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首页> 外文期刊>Differentiation: The Journal of the International Society of Differentiation >Rapid and efficient reprogramming of human amnion-derived cells into pluripotency by three factors OCT4/SOX2/NANOG.
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Rapid and efficient reprogramming of human amnion-derived cells into pluripotency by three factors OCT4/SOX2/NANOG.

机译:通过三种因素OCT4 / SOX2 / NANOG将人类羊膜来源的细胞快速有效地重编程为多能性。

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Reprogramming human somatic cells to pluripotency represents a valuable resource for research aiming at the development of in vitro models for human diseases and regenerative medicines to produce patient-specific induced pluripotent stem (iPS) cells. Seeking appropriate cell resources for higher efficiency and reducing the risk of viral transgene activation, especially oncogene activation, are of significance for iPS cell research. In this study, we tested whether human amnion-derived cells (hADCs) could be rapidly and efficiently reprogrammed into iPS cells by the defined factors: OCT4/SOX2/NANOG. hADCs from normal placenta were isolated and cultured. The 3rd passage cells were infected with the lentiviral vectors for the delivery of OCT4, SOX2, and NANOG. Afterwards, the generated iPSCs were identified by morphology, pluripotency markers, global gene expression profiles, and epigenetic status both in vitro and in vivo. The results showed that we were able to reprogram hADCs by the defined factors (OCT4/SOX2/NANOG). The efficiency was significantly high (about 0.1%), and the typical colonies appeared on the 9th day after infection. They were similar to human embryonic stem (ES) cells in morphology, proliferation, surface markers, gene expression, and the epigenetic status of pluripotent cell-specific genes. Furthermore, these cells were able to differentiate into various cell types of all three germ layers both in vitro and in vivo. These results demonstrate that hADCs were an ideal somatic cell resource for the rapid and efficient generation of iPS cells by OCT4/SOX2/NANOG.
机译:将人类体细胞重编程为多能性代表了一项有价值的研究资源,旨在开发人类疾病和再生药物的体外模型,以产生患者特异性的诱导性多能干(iPS)细胞。寻求合适的细胞资源以提高效率并降低病毒转基因激活(尤其是癌基因激活)的风险,对于iPS细胞研究具有重要意义。在这项研究中,我们测试了是否可以通过定义的因素OCT4 / SOX2 / NANOG将人羊膜来源的细胞(hADC)快速有效地重编程为iPS细胞。分离并培养了来自正常胎盘的hADC。用慢病毒载体感染第三代细胞,以递送OCT4,SOX2和NANOG。然后,通过形态学,多能性标志物,整体基因表达谱和表观遗传学状态在体外和体内鉴定出生成的iPSC。结果表明,我们能够通过定义的因子(OCT4 / SOX2 / NANOG)对hADC进行重新编程。效率非常高(约0.1%),典型的菌落在感染后第9天出现。它们在形态,增殖,表面标记,基因表达以及多能细胞特异性基因的表观遗传状态方面与人类胚胎干(ES)细胞相似。此外,这些细胞能够在体外和体内分化为所有三个胚层的各种细胞类型。这些结果表明,hADC是OCT4 / SOX2 / NANOG快速有效生成iPS细胞的理想体细胞资源。

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