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细胞黏菌玫瑰集胞黏菌和食菌原柄菌变形虫的肌动球蛋白细胞骨架:结构、生化特性及功能

The actomyosin cytoskeleton of amoebae of the cellular slime molds acrasis rosea and protostelium mycophaga: structure, biochemical properties, and function.

作者信息

Hellsten M, Roos UP

机构信息

Institut fur Pflanzenbiologie, Universitat Zurich, Zollikerstrasse 107, Zurich, CH-8008, Switzerland.

出版信息

Fungal Genet Biol. 1998 Jun;24(1-2):123-45. doi: 10.1006/fgbi.1998.1048.

Abstract

In amoebae of the cellular slime molds (mycetozoans) Acrasis rosea and Protostelium mycophaga, bundles of F-actin radiate from the endoplasm-ectoplasm interface into the pseudopodia, where G-actin is also located. We conclude that these actin bundles form a core scaffold driving pseudopod extension which is subsequently completed by filling with a more loosely organized meshwork of F-actin. Some bipolar, elongate amoebae of A. rosea also contained long bundles of F-actin that traverse the cells lengthwise and remotely resemble stress fibers. Rodlets of F-actin were scattered in the body of amoebae of A. rosea or formed star-shaped or polygonal complexes near or around contractile vacuoles, where they may play a role in contraction. In total protein extracts analyzed by SDS-PAGE and immunoblots the actins migrated like the rabbit skeletal muscle control. The relative proportion of actin in total protein extracts was 7.9% for A. rosea and 34.5% for P. mycophaga. We detected four or five isoactins in extracts of both species and we determined that the genome of each species contains approximately six actin genes. Whether they are all expressed or if posttranslational modifications occur remains to be determined. Myosin II was enriched in actomyosin extracts; its Mr was 187.8 kDa for A. rosea and 220.7 kDa for P. mycophaga. Cell models ("ghosts") contracted upon the addition of ATP. We conclude that amoebae of A. rosea and P. mycophaga, although behaving differently from those of Dictyostelium discoideum, contain the basic repertoire of molecules that enable pseudopod extension by actin polymerization and ATP-induced contraction of the cell cortex. Copyright 1998 Academic Press.

摘要

在细胞黏菌(黏菌纲)玫红顶柱黏菌和食菌原柄菌的变形虫中,F-肌动蛋白束从内质-外质界面辐射到伪足中,G-肌动蛋白也位于伪足中。我们得出结论,这些肌动蛋白束形成了一个核心支架,驱动伪足延伸,随后通过填充更松散组织的F-肌动蛋白网络来完成延伸。一些玫红顶柱黏菌的双极、细长变形虫还含有纵向穿过细胞的长F-肌动蛋白束,与应力纤维有一定的相似性。F-肌动蛋白小杆分散在玫红顶柱黏菌变形虫体内,或在收缩泡附近或周围形成星形或多边形复合体,它们可能在收缩中发挥作用。通过SDS-PAGE和免疫印迹分析的总蛋白提取物中,肌动蛋白的迁移情况与兔骨骼肌对照相似。玫红顶柱黏菌总蛋白提取物中肌动蛋白的相对比例为7.9%,食菌原柄菌为34.5%。我们在两个物种的提取物中检测到四到五种肌动蛋白异构体,并确定每个物种的基因组包含大约六个肌动蛋白基因。它们是否全部表达或是否发生翻译后修饰还有待确定。肌球蛋白II在肌动球蛋白提取物中富集;玫红顶柱黏菌的分子量为187.8 kDa,食菌原柄菌为220.7 kDa。添加ATP后,细胞模型(“空壳”)发生收缩。我们得出结论,玫红顶柱黏菌和食菌原柄菌的变形虫虽然行为与盘基网柄菌的变形虫不同,但含有通过肌动蛋白聚合和ATP诱导的细胞皮层收缩来实现伪足延伸的基本分子组成。版权所有1998年学术出版社。

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