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一种新的钾离子通道β亚基,可特异性增强Kv2.2(CDRK)的表达。

A new K+ channel beta subunit to specifically enhance Kv2.2 (CDRK) expression.

作者信息

Fink M, Duprat F, Lesage F, Heurteaux C, Romey G, Barhanin J, Lazdunski M

机构信息

Institut de Pharmacologie Moléculaire et Cellulaire, CNRS, 660, route des Lucioles, Sophia Antipolis 06560 Valbonne, France.

出版信息

J Biol Chem. 1996 Oct 18;271(42):26341-8. doi: 10.1074/jbc.271.42.26341.

DOI:10.1074/jbc.271.42.26341
PMID:8824288
Abstract

Cloned K+ channel beta subunits are hydrophilic proteins which associate to pore-forming alpha subunits of the Shaker subfamily. The resulting alphabeta heteromultimers K+ channels have inactivation kinetics significantly more rapid than those of the corresponding alpha homomultimers. This paper reports the cloning and the brain localization of mKvbeta4 (m for mouse), a new beta subunit. This new beta subunit is highly expressed in the nervous system but is also present in other tissues such as kidney. In contrast with other beta subunits, coexpression of the mKvbeta4 subunit with alpha subunits of Shaker-type K+ channel does not modify the kinetic properties or voltage-dependence of these channels in Xenopus oocytes. Instead, mKvbeta4 associates to Kv2.2 (CDRK), a Shab K+ channel, to specifically enhance (a factor of up to 6) its expression level without changing its elementary conductance or kinetics. It is without effect on another closely related Shab K+ channel Kv2.1 (DRK1). Chimeras between Kv2.1 and Kv2. 2 indicate that the COOH-terminal end of the Kv2.2 protein is essential for its mKvbeta4 sensitivity. The functional results associated with the observation of the co-localization of mKvbeta4 and Kv2.2 transcripts in most brain areas strongly suggest that both subunits interact in vivo to form a slowly-inactivating K+ channel. A chaperone-like effect of mKvbeta4 seems to permit the integration of a larger number of Kv2.2 channels at the plasma membrane.

摘要

克隆的钾离子通道β亚基是亲水性蛋白质,它们与Shaker亚家族的成孔α亚基相关联。由此产生的αβ异源多聚体钾离子通道的失活动力学比相应的α同源多聚体要快得多。本文报道了一种新的β亚基——mKvbeta4(m代表小鼠)的克隆及在脑内的定位。这种新的β亚基在神经系统中高度表达,但在其他组织如肾脏中也有存在。与其他β亚基不同,mKvbeta4亚基与Shaker型钾离子通道的α亚基共表达时,并不会改变非洲爪蟾卵母细胞中这些通道的动力学特性或电压依赖性。相反,mKvbeta4与一种Shab钾离子通道Kv2.2(CDRK)相关联,可特异性增强(高达6倍)其表达水平,而不改变其基本电导率或动力学。它对另一种密切相关的Shab钾离子通道Kv2.1(DRK1)没有影响。Kv2.1和Kv2.2之间的嵌合体表明,Kv2.2蛋白的COOH末端对于其对mKvbeta4的敏感性至关重要。与在大多数脑区观察到的mKvbeta4和Kv2.2转录本共定位相关的功能结果强烈表明,这两个亚基在体内相互作用形成一个缓慢失活的钾离子通道。mKvbeta4的伴侣样作用似乎允许在质膜上整合更多数量的Kv2.2通道。

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