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禽胚胎瓣膜祖细胞的分离与培养。

Isolation and culture of avian embryonic valvular progenitor cells.

作者信息

Mahler Gretchen, Gould Russell, Butcher Johnathan

机构信息

Department of Biomedical Engineering, Cornell University, USA.

出版信息

J Vis Exp. 2010 Oct 27(44):2159. doi: 10.3791/2159.

Abstract

Proper formation and function of embryonic heart valves is critical for developmental progression. The early embryonic heart is a U-shaped tube of endocardium surrounded by myocardium. The myocardium secretes cardiac jelly, a hyaluronan-rich gelatinous matrix, into the atrioventricular (AV) junction and outflow tract (OFT) lumen. At stage HH14 valvulogenesis begins when a subset of endocardial cells receive signals from the myocardium, undergo endocardial to mesenchymal transformation (EMT), and invade the cardiac jelly. At stage HH25 the valvular cushions are fully mesenchymalized, and it is this mesenchyme that eventually forms the valvular and septal apparatus of the heart. Understanding the mechanisms that initiate and modulate the process of EMT and cell differentiation are important because of their connection to serious congenital heart defects. In this study we present methods to isolate pre-EMT endocardial and post-EMT mesenchymal cells, which are the two different cell phenotypes of the prevalvular cushion. Pre-EMT endocardial cells can be cultured with or without the myocardium. Post-EMT AV cushion mesenchymal cells can be cultured inside mechanically constrained or stress-free collagen gels. These 3D in vitro models mimic key valvular morphogenic events and are useful for deconstructing the mechanisms of early and late stage valvulogenesis.

摘要

胚胎心脏瓣膜的正常形成和功能对于发育进程至关重要。早期胚胎心脏是一个由心肌包围的心内膜U形管。心肌向房室(AV)交界处和流出道(OFT)腔分泌心胶,一种富含透明质酸的凝胶状基质。在HH14阶段,瓣膜发生开始,此时一部分心内膜细胞接收来自心肌的信号,经历心内膜到间充质转化(EMT),并侵入心胶。在HH25阶段,瓣膜垫完全间充质化,正是这种间充质最终形成心脏的瓣膜和间隔装置。由于其与严重先天性心脏缺陷的关联,了解启动和调节EMT及细胞分化过程的机制很重要。在本研究中,我们展示了分离前EMT心内膜细胞和后EMT间充质细胞的方法,这是瓣膜前垫的两种不同细胞表型。前EMT心内膜细胞可以在有或没有心肌的情况下培养。后EMT房室垫间充质细胞可以在机械约束或无应力的胶原凝胶内培养。这些三维体外模型模拟关键的瓣膜形态发生事件,有助于解析早期和晚期瓣膜发生的机制。

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