微载体中播种和培养时,在接种后7天之内,被困在微载体中的C2C12细胞的数量增加了1.5倍。此封装技术可能对于培养细胞特别有用,尤其对于需要3D原纤维胶原蛋白环境的贴壁细胞有用。

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