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痘苗病毒DNA拓扑异构酶26个残基的突变分析确定丝氨酸-204对DNA结合和切割很重要。

Mutational analysis of 26 residues of vaccinia DNA topoisomerase identifies Ser-204 as important for DNA binding and cleavage.

作者信息

Wang L K, Wittschieben J, Shuman S

机构信息

Molecular Biology Program, Sloan-Kettering Institute, New York, New York 10021.

出版信息

Biochemistry. 1997 Jul 1;36(26):7944-50. doi: 10.1021/bi970498q.

DOI:10.1021/bi970498q
PMID:9201940
Abstract

Vaccinia DNA topoisomerase, a 314 amino acid type I enzyme, catalyzes the cleavage and rejoining of DNA strands through a DNA-(3'-phosphotyrosyl)-enzyme intermediate formed at a specific target sequence, 5'-(C/T)CCTT downward arrow. To identify amino acids that participate in the DNA binding and transesterification steps, we introduced alanine substitutions at 18 positions within a centrally located 27 amino acid segment (181-RLYKPLLKLTDDSSPEEFLFNKLSERK-207) and at 8 positions near the N-terminus (1-MRALFYKDGK-10). All mutant proteins except two displayed wild-type activity in relaxing supercoiled DNA. F200A and S204A exhibited reduced rates of relaxation and were subjected to a kinetic analysis of the strand cleavage reaction under single-turnover and equilibrium conditions. The F200A and S204A mutations reduced the rate of single-turnover DNA cleavage by factors of 5 and 70, respectively. Both mutations shifted the cleavage-religation equilibrium in favor of the noncovalently bound state. The S204A mutation reduced the affinity of topoisomerase for CCCTT-containing DNA, but did not alter the site-specificity of DNA cleavage. Vaccinia residue Ser-204, which is conserved in all poxvirus topoisomerases, but not in the cellular homologues, may contribute to the unique cleavage site specificity of the poxvirus enzymes. Phe-200 is conserved in all members of the type IB topoisomerase family.

摘要

痘苗病毒DNA拓扑异构酶是一种含314个氨基酸的I型酶,它通过在特定靶序列5'-(C/T)CCTT向下箭头处形成的DNA-(3'-磷酸酪氨酸)-酶中间体催化DNA链的切割和重新连接。为了鉴定参与DNA结合和转酯步骤的氨基酸,我们在位于中心位置的27个氨基酸片段(181-RLYKPLLKLTDDSSPEEFLFNKLSERK-207)内的18个位置以及N端附近的8个位置(1-MRALFYKDGK-10)引入了丙氨酸替代。除两个突变蛋白外,所有突变蛋白在松弛超螺旋DNA时均表现出野生型活性。F200A和S204A的松弛速率降低,并在单周转和平衡条件下对链切割反应进行了动力学分析。F200A和S204A突变分别使单周转DNA切割速率降低了5倍和70倍。这两个突变都使切割-重新连接平衡向非共价结合状态偏移。S204A突变降低了拓扑异构酶对含CCCTT的DNA的亲和力,但没有改变DNA切割的位点特异性。痘苗病毒的Ser-204残基在所有痘病毒拓扑异构酶中保守,但在细胞同源物中不保守,可能有助于痘病毒酶独特的切割位点特异性。Phe-200在IB型拓扑异构酶家族的所有成员中保守。

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引用本文的文献

1
Mutational analysis of vaccinia virus topoisomerase identifies residues involved in DNA binding.痘苗病毒拓扑异构酶的突变分析确定了参与DNA结合的残基。
Nucleic Acids Res. 1997 Sep 15;25(18):3649-56. doi: 10.1093/nar/25.18.3649.