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Generation of iPSCs as a Pooled Culture Using Magnetic Activated Cell Sorting of Newly Reprogrammed Cells

机译:使用新激活的细胞的磁激活细胞分选技术将iPSC作为汇集培养物生成

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摘要

Although significant advancement has been made in the induced pluripotent stem cell (iPSC) field, current methods for iPSC derivation are labor intensive and costly. These methods involve manual selection, expansion, and characterization of multiple clones for each reprogrammed cell sample and therefore significantly hampers the feasibility of studies where a large number of iPSCs need to be derived. To develop higher throughput iPSC reprogramming methods, we generated iPSCs as a pooled culture using rigorous cell surface pluripotent marker selection with TRA-1-60 or SSEA4 antibodies followed by Magnetic Activated Cell Sorting (MACS). We observed that pool-selected cells are similar or identical to clonally derived iPSC lines from the same donor by all criteria examined, including stable expression of endogenous pluripotency genes, normal karyotype, loss of exogenous reprogramming factors, and in vitro spontaneous and lineage directed differentiation potential. This strategy can be generalized for iPSC generation using both integrating and non-integrating reprogramming methods. Our studies provide an attractive alternative to clonal derivation of iPSCs using rigorously selected cell pools and is amenable to automation.
机译:尽管在诱导多能干细胞(iPSC)领域取得了显着进步,但目前用于iPSC衍生的方法是劳动密集型且昂贵的。这些方法涉及对每个重新编程的细胞样品进行多个克隆的手动选择,扩增和表征,因此大大阻碍了需要衍生大量iPSC的研究的可行性。为了开发更高通量的iPSC重编程方法,我们使用TRA-1-60或SSEA4抗体对细胞表面多能性标记进行严格选择,然后进行磁激活细胞分选(MACS),生成了iPSC作为合并培养物。我们观察到,通过所有检查的标准,池选择的细胞与来自同一供体的克隆衍生的iPSC系相似或相同,包括内源多能性基因的稳定表达,正常核型,外源重编程因子的丢失以及体外自发和谱系定向分化潜在。可以使用集成和非集成重编程方法将这种策略推广到iPSC生成。我们的研究为使用严格选择的细胞池的iPSC的克隆衍生提供了有吸引力的替代方法,并且适合自动化。

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