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离子通过G蛋白激活的内向整流钾通道(GIRK1/GIRK5)的渗透。

Ion permeation through a G-protein activated (GIRK1/GIRK5) inwardly rectifying potassium channel.

作者信息

Luchian T, Schreibmayer W

机构信息

Department of Medical Physics and Biophysics, Graz, Austria.

出版信息

Biochim Biophys Acta. 1998 Jan 19;1368(2):167-70. doi: 10.1016/s0005-2736(97)00248-4.

Abstract

In order to further investigate a G-protein activated inwardly rectifying potassium channel subunit, GIRK1 was expressed in Xenopus oocytes (where it coassembles with the endogenous GIRK5). The mechanism underlying ion permeation and rectification were measured in isolated inside-out patches. Single channel current amplitudes under symmetrical K+ concentrations at different holding potentials were evaluated. Inward-rectification of K+-currents through open GIRK1/GIRK5 channels was removed by washing out polyamines and Mg2+ ions. We developed a simple 'two-sites-three-barrier' (2S3B) Eyring rate theory model of K+ ion permeation for GIRK1/GIRK5 channels. The resulting optimized parameter-set will be used as a working model for subsequent investigation regarding K+ permeation process through the GIRK1/GIRK5 channel.

摘要

为了进一步研究一种G蛋白激活的内向整流钾通道亚基,GIRK1在非洲爪蟾卵母细胞中表达(在那里它与内源性GIRK5共同组装)。在分离的内面向外膜片中测量离子渗透和整流的潜在机制。评估了在不同保持电位下对称K+浓度下的单通道电流幅度。通过洗去多胺和Mg2+离子消除了通过开放的GIRK1/GIRK5通道的K+电流的内向整流。我们开发了一个简单的GIRK1/GIRK5通道K+离子渗透的“两点三屏障”(2S3B)艾林速率理论模型。所得的优化参数集将用作后续关于K+通过GIRK1/GIRK5通道渗透过程研究的工作模型。

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