噬菌体λ DNA 在体外的整合重组

Integrative recombination of bacteriophage lambda DNA in vitro.

作者信息

Nash H A

出版信息

Proc Natl Acad Sci U S A. 1975 Mar;72(3):1072-6. doi: 10.1073/pnas.72.3.1072.

DOI:10.1073/pnas.72.3.1072

PMID:1055366

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC432468/

Abstract

An in vitro system for the production of integrative recombinant DNA of bacteriophage lambda is described. The in vitro recombination mimics the in vivo integration of viral DNA into host DNA in its requirement for int gene product, for the presence of a thermolabile component, and for the limitation of the recombination to a pair of specialized sites (attachment sites) on the DNA. The enzymes are extracted from Escherichia coli containing phage lambda gene products. The substrate is the DNA from lambda-attB-attP, a phage variant that contains two attachment sites on the same chromosome. The product is a recombinant phage chromosome that has lost the DNA between the attachment sites. The parental and recombinant DNA are distinguished following transfection to mature phage in spheroplasts. The reaction requires ATP, Mg++, spermidine, and a monovalent cation. Recombination occurs preferentially between attachment sites on the same molecule. The enzymatic activity is completely inhibited by extracts containing xis gene product.

摘要

本文描述了一种用于产生噬菌体λ整合重组DNA的体外系统。该体外重组在对int基因产物的需求、对热不稳定成分的存在以及对重组限于DNA上一对特定位点（附着位点）方面，模拟了病毒DNA在体内整合到宿主DNA的过程。这些酶是从含有噬菌体λ基因产物的大肠杆菌中提取的。底物是来自λ-attB-attP的DNA，这是一种在同一染色体上含有两个附着位点的噬菌体变体。产物是一个在附着位点之间丢失了DNA的重组噬菌体染色体。通过转染到原生质体中形成成熟噬菌体后，可区分亲本DNA和重组DNA。该反应需要ATP、Mg++、亚精胺和一价阳离子。重组优先发生在同一分子上的附着位点之间。含有xis基因产物的提取物可完全抑制酶活性。

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本文引用的文献

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Plasmid ColEl as a molecular vehicle for cloning and amplification of DNA.质粒ColE1作为用于DNA克隆和扩增的分子载体。

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Genome construction between bacterial species in vitro: replication and expression of Staphylococcus plasmid genes in Escherichia coli.体外细菌种间基因组构建：葡萄球菌质粒基因在大肠杆菌中的复制与表达

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