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利用纯化的复制因子重建完整的SV40 DNA复制。

Reconstitution of complete SV40 DNA replication with purified replication factors.

作者信息

Waga S, Bauer G, Stillman B

机构信息

Cold Spring Harbor Laboratory, New York 11724.

出版信息

J Biol Chem. 1994 Apr 8;269(14):10923-34.

PMID:8144677
Abstract

The identification and purification of human cell proteins required for the production of form I DNA following DNA replication from the simian virus 40 (SV40) origin is described. Using these proteins, complete SV40 DNA replication was reconstituted with only purified DNA replication factors: SV40 large tumor antigen (TAg), replication protein A (RPA), DNA topoisomerases I and II, DNA polymerase alpha-primase, replication factor C (RFC), the proliferating cell nuclear antigen (PCNA), DNA polymerase delta, maturation factor 1 (MF1), and DNA ligase I. MF1, a 5' to 3' exonuclease and DNA ligase I were both identified as essential components for production of covalently closed circular relaxed (form I) DNA. MF1 is probably the same exonuclease previously shown by others to function during DNA synthesis on artificial DNA templates or in conjunction with DNA polymerase alpha from the SV40 origin. Combined with these previous studies, our results suggest that MF1 functions to remove an RNA primer attached to every Okazaki fragment during lagging strand DNA synthesis. Interestingly, whereas mammalian DNA ligase I functioned in the reconstituted replication system, mammalian DNA ligase III did not substitute and the phage T4 DNA ligase functioned inefficiently, suggesting that DNA ligase I has a specific role as a replicative DNA ligase in eukaryotic cells.

摘要

本文描述了从猿猴病毒40(SV40)起始点进行DNA复制后产生I型DNA所需的人类细胞蛋白质的鉴定和纯化。利用这些蛋白质,仅用纯化的DNA复制因子就重建了完整的SV40 DNA复制:SV40大T抗原(TAg)、复制蛋白A(RPA)、DNA拓扑异构酶I和II、DNA聚合酶α-引物酶、复制因子C(RFC)、增殖细胞核抗原(PCNA)、DNA聚合酶δ、成熟因子1(MF1)和DNA连接酶I。MF1(一种5'至3'核酸外切酶)和DNA连接酶I均被鉴定为产生共价闭合环状松弛(I型)DNA的必需成分。MF1可能与其他人先前所示的在人工DNA模板上进行DNA合成期间或与来自SV40起始点的DNA聚合酶α一起发挥作用的核酸外切酶相同。结合这些先前的研究,我们的结果表明MF1在滞后链DNA合成期间发挥作用,去除附着在每个冈崎片段上的RNA引物。有趣的是,虽然哺乳动物DNA连接酶I在重建的复制系统中起作用,但哺乳动物DNA连接酶III不能替代,噬菌体T4 DNA连接酶功能效率低下,这表明DNA连接酶I在真核细胞中作为复制性DNA连接酶具有特定作用。

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