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将冷活性碱性磷酸酶活性位点残基替换为来自大肠杆菌的嗜温对应物中发现的残基的影响。

Effects of replacing active site residues in a cold-active alkaline phosphatase with those found in its mesophilic counterpart from Escherichia coli.

作者信息

Gudjónsdóttir Katrín, Asgeirsson Bjarni

机构信息

Department of Biochemistry, Science Institute, University of Iceland, Reykjavik, Iceland.

出版信息

FEBS J. 2008 Jan;275(1):117-27. doi: 10.1111/j.1742-4658.2007.06182.x. Epub 2007 Dec 7.

DOI:10.1111/j.1742-4658.2007.06182.x
PMID:18067583
Abstract

Alkaline phosphatase (AP) from a North Atlantic marine Vibrio bacterium was previously characterized as being kinetically cold-adapted. It is still unknown whether its characteristics originate locally in the active site or are linked to more general structural factors. There are three metal-binding sites in the active site of APs, and all three metal ions participate in catalysis. The amino acid residues that bind the two zinc ions most commonly present are conserved in all known APs. In contrast, two of the residues that bind the third metal ion (numbered 153 and 328 in Escherichia coli AP) are different in various APs. This may explain their different catalytic efficiencies, as the Mg2+ most often present there is important for both structural stability and the reaction mechanism. We have mutated these key residues to the corresponding residues in E. coli AP to obtain the double mutant Asp116/Lys274, and both single mutants. All these mutants displayed reduced substrate affinity and lower overall reaction rates. The Lys274 and Asp116/Lys274 mutants also displayed an increase in global heat stability, which may be due to the formation of a stabilizing salt bridge. Overall, the results show that a single amino acid substitution in the active site is sufficient to alter the structural stability of the cold-active Vibrio AP both locally and globally, and this influences kinetic properties.

摘要

来自北大西洋海洋弧菌的碱性磷酸酶(AP)先前被表征为具有动力学冷适应性。其特性是源于活性位点的局部特征还是与更普遍的结构因素相关,目前仍不清楚。AP的活性位点有三个金属结合位点,所有这三种金属离子都参与催化作用。在所有已知的AP中,结合最常见的两种锌离子的氨基酸残基是保守的。相比之下,结合第三种金属离子的两个残基(在大肠杆菌AP中编号为153和328)在不同的AP中有所不同。这可能解释了它们不同的催化效率,因为那里最常存在的Mg2+对结构稳定性和反应机制都很重要。我们已将这些关键残基突变为大肠杆菌AP中的相应残基,以获得双突变体Asp116/Lys274以及两个单突变体。所有这些突变体均表现出底物亲和力降低和总体反应速率降低。Lys274和Asp116/Lys274突变体还表现出全局热稳定性增加,这可能是由于形成了稳定的盐桥。总体而言,结果表明活性位点中的单个氨基酸取代足以在局部和全局上改变冷活性弧菌AP的结构稳定性,并且这会影响动力学性质。

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