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G-肌动蛋白结构与动力学的核苷酸调控

Nucleotide regulation of the structure and dynamics of G-actin.

作者信息

Saunders Marissa G, Tempkin Jeremy, Weare Jonathan, Dinner Aaron R, Roux Benoît, Voth Gregory A

机构信息

Department of Chemistry, University of Chicago, Chicago, Illinois; Institute for Biophysical Dynamics, University of Chicago, Chicago, Illinois; James Franck Institute, University of Chicago, Chicago, Illinois; Computation Institute, University of Chicago, Chicago, Illinois.

James Franck Institute, University of Chicago, Chicago, Illinois; Department of Statistics, University of Chicago, Chicago, Illinois.

出版信息

Biophys J. 2014 Apr 15;106(8):1710-20. doi: 10.1016/j.bpj.2014.03.012.

Abstract

Actin, a highly conserved cytoskeletal protein found in all eukaryotic cells, facilitates cell motility and membrane remodeling via a directional polymerization cycle referred to as treadmilling. The nucleotide bound at the core of each actin subunit regulates this process. Although the biochemical kinetics of treadmilling has been well characterized, the atomistic details of how the nucleotide affects polymerization remain to be definitively determined. There is increasing evidence that the nucleotide regulation (and other characteristics) of actin cannot be fully described from the minimum energy structure, but rather depends on a dynamic equilibrium between conformations. In this work we explore the conformational mobility of the actin monomer (G-actin) in a coarse-grained subspace using umbrella sampling to bias all-atom molecular-dynamics simulations along the variables of interest. The results reveal that ADP-bound actin subunits are more conformationally mobile than ATP-bound subunits. We used a multiscale analysis method involving coarse-grained and atomistic representations of these simulations to characterize how the nucleotide affects the low-energy states of these systems. The interface between subdomains SD2-SD4, which is important for polymerization, is stabilized in an actin filament-like (F-actin) conformation in ATP-bound G-actin. Additionally, the nucleotide modulates the conformation of the SD1-SD3 interface, a region involved in the binding of several actin-binding proteins.

摘要

肌动蛋白是一种在所有真核细胞中都能找到的高度保守的细胞骨架蛋白,它通过一种被称为踏车行为的定向聚合循环促进细胞运动和膜重塑。结合在每个肌动蛋白亚基核心的核苷酸调节这一过程。尽管踏车行为的生化动力学已经得到了很好的表征,但核苷酸如何影响聚合的原子细节仍有待最终确定。越来越多的证据表明,肌动蛋白的核苷酸调节(以及其他特性)不能从最低能量结构中得到充分描述,而是取决于构象之间的动态平衡。在这项工作中,我们使用伞形抽样在粗粒度子空间中探索肌动蛋白单体(G-肌动蛋白)的构象流动性,以沿着感兴趣的变量对全原子分子动力学模拟施加偏置。结果表明,结合ADP的肌动蛋白亚基比结合ATP的亚基具有更高的构象流动性。我们使用了一种多尺度分析方法,该方法涉及这些模拟的粗粒度和原子表示,以表征核苷酸如何影响这些系统的低能态。对于聚合很重要的亚结构域SD2-SD4之间的界面,在结合ATP的G-肌动蛋白中以肌动蛋白丝样(F-肌动蛋白)构象稳定下来。此外,核苷酸调节SD1-SD3界面的构象,该区域参与几种肌动蛋白结合蛋白的结合。

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本文引用的文献

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The Theory of Ultra-Coarse-Graining. 1. General Principles.超粗粒化理论。1. 一般原理。
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