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大电导钙激活钾(BK)通道α亚基的一种新剪接变体改变人软骨细胞功能。

A New Splice Variant of Large Conductance Ca2+-activated K+ (BK) Channel α Subunit Alters Human Chondrocyte Function.

作者信息

Suzuki Yoshiaki, Ohya Susumu, Yamamura Hisao, Giles Wayne R, Imaizumi Yuji

机构信息

From the Department of Molecular and Cellular Pharmacology, Graduate School of Pharmaceutical Sciences, Nagoya City University, 3-1 Tanabedori, Mizuhoku, Nagoya 467-8603, Japan.

the Department of Pharmacology, Division of Pathological Sciences, Kyoto Pharmaceutical University, Kyoto 607-8414, Japan, and.

出版信息

J Biol Chem. 2016 Nov 11;291(46):24247-24260. doi: 10.1074/jbc.M116.743302. Epub 2016 Oct 7.

Abstract

Large conductance Ca-activated K (BK) channels play essential roles in both excitable and non-excitable cells. For example, in chondrocytes, agonist-induced Ca release from intracellular store activates BK channels, and this hyperpolarizes these cells, augments Ca entry, and forms a positive feed-back mechanism for Ca signaling and stimulation-secretion coupling. In the present study, functional roles of a newly identified splice variant in the BK channel α subunit (BKαΔe2) were examined in a human chondrocyte cell line, OUMS-27, and in a HEK293 expression system. Although BKαΔe2 lacks exon2, which codes the intracellular S0-S1 linker (Glu-127-Leu-180), significant expression was detected in several tissues from humans and mice. Molecular image analyses revealed that BKαΔe2 channels are not expressed on plasma membrane but can traffic to the plasma membrane after forming hetero-tetramer units with wild-type BKα (BKαWT). Single-channel current analyses demonstrated that BKα hetero-tetramers containing one, two, or three BKαΔe2 subunits are functional. These hetero-tetramers have a smaller single channel conductance and exhibit lower trafficking efficiency than BKαWT homo-tetramers in a stoichiometry-dependent manner. Site-directed mutagenesis of residues in exon2 identified Helix2 and the linker to S1 (Trp-158-Leu-180, particularly Arg-178) as an essential segment for channel function including voltage dependence and trafficking. BKαΔe2 knockdown in OUMS-27 chondrocytes increased BK current density and augmented the responsiveness to histamine assayed as cyclooxygenase-2 gene expression. These findings provide significant new evidence that BKαΔe2 can modulate cellular responses to physiological stimuli in human chondrocyte and contribute under pathophysiological conditions, such as osteoarthritis.

摘要

大电导钙激活钾(BK)通道在可兴奋细胞和非可兴奋细胞中均发挥着重要作用。例如,在软骨细胞中,激动剂诱导细胞内储存的钙释放,激活BK通道,这使这些细胞超极化,增加钙内流,并形成钙信号传导和刺激-分泌偶联的正反馈机制。在本研究中,我们在人软骨细胞系OUMS-27和HEK293表达系统中研究了BK通道α亚基中一个新鉴定的剪接变体(BKαΔe2)的功能作用。尽管BKαΔe2缺少编码细胞内S0-S1连接区(Glu-127-Leu-180)的外显子2,但在人和小鼠的多个组织中均检测到了显著表达。分子图像分析显示,BKαΔe2通道并不表达于质膜上,但在与野生型BKα(BKαWT)形成异源四聚体单元后可转运至质膜。单通道电流分析表明,含有一个、两个或三个BKαΔe2亚基的BKα异源四聚体具有功能。这些异源四聚体的单通道电导较小,且与BKαWT同源四聚体相比,以化学计量依赖的方式表现出较低的转运效率。对外显子2中残基进行定点诱变确定,螺旋2和与S1的连接区(Trp-158-Leu-180,尤其是Arg-178)是通道功能(包括电压依赖性和转运)的关键区段。在OUMS-27软骨细胞中敲低BKαΔe2可增加BK电流密度,并增强以环氧合酶-2基因表达测定的对组胺的反应性。这些发现提供了重要的新证据,表明BKαΔe2可调节人软骨细胞对生理刺激的细胞反应,并在骨关节炎等病理生理条件下起作用。

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