A cytological F1 RNAi screen for defects in Drosophila melanogaster female meiosis

Author:

Gilliland William D1ORCID,May Dennis P1,Bowen Amelia O1,Conger Kelly O1,Elrad Doreen1,Marciniak Marcin1,Mashburn Sarah A1,Presbitero Gabrielle1,Welk Lucas F1

Affiliation:

1. Department of Biological Sciences, DePaul University , Chicago, IL 60614 , USA

Abstract

Abstract Genetic screens for recessive alleles induce mutations, make the mutated chromosomes homozygous, and then assay those homozygotes for the phenotype of interest. When screening for genes required for female meiosis, the phenotype of interest has typically been nondisjunction from chromosome segregation errors. As this requires that mutant females be viable and fertile, any mutants that are lethal or sterile when homozygous cannot be recovered by this approach. To overcome these limitations, we have screened the VALIUM22 collection of RNAi constructs that target germline-expressing genes in a vector optimized for germline expression by driving RNAi with GAL4 under control of a germline-specific promoter (nanos or mat-alpha4). This allowed us to test genes that would be lethal if knocked down in all cells, and by examining unfertilized metaphase-arrested mature oocytes, we could identify defects in sterile females. After screening >1,450 lines of the collection for two different defects (chromosome congression and the hypoxic sequestration of Mps1-GFP to ooplasmic filaments), we obtained multiple hits for both phenotypes, identified novel meiotic phenotypes for genes that had been previously characterized in other processes, and identified the first phenotypes to be associated with several previously uncharacterized genes.

Funder

NIH

NIGMS

Publisher

Oxford University Press (OUP)

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