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膜嵌入的 Gloeobacter violaceus 配体门控离子通道 (GLIC) 中孔开放和脱敏的构象转变。

Conformational transitions underlying pore opening and desensitization in membrane-embedded Gloeobacter violaceus ligand-gated ion channel (GLIC).

机构信息

Department of Physiology and Biophysics, School of Medicine, Case Western Reserve University, Cleveland, Ohio 44106, USA.

出版信息

J Biol Chem. 2012 Oct 26;287(44):36864-72. doi: 10.1074/jbc.M112.401067. Epub 2012 Sep 13.

DOI:10.1074/jbc.M112.401067
PMID:22977232
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3481289/
Abstract

Direct structural insight into the mechanisms underlying activation and desensitization remain unavailable for the pentameric ligand-gated channel family. Here, we report the structural rearrangements underlying gating transitions in membrane-embedded GLIC, a prokaryotic homologue, using site-directed spin labeling and electron paramagnetic resonance (EPR) spectroscopy. We particularly probed the conformation of pore-lining second transmembrane segment (M2) under conditions that favor the closed and the ligand-bound desensitized states. The spin label mobility, intersubunit spin-spin proximity, and the solvent-accessibility parameters in the two states clearly delineate the underlying protein motions within M2. Our results show that during activation the extracellular hydrophobic region undergoes major changes involving an outward translational movement, away from the pore axis, leading to an increase in the pore diameter, whereas the lower end of M2 remains relatively immobile. Most notably, during desensitization, the intervening polar residues in the middle of M2 move closer to form a solvent-occluded barrier and thereby reveal the location of a distinct desensitization gate. In comparison with the crystal structure of GLIC, the structural dynamics of the channel in a membrane environment suggest a more loosely packed conformation with water-accessible intrasubunit vestibules penetrating from the extracellular end all the way to the middle of M2 in the closed state. These regions have been implicated to play a major role in alcohol and drug modulation. Overall, these findings represent a key step toward understanding the fundamentals of gating mechanisms in this class of channels.

摘要

直接的结构见解为基础的激活和脱敏的机制仍然不可用的五聚体配体门控通道家族。在这里,我们报告的结构重排在门控转变中膜嵌入 GLIC,一个原核同源物,使用定点自旋标记和电子顺磁共振(EPR)光谱。我们特别探测衬里的第二跨膜片段(M2)的构象在有利于封闭和配体结合脱敏状态的条件下。自旋标记的流动性,亚基间自旋-自旋接近性,和溶剂可及性参数在两种状态下清楚地描绘了 M2 内的潜在蛋白质运动。我们的结果表明,在激活过程中,细胞外的疏水区经历了重大变化,涉及到向外平移运动,远离孔轴,导致孔径增大,而 M2 的下端仍然相对不动。最值得注意的是,在脱敏过程中,M2 中间的中间极性残基移动得更近,形成一个溶剂封闭的屏障,从而揭示了一个独特的脱敏门的位置。与 GLIC 的晶体结构相比,通道在膜环境中的结构动力学表明,一种更松散的包装构象与水可及的亚基前庭从细胞外端一直穿透到 M2 的中间在封闭状态。这些区域被认为在酒精和药物调节中起主要作用。总的来说,这些发现代表了理解这一类通道门控机制基本原理的关键一步。

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