Expanding the Drosophila toolkit for dual control of gene expression

Author:

Zirin Jonathan1ORCID,Jusiak Barbara2ORCID,Lopes Raphael1,Ewen-Campen Benjamin1,Bosch Justin A1ORCID,Risbeck Alexandria1,Forman Corey1,Villalta Christians1,Hu Yanhui1,Perrimon Norbert13ORCID

Affiliation:

1. Department of Genetics, Harvard Medical School

2. Department of Physiology and Biophysics, University of California, Irvine

3. Howard Hughes Medical Institute

Abstract

The ability to independently control gene expression in two different tissues in the same animal is emerging as a major need, especially in the context of inter-organ communication studies. This type of study is made possible by technologies combining the GAL4/UAS and a second binary expression system such as the LexA system or QF system. Here, we describe a resource of reagents that facilitate combined use of the GAL4/UAS and a second binary system in various Drosophila tissues. Focusing on genes with well-characterized GAL4 expression patterns, we generated a set of more than 40 LexA-GAD and QF2 insertions by CRISPR knock-in and verified their tissue specificity in larvae. We also built constructs that encode QF2 and LexA-GAD transcription factors in a single vector. Following successful integration of this construct into the fly genome, FLP/FRT recombination is used to isolate fly lines that express only QF2 or LexA-GAD. Finally, using new compatible shRNA vectors, we evaluated both LexA and QF systems for in vivo gene knockdown and are generating a library of such RNAi fly lines as a community resource. Together, these LexA and QF system vectors and fly lines will provide a new set of tools for researchers who need to activate or repress two different genes in an orthogonal manner in the same animal.

Funder

National Institute of General Medical Sciences

NIH Office of the Director

Damon Runyon Cancer Research Foundation

Howard Hughes Medical Institute

Publisher

eLife Sciences Publications, Ltd

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