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在大鼠脑组织中差异表达的两种大电导钙激活钾通道变体的功能特性

Functional characteristics of two BKCa channel variants differentially expressed in rat brain tissues.

作者信息

Ha T S, Jeong S Y, Cho S W, Jeon H k, Roh G S, Choi W S, Park C S

机构信息

Department of Life Science, Kwangju Institute of Science and Technology, Korea.

出版信息

Eur J Biochem. 2000 Feb;267(3):910-8. doi: 10.1046/j.1432-1327.2000.01076.x.

Abstract

cDNAs encoding large-conductance Ca2+-activated K+ channel alpha-subunit (rSlo) were obtained from rat brain. From the DNA sequence of multiple rslo clones, we identified a specific sequence variation of 81 nucleotides, which is either absent from or present at the N-terminal region of a putative Ca2+-sensing domain of the channel. Transcripts containing such variations were detected in different ratios from several brain regions, and their functional significance was further examined. When heterologously expressed in Xenopus oocytes, both rSlo variants, named rSlo0 and rSlo27, generated Ca2+-activated and voltage-activated K+ currents characteristic of neuronal large-conductance Ca2+-activated K+ (BKCa) channels. Single-channel recordings of the two channels showed almost identical permeation characteristics and steady-state gating behavior. Noticeable differences between rSlo0 and rSlo27 were revealed when the macroscopic currents were measured at various voltages and intracellular Ca2+ concentrations. rSlo27 activated was more rapidly than rSlo0 in the presence of the same voltage stimulus, and the differences in these activation kinetics were dependent on the concentration of intracellular Ca2+. Despite their similar apparent affinities for Ca2+, rSlo0 and rSlo27 showed significant differences in their co-operative gating behavior. The Hill coefficient for intracellular Ca2+ was estimated to be about 3.7 for rSlo27 regardless of the membrane voltage, and that for rSlo0 was reduced from about 5 to 2 as the membrane voltage changed from 40 to 140 mV. As activation of BKCa channels is involved in rapid hyperpolarization of action potentials, the differential processing of rslo transcripts, and the generation of channels with different activation kinetics and Ca2+ cooperativity may be a mechanism for tuning the excitability of neurons in different brain regions.

摘要

编码大电导钙激活钾通道α亚基(rSlo)的互补DNA(cDNA)是从大鼠脑中获得的。通过多个rSlo克隆的DNA序列,我们鉴定出一个81个核苷酸的特定序列变异,该变异在通道假定的钙传感结构域的N端区域要么不存在,要么存在。在几个脑区以不同比例检测到含有此类变异的转录本,并进一步研究了它们的功能意义。当在非洲爪蟾卵母细胞中异源表达时,两种rSlo变体,即rSlo0和rSlo27,均产生神经元大电导钙激活钾(BKCa)通道特有的钙激活和电压激活钾电流。对这两种通道的单通道记录显示,它们的通透特性和稳态门控行为几乎相同。当在不同电压和细胞内钙浓度下测量宏观电流时,rSlo0和rSlo27之间出现了明显差异。在相同电压刺激下,rSlo27比rSlo0激活得更快,这些激活动力学的差异取决于细胞内钙的浓度。尽管rSlo0和rSlo27对钙的表观亲和力相似,但它们在协同门控行为上存在显著差异。无论膜电压如何,rSlo27对细胞内钙的希尔系数估计约为3.7,而当膜电压从40 mV变为140 mV时,rSlo0的希尔系数从约5降至2。由于BKCa通道的激活参与动作电位的快速超极化,rSlo转录本的差异加工以及具有不同激活动力学和钙协同性的通道的产生可能是调节不同脑区神经元兴奋性的一种机制。

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