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Extracellular Matrix Deposited by Synovium-Derived Stem Cells Delays Replicative Senescent Chondrocyte Dedifferentiation and Enhances Redifferentiation

机译:由滑动衍生的干细胞沉积的细胞外基质延迟复制衰老软骨细胞去消化剂增强了再分析

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摘要

The aim of this study was to assess the effect of extracellular matrix (ECM) deposited by synovium-derived stem cells (SDSCs) on articular chondrocyte expansion and maintenance of differentiation status and redifferentiation capacity. Passage 0 (P0) pig articular chondrocytes were expanded for six passages on plastic flasks (Plastic), SDSC-derived ECM (ECM), or substrate switching from either Plastic to ECM (PtoE) or ECM to Plastic (EtoP). Cell morphology, gene expression profiles, and immunophenotypes at each passage were used to characterize differentiation status of expanded cells. Chondrocytes at P0, P2, and P6 were assessed for redifferentiation capacity in a pellet culture system treated with either TGF-β1- or serum-containing medium for 14 days, using histology, immunohistochemistry, biochemistry, western blot, and real-time PCR. We found that ECM not only greatly enhanced chondrocyte expansion but also delayed dedifferentiation of expanded chondrocytes. Intriguingly, compared to a dramatic decrease in CD90+/CD105+ cells and CD90+ cells, CD105+ cells dramatically increased when chondrocytes were plated on Plastic; on the contrary, ECM expansion dramatically increased CD90+ cells and delayed the decrease of CD90+/CD105+ cells. Interestingly, expanded chondrocytes on ECM also acquired a strong redifferentiation capacity, particularly in the pellets treated with TGF-β1. In conclusion, the ratio of CD90 to CD105 may serve as a marker indicative of proliferation and redifferentiation capacity of dedifferentiated chondrocytes. ECM deposited by SDSCs provides a tissue-specific three-dimensional microenvironment for ex vivo expansion of articular chondrocytes while retaining redifferentiation capacity, suggesting that ECM may provide a novel approach for autologous chondrocyte - based cartilage repair.
机译:本研究的目的是评估乳房衍生的干细胞(SDSCS)沉积的细胞外基质(ECM)对关节软骨细胞的膨胀和维持分化状态和再分化能力的影响。通道0(P0)猪关节软骨细胞在塑料烧瓶(塑料),SDSC衍生的ECM(ECM)或从塑料转向ECM(PTOE)或ECM的底物切换到塑料(ETOP)。在每个通道的细胞形态,基因表达谱和免疫蛋白酶型用于表征扩增细胞的分化状态。在P0,P2和P6处的软骨细胞被评估用于用TGF-β1-或血清培养基处理的颗粒培养体系中的重新细胞能力14天,使用组织学,免疫组化,生物化学,蛋白质印迹和实时PCR。我们发现ECM不仅大大增强了软骨细胞扩张,而且延迟了扩张的软骨细胞的消化不异性。有趣的是,与CD90 + / CD105 +细胞和CD90 +细胞的显着降低相比,当软骨细胞镀在塑料上时,CD105 +细胞显着增加;相反,ECM膨胀显着增加了CD90 +细胞,并延迟了CD90 + / CD105 +细胞的降低。有趣的是,ECM的扩展软骨细胞还获得了强大的重新增收能力,特别是在用TGF-β1处理的颗粒中。总之,CD90至CD105的比例可以作为指示消化不良的软骨细胞的增殖和重新细胞能力的标志物。 SDSCS沉积的ECM为特定的三维微环境提供了关节软骨细胞的前体内的三维微环境,同时保持重新细胞能力,表明ECM可以为基于自体软骨细胞的软骨修复提供一种新的方法。

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