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2',3'-环核苷酸3'-磷酸二酯酶中必需残基的鉴定。通过化学修饰和定点诱变研究半胱氨酸和组氨酸残基在酶活性中的作用。

Identification of essential residues in 2',3'-cyclic nucleotide 3'-phosphodiesterase. Chemical modification and site-directed mutagenesis to investigate the role of cysteine and histidine residues in enzymatic activity.

作者信息

Lee J, Gravel M, Gao E, O'Neill R C, Braun P E

机构信息

Department of Biochemistry, McGill University, Montreal, Quebec H3G 1Y6, Canada.

出版信息

J Biol Chem. 2001 May 4;276(18):14804-13. doi: 10.1074/jbc.M009434200. Epub 2001 Feb 5.

DOI:10.1074/jbc.M009434200
PMID:11278504
Abstract

2',3'-Cyclic nucleotide 3'-phosphodiesterase (CNP; EC ) catalyzes in vitro hydrolysis of 3'-phosphodiester bonds in 2',3'-cyclic nucleotides to produce 2'-nucleotides exclusively. N-terminal deletion mapping of the C-terminal two-thirds of recombinant rat CNP1 identified a region that possesses the catalytic domain, with further truncations abolishing activity. Proteolysis and kinetic analysis indicated that this domain forms a compact globular structure and contains all of the catalytically essential features. Subsequently, this catalytic fragment of CNP1 (CNP-CF) was used for chemical modification studies to identify amino acid residues essential for activity. 5,5'-Dithiobis-(2-nitrobenzoic acid) modification studies and kinetic analysis of cysteine CNP-CF mutants revealed the nonessential role of cysteines for enzymatic activity. On the other hand, modification studies with diethyl pyrocarbonate indicated that two histidines are essential for CNPase activity. Consequently, the only two conserved histidines, His-230 and His-309, were mutated to phenylalanine and leucine. All four histidine mutants had k(cat) values 1000-fold lower than wild-type CNP-CF, but K(m) values were similar. Circular dichroism studies demonstrated that the low catalytic activities of the histidine mutants were not due to gross changes in secondary structure. Taken together, these results demonstrate that both histidines assume critical roles for catalysis.

摘要

2',3'-环核苷酸3'-磷酸二酯酶(CNP;EC )在体外催化2',3'-环核苷酸中3'-磷酸二酯键的水解,专一性地生成2'-核苷酸。对重组大鼠CNP1 C端三分之二区域进行N端缺失定位,确定了一个具有催化结构域的区域,进一步截短则会消除活性。蛋白水解和动力学分析表明,该结构域形成紧密的球状结构,并包含所有催化必需的特征。随后,将CNP1的这个催化片段(CNP-CF)用于化学修饰研究,以确定对活性至关重要的氨基酸残基。5,5'-二硫代双(2-硝基苯甲酸)修饰研究以及半胱氨酸CNP-CF突变体的动力学分析揭示了半胱氨酸对酶活性的非必需作用。另一方面,焦碳酸二乙酯修饰研究表明,两个组氨酸对CNP酶活性至关重要。因此,仅有的两个保守组氨酸,即His-230和His-309,被突变为苯丙氨酸和亮氨酸。所有四个组氨酸突变体的k(cat)值比野生型CNP-CF低1000倍,但K(m)值相似。圆二色性研究表明,组氨酸突变体的低催化活性并非由于二级结构的总体变化。综上所述,这些结果表明这两个组氨酸在催化中都起着关键作用。

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