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通过一种基于单细胞的新型心肌细胞诱导方法对心脏祖细胞进行前瞻性鉴定。

Prospective identification of cardiac progenitors by a novel single cell-based cardiomyocyte induction.

作者信息

Yamashita Jun K, Takano Makoto, Hiraoka-Kanie Mina, Shimazu Chikashi, Peishi Yan, Yanagi Kentoku, Nakano Akiko, Inoue Emi, Kita Fumiyo, Nishikawa Shin-Ichi

机构信息

Laboratory of Stem Cell Differentiation, Stem Cell Research Center, Institute for Frontier Medical Sciences, Kyoto University, Kyoto, Japan.

出版信息

FASEB J. 2005 Sep;19(11):1534-6. doi: 10.1096/fj.04-3540fje. Epub 2005 Jul 20.

DOI:10.1096/fj.04-3540fje
PMID:16033809
Abstract

Dissection of cardiomyocyte differentiation process at the cellular level is indispensable in the research for cardiac development and regeneration. Previously, we have established an embryonic stem cell differentiation system that reproduces early vascular development from progenitor cells that express Flk1, a vascular endothelial growth factor receptor, by the combinatory application of 2-dimensional culture and flowcytometry. Here we show that cardiomyocytes can be successfully induced from a single Flk1+ cell on 2-dimensional culture, enabling the direct observation of differentiating cardiomyocytes and the prospective identification of cardiac progenitor potentials. Flk1+ cells could give rise to cardiomyocytes, as well as endothelial cells, from a single cell by the co-culture on OP9 stroma cells in a fusion-independent manner. Among the cell populations in intermediate stages from Flk1+ cells to cardiomyocytes, Flk1+/CXCR4+/vascular endothelial cadherin- cells were cardiac-specific progenitors at the single cell level. Noggin, a bone morphogenetic protein inhibitor, abolished cardiomyocyte differentiation by inhibiting the cardiac progenitor induction. However, wnt inhibitors Dkk-1 or Frizzled-8/Fc chimeric protein augmented, but wnt3a inhibited, cardiomyocyte differentiation. In vitro reproduction of cardiomyocyte differentiation process should be a potent tool for the cellular and molecular elucidation of cardiac development, which would provide various targets for cardiac regeneration.

摘要

在心脏发育和再生研究中,在细胞水平剖析心肌细胞分化过程是必不可少的。此前,我们建立了一个胚胎干细胞分化系统,通过二维培养和流式细胞术的联合应用,从表达血管内皮生长因子受体Flk1的祖细胞中重现早期血管发育。在此我们表明,在二维培养中可以从单个Flk1+细胞成功诱导出心肌细胞,从而能够直接观察分化中的心肌细胞,并前瞻性地鉴定心脏祖细胞潜能。通过在OP9基质细胞上非融合方式共培养,Flk1+细胞可以从单个细胞产生心肌细胞以及内皮细胞。在从Flk1+细胞到心肌细胞的中间阶段细胞群体中,Flk1+/CXCR4+/血管内皮钙黏蛋白阴性细胞在单细胞水平是心脏特异性祖细胞。骨形态发生蛋白抑制剂Noggin通过抑制心脏祖细胞诱导而消除心肌细胞分化。然而,Wnt抑制剂Dkk-1或卷曲蛋白8/Fc嵌合蛋白增强了心肌细胞分化,但Wnt3a抑制了心肌细胞分化。心肌细胞分化过程的体外重现应该是在细胞和分子水平阐明心脏发育的有力工具,这将为心脏再生提供各种靶点。

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