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通过驱动蛋白-1 马达的集体运作检测货物移动中的分数步。

Detection of fractional steps in cargo movement by the collective operation of kinesin-1 motors.

作者信息

Leduc Cécile, Ruhnow Felix, Howard Jonathon, Diez Stefan

机构信息

Max Planck Institute of Molecular Cell Biology and Genetics, Pfotenhauerstrasse 108, D-01307 Dresden, Germany.

出版信息

Proc Natl Acad Sci U S A. 2007 Jun 26;104(26):10847-52. doi: 10.1073/pnas.0701864104. Epub 2007 Jun 14.

Abstract

The stepping behavior of single kinesin-1 motor proteins has been studied in great detail. However, in cells, these motors often do not work alone but rather function in small groups when they transport cellular cargo. Until now, the cooperative interactions between motors in such groups were poorly understood. A fundamental question is whether two or more motors that move the same cargo step in synchrony, producing the same step size as a single motor, or whether the step size of the cargo movement varies. To answer this question, we performed in vitro gliding motility assays, where microtubules coated with quantum dots were driven over a glass surface by a known number of kinesin-1 motors. The motion of individual microtubules was then tracked with nanometer precision. In the case of transport by two kinesin-1 motors, we found successive 4-nm steps, corresponding to half the step size of a single motor. Dwell-time analysis did not reveal any coordination, in the sense of alternate stepping, between the motors. When three motors interacted in collective transport, we identified distinct forward and backward jumps on the order of 10 nm. The existence of the fractional steps as well as the distinct jumps illustrate a lack of synchronization and has implications for the analysis of motor-driven organelle movement investigated in vivo.

摘要

单个驱动蛋白-1 运动蛋白的步进行为已得到详细研究。然而,在细胞中,这些运动蛋白通常并非单独发挥作用,而是在运输细胞货物时以小群体的形式发挥功能。到目前为止,此类群体中运动蛋白之间的协同相互作用还鲜为人知。一个基本问题是,两个或更多运输同一货物的运动蛋白是否同步步进,产生与单个运动蛋白相同的步长,或者货物运动的步长是否会变化。为了回答这个问题,我们进行了体外滑动运动测定,即用已知数量的驱动蛋白-1 运动蛋白在玻璃表面驱动涂有量子点的微管。然后以纳米精度跟踪单个微管的运动。在由两个驱动蛋白-1 运动蛋白进行运输的情况下,我们发现了连续的 4 纳米步长,这相当于单个运动蛋白步长的一半。驻留时间分析并未揭示运动蛋白之间在交替步进意义上的任何协同作用。当三个运动蛋白在集体运输中相互作用时,我们识别出了约 10 纳米量级的明显向前和向后跳跃。分数步长以及明显跳跃的存在说明了缺乏同步性,并对体内研究的运动蛋白驱动的细胞器运动分析具有启示意义。

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