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An enhanced CRISPR repressor for targeted mammalian gene regulation.

Nat Methods

Authors	Nan Yeo Alejandro Chavez Alissa Lance-Byrne Yingleong Chan David Menn Denitsa Milanova Chih-Chung Kuo Xiaoge Guo Sumana Sharma Angela Tung Ryan Cecchi Marcelle Tuttle Swechchha Pradhan Elaine Lim Noah Davidsohn Mo Ebrahimkhani James Collins Nathan Lewis Samira Kiani George Church
Keywords	Humans Gene Expression Regulation Gene Silencing HEK293 Cells Repressor Proteins Recombinant Fusion Proteins RNA, Guide CRISPR-Cas Systems Genes, Synthetic Methyl-CpG-Binding Protein 2 CRISPR-Associated Protein 9
Abstract	The RNA-guided endonuclease Cas9 can be converted into a programmable transcriptional repressor, but inefficiencies in target-gene silencing have limited its utility. Here we describe an improved Cas9 repressor based on the C-terminal fusion of a rationally designed bipartite repressor domain, KRAB-MeCP2, to nuclease-dead Cas9. We demonstrate the system's superiority in silencing coding and noncoding genes, simultaneously repressing a series of target genes, improving the results of single and dual guide RNA library screens, and enabling new architectures of synthetic genetic circuits.
Year of Publication	2018
Journal	Nat Methods
Volume	15
Issue	8
Pages	611-616
Date Published	2018 08
ISSN	1548-7105
DOI	10.1038/s41592-018-0048-5
PubMed ID	30013045
PubMed Central ID	PMC6129399
Links
Grant list	P50 HG005550 / HG / NHGRI NIH HHS / United States R35 GM119850 / GM / NIGMS NIH HHS / United States RM1 HG008525 / HG / NHGRI NIH HHS / United States T32 CA009216 / CA / NCI NIH HHS / United States

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