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A hybrid-membrane migration method to isolate high-purity adipose-derived stem cells from fat tissues

机译:从脂肪组织分离高纯度脂肪干细胞的杂交膜迁移方法

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摘要

Human adipose-derived stem cells (hADSCs) exhibit heterogeneous characteristics, indicating various genotypes and differentiation abilities. The isolated hADSCs can possess different purity levels and divergent properties depending on the purification methods used. We developed a hybrid-membrane migration method that purifies hADSCs from a fat tissue solution with extremely high purity and pluripotency. A primary fat-tissue solution was permeated through the porous membranes with a pore size from 8 to 25 μm, and the membranes were incubated in cell culture medium for 15-18 days. The hADSCs that migrated from the membranes contained an extremely high percentage (e.g., >98%) of cells positive for mesenchymal stem cell markers and showed almost one order of magnitude higher expression of some pluripotency genes (Oct4, Sox2, Klf4 and Nanog) compared with cells isolated using the conventional culture method.
机译:人脂肪来源的干细胞(hADSCs)表现出异质性,表明各种基因型和分化能力。分离的hADSCs可以具有不同的纯度水平和不同的性质,这取决于所使用的纯化方法。我们开发了一种杂交膜迁移方法,可从脂肪组织溶液中纯化hADSCs,具有极高的纯度和多能性。初生脂肪组织溶液渗透通过孔径为8至25μm的多孔膜,并将膜在细胞培养基中孵育15-18天。从膜迁移的hADSCs含有极高百分比(例如,> 98%)的间充质干细胞标记阳性细胞,并且与某些多能性基因(Oct4,Sox2,Klf4和Nanog)相比,其表达量高出近一个数量级。使用常规培养方法分离的细胞。

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