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Processive behaviour of kinesin observed using micro-fabricated cantilevers

机译:使用微型悬臂观察到的驱动蛋白的处理行为

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The mechanical characterization of biomolecular motors requires force sensors with sub-piconewton resolution. The coupling of a nanoscale motor to this type of microscale sensors introduces structural deformations in the motor according to the thermally activated degrees of freedom of the sensor. At present, no simple solution is available to reduce these effects. Here, we exploit the advantages of micro-fabricated cantilevers to produce a force sensor with essentially one degree of freedom and a spring constant of 0.03 pN nm-1 for the study of the molecular motor protein kinesin-1. During processive runs, the cantilever constrains the movement of the cargo binding domain of kinesin in a straight line, parallel to the microtubule track, and excludes specific reaction coordinates such as cargo rotation. In these conditions, we measured a step size of 8.0 ± 0.4 nm and a maximal unloaded velocity of 820 ± 80 nm s~(-1) at saturated adenosine triphosphate (ATP) concentration. We concluded that the motor does not need to rotate its tail as it moves through consecutive stepping cycles.
机译:生物分子马达的机械特性需要具有亚皮秒分辨率的力传感器。纳米级电动机与这种类型的微型传感器的耦合根据传感器的热激活自由度在电动机中引入结构变形。当前,没有简单的解决方案可用来减少这些影响。在这里,我们利用微细悬臂的优势来生产一种力传感器,该力传感器具有一个基本的自由度和0.03 pN nm-1的弹簧常数,用于研究分子运动蛋白kinesin-1。在连续运行过程中,悬臂限制了驱动蛋白的货物结合域在平行于微管轨道的直线上的运动,并排除了诸如货物旋转之类的特定反应坐标。在这些条件下,我们在饱和三磷酸腺苷(ATP)浓度下测量的步长为8.0±0.4 nm,最大空载速度为820±80 nm s〜(-1)。我们得出的结论是,电动机在连续的步进周期中移动时不需要旋转其尾部。

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