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III型限制修饰酶中保守基序的功能分析

Functional analysis of conserved motifs in type III restriction-modification enzymes.

作者信息

Saha S, Ahmad I, Reddy Y V, Krishnamurthy V, Rao D N

机构信息

Department of Biochemistry, Indian Institute of Science, Bangalore.

出版信息

Biol Chem. 1998 Apr-May;379(4-5):511-7. doi: 10.1515/bchm.1998.379.4-5.511.

DOI:10.1515/bchm.1998.379.4-5.511
PMID:9628345
Abstract

EcoP1I and EcoP15I are members of type III restriction-modification enzymes. EcoPI and EcoP15I DNA methyltransferases transfer a methyl group from S-adenosyl-L-methionine (AdoMet) to the N6 position of the second adenine residues in their recognition sequences, 5'-AGACC-3' and 5'-CAGCAG-3' respectively. We have altered various residues in two highly conserved sequences, FxGxG (motif I) and DPPY (motif IV) in these proteins by site-directed mutagenesis. Using a mixture of in vivo and in vitro assays, our results on the mutational analysis of these methyltransferases demonstrate the universal role of motif I in AdoMet binding and a role for motif IV in catalysis. All six cysteine residues in EcoP15I DNA methyltransferase have been substituted with serine and the role of cysteine residues in EcoP15I DNA methyltransferase catalysed reaction assessed. The Res subunits of type III restriction enzymes share a distant sequence similarity with and contain the motifs characteristic of the DEAD box proteins. We have carried out site-directed mutagenesis of the conserved residues in two of the helicase motifs of the EcoP1I restriction enzyme in order to investigate the role of motifs in DNA cleavage by this enzyme. Our findings indicate that certain conserved residues in these motifs are involved in ATP hydrolysis while the other residues are involved in coupling restriction of DNA to ATP hydrolysis. Taken collectively, these results form the basis for a detailed structure-function analysis of EcoP1I and EcoP15I restriction enzymes.

摘要

EcoP1I和EcoP15I是III型限制修饰酶的成员。EcoPI和EcoP15I DNA甲基转移酶分别将一个甲基从S-腺苷-L-甲硫氨酸(AdoMet)转移到其识别序列5'-AGACC-3'和5'-CAGCAG-3'中第二个腺嘌呤残基的N6位置。我们通过定点诱变改变了这些蛋白质中两个高度保守序列FxGxG(基序I)和DPPY(基序IV)中的各种残基。使用体内和体外试验的组合,我们对这些甲基转移酶的突变分析结果证明了基序I在AdoMet结合中的普遍作用以及基序IV在催化中的作用。EcoP15I DNA甲基转移酶中的所有六个半胱氨酸残基都已被丝氨酸取代,并评估了半胱氨酸残基在EcoP15I DNA甲基转移酶催化反应中的作用。III型限制酶的Res亚基与DEAD盒蛋白具有远距离的序列相似性,并包含其特征基序。我们对EcoP1I限制酶的两个解旋酶基序中的保守残基进行了定点诱变,以研究这些基序在该酶切割DNA中的作用。我们的研究结果表明,这些基序中的某些保守残基参与ATP水解,而其他残基则参与将DNA限制与ATP水解偶联。总的来说,这些结果构成了对EcoP1I和EcoP15I限制酶进行详细结构功能分析的基础。

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