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鉴定 Thr29 为一个关键磷酸化位点,该位点可激活白细胞中的人质子通道 Hvcn1。

Identification of Thr29 as a critical phosphorylation site that activates the human proton channel Hvcn1 in leukocytes.

机构信息

Department of Molecular Biophysics and Physiology, Rush University Medical Center, Chicago, Illinois 60612, USA.

出版信息

J Biol Chem. 2010 Feb 19;285(8):5117-21. doi: 10.1074/jbc.C109.082727. Epub 2009 Dec 26.

Abstract

Voltage-gated proton channels and NADPH oxidase function cooperatively in phagocytes during the respiratory burst, when reactive oxygen species are produced to kill microbial invaders. Agents that activate NADPH oxidase also enhance proton channel gating profoundly, facilitating its roles in charge compensation and pH(i) regulation. The "enhanced gating mode" appears to reflect protein kinase C (PKC) phosphorylation. Here we examine two candidates for PKC-delta phosphorylation sites in the human voltage-gated proton channel, H(V)1 (Hvcn1), Thr(29) and Ser(97), both in the intracellular N terminus. Channel phosphorylation was reduced in single mutants S97A or T29A, and further in the double mutant T29A/S97A, by an in vitro kinase assay with PKC-delta. Enhanced gating was evaluated by expressing wild-type (WT) or mutant H(V)1 channels in LK35.2 cells, a B cell hybridoma. Stimulation by phorbol myristate acetate enhanced WT channel gating, and this effect was reversed by treatment with the PKC inhibitor GF109203X. The single mutant T29A or double mutant T29A/S97A failed to respond to phorbol myristate acetate or GF109203X. In contrast, the S97A mutant responded like cells transfected with WT H(V)1. We conclude that under these conditions, direct phosphorylation of the proton channel molecule at Thr(29) is primarily responsible for the enhancement of proton channel gating. This phosphorylation is crucial to activation of the proton conductance during the respiratory burst in phagocytes.

摘要

电压门控质子通道和 NADPH 氧化酶在吞噬细胞的呼吸爆发期间协同作用,此时会产生活性氧物质来杀死微生物入侵者。激活 NADPH 氧化酶的试剂也会深刻增强质子通道的门控作用,促进其在电荷补偿和 pH(i)调节中的作用。这种“增强的门控模式”似乎反映了蛋白激酶 C(PKC)的磷酸化。在这里,我们研究了人类电压门控质子通道 H(V)1(Hvcn1)中两个 PKC-δ磷酸化位点的候选物,即位于细胞内 N 端的 Thr(29)和 Ser(97)。体外激酶测定表明,在单个突变体 S97A 或 T29A 中,以及在双突变体 T29A/S97A 中,通道磷酸化减少。通过表达野生型(WT)或突变型 H(V)1 通道的 LK35.2 细胞(B 细胞杂交瘤)评估增强的门控。佛波醇 12,13-二丁酸酯(PMA)刺激增强了 WT 通道的门控,而 PKC 抑制剂 GF109203X 逆转了这种作用。单个突变体 T29A 或双突变体 T29A/S97A 对佛波醇 12,13-二丁酸酯或 GF109203X 没有反应。相比之下,S97A 突变体的反应类似于转染 WT H(V)1 的细胞。我们的结论是,在这些条件下,质子通道分子 Thr(29)的直接磷酸化主要负责增强质子通道的门控。这种磷酸化对于吞噬细胞呼吸爆发期间质子电导的激活至关重要。

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