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肌球蛋白II和肌动蛋白早期募集到胞质分裂沟的不同途径。

Distinct pathways for the early recruitment of myosin II and actin to the cytokinetic furrow.

作者信息

Zhou Mian, Wang Yu-Li

机构信息

University of Massachusetts Medical School, Department of Physiology, Worcester, MA 01605, USA.

出版信息

Mol Biol Cell. 2008 Jan;19(1):318-26. doi: 10.1091/mbc.e07-08-0783. Epub 2007 Oct 24.

Abstract

Equatorial organization of myosin II and actin has been recognized as a universal event in cytokinesis of animal cells. Current models for the formation of equatorial cortex favor either directional cortical transport toward the equator or localized de novo assembly. However, this process has never been analyzed directly in dividing mammalian cells at a high resolution. Here we applied total internal reflection fluorescence microscope (TIRF-M), coupled with spatial temporal image correlation spectroscopy (STICS) and a new analytical approach termed temporal differential microscopy (TDM), to image the dynamics of myosin II and actin during the assembly of equatorial cortex. Our results indicated distinct and at least partially independent mechanisms for the early equatorial recruitment of myosin and actin filaments. Cortical myosin showed no detectable directional flow during early cytokinesis. In addition to equatorial assembly, we showed that localized inhibition of disassembly contributed to the formation of the equatorial myosin band. In contrast to myosin, actin filaments underwent a striking flux toward the equator. Myosin motor activity was required for the actin flux, but not for actin concentration in the furrow, suggesting that there was a flux-independent, de novo mechanism for actin recruitment along the equator. Our results indicate that cytokinesis involves signals that regulate both assembly and disassembly activities and argue against mechanisms that are coupled to global cortical movements.

摘要

肌球蛋白II和肌动蛋白的赤道组织已被认为是动物细胞胞质分裂中的普遍现象。目前关于赤道皮质形成的模型倾向于要么是向赤道的定向皮质运输,要么是局部从头组装。然而,这一过程从未在处于分裂期的哺乳动物细胞中以高分辨率直接进行分析。在这里,我们应用全内反射荧光显微镜(TIRF-M),结合空间时间图像相关光谱(STICS)和一种称为时间差分显微镜(TDM)的新分析方法,来成像赤道皮质组装过程中肌球蛋白II和肌动蛋白的动态变化。我们的结果表明,肌球蛋白和肌动蛋白丝在赤道早期募集过程中有不同且至少部分独立的机制。在早期胞质分裂过程中,皮质肌球蛋白未显示出可检测到的定向流动。除了赤道组装外,我们还表明,局部抑制解聚有助于赤道肌球蛋白带的形成。与肌球蛋白不同,肌动蛋白丝向赤道有显著的通量。肌动蛋白通量需要肌球蛋白运动活性,但沟内肌动蛋白浓度不需要,这表明沿赤道存在一种与通量无关的肌动蛋白募集的从头机制。我们的结果表明,胞质分裂涉及调节组装和解聚活动的信号,并反对与整体皮质运动相关的机制。

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