4.7 Article

A CRISPR/Cas9 Vector System for Tissue-Specific Gene Disruption in Zebrafish

Journal

DEVELOPMENTAL CELL
Volume 32, Issue 6, Pages 756-764

Publisher

CELL PRESS
DOI: 10.1016/j.devcel.2015.01.032

Keywords

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Funding

  1. NIH [R01 CA103846, R01 HL04880, R01 DK53298, PO1 HL32262, P30 DK49216, U01 HL10001, R24 DK092760]
  2. European Molecular Biology Organization (EMBO) Long-Term Fellowship [EMBO ALTF 263-2013]
  3. NATIONAL CANCER INSTITUTE [R01CA103846] Funding Source: NIH RePORTER
  4. NATIONAL HEART, LUNG, AND BLOOD INSTITUTE [R01HL048801, P01HL032262, U01HL100001] Funding Source: NIH RePORTER
  5. NATIONAL INSTITUTE OF DIABETES AND DIGESTIVE AND KIDNEY DISEASES [R01DK053298, R24DK092760, P30DK049216] Funding Source: NIH RePORTER
  6. OFFICE OF THE DIRECTOR, NATIONAL INSTITUTES OF HEALTH [R24OD017870] Funding Source: NIH RePORTER

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CRISPR/Cas9 technology of genome editing has greatly facilitated the targeted inactivation of genes in vitro and in vivo in a wide range of organisms. In zebrafish, it allows the rapid generation of knockout lines by simply injecting a guide RNA (gRNA) and Cas9 mRNA into one-cell stage embryos. Here, we report a simple and scalable CRISPR-based vector system for tissue-specific gene inactivation in zebrafish. As proof of principle, we used our vector with the gata1 promoter driving Cas9 expression to silence the urod gene, implicated in heme biosynthesis, specifically in the erythrocytic lineage. Urod targeting yielded red fluorescent erythrocytes in zebrafish embryos, recapitulating the phenotype observed in the yquem mutant. While F0 embryos displayed mosaic gene disruption, the phenotype appeared very penetrant in stable F1 fish. This vector system constitutes a unique tool to spatially control gene knockout and greatly broadens the scope of loss-of-function studies in zebrafish.

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