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鉴定液泡 H+-焦磷酸酶底物结合所必需的赖氨酸残基。

Identification of essential lysines involved in substrate binding of vacuolar H+-pyrophosphatase.

机构信息

Department of Life Science and Institute of Bioinformatics and Structural Biology, College of Life Science, National Tsing Hua University, Hsin Chu 30043, Taiwan.

出版信息

J Biol Chem. 2011 Apr 8;286(14):11970-6. doi: 10.1074/jbc.M110.190215. Epub 2011 Feb 3.

DOI:10.1074/jbc.M110.190215
PMID:21292767
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3069399/
Abstract

H+-translocating pyrophosphatase (H+-PPase; EC 3.6.1.1) drives proton transport against an electrochemical potential gradient by hydrolyzing pyrophosphate (PPi) and is found in various endomembranes of higher plants, bacteria, and some protists. H+-PPase contains seven highly conserved lysines. We examined the functional roles of these lysines, which are, for the most part, found in the cytosolic regions of mung bean H+-PPase by site-directed mutagenesis. Construction of mutants that each had a cytosolic and highly conserved lysine substituted with an alanine resulted in dramatic drops in the PPi hydrolytic activity. The effects caused by ions on the activities of WT and mutant H+-PPases suggest that Lys-730 may be in close proximity to the Mg2+-binding site, and the great resistance of the K694A and K695A mutants to fluoride inhibition suggests that these lysines are present in the active site. The modifier fluorescein 5'-isothiocyanate (FITC) labeled a lysine at the H+-PPase active site but did not inhibit the hydrolytic activities of K250A, K250N, K250T, and K250S, which suggested that Lys-250 is essential for substrate binding and may be involved in proton translocation. Analysis of tryptic digests indicated that Lys-711 and Lys-717 help maintain the conformation of the active site. Proteolytic evidence also demonstrated that Lys-250 is the primary target of trypsin and confirmed its crucial role in H+-PPase hydrolysis.

摘要

H+-转运焦磷酸酶(H+-PPase;EC 3.6.1.1)通过水解焦磷酸(PPi)来驱动质子逆电化学势梯度运输,存在于高等植物、细菌和一些原生生物的各种内膜中。H+-PPase 含有七个高度保守的赖氨酸。我们通过定点突变研究了这些赖氨酸的功能作用,这些赖氨酸在绿豆 H+-PPase 的胞质区域大部分被发现。构建每个胞质和高度保守的赖氨酸都被丙氨酸取代的突变体,导致 PPi 水解活性显著下降。离子对 WT 和突变体 H+-PPase 活性的影响表明,Lys-730 可能靠近 Mg2+结合位点,而 K694A 和 K695A 突变体对氟化物抑制的强抗性表明这些赖氨酸存在于活性位点中。修饰荧光素 5'-异硫氰酸酯(FITC)标记 H+-PPase 活性位点的一个赖氨酸,但不抑制 K250A、K250N、K250T 和 K250S 的水解活性,这表明 Lys-250 对底物结合是必需的,并且可能参与质子转运。胰蛋白酶消化分析表明,Lys-711 和 Lys-717 有助于维持活性位点的构象。蛋白水解证据还表明,Lys-250 是胰蛋白酶的主要靶标,并证实了它在 H+-PPase 水解中的关键作用。

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本文引用的文献

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Distance variations between active sites of H(+)-pyrophosphatase determined by fluorescence resonance energy transfer.荧光共振能量转移测定 H(+)-焦磷酸酶活性位点之间的距离变化。
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