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通过单分子膜片钳荧光显微镜探测短杆菌肽离子通道的构象变化。

Probing conformational changes of gramicidin ion channels by single-molecule patch-clamp fluorescence microscopy.

作者信息

Harms Greg S, Orr Galya, Montal Mauricio, Thrall Brian D, Colson Steve D, Lu H Peter

机构信息

Pacific Northwest National Laboratory, Fundamental Science Division, Richland, Washington 99352, USA.

出版信息

Biophys J. 2003 Sep;85(3):1826-38. doi: 10.1016/S0006-3495(03)74611-6.

Abstract

Complex conformational changes influence and regulate the dynamics of ion channels. Such conformational changes are stochastic and often inhomogeneous, which makes it extremely difficult, if not impossible, to characterize them by ensemble-averaged experiments or by single-channel recordings of the electric current that report the open-closed events but do not specifically probe the associated conformational changes. Here, we report our studies on ion channel conformational changes using a new approach, patch-clamp fluorescence microscopy, which simultaneously combines single-molecule fluorescence spectroscopy and single-channel current recordings to probe the open-closed transitions and the conformational dynamics of individual ion channels. We demonstrate patch-clamp fluorescence microscopy by measuring gramicidin ion channel conformational changes in a lipid bilayer formed at a patch-clamp micropipette tip under a buffer solution. By measuring single-pair fluorescence resonance energy transfer and fluorescence self-quenching from dye-labeled gramicidin channels, we observed that the efficiency of single-pair fluorescence resonance energy transfer and self-quenching is widely distributed, which reflects a broad distribution of conformations. Our results strongly suggest a hitherto undetectable correlation between the multiple conformational states of the gramicidin channel and its closed and open states in a lipid bilayer.

摘要

复杂的构象变化影响并调节离子通道的动力学。此类构象变化是随机的,且往往是不均匀的,这使得通过总体平均实验或通过报告开放-关闭事件但不专门探测相关构象变化的单通道电流记录来表征它们变得极其困难,甚至是不可能的。在此,我们报告了我们使用一种新方法——膜片钳荧光显微镜对离子通道构象变化的研究,该方法同时结合了单分子荧光光谱和单通道电流记录,以探测单个离子通道的开放-关闭转变和构象动力学。我们通过测量在缓冲溶液下膜片钳微吸管尖端形成的脂质双层中短杆菌肽离子通道的构象变化来展示膜片钳荧光显微镜。通过测量染料标记的短杆菌肽通道的单对荧光共振能量转移和荧光自猝灭,我们观察到单对荧光共振能量转移和自猝灭的效率分布广泛,这反映了构象的广泛分布。我们的结果有力地表明,在脂质双层中,短杆菌肽通道的多个构象状态与其关闭和开放状态之间存在迄今无法检测到的相关性。

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