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与传统单层技术相比,在藻酸盐珠粒中培养软骨细胞用于组织工程可增强软骨细胞表型。

Expansion of chondrocytes for tissue engineering in alginate beads enhances chondrocytic phenotype compared to conventional monolayer techniques.

作者信息

Lee David A, Reisler Tom, Bader Dan L

机构信息

IRC in Biomedical Materials and Medical Engineering Division, Department of Engineering, Queen Mary, University of London, Mile End Road, London, E1 4NS, UK.

出版信息

Acta Orthop Scand. 2003 Feb;74(1):6-15. doi: 10.1080/00016470310013581.

DOI:10.1080/00016470310013581
PMID:12635786
Abstract

Chondrocytes are known to dedifferentiate when cultured in monolayer culture, which may compromise the efficacy of cartilage repair systems in which cells are expanded by repeat passage in monolayer prior to implantation. We tested the hypothesis that repeat passage in alginate beads can provide sufficient expansion of cells, while producing cells with enhanced chondrocytic phenotype. Bovine articular chondrocytes were seeded in 2% alginate beads or in monolayer. 4 passages at 7-day intervals were performed. Values of 9.1 days for monolayer expansion and 12.5 days for alginate expansion were estimated for a 10-fold increase in cell number. For assessment of chondrocytic and fibroblastic phenotype, expanded cells were seeded in alginate beads or on glass coverslips and cultured for 7 days. On subsequent seeding in alginate, cells which had previously been subcultured in alginate showed higher levels of both DNA and GAG synthesis than cells passaged in monolayer. Furthermore, the alginate-passaged cells retained a chondrocytic phenotype, indicated by synthesis of type II collagen and chondroitin-6-sulphate, while cells passaged inmonolayer synthesised type I collagen, indicating a fibroblastic phenotype. In conclusion, expansion of cells for autologous cartilage repair systems, using subculture within alginate beads, provides a potentially attractive alternative to monolayer expansion.

摘要

已知软骨细胞在单层培养时会发生去分化,这可能会损害软骨修复系统的功效,在该系统中,细胞在植入前通过在单层中反复传代进行扩增。我们测试了这样一个假设,即在藻酸盐珠中反复传代可以使细胞充分扩增,同时产生具有增强软骨细胞表型的细胞。将牛关节软骨细胞接种到2%的藻酸盐珠或单层培养物中。每隔7天进行4次传代。估计细胞数量增加10倍时,单层扩增的时间为9.1天,藻酸盐扩增的时间为12.5天。为了评估软骨细胞和成纤维细胞表型,将扩增后的细胞接种到藻酸盐珠或玻璃盖玻片上,并培养7天。随后接种到藻酸盐中时,先前在藻酸盐中传代培养的细胞比在单层中传代的细胞表现出更高水平的DNA和糖胺聚糖合成。此外,藻酸盐传代的细胞保留了软骨细胞表型,表现为合成II型胶原蛋白和硫酸软骨素-6-硫酸盐,而在单层中传代的细胞合成I型胶原蛋白,表明具有成纤维细胞表型。总之,利用藻酸盐珠中的传代培养来扩增用于自体软骨修复系统的细胞,为单层扩增提供了一种潜在有吸引力的替代方法。

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