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首页> 外文期刊>Journal of Structural Biology >High flexibility of the actomyosin crossbridge resides in skeletal muscle myosin subfragment-2 as demonstrated by a new single molecule assay
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High flexibility of the actomyosin crossbridge resides in skeletal muscle myosin subfragment-2 as demonstrated by a new single molecule assay

机译:一种新的单分子分析表明,肌动球蛋白横桥的高度灵活性存在于骨骼肌肌球蛋白亚片段2中

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Popular views of force generation in muscle indicate that a lever arm in the myosin head initiates displacement of the thin filament. However, this lever arm is attached to the thick filament backbone by a flexible combination of coiled coils and hinges in the myosin subfragment-2 (S2); therefore, efficient force generation depends on tension development in this linking structure. Herein, a single molecule assay is developed to examine the flexibility of the intact S2 relative to that of the myosin head. Fluorescently labeled myosin rod is polymerized onto a single myosin molecule that is bound to actin, and the resulting Brownian motion of the rod is analyzed at video rates by digital image processing. Complete rotations of the rod suggest significant amounts of random coil in the linking structure. The close similarity of twist rates for double-headed and single-headed myosin indicates that most of the flexibility originates at or beyond the first pitch of coiled coil in S2 and most likely at the hinge connecting S2 and the light meromyosin. The myosin head has a smaller but still detectable impact on this flexibility, since the addition of ADP to the rigor crossbridge produces differential effects on the torsional characteristics of double-headed versus single-headed myosin.
机译:在肌肉中产生力的流行观点表明,肌球蛋白头中的杠杆臂促使细丝移位。但是,该杠杆臂通过缠绕的线圈和肌球蛋白亚片段2(S2)中的铰链的灵活组合而连接到粗丝骨架上。因此,有效的力产生取决于该连接结构中张力的产生。本文中,开发了单分子测定法以检查完整S2相对于肌球蛋白头的柔性。将荧光标记的肌球蛋白棒聚合到与肌动蛋白结合的单个肌球蛋白分子上,然后通过数字图像处理以视频速率分析棒的所得布朗运动。杆的完整旋转表明链接结构中存在大量的随机线圈。双头和单头肌球蛋白的扭曲率非常相似,这表明大多数柔韧性源自或超过S2中盘绕线圈的第一个螺距,最有可能源自连接S2和轻质肌球蛋白的铰链。肌球蛋白头对此灵活性具有较小但仍可检测到的影响,因为在严格的跨桥中添加ADP会对双头肌球蛋白与单头肌球蛋白的扭转特性产生不同的影响。

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