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冷冻电镜技术开启 TRP 通道结构生物学新纪元。

Dawning of a new era in TRP channel structural biology by cryo-electron microscopy.

机构信息

Department of Structural Biology, Institute of Biophysics and Physical Biochemistry, University of Regensburg, Universitätsstrasse 31, D-93053, Regensburg, Germany.

出版信息

Pflugers Arch. 2018 Feb;470(2):213-225. doi: 10.1007/s00424-018-2107-2. Epub 2018 Jan 17.

DOI:10.1007/s00424-018-2107-2
PMID:29344776
Abstract

Cryo-electron microscopy (cryo-EM) permits the determination of atomic protein structures by averaging large numbers of individual projection images recorded at cryogenic temperatures-a method termed single-particle analysis. The cryo-preservation traps proteins within a thin glass-like ice layer, making literally a freeze image of proteins in solution. Projections of randomly adopted orientations are merged to reconstruct a 3D density map. While atomic resolution for highly symmetric viruses was achieved already in 2009, the development of new sensitive and fast electron detectors has enabled cryo-EM for smaller and asymmetrical proteins including fragile membrane proteins. As one of the most important structural biology methods at present, cryo-EM was awarded in October 2017 with the Nobel Prize in Chemistry. The molecular understanding of Transient-Receptor-Potential (TRP) channels has been boosted tremendously by cryo-EM single-particle analysis. Several near-atomic and atomic structures gave important mechanistic insights, e.g., into ion permeation and selectivity, gating, as well as into the activation of this enigmatic and medically important membrane protein family by various chemical and physical stimuli. Lastly, these structures have set the starting point for the rational design of TRP channel-targeted therapeutics to counteract life-threatening channelopathies. Here, we attempt a brief introduction to the method, review the latest advances in cryo-EM structure determination of TRP channels, and discuss molecular insights into the channel function based on the wealth of TRP channel cryo-EM structures.

摘要

低温电子显微镜(cryo-EM)通过在低温下记录大量单个投影图像来平均化,从而确定蛋白质的原子结构 - 这种方法称为单颗粒分析。低温保存将蛋白质困在薄的玻璃状冰层中,实际上是溶液中蛋白质的冷冻图像。随机采用的取向的投影合并以重建三维密度图。虽然在 2009 年已经实现了高度对称病毒的原子分辨率,但新型灵敏快速电子探测器的发展使得 cryo-EM 适用于包括脆弱的膜蛋白在内的较小和不对称的蛋白质。作为目前最重要的结构生物学方法之一,cryo-EM 在 2017 年 10 月获得了诺贝尔化学奖。低温电子显微镜单颗粒分析极大地促进了瞬时受体电位(TRP)通道的分子理解。几个近原子和原子结构提供了重要的机械见解,例如,离子渗透和选择性,门控,以及各种化学和物理刺激对这种神秘和医学上重要的膜蛋白家族的激活。最后,这些结构为基于 TRP 通道靶向治疗的合理设计提供了起点,以对抗危及生命的通道病。在这里,我们尝试简要介绍该方法,回顾 TRP 通道 cryo-EM 结构测定的最新进展,并根据丰富的 TRP 通道 cryo-EM 结构讨论分子对通道功能的见解。

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