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POSH刺激ROMK1通道的泛素化和网格蛋白非依赖性内吞作用。

POSH stimulates the ubiquitination and the clathrin-independent endocytosis of ROMK1 channels.

作者信息

Lin Dao-Hong, Yue Peng, Pan Chu-Yang, Sun Peng, Zhang Xin, Han Zeguang, Roos Marcel, Caplan Michael, Giebisch Gerhard, Wang Wen-Hui

机构信息

Department of Pharmacology, New York Medical College, Valhalla, New York 10595, USA.

出版信息

J Biol Chem. 2009 Oct 23;284(43):29614-24. doi: 10.1074/jbc.M109.041582. Epub 2009 Aug 26.

Abstract

POSH (plenty of SH3) is a scaffold protein that has been shown to act as an E3 ubiquitin ligase. Here we report that POSH stimulates the ubiquitination of Kir1.1 (ROMK) and enhances the internalization of this potassium channel. Immunostaining reveals the expression of POSH in the renal cortical collecting duct. Immunoprecipitation of renal tissue lysate with ROMK antibody and glutathione S-transferase pulldown experiments demonstrated the association between ROMK and POSH. Moreover, immunoprecipitation of lysates of HEK293T cells transfected with ROMK1 or with constructs encoding the ROMK-N terminus or ROMK1-C-Terminus demonstrated that POSH binds to ROMK1 on its N terminus. To study the effect of POSH on ROMK1 channels, we measured potassium currents with electrophysiological methods in HEK293T cells and in oocytes transfected or injected with ROMK1 and POSH. POSH decreased potassium currents, and the inhibitory effect of POSH on ROMK channels was dose-dependent. Biotinylation assay further showed that POSH decreased surface expression of ROMK channels in HEK293T cells transfected with ROMK1 and POSH. The effect of POSH on ROMK1 channels was specific because POSH did not inhibit sodium current in oocytes injected with ENaC-alpha, beta, and gamma subunits. Moreover, POSH still decreased the potassium current in oocytes injected with a ROMK1 mutant (R1Delta373-378), in which a clathrin-dependent tyrosine-based internalization signal residing between amino acid residues 373 and 378 is deleted. However, the inhibitory effect of POSH on ROMK channels was absent in cells expressing with dominant negative dynamin and POSHDeltaRING, in which the RING domain was deleted. Expression of POSH also increased the ubiquitination of ROMK1, whereas expression of POSHDeltaRING diminished its ubiquitination in HEK293T cells. The notion that POSH may serve as an E3 ubiquitin ligase is also supported by in vitro ubiquitination assays in which adding POSH increased the ROMK ubiquitination. We conclude that POSH inhibits ROMK channels by enhancing dynamin-dependent and clathrin-independent endocytosis and by stimulating ubiquitination of ROMK channels.

摘要

富含SH3结构域蛋白(POSH)是一种支架蛋白,已被证明可作为E3泛素连接酶发挥作用。在此我们报告,POSH刺激Kir1.1(ROMK)的泛素化,并增强该钾通道的内化。免疫染色显示POSH在肾皮质集合管中表达。用ROMK抗体对肾组织裂解物进行免疫沉淀以及谷胱甘肽S-转移酶下拉实验证明了ROMK与POSH之间的关联。此外,对转染了ROMK1或编码ROMK-N端或ROMK1-C端构建体的HEK293T细胞裂解物进行免疫沉淀表明,POSH在其N端与ROMK1结合。为了研究POSH对ROMK1通道的影响,我们在转染或注射了ROMK1和POSH的HEK293T细胞及卵母细胞中用电生理方法测量了钾电流。POSH降低了钾电流,且POSH对ROMK通道的抑制作用呈剂量依赖性。生物素化分析进一步表明,POSH降低了转染了ROMK1和POSH的HEK293T细胞中ROMK通道的表面表达。POSH对ROMK1通道的作用具有特异性,因为POSH不抑制注射了ENaC-α、β和γ亚基的卵母细胞中的钠电流。此外,POSH仍能降低注射了ROMK1突变体(R1Delta373 - 378)的卵母细胞中的钾电流,该突变体缺失了位于氨基酸残基373和378之间的基于酪氨酸的网格蛋白依赖性内化信号。然而,在表达显性负性发动蛋白和缺失RING结构域的POSHDeltaRING的细胞中,POSH对ROMK通道的抑制作用消失。在HEK293T细胞中,POSH的表达也增加了ROMK1的泛素化,而POSHDeltaRING的表达则减少了其泛素化。体外泛素化分析也支持POSH可能作为E3泛素连接酶的观点,在该分析中加入POSH会增加ROMK的泛素化。我们得出结论,POSH通过增强发动蛋白依赖性和网格蛋白非依赖性内吞作用以及刺激ROMK通道的泛素化来抑制ROMK通道。

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