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单体驱动蛋白-5 Cin8 马达的定向性由环 8、离子强度和微管结构调节。

Directionality of individual kinesin-5 Cin8 motors is modulated by loop 8, ionic strength and microtubule geometry.

机构信息

Department of Chemistry, Ben-Gurion University of the Negev, Beer-Sheva, Israel.

出版信息

EMBO J. 2011 Nov 18;30(24):4942-54. doi: 10.1038/emboj.2011.403.

Abstract

Kinesin-5 motors fulfil essential roles in mitotic spindle morphogenesis and dynamics as slow, processive microtubule (MT) plus-end directed motors. The Saccharomyces cerevisiae kinesin-5 Cin8 was found, surprisingly, to switch directionality. Here, we have examined directionality using single-molecule fluorescence motility assays and live-cell microscopy. On spindles, Cin8 motors mostly moved slowly (∼25 nm/s) towards the midzone, but occasionally also faster (∼55 nm/s) towards the spindle poles. In vitro, individual Cin8 motors could be switched by ionic conditions from rapid (380 nm/s) and processive minus-end to slow plus-end motion on single MTs. At high ionic strength, Cin8 motors rapidly alternated directionalities between antiparallel MTs, while driving steady plus-end relative sliding. Between parallel MTs, plus-end motion was only occasionally observed. Deletion of the uniquely large insert in loop 8 of Cin8 induced bias towards minus-end motility and affected the ionic strength-dependent directional switching of Cin8 in vitro. The deletion mutant cells exhibited reduced midzone-directed motility and efficiency to support spindle elongation, indicating the importance of directionality control for the anaphase function of Cin8.

摘要

驱动蛋白-5 马达在有丝分裂纺锤体形态发生和动力学中起着至关重要的作用,是一种缓慢、连续的微管(MT)正极导向马达。出人意料的是,我们发现酿酒酵母的驱动蛋白-5 Cin8 会改变其运动方向。在这里,我们使用单分子荧光运动分析和活细胞显微镜检查了其运动方向。在纺锤体上,Cin8 马达主要缓慢(约 25nm/s)向中部移动,但偶尔也会更快(约 55nm/s)向纺锤体两极移动。在体外,单个 Cin8 马达可以通过离子条件从快速(380nm/s)和连续的负端转换为在单根 MT 上缓慢的正端运动。在高离子强度下,Cin8 马达在平行 MT 之间快速交替定向,同时驱动稳定的正极相对滑动。在平行 MT 之间,偶尔观察到正极运动。删除 Cin8 环 8 中独特的大插入会导致偏向负端运动,并影响 Cin8 在体外对离子强度依赖性方向转换的影响。缺失突变体细胞表现出向中部定向运动的减少和支持纺锤体伸长的效率降低,这表明方向控制对 Cin8 的后期功能至关重要。

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