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使用商业逆转录酶制剂在植物病毒RNA模板上进行不依赖外源性引物的cDNA合成。

Exogenous primer-independent cDNA synthesis with commercial reverse transcriptase preparations on plant virus RNA templates.

作者信息

Agranovsky A A

机构信息

A. N. Belozersky Laboratory, Moscow State University, Russia.

出版信息

Anal Biochem. 1992 May 15;203(1):163-5. doi: 10.1016/0003-2697(92)90058-f.

Abstract

Upon reverse transcription and cloning manipulations with virion RNAs of several plant viruses, namely beet yellows virus, brome mosaic virus, and potato virus X, we came across a significant background synthesis of cDNA on the virion RNA template in vitro independent of exogenous primers added. When tested with beet yellow virus RNA template, several commercial preparations of avian myeloblastosis virus (AMV) reverse transcriptase showed the background activity monitored by the [alpha-32P]dNTP incorporation in vitro, while the enzyme from murine moloney leukemia virus (MMLV) was found strictly exogenous-primer-dependent. To detect possible nucleic acid contaminations in reverse transcriptase, the enzyme preparations from several commercial sources were incubated with [gamma-32P]ATP and polynucleotide kinase. The labeled material from AMV reverse transcriptase preparations comigrated with a tRNA marker in polyacrylamide gels and was found to be RNase-sensitive. The MMLV reverse transcriptase preparations were free from such a contamination. These results indicate that the exogenous-primer-independent cDNA synthesis by some AMV reverse transcriptases could be due to a contaminating tRNA (or its low-molecular-weight degradation products) serving as an endogenous primer.

摘要

在用几种植物病毒(即甜菜黄化病毒、雀麦花叶病毒和马铃薯X病毒)的病毒粒子RNA进行逆转录和克隆操作时,我们发现在体外病毒粒子RNA模板上存在显著的背景cDNA合成,且不依赖于添加的外源引物。用甜菜黄化病毒RNA模板进行测试时,几种禽成髓细胞瘤病毒(AMV)逆转录酶的商业制剂显示出通过体外[α-32P]dNTP掺入监测的背景活性,而来自鼠莫洛尼白血病病毒(MMLV)的酶则被发现严格依赖外源引物。为了检测逆转录酶中可能的核酸污染,将几种商业来源的酶制剂与[γ-32P]ATP和多核苷酸激酶一起孵育。AMV逆转录酶制剂中的标记物质在聚丙烯酰胺凝胶中与tRNA标记物迁移一致,并且被发现对RNase敏感。MMLV逆转录酶制剂没有这种污染。这些结果表明,一些AMV逆转录酶的不依赖外源引物的cDNA合成可能是由于污染的tRNA(或其低分子量降解产物)作为内源性引物所致。

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