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High-Speed Atomic Force Microscopy Visualization of the Dynamics of the Multienzyme Fatty Acid Synthase

机译:高速原子力显微镜显微镜可视化偏见脂肪酸合成酶的动态

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摘要

Multienzymes, such as the protein metazoan fatty acid synthase (FAS), are giant and highly dynamic molecular machines for critical biosynthetic processes. The molecular architecture of FAS was elucidated by static high-resolution crystallographic analysis, while electron microscopy revealed large-scale conformational variability in FAS with some correlation to functional states in catalysis. However, little is known about time scales of conformational dynamics, the trajectory of motions in individual FAS molecules, and the extent of coupling between catalysis and structural changes. Here, we present an experimental single-molecule approach to film immobilized or selectively tethered FAS in solution at different viewing angles and high spatiotemporal resolution using high-speed atomic force microscopy. Mobility of individual regions of the multienzyme is recognized in video sequences, and correlation of shape features implies a convergence of temporal resolution and velocity of FAS dynamics. Conformational variety can be identified and grouped by reference-free 2D class averaging, enabling the tracking of conformational transitions in movies. The approach presented here is suited for comprehensive studies of the dynamics of FAS and other multienzymes in aqueous solution at the single-molecule level.
机译:诸如蛋白质美观蛋白质脂肪酸合成酶(FAS)的偏酶是用于关键生物合成过程的巨大和高动态的分子机。通过静态高分辨率结晶分析阐明了Fas的分子结构,而电子显微镜揭示了Fas中的大规模构象变化,其与催化中的功能状态相关。然而,关于构象动态的时间尺度,对单个FAS分子中的运动的轨迹以及催化和结构变化之间的偶联程度几乎是知之甚少。在这里,我们在不同观察角度和使用高速原子力显微镜显微镜的不同观察角度和高时的时空分辨率呈现实验单分子方法以在溶液中薄膜固定或选择性地拴住的Fas。在视频序列中识别多酶各个区域的迁移率,形状特征的相关性意味着对Fas动态的时间分辨率和速度的收敛性。可以通过参考的2D类平均来识别和分组构象品种,从而能够跟踪电影中的构象转换。此处呈现的方法适用于单分子水平在水溶液中Fas和其他偏见的动态的综合研究。

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