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鉴定 TRPA1 离子通道的体内二硫键构象。

Identification of in vivo disulfide conformation of TRPA1 ion channel.

机构信息

Department of Pharmacology, School of Medicine, Case Western Reserve University,Cleveland, Ohio 44106, USA.

出版信息

J Biol Chem. 2012 Feb 24;287(9):6169-76. doi: 10.1074/jbc.M111.329748. Epub 2011 Dec 29.

DOI:10.1074/jbc.M111.329748
PMID:22207754
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3307328/
Abstract

TRPA1 (transient receptor potential ankyrin 1) is an ion channel expressed in the termini of sensory neurons and is activated in response to a broad array of noxious exogenous and endogenous thiol-reactive compounds, making it a crucial player in chemical nociception. A number of conserved cysteine residues on the N-terminal domain of the channel have been identified as critical for sensing these electrophilic pungent chemicals, and our recent EM structure with modeled domains predicts that these cysteines form a ligand-binding pocket, allowing for the possibility of disulfide bonding between the cysteine residues. Here, we present a comprehensive mass spectrometry investigation of the in vivo disulfide bonding conformation and in vitro reactivity of 30 of the 31 cysteine residues in the TRPA1 ion channel. Four disulfide bonds were detected in the in vivo TRPA1 structure: Cys-666-Cys-622, Cys-666-Cys-463, Cys-622-Cys-609, and Cys-666-Cys-193. All of the cysteines detected were reactive to N-methylmaleimide (NMM) in vitro, with varying degrees of labeling efficiency. Comparison of the ratio of the labeling efficiency at 300 μM versus 2 mM NMM identified a number of cysteine residues that were outliers from the mean labeling ratio, suggesting that protein conformation changes rendered these cysteines either more or less protected from labeling at the higher NMM concentrations. These results indicate that the activation mechanism of TRPA1 may involve N-terminal conformation changes and disulfide bonding between critical cysteine residues.

摘要

TRPA1(瞬态受体电位锚蛋白 1)是一种在感觉神经元末端表达的离子通道,对广泛的有害外源性和内源性硫醇反应性化合物激活,使其成为化学伤害感受的关键参与者。通道的 N 端结构域中的一些保守半胱氨酸残基被鉴定为感知这些亲电子刺激性化学物质的关键,我们最近的带有建模结构域的 EM 结构预测这些半胱氨酸形成配体结合口袋,允许半胱氨酸残基之间形成二硫键。在这里,我们对 31 个 TRPA1 离子通道中的 30 个半胱氨酸残基的体内二硫键结合构象和体外反应性进行了全面的质谱研究。在体内 TRPA1 结构中检测到四个二硫键:Cys-666-Cys-622、Cys-666-Cys-463、Cys-622-Cys-609 和 Cys-666-Cys-193。所有检测到的半胱氨酸在体外均与 N-甲基马来酰亚胺(NMM)反应,具有不同程度的标记效率。比较 300 μM 和 2 mM NMM 的标记效率比,确定了一些半胱氨酸残基是平均标记比的离群值,表明蛋白质构象变化使这些半胱氨酸在较高的 NMM 浓度下更易或更不易被标记。这些结果表明,TRPA1 的激活机制可能涉及 N 端构象变化和关键半胱氨酸残基之间的二硫键形成。

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本文引用的文献

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Cytoplasmic ankyrin repeats of transient receptor potential A1 (TRPA1) dictate sensitivity to thermal and chemical stimuli.细胞质锚蛋白重复序列的瞬时受体电位 A1(TRPA1)决定了对热和化学刺激的敏感性。
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Molecular architecture and subunit organization of TRPA1 ion channel revealed by electron microscopy.电子显微镜揭示 TRPA1 离子通道的分子结构和亚基组织。
J Biol Chem. 2011 Nov 4;286(44):38168-38176. doi: 10.1074/jbc.M111.288993. Epub 2011 Sep 9.
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