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A serum free approach towards the conservation of chondrogenic phenotype during in vitro cell expansion.

机译:在体外细胞扩增过程中采用无血清方法保护软骨形成表型。

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OBJECTIVE: Functionally viable chondrocytes in sufficient quantity is crucial for the success of matrix associated autologous chondrocyte implantation. This is difficult with conventional methods as chondrocytes dedifferentiate during 2D expansion with the loss of their chondrogenic phenotype. Moreover, established protocols are dependent on the use of serum which is not without its drawbacks. This study sought to address the issue by evaluating the feasibility of serum free, growth factors supplemented chondrocyte media with extracellular matrix (ECM) coatings. DESIGN: Passage 2 human chondrocytes were cultured in serum supplemented media or serum free media with collagen I or fibronectin coatings. Cell attachment and proliferation were assessed in these conditions. The cells were redifferentiated via pellet cultures for 7 and 14 days before being subjected to histological and gene expression analysis. RESULTS: The serum-free, growth factor cocktail supplemented with ECM coating improved long-term chondrocyte proliferation with enhanced basal Sox 9 expression. Upon induction, the redifferentiated chondrocytes expressed aggrecan and collagen II especially so for the cells plated on collagen coated surfaces. The chondrocytic phenotype was better conserved under the serum free conditions but the loss of the hyaline cartilage characteristics was not completely halted given the expression of collagen I. These essential cartilage markers were, however, reduced or absented for cells expanded with serum. Moreover, serum cultures displayed a higher tendency of undergoing hypertrophy given the stronger collagen X gene expression. CONCLUSION: The advocated technique promoted cell expansion with respect to conventional serum supplemented cultures while reducing the loss of the chondrogenic phenotype. This demonstrates the feasibility and potential of the novel concomitant use of serum free media and ECM coatings in the expansion of chondrocytes for cartilage regenerative applications.
机译:目的:足够数量的功能上可行的软骨细胞对于基质相关自体软骨细胞植入的成功至关重要。对于常规方法,这是困难的,因为软骨细胞在2D扩展过程中会去分化,并丧失其软骨形成表型。而且,已建立的方案取决于血清的使用,这并非没有缺点。这项研究试图通过评估无血清,生长因子补充有细胞外基质(ECM)涂层的软骨细胞培养基的可行性来解决这个问题。设计:在胶原蛋白或纤连蛋白涂层的血清补充培养基或不含血清的培养基中培养第2代人软骨细胞。在这些条件下评估细胞附着和增殖。通过沉淀培养将细胞再分化7天和14天,然后进行组织学和基因表达分析。结果:无血清,生长因子混合物加ECM涂层改善了长期软骨细胞增殖,增强了基础Sox 9的表达。诱导后,再分化的软骨细胞表达聚集蛋白聚糖和胶原蛋白II,尤其是对于铺在胶原蛋白涂层表面的细胞。在无血清条件下,软骨细胞表型的保守性更好,但是考虑到胶原蛋白I的表达,透明软骨特性的丧失并没有完全停止。但是,这些必需的软骨标志物对于用血清扩增的细胞会减少或缺失。而且,鉴于胶原蛋白X基因表达更强,血清培养物显示出发生肥大的更高趋势。结论:所提倡的技术相对于传统的血清补充培养物促进了细胞扩增,同时减少了软骨形成表型的丧失。这证明了无血清培养基和ECM涂层在伴随软骨再生应用的软骨细胞扩增中同时使用的可行性和潜力。

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