Dual pattern of cholesterol-induced decoupling of residue-residue interactions of Kir2.2

IF 3 3区生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY

Journal of structural biology Pub Date : 2024-04-17 DOI:10.1016/j.jsb.2024.108091

Katie M. Beverley , Nicolas Barbera , Irena Levitan

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引用次数: 0

Abstract

Cholesterol is a negative regulator of a variety of ion channels. We have previously shown that cholesterol suppresses Kir2.2 channels via residue-residue uncoupling on the inter-subunit interfaces within the close state of the channels (3JYC). In this study, we extend this analysis to the other known structure of Kir2.2 that is closer to the open state of Kir2.2 channels (3SPI) and provide additional analysis of the residue distances between the uncoupled residues and cholesterol binding domains in the two conformation states of the channels. We found that the general phenomenon of cholesterol binding leading to uncoupling between specific residues is conserved in both channel states but the specific pattern of the uncoupling residues is distinct between the two states and implies different mechanisms. Specifically, we found that cholesterol binding in the 3SPI state results in an uncoupling of residues in three distinct regions; the transmembrane domain, membrane-cytosolic interface, and the cytosolic domain, with the first two regions forming an envelope around PI(4,5)P2 and cholesterol binding sites and the distal region overlapping with the subunit-subunit interface characterized in our previous study of the disengaged state. We also found that this uncoupling is dependent upon the number of cholesterol molecules bound to the channel. We further generated a mutant channel Kir2.2^P187V with a single point mutation in a residue proximal to the PI(4,5)P2 binding site, which is predicted to be uncoupled from other residues in its vicinity upon cholesterol binding and found that this mutation abrogates the sensitivity of Kir2.2 to cholesterol changes in the membrane. These findings suggest that cholesterol binding to this conformation state of Kir2.2 channels may destabilize the PI(4,5)P2 interactions with the channels while in the disengaged state the destabilization occurs where the subunits interact. These findings give insight into the structural mechanistic basis for the functional effects of cholesterol binding to the Kir2.2 channel.

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胆固醇诱导 Kir2.2 的残基-残基相互作用解耦的双重模式

胆固醇是多种离子通道的负调控因子。我们以前的研究表明，胆固醇通过通道关闭状态下亚基间界面上的残基-残基解偶联来抑制 Kir2.2 通道 (3JYC)。在本研究中，我们将这一分析扩展到更接近 Kir2.2 通道开放状态的另一种已知 Kir2.2 结构 (3SPI)，并对通道两种构象状态中未耦合残基与胆固醇结合域之间的残基距离进行了补充分析。我们发现，胆固醇结合导致特定残基之间解偶联的一般现象在两种通道状态下都是一致的，但两种状态下解偶联残基的特定模式是不同的，这意味着不同的机制。具体来说，我们发现在 3SPI 状态下，胆固醇结合会导致三个不同区域的残基解偶联：跨膜结构域、膜-细胞膜界面和细胞膜结构域，前两个区域围绕 PI(4,5)P2 和胆固醇结合位点形成一个包膜，远端区域则与我们之前对脱离状态的研究中所描述的亚基-亚基界面重叠。我们还发现，这种脱钩取决于与通道结合的胆固醇分子的数量。我们进一步生成了一个突变通道 Kir2.2P187V，它在 PI（4,5）P2 结合位点近端的一个残基上发生了单点突变，据预测，该位点在胆固醇结合时会与其附近的其他残基脱钩。这些发现表明，胆固醇结合到 Kir2.2 通道的这种构象状态可能会破坏 PI(4,5)P2 与通道的相互作用，而在脱离状态下，破坏稳定的作用发生在亚基相互作用的地方。这些发现使人们深入了解了胆固醇与 Kir2.2 通道结合产生功能效应的结构机理基础。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Journal of structural biology 生物-生化与分子生物学

CiteScore

6.30

自引率

3.30%

发文量

审稿时长

65 days

期刊介绍： Journal of Structural Biology (JSB) has an open access mirror journal, the Journal of Structural Biology: X (JSBX), sharing the same aims and scope, editorial team, submission system and rigorous peer review. Since both journals share the same editorial system, you may submit your manuscript via either journal homepage. You will be prompted during submission (and revision) to choose in which to publish your article. The editors and reviewers are not aware of the choice you made until the article has been published online. JSB and JSBX publish papers dealing with the structural analysis of living material at every level of organization by all methods that lead to an understanding of biological function in terms of molecular and supermolecular structure. Techniques covered include: • Light microscopy including confocal microscopy • All types of electron microscopy • X-ray diffraction • Nuclear magnetic resonance • Scanning force microscopy, scanning probe microscopy, and tunneling microscopy • Digital image processing • Computational insights into structure