CRISPR-Cas9-based mutagenesis frequently provokes on-target mRNA misregulation

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Rubina Tuladhar
Yunku Yeu
John Tyler Piazza
Zhen Tan
Jean Rene Clemenceau
Xiaofeng Wu
Quinn Barrett
Jeremiah Herbert
David H. Mathews
James Kim
Tae Hyun Hwang
Lawrence Lum
机构
[1] University of Texas Southwestern Medical Center,Department of Cell Biology
[2] Cleveland Clinic Lerner Research Institute,Department of Quantitative Health Sciences
[3] University of Rochester Medical Center,Department of Biochemistry and Biophysics
[4] University of Texas Southwestern Medical Center,Department of Internal Medicine
[5] University of Texas Southwestern Medical Center,Hamon Center for Therapeutic Oncology Research Department of Biochemistry
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The introduction of insertion-deletions (INDELs) by non-homologous end-joining (NHEJ) pathway underlies the mechanistic basis of CRISPR-Cas9-directed genome editing. Selective gene ablation using CRISPR-Cas9 is achieved by installation of a premature termination codon (PTC) from a frameshift-inducing INDEL that elicits nonsense-mediated decay (NMD) of the mutant mRNA. Here, by examining the mRNA and protein products of CRISPR targeted genes in a cell line panel with presumed gene knockouts, we detect the production of foreign mRNAs or proteins in ~50% of the cell lines. We demonstrate that these aberrant protein products stem from the introduction of INDELs that promote internal ribosomal entry, convert pseudo-mRNAs (alternatively spliced mRNAs with a PTC) into protein encoding molecules, or induce exon skipping by disruption of exon splicing enhancers (ESEs). Our results reveal challenges to manipulating gene expression outcomes using INDEL-based mutagenesis and strategies useful in mitigating their impact on intended genome-editing outcomes.
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