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来自……的液泡和高尔基体V-ATP酶的结构比较。 (原文中“from”后面缺少具体内容)

Structural comparison of the vacuolar and Golgi V-ATPases from .

作者信息

Vasanthakumar Thamiya, Bueler Stephanie A, Wu Di, Beilsten-Edmands Victoria, Robinson Carol V, Rubinstein John L

机构信息

Molecular Medicine Program, The Hospital for Sick Children, Toronto, ON M5G 0A4, Canada.

Department of Biochemistry, University of Toronto, Toronto, ON M5S 1A8, Canada.

出版信息

Proc Natl Acad Sci U S A. 2019 Apr 9;116(15):7272-7277. doi: 10.1073/pnas.1814818116. Epub 2019 Mar 25.

Abstract

Proton-translocating vacuolar-type ATPases (V-ATPases) are necessary for numerous processes in eukaryotic cells, including receptor-mediated endocytosis, protein maturation, and lysosomal acidification. In mammals, V-ATPase subunit isoforms are differentially targeted to various intracellular compartments or tissues, but how these subunit isoforms influence enzyme activity is not clear. In the yeast , isoform diversity is limited to two different versions of the proton-translocating subunit a: Vph1p, which is targeted to the vacuole, and Stv1p, which is targeted to the Golgi apparatus and endosomes. We show that purified V-ATPase complexes containing Vph1p have higher ATPase activity than complexes containing Stv1p and that the relative difference in activity depends on the presence of lipids. We also show that V complexes containing Stv1p could be readily purified without attached V regions. We used this effect to determine structures of the membrane-embedded V region with Stv1p at 3.1-Å resolution, which we compare with a structure of the V region with Vph1p that we determine to 3.2-Å resolution. These maps reveal differences in the surface charge near the cytoplasmic proton half-channel. Both maps also show the presence of bound lipids, as well as regularly spaced densities that may correspond to ergosterol or bound detergent, around the c-ring.

摘要

质子转运型液泡型ATP酶(V-ATP酶)对于真核细胞中的众多过程是必需的,包括受体介导的内吞作用、蛋白质成熟和溶酶体酸化。在哺乳动物中,V-ATP酶亚基异构体被差异性地靶向到各种细胞内区室或组织,但这些亚基异构体如何影响酶活性尚不清楚。在酵母中,异构体多样性仅限于质子转运亚基a的两种不同版本:靶向液泡的Vph1p和靶向高尔基体和内体的Stv1p。我们发现,含有Vph1p的纯化V-ATP酶复合物比含有Stv1p的复合物具有更高的ATP酶活性,并且活性的相对差异取决于脂质的存在。我们还发现,含有Stv1p的V复合物可以很容易地在没有附着V区域的情况下被纯化。我们利用这一效应以3.1埃的分辨率确定了含有Stv1p的膜嵌入V区域的结构,并将其与我们确定为3.2埃分辨率的含有Vph1p的V区域结构进行比较。这些图谱揭示了细胞质质子半通道附近表面电荷的差异。两张图谱还显示了c环周围存在结合的脂质以及可能对应于麦角固醇或结合去污剂的规则间隔密度。

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