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Dissection of Kinesins Processivity

机译:剖析驱动蛋白的生产力

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摘要

The protein family of kinesins contains processive motor proteins that move stepwise along microtubules. This mechanism requires the precise coupling of the catalytic steps in the two heads, and their precise mechanical coordination. Here we show that these functionalities can be uncoupled in chimera of processive and non-processive kinesins. A chimera with the motor domain of Kinesin-1 and the dimerization domain of a non-processive Kinesin-3 motor behaves qualitatively as conventional kinesin and moves processively in TIRF and bead motility assays, suggesting that spatial proximity of two Kinein-1 motor domains is sufficient for processive behavior. In the reverse chimera, the non-processive motor domains are unable to step along microtubules, despite the presence of the Kinesin-1 neck coiled coil. Still, ATP-binding to one head of these chimera induces ADP-release from the partner head, a characteristic feature of alternating site catalysis. These results show that processive movement of kinesin dimers requires elements in the motor head that respond to ADP-release and induce stepping, in addition to a proper spacing of the motor heads via the neck coiled coil.
机译:驱动蛋白的蛋白质家族包含沿微管逐步移动的过程性运动蛋白。该机理需要两个头中催化步骤的精确耦合,以及它们的精确机械配合。在这里,我们显示这些功能可以在进行性和非进行性驱动蛋白的嵌合体中解偶联。具有Kinesin-1马达结构域和非进行性Kinesin-3马达二聚化域的嵌合体在质量上与常规kinesin相同,并且在TIRF和磁珠运动性试验中进行性移动,这表明两个Kinein-1马达域在空间上接近足以进行行为举止。在反向嵌合体中,尽管存在Kinesin-1颈绕线圈,但非持续性运动域仍无法沿着微管运动。仍然,与这些嵌合体的一个头部结合的ATP诱导从伴侣头部释放ADP,这是交替位点催化的特征。这些结果表明,驱动蛋白二聚体的进行性运动需要马达头中的元件响应ADP释放并引起步进,此外还需要通过颈部螺旋线圈适当地隔开马达头。

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