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神经递质-钠同向转运体在脂质双分子层中的构象动力学

Conformational dynamics of a neurotransmitter:sodium symporter in a lipid bilayer.

作者信息

Adhikary Suraj, Deredge Daniel J, Nagarajan Anu, Forrest Lucy R, Wintrode Patrick L, Singh Satinder K

机构信息

Department of Cellular and Molecular Physiology, Yale University School of Medicine, New Haven, CT 06520.

Department of Pharmaceutical Sciences, University of Maryland School of Pharmacy, Baltimore, MD 21201.

出版信息

Proc Natl Acad Sci U S A. 2017 Mar 7;114(10):E1786-E1795. doi: 10.1073/pnas.1613293114. Epub 2017 Feb 21.

Abstract

Neurotransmitter:sodium symporters (NSSs) are integral membrane proteins responsible for the sodium-dependent reuptake of small-molecule neurotransmitters from the synaptic cleft. The symporters for the biogenic amines serotonin (SERT), dopamine (DAT), and norepinephrine (NET) are targets of multiple psychoactive agents, and their dysfunction has been implicated in numerous neuropsychiatric ailments. LeuT, a thermostable eubacterial NSS homolog, has been exploited as a model protein for NSS members to canvass the conformational mechanism of transport with a combination of X-ray crystallography, cysteine accessibility, and solution spectroscopy. Despite yielding remarkable insights, these studies have primarily been conducted with protein in the detergent-solubilized state rather than embedded in a membrane mimic. In addition, solution spectroscopy has required site-specific labeling of nonnative cysteines, a labor-intensive process occasionally resulting in diminished transport and/or binding activity. Here, we overcome these limitations by reconstituting unlabeled LeuT in phospholipid bilayer nanodiscs, subjecting them to hydrogen-deuterium exchange coupled with mass spectrometry (HDX-MS), and facilitating interpretation of the data with molecular dynamics simulations. The data point to changes of accessibility and dynamics of structural elements previously implicated in the transport mechanism, in particular transmembrane helices (TMs) 1a and 7 as well as extracellular loops (ELs) 2 and 4. The results therefore illuminate the value of this strategy for interrogating the conformational mechanism of the more clinically significant mammalian membrane proteins including SERT and DAT, neither of which tolerates complete removal of endogenous cysteines, and whose activity is heavily influenced by neighboring lipids.

摘要

神经递质

钠同向转运体(NSSs)是整合膜蛋白,负责从突触间隙中对小分子神经递质进行钠依赖性再摄取。生物胺5-羟色胺(SERT)、多巴胺(DAT)和去甲肾上腺素(NET)的同向转运体是多种精神活性药物的作用靶点,其功能障碍与众多神经精神疾病有关。LeuT是一种耐热的真细菌NSS同源物,已被用作NSS成员的模型蛋白,通过结合X射线晶体学、半胱氨酸可及性和溶液光谱学来探究转运的构象机制。尽管取得了显著的见解,但这些研究主要是在去污剂溶解状态下的蛋白质上进行的,而不是嵌入膜模拟物中。此外,溶液光谱学需要对非天然半胱氨酸进行位点特异性标记,这是一个劳动密集型过程,偶尔会导致转运和/或结合活性降低。在这里,我们通过在磷脂双层纳米盘中重组未标记的LeuT、使其进行氢-氘交换并结合质谱(HDX-MS)以及通过分子动力学模拟促进数据解释来克服这些限制。数据表明,先前与转运机制有关的结构元件的可及性和动力学发生了变化,特别是跨膜螺旋(TMs)1a和7以及细胞外环(ELs)2和4。因此,这些结果阐明了该策略对于探究更具临床意义的哺乳动物膜蛋白(包括SERT和DAT)的构象机制的价值,这两种蛋白都不能完全去除内源性半胱氨酸,并且其活性受到相邻脂质的严重影响。

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