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血小板衍生生长因子、转化生长因子-β和异型细胞间相互作用介导内皮细胞诱导的10T1/2细胞募集及其向平滑肌命运的分化。

PDGF, TGF-beta, and heterotypic cell-cell interactions mediate endothelial cell-induced recruitment of 10T1/2 cells and their differentiation to a smooth muscle fate.

作者信息

Hirschi K K, Rohovsky S A, D'Amore P A

机构信息

Harvard Medical School and Children's Hospital, Boston, Massachusetts 02115, USA.

出版信息

J Cell Biol. 1998 May 4;141(3):805-14. doi: 10.1083/jcb.141.3.805.

DOI:10.1083/jcb.141.3.805
PMID:9566978
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2132737/
Abstract

We aimed to determine if and how endothelial cells (EC) recruit precursors of smooth muscle cells and pericytes and induce their differentiation during vessel formation. Multipotent embryonic 10T1/2 cells were used as presumptive mural cell precursors. In an under-agarose coculture, EC induced migration of 10T1/2 cells via platelet-derived growth factor BB. 10T1/2 cells in coculture with EC changed from polygonal to spindle-shaped, reminiscent of smooth muscle cells in culture. Immunohistochemical and Western blot analyses were used to examine the expression of smooth muscle (SM)-specific markers in 10T1/2 cells cultured in the absence and presence of EC. SM-myosin, SM22alpha, and calponin proteins were undetectable in 10T1/2 cells cultured alone; however, expression of all three SM-specific proteins was significantly induced in 10T1/2 cells cocultured with EC. Treatment of 10T1/2 cells with TGF-beta induced phenotypic changes and changes in SM markers similar to those seen in the cocultures. Neutralization of TGF-beta in the cocultures blocked expression of the SM markers and the shape change. To assess the ability of 10T1/2 cells to contribute to the developing vessel wall in vivo, prelabeled 10T1/2 cells were grown in a collagen matrix and implanted subcutaneously into mice. The fluorescently marked cells became incorporated into the medial layer of developing vessels where they expressed SM markers. These in vitro and in vivo observations shed light on the cell-cell interactions that occur during vessel development, as well as in pathologies in which developmental processes are recapitulated.

摘要

我们旨在确定内皮细胞(EC)是否以及如何招募平滑肌细胞和周细胞的前体细胞,并在血管形成过程中诱导它们分化。多能胚胎10T1/2细胞被用作假定的壁细胞前体细胞。在琼脂糖下共培养中,EC通过血小板衍生生长因子BB诱导10T1/2细胞迁移。与EC共培养的10T1/2细胞从多边形变为纺锤形,类似于培养中的平滑肌细胞。免疫组织化学和蛋白质印迹分析用于检测在有无EC的情况下培养的10T1/2细胞中平滑肌(SM)特异性标志物的表达。单独培养的10T1/2细胞中检测不到SM肌球蛋白、SM22α和钙调蛋白;然而,与EC共培养的10T1/2细胞中所有三种SM特异性蛋白的表达均显著诱导。用转化生长因子-β(TGF-β)处理10T1/2细胞诱导了表型变化以及SM标志物的变化,类似于共培养中所见。在共培养中中和TGF-β可阻断SM标志物的表达和形状变化。为了评估10T1/2细胞在体内对发育中的血管壁的贡献能力,将预先标记的10T1/2细胞在胶原基质中培养并皮下植入小鼠体内。荧光标记的细胞整合到发育中血管的中层,在那里它们表达SM标志物。这些体外和体内观察结果揭示了血管发育过程中以及重现发育过程的病理情况下发生的细胞间相互作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cc16/2132737/d04cfa736417/JCB29456.f7.jpg
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