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Individual dimers of the mitotic kinesin motor Eg5 step processively and support substantial loads in vitro

机译:有丝分裂驱动蛋白Eg5的单个二聚体逐步进行并在体外支持大量负荷

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摘要

Eg5, a member of the kinesin superfamily of microtubule-based motors, is essential for bipolar spindle assembly and maintenance during mitosis, yet little is known about the mechanisms by which it accomplishes these tasks. Here, we used an automated optical trapping apparatus in conjunction with a novel motility assay that employed chemically modified surfaces to probe the mechanochemistry of Eg5. Individual dimers, formed by a recombinant human construct Eg5–513–5His, stepped processively along microtubules in 8-nm increments, with short run lengths averaging approximately eight steps. By varying the applied load (with a force clamp) and the ATP concentration, we found that the velocity of Eg5 was slower and less sensitive to external load than that of conventional kinesin, possibly reflecting the distinct demands of spindle assembly as compared with vesicle transport. The Eg5–513–5His velocity data were described by a minimal, three-state model where a force-dependent transition follows nucleotide binding.
机译:Eg5是基于微管的电机驱动蛋白超家族的成员,对于有丝分裂期间的双极纺锤体组装和维护至关重要,但对其完成这些功能的机制知之甚少。在这里,我们使用了一种自动光学捕获设备,并结合了采用化学修饰表面探测Eg5力学化学的新型运动测定法。由重组人类构建体Eg5-513-5His形成的单个二聚体,以8 nm的增量沿微管进行性步进,平均短运行时间约为8步。通过改变施加的载荷(用力钳)和ATP浓度,我们发现Eg5的速度比常规驱动蛋白的速度更慢,对外部载荷的敏感性更低,这可能反映了与囊泡运输相比,纺锤体装配的独特需求。 Eg5-513-5His的速度数据由最小的三态模型描述,该模型中核苷酸结合后发生了力依赖性转变。

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