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. 2017 Jun;14(6):600-606.
doi: 10.1038/nmeth.4284. Epub 2017 May 1.

Mapping the genomic landscape of CRISPR-Cas9 cleavage

Peter Cameron  1 Chris K Fuller  1 Paul D Donohoue  1 Brittnee N Jones  1 Matthew S Thompson  1 Matthew M Carter  1 Scott Gradia  1 Bastien Vidal  1 Elizabeth Garner  1 Euan M Slorach  1 Elaine Lau  1 Lynda M Banh  1 Alexandra M Lied  1 Leslie S Edwards  1 Alexander H Settle  1 Daniel Capurso  1 Victor Llaca  2 Stéphane Deschamps  2 Mark Cigan  2 Joshua K Young  2 Andrew P May  1
Affiliations

Mapping the genomic landscape of CRISPR-Cas9 cleavage

Peter Cameron et al. Nat Methods. 2017 Jun.

Erratum in

  • Author Correction: Mapping the genomic landscape of CRISPR-Cas9 cleavage.
    Cameron P, Fuller CK, Donohoue PD, Jones BN, Thompson MS, Carter MM, Gradia S, Vidal B, Garner E, Slorach EM, Lau E, Banh LM, Lied AM, Edwards LS, Settle AH, Capurso D, Llaca V, Deschamps S, Cigan M, Young JK, May AP. Cameron P, et al. Nat Methods. 2023 Dec;20(12):2068. doi: 10.1038/s41592-023-02114-4. Nat Methods. 2023. PMID: 37945910 No abstract available.

Abstract

RNA-guided CRISPR-Cas9 endonucleases are widely used for genome engineering, but our understanding of Cas9 specificity remains incomplete. Here, we developed a biochemical method (SITE-Seq), using Cas9 programmed with single-guide RNAs (sgRNAs), to identify the sequence of cut sites within genomic DNA. Cells edited with the same Cas9-sgRNA complexes are then assayed for mutations at each cut site using amplicon sequencing. We used SITE-Seq to examine Cas9 specificity with sgRNAs targeting the human genome. The number of sites identified depended on sgRNA sequence and nuclease concentration. Sites identified at lower concentrations showed a higher propensity for off-target mutations in cells. The list of off-target sites showing activity in cells was influenced by sgRNP delivery, cell type and duration of exposure to the nuclease. Collectively, our results underscore the utility of combining comprehensive biochemical identification of off-target sites with independent cell-based measurements of activity at those sites when assessing nuclease activity and specificity.

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