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真核生物复制叉处的滞后链DNA合成涉及增殖细胞核抗原对FEN-1的结合和刺激。

Lagging strand DNA synthesis at the eukaryotic replication fork involves binding and stimulation of FEN-1 by proliferating cell nuclear antigen.

作者信息

Li X, Li J, Harrington J, Lieber M R, Burgers P M

机构信息

Department of Biochemistry, Washington University School of Medicine, St. Louis, Missouri 63110, USA.

出版信息

J Biol Chem. 1995 Sep 22;270(38):22109-12. doi: 10.1074/jbc.270.38.22109.

Abstract

The 5'-->3'-exonuclease domain of Escherichia coli DNA polymerase I is required for the completion of lagging strand DNA synthesis, and yet this domain is not present in any of the eukaryotic DNA polymerases. Recently, the gene encoding the functional and evolutionary equivalent of this 5'-->3'-exonuclease domain has been identified. It is called FEN-1 in mouse and human cells and RTH1 in Saccharomyces cerevisiae. This 42-kDa enzyme is required for Okazaki fragment processing. Here we report that FEN-1 physically interacts with proliferating cell nuclear antigen (PCNA), the processivity factor for DNA polymerases delta and epsilon. Through protein-protein interactions, PCNA focuses FEN-1 on branched DNA substrates (flap structures) and on nicked DNA substrates, thereby stimulating its activity 10-50-fold but only if PCNA can functionally assemble as a toroidal trimer around the DNA. This interaction is important in the physical orchestration of lagging strand synthesis and may have implications for how PCNA stimulates other members of the FEN-1 nuclease family in a broad range of DNA metabolic transactions.

摘要

大肠杆菌DNA聚合酶I的5'→3'核酸外切酶结构域是后随链DNA合成完成所必需的,然而该结构域在任何真核DNA聚合酶中都不存在。最近,编码这种5'→3'核酸外切酶结构域功能和进化等效物的基因已被鉴定。在小鼠和人类细胞中它被称为FEN-1,在酿酒酵母中被称为RTH1。这种42 kDa的酶是冈崎片段加工所必需的。在此我们报道,FEN-1与增殖细胞核抗原(PCNA)发生物理相互作用,PCNA是DNA聚合酶δ和ε的持续合成因子。通过蛋白质-蛋白质相互作用,PCNA将FEN-1聚焦于分支DNA底物(瓣状结构)和带切口的DNA底物上,从而将其活性提高10至50倍,但前提是PCNA能够作为环形三聚体围绕DNA进行功能性组装。这种相互作用在协调后随链合成的物理过程中很重要,并且可能对PCNA在广泛的DNA代谢过程中如何刺激FEN-1核酸酶家族的其他成员具有启示意义。

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