Xie Lai-Hua, John Scott A, Weiss James N
Cardiovascular Research Laboratory, Department of Medicine, University of California at Los Angeles, School of Medicine, Los Angeles, CA 90095, USA.
J Gen Physiol. 2002 Jul;120(1):53-66. doi: 10.1085/jgp.20028576.
Inward rectification in strong inward rectifiers such as Kir2.1 is attributed to voltage-dependent block by intracellular polyamines and Mg(2+). Block by the polyamine spermine has a complex voltage dependence with shallow and steep components and complex concentration dependence. To understand the mechanism, we measured macroscopic Kir2.1 currents in excised inside-out giant patches from Xenopus oocytes expressing Kir2.1, and single channel currents in the inside-out patches from COS7 cells transfected with Kir2.1. We found that as spermine concentration or voltage increased, the shallow voltage-dependent component of spermine block at more negative voltages was caused by progressive reduction in the single channel current amplitude, without a decrease in open probability. We attributed this effect to spermine screening negative surface charges involving E224 and E299 near the inner vestibule of the channel, thereby reducing K ion permeation rate. This idea was further supported by experiments in which increasing ionic strength also decreased Kir2.1 single channel amplitude, and by mutagenesis experiments showing that this component of spermine block decreased when E224 and E299, but not D172, were neutralized. The steep voltage-dependent component of block at more depolarized voltages was attributed to spermine migrating deeper into the pore and causing fast open channel block. A quantitative model incorporating both features showed excellent agreement with the steady-state and kinetic data. In addition, this model accounts for previously described substate behavior induced by a variety of Kir2.1 channel blockers.
在诸如Kir2.1这类强内向整流器中,内向整流作用归因于细胞内多胺和Mg(2+)对电压依赖性的阻断。多胺精胺的阻断具有复杂的电压依赖性,包括浅部和陡部成分以及复杂的浓度依赖性。为了理解其机制,我们测量了表达Kir2.1的非洲爪蟾卵母细胞中切除的内向外膜片上的宏观Kir2.1电流,以及转染了Kir2.1的COS7细胞的内向外膜片上的单通道电流。我们发现,随着精胺浓度或电压的增加,在更负电压下精胺阻断的浅电压依赖性成分是由单通道电流幅度的逐渐降低引起的,而开放概率并未降低。我们将这种效应归因于精胺屏蔽了通道内前庭附近涉及E224和E299的负表面电荷,从而降低了钾离子的渗透速率。增加离子强度也会降低Kir2.1单通道幅度的实验以及诱变实验进一步支持了这一观点,诱变实验表明,当E224和E299而非D172被中和时,精胺阻断的这一成分会降低。在更正的电压下,阻断的陡电压依赖性成分归因于精胺向孔内更深部位迁移并导致快速的开放通道阻断。一个包含这两个特征的定量模型与稳态和动力学数据显示出极好的一致性。此外,该模型解释了先前描述的由多种Kir2.1通道阻滞剂诱导的亚状态行为。