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神经元中的V-ATP酶V0扇区亚基a1是钙调蛋白的作用靶点。

V-ATPase V0 sector subunit a1 in neurons is a target of calmodulin.

作者信息

Zhang Wei, Wang Dong, Volk Elzi, Bellen Hugo J, Hiesinger Peter Robin, Quiocho Florante A

机构信息

Verna and Marrs McLean Department of Biochemistry and Molecular Biology, Houston, Texas 77030.

Department of Physiology and Green Center Division for Systems Biology, University of Texas Southwestern Medical Center, Dallas, Texas 75390.

出版信息

J Biol Chem. 2008 Jan 4;283(1):294-300. doi: 10.1074/jbc.M708058200. Epub 2007 Oct 12.

Abstract

The V(0) complex forms the proteolipid pore of a vesicular ATPase that acidifies vesicles. In addition, an independent function in membrane fusion has been suggested in vacuolar fusion in yeast and synaptic vesicle exocytosis in fly neurons. Evidence for a direct role in secretion has also recently been presented in mouse and worm. The molecular mechanisms of how the V(0) components might act or are regulated are largely unknown. Here we report the identification and characterization of a calmodulin-binding site in the large cytosolic N-terminal region of the Drosophila protein V100, the neuron-specific V(0) subunit a1. V100 forms a tight complex with calmodulin in a Ca(2+)-dependent manner. Mutations in the calmodulin-binding site in Drosophila lead to a loss of calmodulin recruitment to synapses. Neuronal expression of a calmodulin-binding deficient V100 uncovers an incomplete rescue at low levels and cellular toxicity at high levels. Our results suggest a vesicular ATPase V(0)-dependent function of calmodulin at synapses.

摘要

V(0)复合物构成了使囊泡酸化的囊泡ATP酶的蛋白脂质孔。此外,在酵母的液泡融合和果蝇神经元的突触小泡胞吐作用中,有人提出它在膜融合中具有独立功能。最近在小鼠和蠕虫中也有证据表明它在分泌中起直接作用。V(0)组分如何发挥作用或受到调控的分子机制在很大程度上尚不清楚。在这里,我们报告了在果蝇蛋白V100(神经元特异性V(0)亚基a1)的大的胞质N端区域中钙调蛋白结合位点的鉴定和表征。V100以Ca(2+)依赖的方式与钙调蛋白形成紧密复合物。果蝇中钙调蛋白结合位点的突变导致钙调蛋白向突触募集的丧失。钙调蛋白结合缺陷型V100的神经元表达在低水平时显示不完全拯救,在高水平时显示细胞毒性。我们的结果表明钙调蛋白在突触处具有依赖于囊泡ATP酶V(

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