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Rol; D) ecd1 29oC day 4; E) c587 alone 29oC day 8; F) c587::USP RNAi 29oC day 8; G) c587::EcR RNAi 29oC day 8; H) c587::E75 RNAi 29oC day 8. Green, somatic cells (anti-Tj), magenta, cell membranes and spectrosome/fusome (anti-Hts and anti-FasIII). I) Time course showing the number of GSCs present in germaria from controls and flies in which ecdysone signaling was AVP custom synthesis reduced for the duration shown as described. J-K) Control germaria usual have two to three GSCs (J, dashed outline), whereas c587:USP RNAi flies after 8 days at 29uC usually have only one (K, dashed outline), white: cell membranes and spectrosome/fusome (anti-Hts and anti-FasIII). Asterisk marks the position of the cap cells. L) The number of cap cells was counted in germaria from controls and flies in which ecdysone signaling was reduced for the duration shown. Cap cell number is not affected by reducing ecdysteroid signaling. Error bars indicate s.d. Scale 1326631 bar: 10 mm. doi:10.1371/journal.pone.0046109.gAs steroid hormone signaling is a key regulator of developmental transitions we investigated whether ecdysone controls events in early Drosophila oogenesis. We show that ecdysteroid signaling is important for several steps of early female gametogenesis downstream from the GSC including 16-cell cyst formation, meiotic entry, and follicle formation. Steroid signaling acts in the somatic cells enveloping germline cysts in females but not in structurally similar male somatic cells. Gametogenesis diverges in the two sexes during cyst formation. For example, male meiosis lacks recombination and requires male-specific cell cycle genes (reviewed in [19,20]). Our results argue that ecdysone-mediated signaling represents an early branch point between male and female germline development. Thus, in Drosophila, as well as mammals, sexually dimorphic steroid hormone signaling acts at the time development diverges between male and female germ cells.Results Early Oogenesis Requires Nuclear Hormone Receptor Function within Somatic CellsTo investigate whether ecdysone signaling is required for early oogenesis, we reduced whole fly hormone levels using a temperature sensitive ecdysoneless mutant (ecd1). ecd mutant flies were maintained at 18uC to provide essential signaling during development then moved to the restrictive temperature of 29uC, which reduces circulating ecdysone to 30 of wild-type levels [17]. Additionally, we used RNAi to knock down expression ofecdysone receptor genes (ultraspiracle, usp and the ecdysone receptor, EcR) or the early ecdysone effector gene (E75). To identify the ecdysone-responsive cell population, ecdysone-signaling Arg8-vasopressin site activity was reduced in a limited group of cells. Knock down was confined to escort and undifferentiated follicle cells by driving RNAi expression using a GAL4 driver line (c587) expressed in these somatic cell types but not in germ cells (Fig. S1A ). RNAi expression was prevented during development using a temperature sensitive gal80 repressor and by maintaining flies at 20oC. When adult animals were switched to 29uC for 8 days, RNAi-mediated gene knock down occurred in the somatic cells of the germarium. For example, the Usp co-receptor is expressed in both somatic and germ cells of the germarium (Fig. 1B). RNAi directed against Usp driven by the c587 GAL4 line eliminated Usp antibody staining specifically in somatic cells, but not germ cells (Fig. S1C, D). The effects on early oogenesis of reducing ecdysone synthesis or knocking down pathway recepto.Rol; D) ecd1 29oC day 4; E) c587 alone 29oC day 8; F) c587::USP RNAi 29oC day 8; G) c587::EcR RNAi 29oC day 8; H) c587::E75 RNAi 29oC day 8. Green, somatic cells (anti-Tj), magenta, cell membranes and spectrosome/fusome (anti-Hts and anti-FasIII). I) Time course showing the number of GSCs present in germaria from controls and flies in which ecdysone signaling was reduced for the duration shown as described. J-K) Control germaria usual have two to three GSCs (J, dashed outline), whereas c587:USP RNAi flies after 8 days at 29uC usually have only one (K, dashed outline), white: cell membranes and spectrosome/fusome (anti-Hts and anti-FasIII). Asterisk marks the position of the cap cells. L) The number of cap cells was counted in germaria from controls and flies in which ecdysone signaling was reduced for the duration shown. Cap cell number is not affected by reducing ecdysteroid signaling. Error bars indicate s.d. Scale 1326631 bar: 10 mm. doi:10.1371/journal.pone.0046109.gAs steroid hormone signaling is a key regulator of developmental transitions we investigated whether ecdysone controls events in early Drosophila oogenesis. We show that ecdysteroid signaling is important for several steps of early female gametogenesis downstream from the GSC including 16-cell cyst formation, meiotic entry, and follicle formation. Steroid signaling acts in the somatic cells enveloping germline cysts in females but not in structurally similar male somatic cells. Gametogenesis diverges in the two sexes during cyst formation. For example, male meiosis lacks recombination and requires male-specific cell cycle genes (reviewed in [19,20]). Our results argue that ecdysone-mediated signaling represents an early branch point between male and female germline development. Thus, in Drosophila, as well as mammals, sexually dimorphic steroid hormone signaling acts at the time development diverges between male and female germ cells.Results Early Oogenesis Requires Nuclear Hormone Receptor Function within Somatic CellsTo investigate whether ecdysone signaling is required for early oogenesis, we reduced whole fly hormone levels using a temperature sensitive ecdysoneless mutant (ecd1). ecd mutant flies were maintained at 18uC to provide essential signaling during development then moved to the restrictive temperature of 29uC, which reduces circulating ecdysone to 30 of wild-type levels [17]. Additionally, we used RNAi to knock down expression ofecdysone receptor genes (ultraspiracle, usp and the ecdysone receptor, EcR) or the early ecdysone effector gene (E75). To identify the ecdysone-responsive cell population, ecdysone-signaling activity was reduced in a limited group of cells. Knock down was confined to escort and undifferentiated follicle cells by driving RNAi expression using a GAL4 driver line (c587) expressed in these somatic cell types but not in germ cells (Fig. S1A ). RNAi expression was prevented during development using a temperature sensitive gal80 repressor and by maintaining flies at 20oC. When adult animals were switched to 29uC for 8 days, RNAi-mediated gene knock down occurred in the somatic cells of the germarium. For example, the Usp co-receptor is expressed in both somatic and germ cells of the germarium (Fig. 1B). RNAi directed against Usp driven by the c587 GAL4 line eliminated Usp antibody staining specifically in somatic cells, but not germ cells (Fig. S1C, D). The effects on early oogenesis of reducing ecdysone synthesis or knocking down pathway recepto.

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Author: bet-bromodomain.