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Engineering of bacteriophage T4 genome using CRISPR-Cas9

Synthetic Biology. 2017; 
Pan Tao,* Xiaorong Wu, Wei-Chun Tang, Jingen Zhu, and Venigalla Rao*
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Gene Synthesis A DNA fragment containing a multiple mutations in the g56 gene between amino acids 121 and 158 was synthesized by Genscript (Piscataway, NJ). The DNA was inserted into the pET-28b DNA linearized with BglII and BamHI to generate the g56 donor plasmid. Get A Quote

摘要

: Bacteriophages likely constitute the largest biomass on Earth. However, very few phage genomes have been well-characterized, the tailed phage T4 genome being one of them. Even in T4, much of the genome remained uncharacterized. The classical genetic strategies are tedious, compounded by genome modifications such as cytosine hydroxylmethylation and glucosylation which makes T4 DNA resistant to most restriction endonucleases. Here, using the type-II CRISPR-Cas9 system, we report the editing of both modified (ghm-Cytosine) and unmodified (Cytosine) T4 genomes. The modified genome, however, is less susceptible to Cas9 nuclease attack when compared to the unmodified genome. The efficiency of restriction of modifie... More

关键词

: genome engineering, T4 bacteriophage, CRISPR, Cas9 nuclease, genome editing