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逆转录酶在体外以RNA为引物起始莫洛尼鼠白血病病毒正链的合成

RNA-primed initiation of Moloney murine leukemia virus plus strands by reverse transcriptase in vitro.

作者信息

Finston W I, Champoux J J

出版信息

J Virol. 1984 Jul;51(1):26-33. doi: 10.1128/JVI.51.1.26-33.1984.

Abstract

A 190-base-pair DNA-RNA hybrid containing the Moloney murine leukemia virus origin of plus-strand DNA synthesis was constructed and used as a source of template-primer for the reverse transcriptase in vitro. Synthesis was shown to initiate precisely at the known plus-strand origin. The observation that some of the origin fragments retained ribonucleotide residues on their 5' ends suggests that the primer for chain initiation is an RNA molecule left behind by RNase H during the degradation of the RNA moiety of the DNA-RNA hybrid. If the RNase H is responsible for creating the correct primer terminus, then it must possess a specific endonucleolytic activity capable of recognizing the sequence in the RNA where plus strands are initiated. The 16-base RNase A-resistant fragment which spans the plus-strand origin can also serve as a source of the specific plus-strand primer RNA. Evidence is presented that some of the plus-strand origin fragments synthesized in the endogenous reaction contain 5' ribonucleotides, suggesting that specific RNA primers for plus-strand initiation may be generated during reverse transcription in vivo as well.

摘要

构建了一个包含莫洛尼鼠白血病病毒正链 DNA 合成起始位点的 190 个碱基对的 DNA - RNA 杂交体,并将其用作体外逆转录酶的模板 - 引物来源。结果表明合成精确起始于已知的正链起始位点。一些起始位点片段在其 5' 末端保留核糖核苷酸残基的观察结果表明,链起始的引物是 RNase H 在降解 DNA - RNA 杂交体的 RNA 部分过程中留下的 RNA 分子。如果 RNase H 负责产生正确的引物末端,那么它必须具有一种能够识别正链起始处 RNA 序列的特异性内切核酸酶活性。跨越正链起始位点的 16 个碱基的抗 RNase A 片段也可作为特异性正链引物 RNA 的来源。有证据表明,在内源反应中合成的一些正链起始位点片段含有 5' 核糖核苷酸,这表明在体内逆转录过程中也可能产生用于正链起始的特异性 RNA 引物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7646/254394/f3bca27115c9/jvirol00130-0037-a.jpg

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