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均聚物尾巴介导的连接 PCR:一种用于 DNA 克隆和文库构建的简化、高效的方法。

Homopolymer tail-mediated ligation PCR: a streamlined and highly efficient method for DNA cloning and library construction.

机构信息

Department of Molecular Biology and Microbiology, Tufts University School of Medicine, Boston, MA 02111, USA.

出版信息

Biotechniques. 2013 Jan;54(1):25-34. doi: 10.2144/000113981.

Abstract

The amplification of DNA fragments, cloned between user-defined 5' and 3' end sequences, is a prerequisite step in the use of many current applications including massively parallel sequencing (MPS). Here we describe an improved method, called homopolymer tail-mediated ligation PCR (HTML-PCR), that requires very little starting template, minimal hands-on effort, is cost-effective, and is suited for use in high-throughput and robotic methodologies. HTML-PCR starts with the addition of homopolymer tails of controlled lengths to the 3' termini of a double-stranded genomic template. The homopolymer tails enable the annealing-assisted ligation of a hybrid oligonucleotide to the template's recessed 5' ends. The hybrid oligonucleotide has a user-defined sequence at its 5' end. This primer, together with a second primer composed of a longer region complementary to the homopolymer tail and fused to a second 5' user-defined sequence, are used in a PCR reaction to generate the final product. The user-defined sequences can be varied to enable compatibility with a wide variety of downstream applications. We demonstrate our new method by constructing MPS libraries starting from nanogram and sub-nanogram quantities of Vibrio cholerae and Streptococcus pneumoniae genomic DNA.

摘要

在使用许多当前应用程序(包括大规模平行测序(MPS))中,用户定义的 5'和 3'末端序列之间克隆的 DNA 片段的扩增是前提步骤。在这里,我们描述了一种称为同源多聚尾介导连接 PCR(HTML-PCR)的改进方法,该方法需要很少的起始模板,很少的手工操作,具有成本效益,并且适合高通量和机器人方法学使用。HTML-PCR 首先在双链基因组模板的 3'末端添加长度受控的同源多聚尾。同源多聚尾允许退火辅助连接杂交寡核苷酸到模板的凹入 5'末端。该杂交寡核苷酸在其 5'末端具有用户定义的序列。该引物与第二引物一起使用,第二引物由与同源多聚尾互补的较长区域组成,并融合到第二 5'用户定义序列,用于 PCR 反应以生成最终产物。用户定义的序列可以改变以实现与各种下游应用程序的兼容性。我们通过从纳米克和亚纳克数量的霍乱弧菌和肺炎链球菌基因组 DNA 开始构建 MPS 文库来证明我们的新方法。

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