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Kv1.2依赖于运输的磷酸化调节电压门控钾通道的细胞表面表达。

Trafficking-dependent phosphorylation of Kv1.2 regulates voltage-gated potassium channel cell surface expression.

作者信息

Yang Jae-Won, Vacher Helene, Park Kang-Sik, Clark Eliana, Trimmer James S

机构信息

Section of Neurobiology, Physiology, and Behavior, College of Biological Sciences, School of Medicine, University of California, Davis, CA 95616, USA.

出版信息

Proc Natl Acad Sci U S A. 2007 Dec 11;104(50):20055-60. doi: 10.1073/pnas.0708574104. Epub 2007 Dec 3.

Abstract

Kv1.2 alpha-subunits are components of low-threshold, rapidly activating voltage-gated potassium (Kv) channels in mammalian neurons. Expression and localization of Kv channels is regulated by trafficking signals encoded in their primary structure. Kv1.2 is unique in lacking strong trafficking signals and in exhibiting dramatic cell-specific differences in trafficking, which is suggestive of conditional trafficking signals. Here we show that a cluster of cytoplasmic C-terminal phosphorylation sites regulates Kv1.2 trafficking. Using tandem MS to analyze Kv1.2 purified from rat, human, and mouse brain, we identified in each sample in vivo phosphoserine (pS) phosphorylation sites at pS434, pS440, and pS441, as well as doubly phosphorylated pS440/pS441. We also found these sites, as well as pS449, on recombinant Kv1.2 expressed in heterologous cells. We found that phosphorylation at pS440/pS441 is present only on the post-endoplasmic reticulum (ER)/cell surface pool of Kv1.2 and is not detectable on newly synthesized and ER-localized Kv1.2, on which we did observe pS449 phosphorylation. Elimination of PS440/PS441 phosphorylation by mutation reduces cell-surface expression efficiency and functional expression of homomeric Kv1.2 channels. Interestingly, mutation of S449 reduces phosphorylation at pS440/pS441 and also decreases Kv1.2 cell-surface expression efficiency and functional expression. These mutations also suppress trafficking of Kv1.2/Kv1.4 heteromeric channels, suggesting that incorporation of Kv1.2 into heteromeric complexes confers conditional phosphorylation-dependent trafficking to diverse Kv channel complexes. These data support Kv1.2 phosphorylation at these clustered C-terminal sites as playing an important role in regulating trafficking of Kv1.2-containing Kv channels.

摘要

Kv1.2α亚基是哺乳动物神经元中低阈值、快速激活的电压门控钾(Kv)通道的组成部分。Kv通道的表达和定位受其一级结构中编码的转运信号调控。Kv1.2的独特之处在于缺乏强大的转运信号,且在转运过程中表现出显著的细胞特异性差异,这提示存在条件性转运信号。在此,我们表明细胞质C末端磷酸化位点簇调节Kv1.2的转运。利用串联质谱分析从大鼠、人类和小鼠大脑中纯化的Kv1.2,我们在每个样本中鉴定出体内丝氨酸磷酸化(pS)位点pS434、pS440和pS441,以及双磷酸化的pS440/pS441。我们还在异源细胞中表达的重组Kv1.2上发现了这些位点以及pS449。我们发现pS440/pS441处的磷酸化仅存在于Kv1.2的内质网(ER)后/细胞表面池,而在新合成的和ER定位的Kv1.2上无法检测到,我们在后者上观察到了pS449磷酸化。通过突变消除PS440/PS441磷酸化会降低同源Kv1.2通道的细胞表面表达效率和功能表达。有趣的是,S449突变会降低pS440/pS441处的磷酸化,也会降低Kv1.2细胞表面表达效率和功能表达。这些突变还抑制Kv1.2/Kv1.4异源通道的转运,表明将Kv1.2纳入异源复合物赋予了不同Kv通道复合物条件性磷酸化依赖性转运。这些数据支持Kv1.2在这些成簇的C末端位点的磷酸化在调节含Kv1.2的Kv通道的转运中起重要作用。

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