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Stoichiometry and turnover in single, functioning membrane protein complexes

机译:单一功能膜蛋白复合物的化学计量和周转率

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Many essential cellular processes are carried out by complex biological machines located in the cell membrane. The bacterial flagellar motor is a large membrane-spanning protein complex that functions as an ion-driven rotary motor to propel cells through liquid media(1-3). Within the motor, MotB is a component of the stator that couples ion flow to torque generation and anchors the stator to the cell wall(4,5). Here we have investigated the protein stoichiometry, dynamics and turnover of MotB with single-molecule precision in functioning bacterial flagellar motors in Escherichia coli. We monitored motor function by rotation of a tethered cell body(6), and simultaneously measured the number and dynamics of MotB molecules labelled with green fluorescent protein (GFP - MotB) in the motor by total internal reflection fluorescence microscopy. Counting fluorophores by the stepwise photobleaching of single GFP molecules showed that each motor contains similar to 22 copies of GFP - MotB, consistent with similar to 11 stators each containing two MotB molecules. We also observed a membrane pool of similar to 200 GFP - MotB molecules diffusing at similar to 0.008 mu m(2) s(-1). Fluorescence recovery after photobleaching and fluorescence loss in photobleaching showed turnover of GFP MotB between the membrane pool and motor with a rate constant of the order of 0.04 s(-1): the dwell time of a given stator in the motor is only similar to 0.5 min. This is the first direct measurement of the number and rapid turnover of protein subunits within a functioning molecular machine.
机译:许多基本的细胞过程是由位于细胞膜中的复杂生物机器完成的。细菌鞭毛马达是一种跨膜的大蛋白复合物,可作为离子驱动的旋转马达来推动细胞通过液体介质(1-3)。在电动机内部,MotB是定子的一个组件,该组件将离子流耦合到转矩产生并将定子锚定到单元壁上(4,5)。在这里,我们研究了功能化细菌鞭毛马达在大肠杆菌中的单分子精度的MotB的蛋白质化学计量,动力学和周转率。我们通过束缚的细胞体的旋转来监测运动功能(6),并通过全内反射荧光显微镜同时测量在运动中被绿色荧光蛋白(GFP-MotB)标记的MotB分子的数量和动力学。通过单个GFP分子的逐步光漂白对荧光团进行计数显示,每个电机包含接近22个拷贝的GFP-MotB,与类似于11个定子(每个定子包含两个MotB分子)一致。我们还观察到一个类似于200 GFP-MotB分子的膜池,其扩散速率接近0.008μm(2)s(-1)。光漂白后的荧光恢复和光漂白中的荧光损失表明,膜池和电机之间的GFP MotB的转换速率常数约为0.04 s(-1):给定定子在电机中的停留时间仅约为0.5分钟这是对功能分子机器内蛋白质亚基的数量和快速转换的首次直接测量。

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