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棕榈酰化和应激轴调节插入(STREX)的膜结合控制蛋白激酶 C 对 BK 通道的调节。

Palmitoylation and membrane association of the stress axis regulated insert (STREX) controls BK channel regulation by protein kinase C.

机构信息

Division of Experimental Cardiology, Mannheim Medical Faculty, Heidelberg University, D-68167 Mannheim, Germany.

出版信息

J Biol Chem. 2012 Sep 14;287(38):32161-71. doi: 10.1074/jbc.M112.386359. Epub 2012 Jul 29.

Abstract

Large-conductance, calcium- and voltage-gated potassium (BK) channels play an important role in cellular excitability by controlling membrane potential and calcium influx. The stress axis regulated exon (STREX) at splice site 2 inverts BK channel regulation by protein kinase A (PKA) from stimulatory to inhibitory. Here we show that palmitoylation of STREX controls BK channel regulation also by protein kinase C (PKC). In contrast to the 50% decrease of maximal channel activity by PKC in the insertless (ZERO) splice variant, STREX channels were completely resistant to PKC. STREX channel mutants in which Ser(700), located between the two regulatory domains of K(+) conductance (RCK) immediately downstream of the STREX insert, was replaced by the phosphomimetic amino acid glutamate (S700E) showed a ∼50% decrease in maximal channel activity, whereas the S700A mutant retained its normal activity. BK channel inhibition by PKC, however, was effectively established when the palmitoylation-mediated membrane-anchor of the STREX insert was removed by either pharmacological inhibition of palmitoyl transferases or site-directed mutagenesis. These findings suggest that STREX confers a conformation on BK channels where PKC fails to phosphorylate and to inhibit channel activity. Importantly, PKA which inhibits channel activity by disassembling the STREX insert from the plasma membrane, allows PKC to further suppress the channel gating independent from voltage and calcium. Our results present an important example for the cross-talk between ion channel palmitoylation and phosphorylation in regulation of cellular excitability.

摘要

大电导、钙和电压门控钾 (BK) 通道通过控制膜电位和钙内流在细胞兴奋性中起重要作用。剪接位点 2 处的应激轴调节外显子 (STREX) 将蛋白激酶 A (PKA) 对 BK 通道的调节从刺激转变为抑制。本文表明,STREX 的棕榈酰化也通过蛋白激酶 C (PKC) 控制 BK 通道的调节。与插入缺失 (ZERO) 剪接变体中 PKC 使最大通道活性降低 50%形成对比,STREX 通道对 PKC 完全不敏感。位于 K(+)电导两个调节域 (RCK) 之间的 Ser(700)(紧邻 STREX 插入的下游)的 STREX 通道突变体中,将丝氨酸突变为磷酸模拟氨基酸谷氨酸 (S700E) 可使最大通道活性降低约 50%,而 S700A 突变体则保留其正常活性。然而,当通过药理学抑制棕榈酰转移酶或定点突变去除 STREX 插入的棕榈酰化介导的膜锚时,PKC 对 BK 通道的抑制作用得以有效建立。这些发现表明,STREX 赋予 BK 通道一种构象,使 PKC 无法磷酸化并抑制通道活性。重要的是,通过将 STREX 插入物从质膜上分离出来抑制通道活性的 PKA,使 PKC 能够进一步独立于电压和钙来抑制通道门控。我们的研究结果提供了一个重要的例子,说明了离子通道棕榈酰化和磷酸化在调节细胞兴奋性中的相互作用。

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