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Microscopy of single FoF1-ATP synthases The unraveling of motors, gears, and controls

机译:单个FoF1-ATP合酶的显微镜检查电机,齿轮和控件的分解

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摘要

Optical microscopy of single F1-ATPase and FoF1-ATP synthases started 15 years ago. Direct demonstration of ATP-driven subunit rotation by videomicroscopy became the new exciting tool to analyze the conformational changes of this enzyme during catalysis. Stimulated by these experiments, technical improvements for higher time resolution, better angular resolution, and reduced viscous drag were developed rapidly. Optics and single-molecule enzymology were entangled to benefit both biochemists and microscopists. Today, several single-molecule microscopy methods are established including controls for the precise nanomanipulation of individual enzymes in vitro. Forster resonance energy transfer, which has been used for simultaneous monitoring of conformational changes of different parts of this rotary motor, is one of them and may become the tool for the analysis of single FoF1-ATP synthases in membranes of living cells. Here, breakthrough experiments are critically reviewed and challenges are discussed for the future microscopy of single ATP synthesizing enzymes at work
机译:单个F1-ATPase和FoF1-ATP合酶的光学显微镜始于15年前。通过视频显微镜直接证明ATP驱动的亚基旋转成为分析该酶催化过程中构象变化的令人兴奋的新工具。通过这些实验,迅速开发出了更高的时间分辨率,更好的角度分辨率和减少的粘性阻力的技术改进。光学和单分子酶学纠缠在一起,有利于生物化学家和显微学家。如今,已建立了几种单分子显微镜方法,包括用于体外精确控制单个酶的对照。 Forster共振能量转移已被用于同时监测该旋转电机不同部分的构象变化,是其中之一,并且可能成为分析活细胞膜中单个FoF1-ATP合成酶的工具。在这里,对突破性的实验进行了严格的审查,并讨论了未来工作中单个ATP合成酶的显微技术面临的挑战

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