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胡萝卜液泡H⁺-ATPase 69-kDa亚基的cDNA序列。与F₀F₁-ATPases的β链的同源性。

The cDNA sequence of the 69-kDa subunit of the carrot vacuolar H+-ATPase. Homology to the beta-chain of F0F1-ATPases.

作者信息

Zimniak L, Dittrich P, Gogarten J P, Kibak H, Taiz L

机构信息

Biology Department, Thimann Laboratories, University of California, Santa Cruz 95064.

出版信息

J Biol Chem. 1988 Jul 5;263(19):9102-12.

PMID:2897965
Abstract

Vacuolar ATPases constitute a novel class of N-ethylmaleimide- and nitrate-sensitive proton pumps associated with the endomembrane system of eukaryotic cells. They resemble F0F1-ATPases in that they are large multimeric proteins, 400-500 kDa, composed of three to nine different subunits. Previous studies have indicated that the active site is located on the approximately 70-kDa subunit. Using antibodies to the approximately 70-kDa subunit of corn to screen a carrot root lambda gt11 cDNA library, we have isolated cDNA clones of the carrot 69-kDa subunit. The complete primary structure of the 69-kDa subunit was then determined from the nucleotide sequence of its cDNA. The 69-kDa subunit consists of 623 amino acids (Mr 68,835), with no obvious membrane-spanning regions. The carrot cDNA sequence was over 70% homologous with exons of a Neurospora 69-kDa genomic clone. The protein sequence of the carrot 69-kDa subunit also exhibited 34.3% identity to four representative F0F1-ATPase beta-chains over a 275-amino-acid core stretch of similar sequence. Alignment studies revealed several regions which were highly homologous to beta-chains, including sequences previously implicated in catalytic function. This provides definitive evidence that the vacuolar ATPase is closely related to the F0F1-type ATPases. A major functional difference between the 69-kDa and beta-subunits is the location of 3 critical cysteine residues: two in the putative catalytic region (Cys-248 and Cys-256) and one in the proposed Mg2+-binding site (Cys-279). These cysteines (and two others) probably account for the sensitivity of the vacuolar H+-ATPase to the sulfhydryl reagent, N-ethylmaleimide. It is proposed that the two ATPases may have arisen from a common ancestor by the insertion or deletion of a large stretch of nonhomologous sequence near the amino-terminal end of the subunit.

摘要

液泡ATP酶构成了一类新型的对N - 乙基马来酰亚胺和硝酸盐敏感的质子泵,与真核细胞的内膜系统相关。它们类似于F0F1 - ATP酶,因为它们是大型多聚体蛋白,分子量为400 - 500 kDa,由三到九个不同的亚基组成。先前的研究表明,活性位点位于大约70 kDa的亚基上。利用针对玉米大约70 kDa亚基的抗体筛选胡萝卜根λgt11 cDNA文库,我们分离出了胡萝卜69 kDa亚基的cDNA克隆。然后根据其cDNA的核苷酸序列确定了69 kDa亚基的完整一级结构。69 kDa亚基由623个氨基酸组成(分子量68,835),没有明显的跨膜区域。胡萝卜cDNA序列与粗糙脉孢菌69 kDa基因组克隆的外显子有超过70%的同源性。胡萝卜69 kDa亚基的蛋白质序列在275个氨基酸的相似序列核心区域与四个代表性的F0F1 - ATP酶β链也有34.3%的同一性。比对研究揭示了几个与β链高度同源的区域,包括先前与催化功能有关的序列。这提供了确凿的证据表明液泡ATP酶与F0F1型ATP酶密切相关。69 kDa亚基和β亚基之间的一个主要功能差异是3个关键半胱氨酸残基的位置:两个在假定的催化区域(Cys - 248和Cys - 256),一个在提议的Mg2 +结合位点(Cys - 279)。这些半胱氨酸(以及另外两个)可能解释了液泡H + - ATP酶对巯基试剂N - 乙基马来酰亚胺的敏感性。有人提出这两种ATP酶可能是由一个共同的祖先通过在亚基氨基末端附近插入或缺失一大段非同源序列而产生的。

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