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N the pupal thorax, however, the increased (-)-Indolactam V web pigmentation and thickness of the adult cuticle precluded us from visualizing the GFP marker to positively identify these regions as tsc1 or tsc2 mutant (Fig. 1E, F). Nonetheless, consistent with the idea that TSC1/2-dependent regulation of Rheb contributes to control of pigmentation, overexpression of TSC1 and TSC2 strongly suppressed the pigmentation and growth phenotypes in Rheb overexpressing flies (Fig. 1G), while knockdown of tsc2 by RNAi significantly enhanced the Rheb-induced pigmentation (Fig. 1H, and Fig. S1D) on the adult thorax. Pigmentation of the pupal cuticle begins at the late stages of metamorphosis (stages P10) [14], proceeding as an anteriorposterior wave of mechanosensory bristle pigmentation, followed by post-eclosion cuticular tanning [15]. We therefore evaluated the onset of pigmentation in either Rheb overexpressing or tsc1 mutant mechanosensory bristles. We saw that while the lateral thoracic mechanosensory bristles, which are outside the pannierGal4 expression domain, were unpigmented in stage P10 pannierGal4, UAS-Rheb pupa, the dorsal bristles within the pannier-Gal4 expression domain were strikingly dark along a broad dorsal stripe (Fig. 1I). Similarly, we found that in tsc1 MARCM clones (which could be definitively identified by strong GFP expression at this developmental stage), mechanosensory bristle pigmentation initiated earlier than in neighboring wildtype bristles (Fig. 1J ). In contrast, pigmentation was delayed compared to wildtype bristles in marked rheb, tsc1 double mutant clones (Fig. 1N, O), suggesting that rheb is required for the precocious pigmentation in tsc1 clones. Taken together, we conclude that Rheb activity is a limiting factor in the timing and degree of adult pigmentation on the thorax and abdomen.Rheb induced pigmentation, we knocked down s6k1 by RNAi in the thorax with pannier-Gal4. s6k1RNAi stunts mechanosensory bristle growth in both wildtype and Rheb overexpressing flies, but does not suppress melanization in wildtype flies. However, s6k1RNAi potently suppresses cuticular pigmentation in Rheb overexpressing flies (Fig. 2F). To assess whether S6K1 activity was sufficient to drive increased pigmentation on the thorax, we crossed pannier-Gal4 to UAS transgenes encoding S6 kinase mutants that mimic an activating phosphorylation (S6K1TE) [18]. This activated form of S6K1 markedly enhanced Rhebdependent pigmentation (Fig. S1I, J). Furthermore, overexpression of the S6K1TE or S6K1STDETE mutant (both which possesses the T398 to E amino acid substitution in the linker domain) results in a mild increased pigmentation 374913-63-0 manufacturer phenotype on the thorax when pupae are grown at 29uC (Fig. 2G). We hypothesized that since TORC1 activation promotes both S6K1 activity and releases repression on eIF4E, that activation of S6K1 alone was perhaps not sufficient to fully recapitulate the pigmentation phenotype caused by Rheb. We therefore asked whether combined expression of S6K1TE and eIF4E could yield a robust increase in pigmentation on the thorax. Indeed, we find that while overexpression of eIF4E alone has no effect, eIF4E overexpression enhanced the increased pigmentation phenotype resulting from S6K1TE overexpression at 29uC (Fig. 2H). Due to severe distortion of thorax morphology, we were unable to assess whether overexpression of 4E-BP, which acts an inhibitor of eIF4E, could suppress Rheb-induced pigmentation. Taken together, our findings lead us to conclude t.N the pupal thorax, however, the increased pigmentation and thickness of the adult cuticle precluded us from visualizing the GFP marker to positively identify these regions as tsc1 or tsc2 mutant (Fig. 1E, F). Nonetheless, consistent with the idea that TSC1/2-dependent regulation of Rheb contributes to control of pigmentation, overexpression of TSC1 and TSC2 strongly suppressed the pigmentation and growth phenotypes in Rheb overexpressing flies (Fig. 1G), while knockdown of tsc2 by RNAi significantly enhanced the Rheb-induced pigmentation (Fig. 1H, and Fig. S1D) on the adult thorax. Pigmentation of the pupal cuticle begins at the late stages of metamorphosis (stages P10) [14], proceeding as an anteriorposterior wave of mechanosensory bristle pigmentation, followed by post-eclosion cuticular tanning [15]. We therefore evaluated the onset of pigmentation in either Rheb overexpressing or tsc1 mutant mechanosensory bristles. We saw that while the lateral thoracic mechanosensory bristles, which are outside the pannierGal4 expression domain, were unpigmented in stage P10 pannierGal4, UAS-Rheb pupa, the dorsal bristles within the pannier-Gal4 expression domain were strikingly dark along a broad dorsal stripe (Fig. 1I). Similarly, we found that in tsc1 MARCM clones (which could be definitively identified by strong GFP expression at this developmental stage), mechanosensory bristle pigmentation initiated earlier than in neighboring wildtype bristles (Fig. 1J ). In contrast, pigmentation was delayed compared to wildtype bristles in marked rheb, tsc1 double mutant clones (Fig. 1N, O), suggesting that rheb is required for the precocious pigmentation in tsc1 clones. Taken together, we conclude that Rheb activity is a limiting factor in the timing and degree of adult pigmentation on the thorax and abdomen.Rheb induced pigmentation, we knocked down s6k1 by RNAi in the thorax with pannier-Gal4. s6k1RNAi stunts mechanosensory bristle growth in both wildtype and Rheb overexpressing flies, but does not suppress melanization in wildtype flies. However, s6k1RNAi potently suppresses cuticular pigmentation in Rheb overexpressing flies (Fig. 2F). To assess whether S6K1 activity was sufficient to drive increased pigmentation on the thorax, we crossed pannier-Gal4 to UAS transgenes encoding S6 kinase mutants that mimic an activating phosphorylation (S6K1TE) [18]. This activated form of S6K1 markedly enhanced Rhebdependent pigmentation (Fig. S1I, J). Furthermore, overexpression of the S6K1TE or S6K1STDETE mutant (both which possesses the T398 to E amino acid substitution in the linker domain) results in a mild increased pigmentation phenotype on the thorax when pupae are grown at 29uC (Fig. 2G). We hypothesized that since TORC1 activation promotes both S6K1 activity and releases repression on eIF4E, that activation of S6K1 alone was perhaps not sufficient to fully recapitulate the pigmentation phenotype caused by Rheb. We therefore asked whether combined expression of S6K1TE and eIF4E could yield a robust increase in pigmentation on the thorax. Indeed, we find that while overexpression of eIF4E alone has no effect, eIF4E overexpression enhanced the increased pigmentation phenotype resulting from S6K1TE overexpression at 29uC (Fig. 2H). Due to severe distortion of thorax morphology, we were unable to assess whether overexpression of 4E-BP, which acts an inhibitor of eIF4E, could suppress Rheb-induced pigmentation. Taken together, our findings lead us to conclude t.

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