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Improving FRET-based monitoring of single chemomechanical rotary motors at work

机译:改进基于FRET的单一化学机械旋转电动机监控工作

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摘要

Protein dynamics are observable in real time using internal distance measurements of reference positions. Based on F?rster resonance energy transfer (FRET) as the distance ruler between two fluorescent markers, investigations of single molecules one at a time have modified our views of protein conformational changes. X-ray crystallography provides trapped conformations at atomic resolution and NMR can add information about flexible parts of proteins, but the pathways between these structures including unknown conformations are often not directly accessible. Especially for membrane enzymes comprising multiple subunits, limited structural information requires alternative experimental methods to follow conformational pathways. Herein we summarize the knowledge gathered from single-molecule FRET studies of the membrane-embedded rotary nanomotor F_oF_1-ATP synthase. In addition, new ideas and concepts to shift and extend the current limitations of the confocal FRET detection approach using freely diffusing, liposome-reconstituted, individual enzymes are discussed: nanodiamonds as new fluorophores, optimized laser excitation schemes, Hidden Markov Models for software-based FRET trajectory analysis, and application of the anti-Brownian electrokinetic trap (ABELtrap) to keep the single enzyme in focus.
机译:使用基准位置的内距离测量,实时观察蛋白质动力学。基于F?奔跑共振能量转移(FRET)作为两个荧光标记之间的距离尺寸,一次调查单个分子的调查修改了我们对蛋白质构象变化的看法。 X射线晶体术以原子分辨率提供捕获的构象,NMR可以添加有关蛋白质柔性部分的信息,但这些结构之间的途径通常不可直接访问。特别是对于包含多个亚基的膜酶,有限的结构信息需要替代的实验方法来遵循构象途径。在此,我们总结了从膜嵌入式旋转纳米运动F_OF_1-ATP合酶F_OF_1-ATP合酶的单分子FRET研究中收集的知识。此外,讨论了新的思路和概念,使用自由漫射,脂质体重构,脂质体重构,单个酶的当前局限性,脂质体重构,单独的酶:纳米金刚石作为新的荧光团,优化的激光激发方案,隐马尔可夫基于软件的Markov模型尺寸轨迹分析,抗褐色电动捕集器(abeltrap)在焦点中保持单一酶的应用。

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