4.3 Article

A Versatile Two-Step CRISPR- and RMCE-Based Strategy for Efficient Genome Engineering in Drosophila

Journal

G3-GENES GENOMES GENETICS
Volume 4, Issue 12, Pages 2409-2418

Publisher

GENETICS SOCIETY AMERICA
DOI: 10.1534/g3.114.013979

Keywords

Drosophila; CRISPR/Cas9; homologous recombination; RMCE; muscle

Funding

  1. Max Planck Society, a Career Development Award from the Human Frontier Science Program
  2. EMBO
  3. European Research Council under European Union/ERC [310939]
  4. European Research Council (ERC) [310939] Funding Source: European Research Council (ERC)

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The development of clustered, regularly interspaced, short palindromic repeats (CRISPR)/CRISPR-associated (Cas) technologies promises a quantum leap in genome engineering of model organisms. However, CRISPR-mediated gene targeting reports in Drosophila melanogaster are still restricted to a few genes, use variable experimental conditions, and vary in efficiency, questioning the universal applicability of the method. Here, we developed an efficient two-step strategy to flexibly engineer the fly genome by combining CRISPR with recombinase-mediated cassette exchange (RMCE). In the first step, two sgRNAs, whose activity had been tested in cell culture, were co-injected together with a donor plasmid into transgenic Act5C-Cas9, Ligase4 mutant embryos and the homologous integration events were identified by eye fluorescence. In the second step, the eye marker was replaced with DNA sequences of choice using RMCE enabling flexible gene modification. We applied this strategy to engineer four different locations in the genome, including a gene on the fourth chromosome, at comparably high efficiencies. Our data suggest that any fly laboratory can engineer their favorite gene for a broad range of applications within approximately 3 months.

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