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Effective Blocking of Microbial Transcriptional Initiation by dCas9-NG-Mediated CRISPR Interference

Authors
Kim, BumjoonKim, Hyun JuLee, Sang Jun
Issue Date
Dec-2020
Publisher
KOREAN SOC MICROBIOLOGY & BIOTECHNOLOGY
Keywords
CRISPR interference; PAM sequence; dCas9-NG; gal promoter; D-galactose
Citation
JOURNAL OF MICROBIOLOGY AND BIOTECHNOLOGY, v.30, no.12, pp 1919 - 1926
Pages
8
Journal Title
JOURNAL OF MICROBIOLOGY AND BIOTECHNOLOGY
Volume
30
Number
12
Start Page
1919
End Page
1926
URI
https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/48933
DOI
10.4014/jmb.2008.08058
ISSN
1017-7825
1738-8872
Abstract
CRISPR interference (CRISPRi) has been developed as a transcriptional control tool by inactivating the DNA cleavage ability of Cas9 nucleases to produce dCas9 (deactivated Cas9), and leaving dCas9 the ability to specifically bind to the target DNA sequence. CRISPR/Cas9 technology has limitations in designing target-specific single-guide RNA (sgRNA) due to the dependence of protospacer adjacent motif (PAM) (5'-NGG) for binding target DNAs. Reportedly, Cas9-NG recognizing 5'-NG as the PAM sequence has been constructed by removing the dependence on the last base G of PAM through protein engineering of Cas9. In this study, a dCas9-NG protein was engineered by introducing two active site mutations in Cas9-NG, and its ability to regulate transcription was evaluated in the gal promoter in E. coli. Analysis of cell growth rate, D-galactose consumption rate, and gal transcripts confirmed that dCas9-NG can completely repress the promoter by recognizing DNA targets with PAM of 5'-NGG, NGA, NGC, NGT, and NAG. Our study showed possible PAM sequences for dCas9-NG and provided information on target-specific sgRNA design for regulation of both gene expression and cellular metabolism.
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Lee, Sang Jun
생명공학대학 (시스템생명공학과)
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