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人瘢痕组织中的皮肤源性干细胞:一种新型的分离和增殖技术及其向神经前体细胞分化的潜能。

Skin-derived stem cells in human scar tissues: a novel isolation and proliferation technique and their differentiation potential to neurogenic progenitor cells.

机构信息

Department of Bioscience and Biotechnology, Bio-Organ Research Center, Konkuk University, Seoul, Korea.

出版信息

Tissue Eng Part C Methods. 2010 Aug;16(4):619-29. doi: 10.1089/ten.TEC.2009.0275.

Abstract

Adult tissues contain stem cells that can transdifferentiate into other cell lineages besides forming differentiated cells of their own tissue of origin. However, human adult skin-derived stem cells have a very low efficiency. Here we established a novel culture system involving bone morphogenetic protein-4 and a floating culture system with sphere-producing medium that can enrich adult stem-cell populations in vitro. Adult stem cells were isolated from useless human scar tissue. Like mesenchymal stem cells, cultured human scar tissue-derived stem cells (hSTSCs) altered their morphology and significantly increased the number of Nestin-positive cells in proportion to the alkaline phosphatase-positive cell ratio. Moreover, the expression of the pluripotency regulator Oct-4 and its target transcripts, Sox-2, c-kit, and Rex-1, was also stimulated by this culture system. Differentiation of neurogenic progenitor cells using basic fibroblast growth factor and Neurogen 2 was successfully performed in vitro more rapidly than previous reports. Neuronal differentiation results showed that our hSTSCs expressed marker of neurogenic genes, such as glial fibrillary acid protein, neural cell adhesion molecules, neuron filament-M, and microtubule-associated protein 2. These results suggest that bone morphogenetic protein-4 and the floating culture system with sphere-producing medium induced significant proliferation of hSTSCs and mediated reprogramming of the cells from adult somatic tissue into precursor state to some degree. It is thought that this new culture system might be a simple, effective, and easily manageable process for regenerative tissue repair and autotransplantation.

摘要

成人组织中含有干细胞,除了形成自身组织来源的分化细胞外,还可以转分化为其他细胞谱系。然而,人类成年皮肤来源的干细胞的效率非常低。在这里,我们建立了一种新的培养体系,涉及骨形态发生蛋白-4 和一个带有球体产生培养基的悬浮培养体系,可在体外富集成年干细胞群体。成体干细胞从无用的人瘢痕组织中分离出来。与间充质干细胞一样,培养的人瘢痕组织来源的干细胞(hSTSCs)改变了它们的形态,并显著增加了巢蛋白阳性细胞的数量,与碱性磷酸酶阳性细胞的比例成正比。此外,多能性调节因子 Oct-4 及其靶转录物 Sox-2、c-kit 和 Rex-1 的表达也受到这种培养体系的刺激。使用碱性成纤维细胞生长因子和 Neurogen 2 体外更快速地成功进行了神经祖细胞的分化,比以前的报道更快。神经元分化结果表明,我们的 hSTSCs 表达神经基因的标志物,如神经胶质纤维酸性蛋白、神经细胞黏附分子、神经元丝-M 和微管相关蛋白 2。这些结果表明,骨形态发生蛋白-4 和带有球体产生培养基的悬浮培养体系诱导 hSTSCs 显著增殖,并在一定程度上介导了来自成体体细胞的细胞重编程为前体细胞状态。人们认为,这种新的培养系统可能是一种简单、有效和易于管理的组织修复和自体移植的过程。

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