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人鼻软骨细胞在大孔微载体上的扩增可增强再分化。

Expansion of human nasal chondrocytes on macroporous microcarriers enhances redifferentiation.

作者信息

Malda J, Kreijveld E, Temenoff J S, van Blitterswijk C A, Riesle J

机构信息

IsoTis NV, PO Box 98, 3720 AB, Bilthoven, The Netherlands.

出版信息

Biomaterials. 2003 Dec;24(28):5153-61. doi: 10.1016/s0142-9612(03)00428-9.

DOI:10.1016/s0142-9612(03)00428-9
PMID:14568432
Abstract

Articular cartilage has a limited capacity for self-repair. To overcome this problem, it is expected that functional cartilage replacements can be created from expanded chondrocytes seeded in biodegradable scaffolds. Expansion of chondrocytes in two-dimensional culture systems often results in dedifferentiation. This investigation focuses on the post-expansion phenotype of human nasal chondrocytes expanded on macroporous gelatin CultiSpher G microcarriers. Redifferentiation was evaluated in vitro via pellet cultures in three different culture media. Furthermore, the chondrogenic potential of expanded cells seeded in polyethylene glycol terephthalate/ polybuthylene terephthalate (PEGT/PBT) scaffolds, cultured for 14 days in vitro, and subsequently implanted subcutaneously in nude mice, was assessed. Chondrocytes remained viable during microcarrier culture and yielded doubling times (1.07+/-0.14 days) comparable to T-flask expansion (1.20+/-0.36 days). Safranin-O staining from pellet culture in different media demonstrated that production of GAG per cell was enhanced by microcarrier expansion. Chondrocyte-polymer constructs with cells expanded on microcarriers contained significantly more proteoglycans after subcutaneous implantation (288.5+/-29.2 microg) than those with T-flask-expanded cells (164.0+/-28.7 microg). Total collagen content was similar between the two groups. This study suggests that macroporous gelatin microcarriers are effective matrices for nasal chondrocyte expansion, while maintaining the ability of chondrocyte differentiation. Although the exact mechanism by which chondrocyte redifferentiation is induced through microcarrier expansion has not yet been elucidated, this technique shows promise for cartilage tissue engineering approaches.

摘要

关节软骨的自我修复能力有限。为克服这一问题,人们期望能利用接种于可生物降解支架上的扩增软骨细胞构建功能性软骨替代物。在二维培养系统中扩增软骨细胞常常会导致去分化。本研究聚焦于在大孔明胶CultiSpher G微载体上扩增的人鼻软骨细胞扩增后的表型。通过在三种不同培养基中进行微团培养在体外评估再分化情况。此外,还评估了接种于聚对苯二甲酸乙二醇酯/聚对苯二甲酸丁二醇酯(PEGT/PBT)支架上、体外培养14天、随后皮下植入裸鼠体内的扩增细胞的软骨形成潜力。软骨细胞在微载体培养过程中保持存活,其倍增时间(1.07±0.14天)与在T型瓶中扩增时(1.20±0.36天)相当。不同培养基中微团培养的番红O染色表明,微载体扩增可提高每细胞糖胺聚糖的产量。微载体上扩增的细胞构建的软骨细胞-聚合物复合物在皮下植入后所含蛋白聚糖(288.5±29.2微克)明显多于T型瓶扩增细胞构建的复合物(164.0±28.7微克)。两组之间的总胶原蛋白含量相似。本研究表明,大孔明胶微载体是鼻软骨细胞扩增的有效基质,同时能保持软骨细胞的分化能力。尽管通过微载体扩增诱导软骨细胞再分化的确切机制尚未阐明,但该技术在软骨组织工程方法中显示出了前景。

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