| Literature DB >> 28968490 |
Hua Bai1,2, Aihua Deng1, Shuwen Liu1, Di Cui1,2, Qidi Qiu1,2, Laiyou Wang1,2, Zhao Yang1, Jie Wu1, Xiuling Shang1, Yun Zhang1, Tingyi Wen1,3.
Abstract
Scarless genetic manipulation of genomes is an essential tool for biological research. The restriction-modification (R-M) system is a defense system in bacteria that protects against invading genomes on the basis of its ability to distinguish foreign DNA from self DNA. Here, we designed an R-M system-mediated genome editing (RMGE) technique for scarless genetic manipulation in different microorganisms. For bacteria with Type IV REase, an RMGE technique using the inducible DNA methyltransferase gene, bceSIIM (RMGE-bceSIIM), as the counter-selection cassette was developed to edit the genome of Escherichia coli. For bacteria without Type IV REase, an RMGE technique based on a restriction endonuclease (RMGE-mcrA) was established in Bacillus subtilis. These techniques were successfully used for gene deletion and replacement with nearly 100% counter-selection efficiencies, which were higher and more stable compared to conventional methods. Furthermore, precise point mutation without limiting sites was achieved in E. coli using RMGE-bceSIIM to introduce a single base mutation of A128C into the rpsL gene. In addition, the RMGE-mcrA technique was applied to delete the CAN1 gene in Saccharomyces cerevisiae DAY414 with 100% counter-selection efficiency. The effectiveness of the RMGE technique in E. coli, B. subtilis, and S. cerevisiae suggests the potential universal usefulness of this technique for microbial genome manipulation.Entities:
Keywords: Bacillus subtilis; Escherichia coli; Saccharomyces cerevisiae; counter-selection cassette; restriction-modification (R-M) system; scarless genome editing
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Year: 2017 PMID: 28968490 DOI: 10.1021/acssynbio.7b00254
Source DB: PubMed Journal: ACS Synth Biol ISSN: 2161-5063 Impact factor: 5.110