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无间充质培养中肺芽上皮分支形态发生的延时观察及其与肌动蛋白丝定位的关系。

Time-lapse observation of branching morphogenesis of the lung bud epithelium in mesenchyme-free culture and its relationship with the localization of actin filaments.

作者信息

Miura T, Shiota K

机构信息

Department of Anatomy and Developmental Biology, Kyoto University Graduate School of Medicine, Japan.

出版信息

Int J Dev Biol. 2000 Dec;44(8):899-902.

PMID:11206330
Abstract

It has been shown that branching morphogenesis of the lung bud is mediated by epithelial-mesenchymal interaction via such molecules as FGF10, BMP4 and Shh. However, a recent study showed that the isolated lung epithelium still undergoes branching morphogenesis in vitro even in the absence of mesenchyme (Nogawa and Ito, 1995). In the present study, we observed in vitro the dynamic movement of the isolated lung epithelium of the fetal mouse using time-lapse recording, and investigatedthe roles of actinfilaments in branching of the lung bud. First, time-lapse observation of the initial phase of lung branching morphogenesis revealed that at the sites of cleft formation, the epithelial surface was retracted inward from its original position. From this observation we assumed that there should be some structures which exert a physical force on the epithelium, and the localization and arrangement of actin fibers in the cultured lung epithelium were examined at various stages of branching morphogenesis. At the prebudding (6 h) and onset-budding (24 h) stages, no specific localization of actin filaments was observed in the lung bud epithelium, but at the postbudding stage (48 h) they were localized densely in the cells at the tip of the branched lung epithelium. The cell density was not different between the tip and cleft regions of the lung bud epithelium. When cultured with FGF-soaked beads, an actin-rich region was induced at the tip of the lung bud which was growing toward an FGF-soaked bead. These results indicate that actin fibers do not play a significant part in cleft formation but can be secondarily induced by FGF in the surrounding matrix and play some roles at later shaping of the branch in lung morphogenesis.

摘要

已经表明,肺芽的分支形态发生是由上皮-间充质相互作用通过诸如FGF10、BMP4和Shh等分子介导的。然而,最近的一项研究表明,即使在没有间充质的情况下,分离的肺上皮在体外仍会发生分支形态发生(Nogawa和Ito,1995)。在本研究中,我们使用延时记录在体外观察了胎鼠分离肺上皮的动态运动,并研究了肌动蛋白丝在肺芽分支中的作用。首先,对肺分支形态发生初始阶段的延时观察表明,在裂隙形成部位,上皮表面从其原始位置向内回缩。基于这一观察结果,我们推测应该存在一些对上皮施加物理力的结构,并在分支形态发生的各个阶段检查了培养的肺上皮中肌动蛋白纤维的定位和排列。在出芽前(6小时)和开始出芽(24小时)阶段,在肺芽上皮中未观察到肌动蛋白丝的特异性定位,但在出芽后阶段(48小时),它们密集地定位在分支肺上皮尖端的细胞中。肺芽上皮尖端和裂隙区域的细胞密度没有差异。当与浸泡有FGF的珠子一起培养时,在朝着浸泡有FGF的珠子生长的肺芽尖端诱导出一个富含肌动蛋白的区域。这些结果表明,肌动蛋白纤维在裂隙形成中不起重要作用,但可被周围基质中的FGF继发性诱导,并在肺形态发生后期的分支塑形中发挥一些作用。

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