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Programmable transcriptional repression in mycobacteria using an orthogonal CRISPR interference platform.

Nat Microbiol. 2017; 
RockJeremy M,HopkinsForrest F,ChavezAlejandro,DialloMarieme,ChaseMichael R,GerrickElias R,PritchardJustin R,ChurchGeorge M,RubinEric J,SassettiChristopher M,SchnappingerDirk,FortuneSar
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Codon Optimization Cas9 nuclease activity was inactivated by making the homologous D10A and H840A (S. pyogenes numbering) mutations in the RuvC and HNH nuclease domains foreach Cas9 protein. dcas9 alleles were then codon optimized for mycobacterial expression with Jcat (ref. 43) and synthesized by Genscript. Get A Quote

摘要

The development of new drug regimens that allow rapid, sterilizing treatment of tuberculosis has been limited by the complexity and time required for genetic manipulations in Mycobacterium tuberculosis. CRISPR interference (CRISPRi) promises to be a robust, easily engineered and scalable platform for regulated gene silencing. However, in M. tuberculosis, the existing Streptococcus pyogenes Cas9-based CRISPRi system is of limited utility because of relatively poor knockdown efficiency and proteotoxicity. To address these limitations, we screened eleven diverse Cas9 orthologues and identified four that are broadly functional for targeted gene knockdown in mycobacteria. The most efficacious of these prot... More

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