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通过Qβ复制酶将宿主细胞RNA进化为高效模板RNA:无模板反应中RNA的起源

Evolution of host cell RNA into efficient template RNA by Q beta replicase: the origin of RNA in untemplated reactions.

作者信息

Moody M D, Burg J L, DiFrancesco R, Lovern D, Stanick W, Lin-Goerke J, Mahdavi K, Wu Y, Farrell M P

机构信息

Gene-Trak, Incorporated, Framingham, Massachusetts 01701.

出版信息

Biochemistry. 1994 Nov 22;33(46):13836-47. doi: 10.1021/bi00250a038.

Abstract

Q beta replicase can replicate a single molecule of certain species of RNA to 10(14) copies in minutes. This replication ability has been used for in vitro studies of molecular evolution and is currently being utilized as a method of amplifying RNAs that contain probe sequences. It has been observed that Q beta replicase can produce replicatable RNA even in the absence of exogenously added template RNA. The origin of this RNA has been ascribed either to contamination with replicatable RNA or to an ability of Q beta replicase to synthesize RNA de novo from the nucleotides present in the reaction. Technologies that employ Q beta replicase require a thorough understanding of the conditions that lead to this so-called spontaneous RNA production. We have created an expression system and purification method with which we produce gram quantities of highly purified Q beta replicase, and we have identified reaction conditions that prevent the amplification of RNA in assays that do not contain added RNA. However, when these reaction conditions are relaxed, spontaneous RNA replication is seen in up to 100% of the assays. To understand the origin of this RNA, we have cloned several spontaneously produced RNAs. Sequence analysis of one of these RNAs shows that it arose by the evolution of Escherichia coli tRNA into a replicatable template and not by de novo synthesis from nucleoside triphosphates in the reaction.

摘要

Qβ复制酶能在数分钟内将某些种类的单个RNA分子复制成10¹⁴个拷贝。这种复制能力已被用于分子进化的体外研究,目前正被用作一种扩增含有探针序列的RNA的方法。据观察,即使在没有外源添加模板RNA的情况下,Qβ复制酶也能产生可复制的RNA。这种RNA的来源要么归因于可复制RNA的污染,要么归因于Qβ复制酶从反应中存在的核苷酸从头合成RNA的能力。采用Qβ复制酶的技术需要深入了解导致这种所谓自发RNA产生的条件。我们创建了一个表达系统和纯化方法,用此方法我们能生产克级量的高度纯化的Qβ复制酶,并且我们已经确定了在不含有添加RNA的测定中防止RNA扩增的反应条件。然而,当这些反应条件放宽时,在高达100%的测定中会出现自发RNA复制。为了了解这种RNA的来源,我们克隆了几种自发产生的RNA。对其中一种RNA的序列分析表明,它是由大肠杆菌tRNA进化成可复制模板而产生的,而不是由反应中的核苷三磷酸从头合成产生的。

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