Your search keyword '"WRPW"' showing total 2 results

1. Evidence That Runt Acts as a Counter-Repressor of Groucho During Drosophila melanogaster Primary Sex Determination

Author

Young-Ho Jung, James W. Erickson, and Sharvani Mahadeveraju

Subjects

Male, Core Binding Factor alpha Subunits, X-signal element, Repressor, QH426-470, Genetic Switch, X-chromosome counting, WRPW, 03 medical and health sciences, 0302 clinical medicine, WRPY, Genetics, Animals, Drosophila Proteins, X:A ratio, Promoter Regions, Genetic, Molecular Biology, Transcription factor, Genetics (clinical), 030304 developmental biology, Regulator gene, 0303 health sciences, biology, Runt, Gene Expression Regulation, Developmental, RNA-Binding Proteins, biology.organism_classification, Cell biology, deadpan, Genetics of Sex, Drosophila melanogaster, 030220 oncology & carcinogenesis, Primary sex determination, Female, Transcription Factors

Abstract

Runx proteins are bifunctional transcription factors that both repress and activate transcription in animal cells. Typically, Runx proteins work in concert with other transcriptional regulators, including co-activators and co-repressors to mediate their biological effects. In Drosophila melanogaster the archetypal Runx protein, Runt, functions in numerous processes including segmentation, neurogenesis and sex determination. During primary sex determination Runt acts as one of four X-linked signal element (XSE) proteins that direct female-specific activation of the establishment promoter (Pe) of the master regulatory gene Sex-lethal (Sxl). Successful activation of SxlPe requires that the XSE proteins overcome the repressive effects of maternally deposited Groucho (Gro), a potent co-repressor of the Gro/TLE family. Runx proteins, including Runt, contain a C-terminal peptide, VWRPY, known to bind to Gro/TLE proteins to mediate transcriptional repression. We show that Runt’s VWRPY co-repressor-interaction domain is needed for Runt to activate SxlPe. Deletion of the Gro-interaction domain eliminates Runt-ability to activate SxlPe, whereas replacement with a higher affinity, VWRPW, sequence promotes Runt-mediated transcription. This suggests that Runt may activate SxlPe by antagonizing Gro function, a conclusion consistent with earlier findings that Runt is needed for Sxl expression only in embryonic regions with high Gro activity. Surprisingly we found that Runt is not required for the initial activation of SxlPe. Instead, Runt is needed to keep SxlPe active during the subsequent period of high-level Sxl transcription suggesting that Runt helps amplify the difference between female and male XSE signals by counter-repressing Gro in female, but not in male, embryos.

Published

2020

2. Maternal Groucho and bHLH repressors amplify the dose-sensitive X chromosome signal in Drosophila sex determination

Author

Sharvani Mahadevaraju, Frank W. Avila, Hong Lu, Dun Yang, Elena Kozhina, and James W. Erickson

Subjects

Genetic switch, Embryo, Nonmammalian, Time Factors, X Chromosome, Molecular Sequence Data, Repressor, Models, Biological, Article, WRPW, Dosage Compensation, Genetic, Basic Helix-Loop-Helix Transcription Factors, Animals, Drosophila Proteins, X chromosome-counting, X:A ratio, Transgenes, Promoter Regions, Genetic, Psychological repression, Molecular Biology, X chromosome, Genetics, Dosage compensation, Binding Sites, biology, Scute, Base Sequence, Gene Expression Regulation, Developmental, Nuclear Proteins, RNA-Binding Proteins, Hes, Cell Biology, Sex Determination Processes, biology.organism_classification, Helix–loop–helix, Repression, DNA-Binding Proteins, Repressor Proteins, Drosophila melanogaster, Mutation, Female, Corepressor, Drosophila Protein, Developmental Biology, Protein Binding

Abstract

In Drosophila, XX embryos are fated to develop as females, and XY embryos as males, because the diplo-X dose of four X-linked signal element genes, XSEs, activates the Sex-lethal establishment promoter, SxlPe, whereas the haplo-X XSE dose leaves SxlPe off. The threshold response of SxlPe to XSE concentrations depends in part on the bHLH repressor, Deadpan, present in equal amounts in XX and XY embryos. We identified canonical and non-canonical DNA-binding sites for Dpn at SxlPe and found that cis-acting mutations in the Dpn-binding sites caused stronger and earlier Sxl expression than did deletion of dpn implicating other bHLH repressors in Sxl regulation. Maternal Hey encodes one such bHLH regulator but the E(spl) locus does not. Elimination of the maternal corepressor Groucho also caused strong ectopic Sxl expression in XY, and premature Sxl activation in XX embryos, but Sxl was still expressed differently in the sexes. Our findings suggest that Groucho and associated maternal and zygotic bHLH repressors define the threshold XSE concentrations needed to activate SxlPe and that they participate directly in sex signal amplification. We present a model in which the XSE signal is amplified by a feedback mechanism that interferes with Gro-mediated repression in XX, but not XY embryos.

Published

2008