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钾离子通道CD环中亮氨酸与异亮氨酸残基诱导的动力学差异的结构基础。

Structural Basis for Differences in Dynamics Induced by Leu Versus Ile Residues in the CD Loop of Kir Channels.

作者信息

Lü Shouqin, An Hailong, Zhang Hailin, Long Mian

机构信息

Center of Biomechanics and Bioengineering, Institute of Mechanics, Chinese Academy of Sciences, Beijing, 100190, China.

Key Laboratory of Microgravity (National Microgravity Laboratory), Institute of Mechanics, Chinese Academy of Sciences, Beijing, 100190, China.

出版信息

Mol Neurobiol. 2016 Nov;53(9):5948-5961. doi: 10.1007/s12035-015-9466-x. Epub 2015 Oct 31.

Abstract

The effect of the conserved Leu/Ile site in the CD loop on the gating dynamics of Kir channels and corresponding micro-structural mechanism remains unclear. Molecular dynamics simulations were performed to investigate the structural mechanism of chicken Kir2.2. Compared to WT, the I223L mutant channel bound to PIP more strongly, was activated more rapidly, and maintained the activation state more stably after PIP dissociation. Cellular electrophysiology assays of mouse Kir2.1 and human Kir2.2 indicated that, consistent with simulations, the Leu residue increased the channel responses to PIP through increased binding affinity and faster activation kinetics, and the deactivation kinetics decreased upon PIP inhibition. The Ile residue induced the opposite responses. This difference was attributed to the distinct hydrophobic side chain symmetries of Leu and Ile; switching between these residues caused the interaction network to redistribute and offered effective conformation transduction in the Leu systems, which had more rigid and independent subunits.

摘要

CD环中保守的亮氨酸/异亮氨酸位点对Kir通道门控动力学的影响及其相应的微观结构机制尚不清楚。进行了分子动力学模拟以研究鸡Kir2.2的结构机制。与野生型相比,I223L突变通道与磷脂酰肌醇(PIP)结合更强,激活更快,且在PIP解离后更稳定地维持激活状态。对小鼠Kir2.1和人Kir2.2的细胞电生理分析表明,与模拟结果一致,亮氨酸残基通过增加结合亲和力和更快的激活动力学增强了通道对PIP的反应,并且在PIP抑制后失活动力学降低。异亮氨酸残基则引发相反的反应。这种差异归因于亮氨酸和异亮氨酸不同的疏水侧链对称性;这些残基之间的切换导致相互作用网络重新分布,并在具有更刚性和独立亚基的亮氨酸系统中提供有效的构象转导。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7f29/5085999/8d479a1384ad/12035_2015_9466_Fig1_HTML.jpg

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