Captured Segment Exchange: A Strategy for Custom Engineering Large Genomic Regions in Drosophila melanogaster

Author:

Bateman Jack R1,Palopoli Michael F1,Dale Sarah T1,Stauffer Jennifer E1,Shah Anita L1,Johnson Justine E1,Walsh Conor W1,Flaten Hanna1,Parsons Christine M1

Affiliation:

1. Biology Department, Bowdoin College, Brunswick, Maine 04011

Abstract

Abstract Site-specific recombinases (SSRs) are valuable tools for manipulating genomes. In Drosophila, thousands of transgenic insertions carrying SSR recognition sites have been distributed throughout the genome by several large-scale projects. Here we describe a method with the potential to use these insertions to make custom alterations to the Drosophila genome in vivo. Specifically, by employing recombineering techniques and a dual recombinase-mediated cassette exchange strategy based on the phiC31 integrase and FLP recombinase, we show that a large genomic segment that lies between two SSR recognition-site insertions can be “captured” as a target cassette and exchanged for a sequence that was engineered in bacterial cells. We demonstrate this approach by targeting a 50-kb segment spanning the tsh gene, replacing the existing segment with corresponding recombineered sequences through simple and efficient manipulations. Given the high density of SSR recognition-site insertions in Drosophila, our method affords a straightforward and highly efficient approach to explore gene function in situ for a substantial portion of the Drosophila genome.

Publisher

Oxford University Press (OUP)

Subject

Genetics

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