重叠延伸 PCR 克隆:一种创建重组质粒的简单可靠方法。
Overlap extension PCR cloning: a simple and reliable way to create recombinant plasmids.
机构信息
Department of Biochemistry, Center for Fundamental and Applied Molecular Evolution, Emory University, Atlanta, Georgia 30322, USA.
出版信息
Biotechniques. 2010 Jun;48(6):463-5. doi: 10.2144/000113418.
Abstract
Here we describe a straightforward, efficient, and reliable way to clone an insert of choice into a plasmid of choice without restriction endonucleases or T4 DNA ligase. Chimeric primers containing plasmid sequence at the 5' ends and insert sequence at the 3' ends were used to PCR-amplify insertion sequences of various sizes, namely the genes for GFP (gfp), beta-d-glucuronidase (gusA), and beta-galactosidase (lacZ), as well as the entire luxABCDE operon. These inserts were employed as mega-primers in a second PCR with a circular plasmid template. The original plasmid templates were then destroyed in restriction digests with DpnI, and the overlap extension PCR products were used to transform competent Escherichia coli cells. Phusion DNA polymerase was used for the amplification and fusion reactions, so both reactions were easy to monitor and optimize.
摘要
在这里,我们描述了一种简单、高效、可靠的方法,无需限制酶或 T4 DNA 连接酶,即可将选择的插入片段克隆到选择的质粒中。在 5' 端含有质粒序列,在 3' 端含有插入序列的嵌合引物被用于 PCR 扩增各种大小的插入序列,即 GFP(gfp)、β-d-葡萄糖醛酸酶(gusA)和β-半乳糖苷酶(lacZ)的基因,以及整个 luxABCDE 操纵子。这些插入物被用作第二轮 PCR 的 mega-引物,使用环状质粒模板。然后用 DpnI 进行限制消化破坏原始质粒模板,并将重叠延伸 PCR 产物用于转化感受态大肠杆菌细胞。Phusion DNA 聚合酶用于扩增和融合反应,因此这两个反应都很容易监测和优化。
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