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Probing nanosecond protein motions of calmodulin by single-molecule fluorescence anisotropy

机译:通过单分子荧光各向异性探测钙调蛋白的纳秒蛋白质运动

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We report a single-molecule fluorescence anisotropy study of calmodulin, a regulatory protein for calcium-dependent cell signaling. Calmodulin in this study contains a site-specifically inserted tetra-cysteine motif that reacted with FlAsH, a biarsenic fluorescein derivative that can be rotationally locked to the host protein. A photon time-stamping technique was employed that combined the capability for both subnanosecond time resolution of time-correlated single photon counting and single-molecule time trajectory recording. The study provided direct characterization of the nanosecond motions of calmodulin tethered to a biologically compatible surface under physiological buffer solution. The unique technical approaches are applicable to single-molecule study of protein conformational dynamics and protein-protein interactions at a wide range of time scales and without the signal convolution of probe-dye molecular motions. (C) 2004 American Institute of Physics.
机译:我们报告钙调蛋白,钙依赖细胞信号的调节蛋白的单分子荧光各向异性研究。这项研究中的钙调蛋白含有一个特定位点插入的四半胱氨酸基序,该基序与FlAsH反应,FlAsH是一种双砷荧光素衍生物,可以旋转锁定在宿主蛋白上。采用了一种光子时间戳技术,该技术结合了时间相关的单光子计数和单分子时间轨迹记录的亚纳秒时间分辨能力。该研究提供了在生理缓冲溶液中钙调蛋白束缚到生物相容性表面的纳秒运动的直接特征。独特的技术方法适用于在宽范围的时间范围内进行蛋白质构象动力学和蛋白质-蛋白质相互作用的单分子研究,而无需进行探针染料分子运动的信号卷积。 (C)2004美国物理研究所。

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