A Highly Efficient CRISPR-Cas9-Mediated Large Genomic Deletion in Bacillus subtilis

被引:64
|
作者
So, Younju [1 ,2 ]
Park, Soo-Young [3 ]
Park, Eun-Hye [3 ]
Park, Seung-Hwan [1 ,2 ]
Kim, Eui-Joong [3 ]
Pan, Jae-Gu [1 ]
Choi, Soo-Keun [1 ,2 ]
机构
[1] Korea Res Inst Biosci & Biotechnol, Infect Dis Res Ctr, Daejeon, South Korea
[2] Korea Univ Sci & Technol UST, KRIBB Sch Biotechnol, Dept Biosyst & Bioengn, Daejeon, South Korea
[3] Genofocus Inc, Daejeon, South Korea
来源
关键词
CRISPR-Cas9; Bacillus subtilis; genome engineering; large genomic deletion; genomic point mutation; gene insertion; MARKER-FREE DELETIONS; CRISPR-CAS SYSTEMS; HETEROLOGOUS HOST; ESCHERICHIA-COLI; PLASMID; RNA; DNA; PROMOTER; VECTOR;
D O I
10.3389/fmicb.2017.01167
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
In Bacillus subtilis, large genomic deletions have been carried out for genome reduction, antibiotic overproduction, and heterologous protein overexpression. In view of the eco-friendliness of B. subtilis, it is critical that engineering preserves its food-grade status and avoids leaving foreign DNA in the genome. Existing methods of generating large genomic deletions leave antibiotic resistance markers or display low mutation efficiency. In this study, we introduced a clustered regularly interspaced short palindromic repeat-derived genome engineering technique to develop a highly efficient method of generating large genomic deletions in B. subtilis without any trace of foreign DNA. Using our system, we produced 38 kb plipastatin-synthesizing pps operon deletion with 80% efficiency. The significant increase in mutation efficiency was due to plasmids-delivered Streptococcus pyogenes-originated SpCas9, target-specific sgRNA and a donor DNA template, which produces SpCas9/sgRNA endonuclease complex continuously for attacking target chromosome until the mutagenic repair occurs. Our system produced single-gene deletion in spo0A (similar to 100%), point mutation (similar to 68%) and GFP gene insertion (similar to 97%) in sigE and demonstrated its broad applicability for various types of site-directed mutagenesis in B. subtilis.
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收藏
页数:12
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