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嗜热栖热菌HB8中的Nudix水解酶Ndx1是一种具有新活性的二腺苷六磷酸水解酶。

The Nudix hydrolase Ndx1 from Thermus thermophilus HB8 is a diadenosine hexaphosphate hydrolase with a novel activity.

作者信息

Iwai Takayoshi, Kuramitsu Seiki, Masui Ryoji

机构信息

Department of Biology, Graduate School of Science, Osaka University, Toyonaka, Osaka 560-0043.

出版信息

J Biol Chem. 2004 May 21;279(21):21732-9. doi: 10.1074/jbc.M312018200. Epub 2004 Mar 15.

DOI:10.1074/jbc.M312018200
PMID:15024014
Abstract

The ndx1 gene, which encodes a Nudix protein, was cloned from the extremely thermophilic bacterium Thermus thermophilus HB8. This gene encodes a 126-amino acid protein that includes the characteristic Nudix motif conserved among Nudix proteins. Ndx1 was overexpressed in Escherichia coli and purified. Ndx1 was stable up to 95 degrees C and at extreme pH. Size exclusion chromatography indicated that Ndx1 was monomeric in solution. Ndx1 specifically hydrolyzed (di)adenosine polyphosphates but not ATP or diadenosine triphosphate, and it always generated ATP as the product. Diadenosine hexaphosphate (Ap(6)A), the most preferred substrate, was hydrolyzed to produce two ATP molecules, which is a novel hydrolysis mode for Ap(6)A, with a K(m) of 1.4 microm and a k(cat) of 4.1 s(-1). These results indicate that Ndx1 is a (di)adenosine polyphosphate hydrolase. Ndx1 activity required the presence of the divalent cations Mn(2+), Mg(2+), Zn(2+), and Co(2+), whereas Ca(2+), Ni(2+), and Cu(2+) were not able to activate Ndx1. Fluoride ion inhibited Ndx1 activity via a non-competitive mechanism. Optimal activity for Ap(6)A was observed at around pH 8.0 and about 70 degrees C. We found two important residues with pK(a) values of 6.1 and 9.6 in the free enzyme and pK(a) values of 7.9 and 10.0 in the substrate-enzyme complex. Kinetic studies of proteins with amino acid substitutions suggested that Glu-46 and Glu-50 were conserved residues in the Nudix motif and were involved in catalysis. Trp-26 was likely involved in enzyme-substrate interactions based on fluorescence measurements. Based on these results, the mechanism of substrate recognition and catalysis are discussed.

摘要

从嗜热栖热菌HB8中克隆出了编码Nudix蛋白的ndx1基因。该基因编码一种含126个氨基酸的蛋白质,其中包括Nudix蛋白中保守的特征性Nudix基序。Ndx1在大肠杆菌中过量表达并得以纯化。Ndx1在高达95摄氏度和极端pH条件下仍保持稳定。尺寸排阻色谱表明Ndx1在溶液中呈单体状态。Ndx1特异性水解(二)腺苷多磷酸,但不水解ATP或二腺苷三磷酸,且其产物总是ATP。最适宜的底物二腺苷六磷酸(Ap(6)A)被水解生成两个ATP分子,这是Ap(6)A一种新的水解模式,其米氏常数(K(m))为1.4微摩尔,催化常数(k(cat))为4.1秒-1。这些结果表明Ndx1是一种(二)腺苷多磷酸水解酶。Ndx1的活性需要二价阳离子Mn(2+)、Mg(2+)、Zn(2+)和Co(2+)的存在,而Ca(2+)、Ni(2+)和Cu(2+)不能激活Ndx1。氟离子通过非竞争性机制抑制Ndx1的活性。在pH约8.0和70摄氏度左右观察到Ap(6)A的最佳活性。我们发现游离酶中有两个重要残基,其pK(a)值分别为6.1和9.6,在底物 - 酶复合物中pK(a)值分别为7.9和10.0。对氨基酸替换后的蛋白质进行动力学研究表明,Glu - 46和Glu - 50是Nudix基序中的保守残基,参与催化作用。基于荧光测量,Trp - 26可能参与酶 - 底物相互作用。基于这些结果,讨论了底物识别和催化机制。

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