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人类REV1蛋白的脱氧胞苷转移酶活性与保守的聚合酶结构域密切相关。

Deoxycytidyl transferase activity of the human REV1 protein is closely associated with the conserved polymerase domain.

作者信息

Masuda Y, Takahashi M, Tsunekuni N, Minami T, Sumii M, Miyagawa K, Kamiya K

机构信息

Research Institute for Radiation Biology and Medicine, Hiroshima University, 1-2-3 Kasumi, Minami-ku, Hiroshima 734-8553, Japan.

出版信息

J Biol Chem. 2001 May 4;276(18):15051-8. doi: 10.1074/jbc.M008082200. Epub 2001 Jan 22.

Abstract

The REV1 protein is a member of the growing family of translesion DNA polymerases. A cDNA of the human REV1 gene that we had originally isolated encoded 1250 amino acids residues, which was one amino acid shorter than previously reported ones. The shorter form of REV1 was named REV1S. All individuals examined expressed equivalent amounts of REV1S and REV1 mRNA, suggesting that the REV1S mRNA is a splicing variant. We show that the REV1S protein also possesses deoxycytidyl transferase activity that inserts a dCMP opposite a DNA template apurinic/apyrimidinic site. Deletion and point mutation analysis of the REV1S protein revealed that the domain required for deoxycytidyl transferase and DNA binding activities of the REV1S protein are located in a conserved domain of translesion DNA polymerases. This result indicates that the structure of the catalytic site of the deoxycytidyl transferase closely resembles that of the translesion DNA polymerases. Therefore, the molecular mechanism of the dCMP transfer reaction of the REV1S protein and maybe also the REV1 protein might be the same as that of the dNTP transfer reaction of the translesion DNA polymerases.

摘要

REV1蛋白是不断增加的跨损伤DNA聚合酶家族的成员之一。我们最初分离的人类REV1基因的cDNA编码1250个氨基酸残基,比之前报道的少一个氨基酸。REV1的较短形式被命名为REV1S。所有检测的个体表达等量的REV1S和REV1 mRNA,这表明REV1S mRNA是一种剪接变体。我们发现REV1S蛋白也具有脱氧胞苷转移酶活性,可在DNA模板的无嘌呤/无嘧啶位点对面插入一个dCMP。对REV1S蛋白的缺失和点突变分析表明,REV1S蛋白的脱氧胞苷转移酶和DNA结合活性所需的结构域位于跨损伤DNA聚合酶的保守结构域中。这一结果表明,脱氧胞苷转移酶催化位点的结构与跨损伤DNA聚合酶的结构非常相似。因此,REV1S蛋白以及可能还有REV1蛋白的dCMP转移反应的分子机制可能与跨损伤DNA聚合酶的dNTP转移反应的分子机制相同。

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