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痘苗拓扑异构酶和Cre重组酶催化含3'-对硝基苯磷酸酯的活化DNA底物的直接连接。

Vaccinia topoisomerase and Cre recombinase catalyze direct ligation of activated DNA substrates containing a 3'-para-nitrophenyl phosphate ester.

作者信息

Woodfield G, Cheng C, Shuman S, Burgin A B

机构信息

Biology Department, San Diego State University, 5500 Campanile Drive, San Diego, CA 92182-4614, USA.

出版信息

Nucleic Acids Res. 2000 Sep 1;28(17):3323-31. doi: 10.1093/nar/28.17.3323.

Abstract

DNA topoisomerases and DNA site-specific recombinases are involved in a diverse set of cellular processes but both function by making transient breaks in DNA. Type IB topoisomerases and tyrosine recombinases cleave DNA by transesterification of an active site tyrosine to generate a DNA-3'-phosphotyrosyl-enzyme adduct and a free 5'-hydroxyl (5'-OH). Strand ligation results when the 5'-OH attacks the covalent complex and displaces the enzyme. We describe the synthesis of 3'-phospho-(para-nitrophenyl) oligonucleotides (3'-pNP DNAs), which mimic the natural 3'-phosphotyrosyl intermediate, and demonstrate that such pre-activated strands are substrates for DNA ligation by vaccinia topoisomerase and Cre recombinase. Ligation occurs by direct attack of a 5'-OH strand on the 3'-pNP DNA (i.e., without a covalent protein-DNA intermediate) and generates free para-nitrophenol as a product. The chromogenic DNA substrate allows ligation to be studied in real-time and in the absence of competing cleavage reactions and can be exploited for high-throughput screening of topoisomerase/recombinase inhibitors.

摘要

DNA拓扑异构酶和DNA位点特异性重组酶参与多种细胞过程,但二者均通过使DNA产生瞬时断裂来发挥作用。IB型拓扑异构酶和酪氨酸重组酶通过活性位点酪氨酸的转酯作用切割DNA,生成DNA-3'-磷酸酪氨酸 - 酶加合物和游离的5'-羟基(5'-OH)。当5'-OH攻击共价复合物并置换酶时,发生链连接。我们描述了3'-磷酸 - (对硝基苯基)寡核苷酸(3'-pNP DNA)的合成,其模拟天然的3'-磷酸酪氨酸中间体,并证明这种预激活的链是牛痘拓扑异构酶和Cre重组酶进行DNA连接的底物。连接通过5'-OH链对3'-pNP DNA的直接攻击发生(即,没有共价蛋白质 - DNA中间体),并产生游离的对硝基苯酚作为产物。这种发色DNA底物允许在无竞争性切割反应的情况下实时研究连接反应,并且可用于高通量筛选拓扑异构酶/重组酶抑制剂。

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