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锌离子对电压门控质子通道的抑制作用的分子机制

Molecular mechanism of Zn2+ inhibition of a voltage-gated proton channel.

作者信息

Qiu Feng, Chamberlin Adam, Watkins Briana M, Ionescu Alina, Perez Marta Elena, Barro-Soria Rene, González Carlos, Noskov Sergei Y, Larsson H Peter

机构信息

Department of Physiology and Biophysics, University of Miami, Miami, FL 33136.

Centre for Molecular Simulation, Department of Biological Sciences, University of Calgary, Calgary, AB, Canada T2N 2N4.

出版信息

Proc Natl Acad Sci U S A. 2016 Oct 4;113(40):E5962-E5971. doi: 10.1073/pnas.1604082113. Epub 2016 Sep 19.

Abstract

Voltage-gated proton (Hv1) channels are involved in many physiological processes, such as pH homeostasis and the innate immune response. Zn is an important physiological inhibitor of Hv1. Sperm cells are quiescent in the male reproductive system due to Zn inhibition of Hv1 channels, but become active once introduced into the low-Zn-concentration environment of the female reproductive tract. How Zn inhibits Hv1 is not completely understood. In this study, we use the voltage clamp fluorometry technique to identify the molecular mechanism of Zn inhibition of Hv1. We find that Zn binds to both the activated closed and resting closed states of the Hv1 channel, thereby inhibiting both voltage sensor motion and gate opening. Mutations of some Hv1 residues affect only Zn inhibition of the voltage sensor motion, whereas mutations of other residues also affect Zn inhibition of gate opening. These effects are similar in monomeric and dimeric Hv1 channels, suggesting that the Zn-binding sites are localized within each subunit of the dimeric Hv1. We propose that Zn binding has two major effects on Hv1: (i) at low concentrations, Zn binds to one site and prevents the opening conformational change of the pore of Hv1, thereby inhibiting proton conduction; and (ii) at high concentrations, Zn, in addition, binds to a second site and inhibits the outward movement of the voltage sensor of Hv1. Elucidating the molecular mechanism of how Zn inhibits Hv1 will further our understanding of Hv1 function and might provide valuable information for future drug development for Hv1 channels.

摘要

电压门控质子(Hv1)通道参与许多生理过程,如pH稳态和先天免疫反应。锌是Hv1的一种重要生理抑制剂。由于锌对Hv1通道的抑制作用,精子细胞在雄性生殖系统中处于静止状态,但一旦进入雌性生殖道的低锌浓度环境中就会变得活跃。锌如何抑制Hv1尚未完全了解。在本研究中,我们使用电压钳荧光测定技术来确定锌抑制Hv1的分子机制。我们发现锌与Hv1通道的激活关闭状态和静息关闭状态都结合,从而抑制电压感受器运动和门控开放。一些Hv1残基的突变仅影响锌对电压感受器运动的抑制,而其他残基的突变也影响锌对门控开放的抑制。这些效应在单体和二聚体Hv1通道中相似,表明锌结合位点位于二聚体Hv1的每个亚基内。我们提出锌结合对Hv1有两个主要影响:(i)在低浓度下,锌结合到一个位点并阻止Hv1孔的开放构象变化,从而抑制质子传导;(ii)在高浓度下,锌还结合到第二个位点并抑制Hv1电压感受器的向外运动。阐明锌抑制Hv1的分子机制将加深我们对Hv1功能的理解,并可能为未来开发针对Hv1通道的药物提供有价值的信息。

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