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小牛胸腺核糖核酸酶HI对冈崎片段上RNA引物进行结构特异性切割。

Structure-specific cleavage of the RNA primer from Okazaki fragments by calf thymus RNase HI.

作者信息

Huang L, Kim Y, Turchi J J, Bambara R A

机构信息

Department of Biochemistry, University of Rochester, School of Medicine and Dentistry, New York 14642.

出版信息

J Biol Chem. 1994 Oct 14;269(41):25922-7.

PMID:7523396
Abstract

Cleavage specificity of RNase HI was examined on model Okazaki fragments, to determine the likely role of this nuclease in lagging strand DNA replication. Each substrate was prepared by annealing a short RNA primer, made by transcription in vitro, to a single-stranded synthetic DNA template, and subsequently extending the primer by DNA polymerization. The calf thymus RNase HI makes a structure-specific endonucleolytic cleavage in the RNA primer, releasing it intact, and leaving a mono-ribonucleotide at the 5' terminus of the RNA-DNA junction. This specific cleavage, one nucleotide upstream of the RNA-DNA junction, is RNA primer sequence- and length-independent. Cleavage specificity is lost if the RNA primer is not extended with DNA, or if the substrate has a nick at the RNA-DNA junction. In addition, the cleavage at a single site requires Mg2+. Cleavage in the presence of Mn2+ is less specific. Neither human immunodeficiency virus reverse transcriptase nor Escherichia coli RNases H perform such a structure-specific cleavage before an RNA-DNA junction. Our work indicates that calf RNase HI is designed to recognize Okazaki fragments. It has the specificity to remove their initiator RNA segments, except for one ribonucleotide, by a single endonucleolytic cleavage in vivo.

摘要

在模型冈崎片段上检测了核糖核酸酶HI(RNase HI)的切割特异性,以确定这种核酸酶在滞后链DNA复制中可能发挥的作用。每个底物的制备方法是,将通过体外转录制备的短RNA引物与单链合成DNA模板退火,随后通过DNA聚合反应延伸引物。小牛胸腺RNase HI在RNA引物中进行结构特异性的内切核酸酶切割,完整释放引物,并在RNA-DNA连接点的5'末端留下一个单核糖核苷酸。这种在RNA-DNA连接点上游一个核苷酸处的特异性切割与RNA引物序列和长度无关。如果RNA引物没有用DNA延伸,或者底物在RNA-DNA连接点处有切口,切割特异性就会丧失。此外,在单个位点的切割需要Mg2+。在Mn2+存在下的切割特异性较低。人类免疫缺陷病毒逆转录酶和大肠杆菌RNases H在RNA-DNA连接点之前都不会进行这种结构特异性切割。我们的工作表明,小牛RNase HI旨在识别冈崎片段。它具有在体内通过一次内切核酸酶切割去除其起始RNA片段(除了一个核糖核苷酸)的特异性。

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