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利用 T4 复制体进行等温 DNA 扩增:环形切口内切酶依赖性扩增和基于引物酶的全基因组扩增。

Isothermal DNA amplification using the T4 replisome: circular nicking endonuclease-dependent amplification and primase-based whole-genome amplification.

机构信息

Department of Biochemistry, University of Cambridge, Cambridge, UK.

出版信息

Nucleic Acids Res. 2010 Dec;38(22):e201. doi: 10.1093/nar/gkq795. Epub 2010 Oct 4.

Abstract

In vitro reconstitution of the bacteriophage T4 replication machinery provides a novel system for fast and processive isothermal DNA amplification. We have characterized this system in two formats: (i) in circular nicking endonuclease-dependent amplification (cNDA), the T4 replisome is supplemented with a nicking endonuclease (Nb.BbvCI) and a reverse primer to generate a well-defined uniform double-stranded linear product and to achieve up to 1100-fold linear amplification of a plasmid in 1 h. (ii) The T4 replisome with its primase (gp61) can also support priming and exponential amplification of genomic DNA in primase-based whole-genome amplification (T4 pWGA). Low amplification biases between 4.8 and 9.8 among eight loci for 0.3-10 ng template DNA suggest that this method is indeed suitable for uniform whole-genome amplification. Finally, the utility of the T4 replisome for isothermal DNA amplification is demonstrated in various applications, including incorporation of functional tags for DNA labeling and immobilization; template generation for in vitro transcription/translation and sequencing; and colony screening and DNA quantification.

摘要

体外重建噬菌体 T4 复制机制为快速、连续的等温 DNA 扩增提供了一种新系统。我们以两种形式对该系统进行了特征描述:(i)在环形切口内切酶依赖性扩增(cNDA)中,T4 复制体与切口内切酶(Nb.BbvCI)和反向引物一起补充,以产生明确定义的均匀双链线性产物,并在 1 小时内实现质粒的高达 1100 倍的线性扩增。(ii)T4 复制体及其引发酶(gp61)也可以在基于引发酶的全基因组扩增(T4 pWGA)中支持基因组 DNA 的引发和指数扩增。在模板 DNA 为 0.3-10ng 时,8 个基因座之间的扩增偏差低至 4.8 至 9.8,表明该方法确实适用于均匀的全基因组扩增。最后,T4 复制体在各种应用中的等温 DNA 扩增的实用性得到了证明,包括用于 DNA 标记和固定的功能标签的掺入;体外转录/翻译和测序的模板生成;以及菌落筛选和 DNA 定量。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8b8f/3001092/32ecd06556f7/gkq795f1.jpg

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