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Mesenchymal stem cells as an appropriate feeder layer for prolonged in vitro culture of human induced pluripotent stem cells

机译:间充质干细胞作为适当的饲养层,可延长人诱导的多能干细胞的体外培养

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Feeder layers have been applied extensively to support the growth and stemness potential of stem cells for in vitro cultures. Mouse embryonic fibroblast and mouse fibroblast cell line (SNL) are common feeder cells for human induced pluripotent stem cells (hiPSCs) culture. Because of some problems in the use of these animal feeders and in order to simplify the therapeutic application of hiPSCs, we tested human adult bone marrow mesenchymal stem cells (hMSCs) as a potent feeder system. This method benefits from prevention of possible contamination of animal origin feeder systems. hiPSCs transferred onto mitotically inactivated hMSCs and passaged every 5 days. Prior to this culture, MSCs were characterized by flow cytometry of their surface markers andevaluation of their osteogenic and adipogenic differentiation potentials. The morphology, expressions of some specific pluripotency markers such as SSEA-3, NANOG and TRA-1-60, alkaline phosphates activity, formation embryoid bodies and their differentiation potentials of iPSCs on SNL and MSC feeder layers were evaluated. To investigate the prolonged maintenance of pluripotency, the quantitative transcriptions of some pluripotency markers including OCT4, SOX2, NANOG and REX1 were compared in the iPS clones on SNL or MSC feeders. Human iPSCs cultured on human MSCs feeder were slightly thinner and flatter than ones on the other feeder system. Interestingly MSCs supported the prolonged in vitro proliferation of hiPSCs along with maintenance of their pluripotency. Altogether our results suggest human mesenchymal stem cells as an appropriate feeder layer for human iPSCs culture for clinical applications and cell therapy.
机译:饲养层已广泛应用于支持干细胞在体外培养中的生长和干性潜力。小鼠胚胎成纤维细胞和小鼠成纤维细胞系(SNL)是人类诱导的多能干细胞(hiPSC)培养的常见饲养细胞。由于在使用这些动物饲养器时存在一些问题,并且为了简化hiPSC的治疗应用,我们测试了人类成人骨髓间充质干细胞(hMSCs)作为有效的饲养器系统。该方法得益于防止动物源进料系统可能受到的污染。 hiPSC转移到有丝分裂失活的hMSC上,每5天传代一次。在此培养之前,通过流式细胞术对其表面标志物进行表征,并评估其成骨和成脂分化潜能。评估了SSEA-3,NANOG和TRA-1-60等特定多能性标记物的形态,表达,碱性磷酸酶活性,形成胚状体及其在SNL和MSC饲养层上iPSC的分化潜能。为了研究多能性的长期维持,在SNL或MSC饲养器上的iPS克隆中比较了一些多能性标志物的定量转录,包括OCT4,SOX2,NANOG和REX1。在人类MSCs饲养者上培养的人类iPSC比其他饲养者系统上的人类iPSC稍薄和平坦。有趣的是,MSC支持hiPSC的长时间体外增殖以及维持其多能性。总的来说,我们的结果表明人间充质干细胞可以作为人iPSCs培养物的合适饲养层,用于临床应用和细胞治疗。

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