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人类复制蛋白A的亚基通过DNA聚合酶合成的光反应性引物发生交联。

Subunits of human replication protein A are crosslinked by photoreactive primers synthesized by DNA polymerases.

作者信息

Lavrik O I, Nasheuer H P, Weisshart K, Wold M S, Prasad R, Beard W A, Wilson S H, Favre A

机构信息

Institut Jacques Monod CNRS, 75251 Paris Cedex 05, France.

出版信息

Nucleic Acids Res. 1998 Jan 15;26(2):602-7. doi: 10.1093/nar/26.2.602.

Abstract

Human replication protein A (huRPA) is a multisubunit protein which is involved in DNA replication, repair and recombination processes. It exists as a stable heterotrimer consisting of p70, p32 and p14 subunits. To understand the contribution of huRPA subunits to DNA binding we applied the photoaffinity labeling technique. The photoreactive oligonucleotide was synthesized in situ by DNA polymerases. 5-[N-(2-nitro-5-azidobenzoyl)-trans -3-aminopropenyl-1]deoxyuridine-5'-triphosphate (NABdUTP) was used as substrate for elongation of a radiolabeled primer logical ortemplate either by human DNA polymerase alpha primase (polalpha), human DNA polymerase beta (polbeta) or Klenow fragment of Escherichia coli DNA polymerase I (KF). The polymerase was incubated with NABdUTP and radiolabeled primer-template in the presence or absence of huRPA. The reaction mixtures were then irradiated with monochromatic UV light (315 nm) and the crosslinked products were separated by SDS-PAGE. The results clearly demonstrate crosslinking of the huRPA p70 and p32 subunits with DNA. The p70 subunit appears to bind to the single-stranded part of the DNA duplex, the p32 subunit locates near the 3'-end of the primer, while the p14 subunit locates relatively far from the 3'-end of the primer. This approach opens new possibilities for analysis of huRPA loading on DNA in the course of DNA replication and DNA repair.

摘要

人类复制蛋白A(huRPA)是一种多亚基蛋白,参与DNA复制、修复和重组过程。它以由p70、p32和p14亚基组成的稳定异源三聚体形式存在。为了了解huRPA亚基对DNA结合的贡献,我们应用了光亲和标记技术。光反应性寡核苷酸由DNA聚合酶原位合成。5-[N-(2-硝基-5-叠氮苯甲酰基)-反式-3-氨基丙烯基-1]脱氧尿苷-5'-三磷酸(NABdUTP)用作底物,通过人DNA聚合酶α引发酶(polα)、人DNA聚合酶β(polβ)或大肠杆菌DNA聚合酶I的Klenow片段(KF)延伸放射性标记的引物或模板。将聚合酶与NABdUTP和放射性标记的引物-模板在有或无huRPA的情况下孵育。然后用单色紫外光(315 nm)照射反应混合物,交联产物通过SDS-PAGE分离。结果清楚地证明了huRPA的p70和p32亚基与DNA的交联。p70亚基似乎与DNA双链的单链部分结合,p32亚基位于引物的3'-末端附近,而p14亚基位于离引物的3'-末端相对较远的位置。这种方法为分析DNA复制和DNA修复过程中huRPA在DNA上的加载开辟了新的可能性。

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本文引用的文献

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