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VMA7编码酿酒酵母液泡H(+) -ATP酶复合体的一个新的14 kDa亚基。

VMA7 encodes a novel 14-kDa subunit of the Saccharomyces cerevisiae vacuolar H(+)-ATPase complex.

作者信息

Graham L A, Hill K J, Stevens T H

机构信息

Institute of Molecular Biology, University of Oregon, Eugene 97403.

出版信息

J Biol Chem. 1994 Oct 21;269(42):25974-7.

PMID:7929308
Abstract

The Saccharomyces cerevisiae vacuolar proton-translocating ATPase (V-ATPase) is composed of at least 10 subunits belonging to either the peripheral V1 or integral membrane V0 subcomplex. We have characterized a novel 14-kDa V-ATPase subunit (Vma7p), encoded by the VMA7 gene, which exhibits features common to both V1 and V0 subunit proteins. Vma7p is a hydrophilic protein of 118 amino acids with a predicted molecular mass of 13,452 Da. Vacuolar membranes isolated from a vma7 delta null mutant contained no V-ATPase activity. Western analysis of vma7 delta cells revealed greatly reduced levels of the remaining V0 complex V-ATPase subunits, but normal levels of the V1 subunits. However, the V1 subunits failed to associate with the vacuolar membrane. Unlike the integral membrane subunits of the V0 complex, Vma7p was easily stripped from vacuolar membranes. Density gradient fractionation revealed that Vma7p associated only with the fully assembled V-ATPase and did not associate with a separate lower density V0 subcomplex fraction. The unique properties of the Vma7p may reflect a critical role in stabilizing the V0 complex and bridging the V1 and V0 complexes to form a functional V-ATPase complex.

摘要

酿酒酵母液泡质子转运ATP酶(V-ATP酶)由至少10个亚基组成,这些亚基属于外周V1或整合膜V0亚复合体。我们鉴定了一种由VMA7基因编码的新型14 kDa V-ATP酶亚基(Vma7p),它具有V1和V0亚基蛋白共有的特征。Vma7p是一种由118个氨基酸组成的亲水蛋白,预测分子量为13452 Da。从vma7Δ缺失突变体中分离的液泡膜没有V-ATP酶活性。对vma7Δ细胞的蛋白质免疫印迹分析显示,剩余的V0复合体V-ATP酶亚基水平大幅降低,但V1亚基水平正常。然而,V1亚基未能与液泡膜结合。与V0复合体的整合膜亚基不同,Vma7p很容易从液泡膜上剥离。密度梯度分级分离显示,Vma7p仅与完全组装好的V-ATP酶结合,而不与单独的低密度V0亚复合体组分结合。Vma7p的独特性质可能反映了其在稳定V0复合体以及连接V1和V0复合体以形成功能性V-ATP酶复合体方面的关键作用。

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