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黑腹果蝇DNA聚合酶α的50-kDa引发酶亚基。基因的分子特征及过表达蛋白的功能分析。

The 50-kDa primase subunit of Drosophila melanogaster DNA polymerase alpha. Molecular characterization of the gene and functional analysis of the overexpressed protein.

作者信息

Bakkenist C J, Cotterill S

机构信息

Marie Curie Research Institute, Oxted, Surrey, United Kingdom.

出版信息

J Biol Chem. 1994 Oct 28;269(43):26759-66.

PMID:7929411
Abstract

The gene encoding the 50-kDa subunit of Drosophila melanogaster DNA polymerase alpha has been cloned. A comparison of the predicted polypeptide sequence of the Drosophila protein with the equivalent subunits from mouse and yeast suggests that they are closely related and defines three conserved regions which are likely to be important for enzyme activity. The expression patterns of both the 50-kDa protein and its transcript (a single RNA message of 1.6 kilobases) throughout development are consistent with a role of the protein in DNA replication. When overexpressed and purified the 50-kDa subunit displays DNA primase activity. The products of the reaction, mainly oligoribonucleotides 12-14 nucleotides in length, plus dimers and some trimers, are similar to those synthesized by either the intact DNA polymerase alpha, or the biochemically isolated primase heterodimer. The isolated primase also shows similar sensitivity to antibodies, magnesium and monovalent cations, and the same nucleotide requirements as complexed forms of the primase. The isolated subunit, however, is more thermally labile, suggesting a role for the additional subunits in DNA polymerase alpha in stabilizing the primase activity of the 50-kDa primase subunit.

摘要

果蝇DNA聚合酶α 50-kDa亚基的编码基因已被克隆。将果蝇蛋白的预测多肽序列与来自小鼠和酵母的等效亚基进行比较,结果表明它们密切相关,并确定了三个保守区域,这些区域可能对酶活性很重要。在整个发育过程中,50-kDa蛋白及其转录本(一条1.6千碱基的单一RNA信息)的表达模式与该蛋白在DNA复制中的作用一致。当50-kDa亚基过表达并纯化后,它表现出DNA引发酶活性。反应产物主要是长度为12 - 14个核苷酸的寡核糖核苷酸,加上二聚体和一些三聚体,与完整的DNA聚合酶α或生化分离的引发酶异二聚体合成的产物相似。分离出的引发酶对抗体、镁和单价阳离子也表现出相似的敏感性,并且与引发酶的复合形式具有相同的核苷酸需求。然而,分离出的亚基热稳定性较差,这表明DNA聚合酶α中的其他亚基在稳定50-kDa引发酶亚基的引发酶活性方面发挥了作用。

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