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利用CRISPR-Cas系统筛选基因编辑噬菌体

Selection of Genetically Modified Bacteriophages Using the CRISPR-Cas System.

作者信息

Manor Miriam, Qimron Udi

机构信息

Department of Clinical Microbiology and Immunology, Sackler School of Medicine, Tel Aviv University, Tel Aviv, Israel.

出版信息

Bio Protoc. 2017 Aug 5;7(15). doi: 10.21769/BioProtoc.2431.

DOI:10.21769/BioProtoc.2431
PMID:28804739
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5553622/
Abstract

We present a CRISPR-Cas based technique for deleting genes from the T7 bacteriophage genome. A DNA fragment encoding homologous arms to the target gene to be deleted is first cloned into a plasmid. The T7 phage is then propagated in harboring this plasmid. During this propagation, some phage genomes undergo homologous recombination with the plasmid, thus deleting the targeted gene. To select for these genomes, the CRISPR-Cas system is used to cleave non-edited genomes, enabling isolation of the desired recombinant phages. This protocol allows seamless deletion of desired genes in a T7 phage, and can be expanded to other phages and other types of genetic manipulations as well.

摘要

我们提出了一种基于CRISPR-Cas的技术,用于从T7噬菌体基因组中删除基因。首先将编码与待删除靶基因同源臂的DNA片段克隆到质粒中。然后让T7噬菌体在含有该质粒的宿主中繁殖。在这个繁殖过程中,一些噬菌体基因组会与质粒进行同源重组,从而删除目标基因。为了筛选这些基因组,使用CRISPR-Cas系统切割未编辑的基因组,从而能够分离出所需的重组噬菌体。该方案允许在T7噬菌体中无缝删除所需基因,并且也可以扩展到其他噬菌体和其他类型的基因操作。

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