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Adhesion strength-based, label-free isolation of human pluripotent stem cells

机译:基于粘附力的无标记人多能干细胞分离

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We demonstrate substantial differences in 'adhesive signature' between human pluripotent stem cells (hPSCs), partially reprogrammed cells, somatic cells and hPSC-derived differentiated progeny. We exploited these differential adhesion strengths to rapidly (over ~10 min) and efficiently isolate fully reprogrammed induced hPSCs (hiPSCs) as intact colonies from heterogeneous reprogramming cultures and from differentiated progeny using microfluidics. hiPSCs were isolated label free, enriched to 95%-99% purity with >80% survival, and had normal transcriptional profiles, differentiation potential and karyotypes. We also applied this strategy to isolate hPSCs (hiPSCs and human embryonic stem cells) during routine culture and show that it may be extended to isolate hPSC-derived lineage-specific stem cells or differentiated cells.
机译:我们证明了人类多能干细胞(hPSCs),部分重编程的细胞,体细胞和hPSC衍生的分化后代之间的“粘附性特征”存在实质性差异。我们利用这些不同的粘附强度快速(约10分钟以上)并从异质重编程培养物和使用微流控技术从分化后代中有效分离出完整重编程的诱导hPSC(hiPSC)作为完整菌落。 hiPSCs不含标签,纯度提高到95%-99%,存活率> 80%,并具有正常的转录谱,分化潜能和核型。我们还应用此策略在常规培养过程中分离了hPSC(hiPSC和人类胚胎干细胞),并表明它可以扩展为分离hPSC衍生的谱系特异性干细胞或分化的细胞。

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