Evaluation of CRISPR gene-editing tools in zebrafish

José M Uribe-Salazar; Gulhan Kaya; Aadithya Sekar; KaeChandra Weyenberg; Cole Ingamells; Megan Y Dennis

doi:10.1186/s12864-021-08238-1

Evaluation of CRISPR gene-editing tools in zebrafish

BMC Genomics. 2022 Jan 6;23(1):12. doi: 10.1186/s12864-021-08238-1.

Authors

José M Uribe-Salazar^{1

2}, Gulhan Kaya¹, Aadithya Sekar¹, KaeChandra Weyenberg¹, Cole Ingamells¹, Megan Y Dennis^{3

4}

Affiliations

¹ Genome Center, MIND Institute, and Department of Biochemistry & Molecular Medicine, School of Medicine, University of California, Davis, Davis, CA, USA.
² Integrative Genetics and Genomics Graduate Group, University of California, Davis, Davis, CA, USA.
³ Genome Center, MIND Institute, and Department of Biochemistry & Molecular Medicine, School of Medicine, University of California, Davis, Davis, CA, USA. mydennis@ucdavis.edu.
⁴ Integrative Genetics and Genomics Graduate Group, University of California, Davis, Davis, CA, USA. mydennis@ucdavis.edu.

Abstract

Background: Zebrafish have practical features that make them a useful model for higher-throughput tests of gene function using CRISPR/Cas9 editing to create 'knockout' models. In particular, the use of G₀ mosaic mutants has potential to increase throughput of functional studies significantly but may suffer from transient effects of introducing Cas9 via microinjection. Further, a large number of computational and empirical tools exist to design CRISPR assays but often produce varied predictions across methods leaving uncertainty in choosing an optimal approach for zebrafish studies.

Methods: To systematically assess accuracy of tool predictions of on- and off-target gene editing, we subjected zebrafish embryos to CRISPR/Cas9 with 50 different guide RNAs (gRNAs) targeting 14 genes. We also investigate potential confounders of G₀-based CRISPR screens by assaying control embryos for spurious mutations and altered gene expression.

Results: We compared our experimental in vivo editing efficiencies in mosaic G₀ embryos with those predicted by eight commonly used gRNA design tools and found large discrepancies between methods. Assessing off-target mutations (predicted in silico and in vitro) found that the majority of tested loci had low in vivo frequencies (< 1%). To characterize if commonly used 'mock' CRISPR controls (larvae injected with Cas9 enzyme or mRNA with no gRNA) exhibited spurious molecular features that might exacerbate studies of G₀ mosaic CRISPR knockout fish, we generated an RNA-seq dataset of various control larvae at 5 days post fertilization. While we found no evidence of spontaneous somatic mutations of injected larvae, we did identify several hundred differentially-expressed genes with high variability between injection types. Network analyses of shared differentially-expressed genes in the 'mock' injected larvae implicated a number of key regulators of common metabolic pathways, and gene-ontology analysis revealed connections with response to wounding and cytoskeleton organization, highlighting a potentially lasting effect from the microinjection process that requires further investigation.

Conclusion: Overall, our results provide a valuable resource for the zebrafish community for the design and execution of CRISPR/Cas9 experiments.

Keywords: CIRCLE-seq; CRISPR; Cas9; Danio rerio; Gene knockout; RNA-seq; Zebrafish.

MeSH terms

Animals
CRISPR-Associated Protein 9 / genetics
CRISPR-Cas Systems / genetics
Gene Editing*
RNA, Guide, CRISPR-Cas Systems / genetics
Zebrafish* / genetics

Substances

RNA, Guide, CRISPR-Cas Systems
CRISPR-Associated Protein 9

Grants and funding

DP2 MH119424/MH/NIMH NIH HHS/United States