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Impact-Free Measurement of Microtubule Rotations on Kinesin and Cytoplasmic-Dynein Coated Surfaces

机译:驱动蛋白和胞质-动力蛋白涂层表面上微管旋转的无冲击测量。

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摘要

Knowledge about the three-dimensional stepping of motor proteins on the surface of microtubules (MTs) as well as the torsional components in their power strokes can be inferred from longitudinal MT rotations in gliding motility assays. In previous studies, optical detection of these rotations relied on the tracking of rather large optical probes present on the outer MT surface. However, these probes may act as obstacles for motor stepping and may prevent the unhindered rotation of the gliding MTs. To overcome these limitations, we devised a novel, impact-free method to detect MT rotations based on fluorescent speckles within the MT structure in combination with fluorescence-interference contrast microscopy. We (i) confirmed the rotational pitches of MTs gliding on surfaces coated by kinesin-1 and kinesin-8 motors, (ii) demonstrated the superiority of our method over previous approaches on kinesin-8 coated surfaces at low ATP concentration, and (iii) identified MT rotations driven by mammalian cytoplasmic dynein, indicating that during collective motion cytoplasmic dynein side-steps with a bias in one direction. Our novel method is easy to implement on any state-of-the-art fluorescence microscope and allows for high-throughput experiments.
机译:可以从滑行运动分析中的纵向MT旋转推断出有关微管(MT)上运动蛋白的三维步进以及其动力冲程中的扭转成分的知识。在先前的研究中,对这些旋转的光学检测依赖于对MT外表面上存在的相当大的光学探针的跟踪。但是,这些探针可能会成为电动机步进的障碍,并且可能会阻止滑动MT不受阻碍地旋转。为了克服这些限制,我们设计了一种新颖的,无冲击的方法,结合荧光干涉对比显微镜,根据MT结构内的荧光斑点检测MT旋转。我们(i)确认了MTs在由kinesin-1和kinesin-8电机涂覆的表面上滑动的旋转螺距,(ii)在低ATP浓度下证明了我们的方法优于先前在kinesin-8涂覆表面上的方法,以及(iii) )确定了由哺乳动物细胞质动力蛋白驱动的MT旋转,这表明在集体运动过程中,细胞质动力蛋白的回避在一个方向上偏向。我们的新方法很容易在任何最新型的荧光显微镜上实施,并允许进行高通量实验。

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