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Fig. S8 Autophagic flux in ttis450 larvae is not abrogated by Tor pathway activation. (A–D) Enhancing Torc1 activity by ablating Tsc2 activity in ttis450 larvae does not change their gross morphology at 120 hpf. Compound mutants (ttis450;Tsc2vu242/vu242) (D) are essentially indistinguishable from ttis450 larvae (C). Other panels show WT (A) and Tsc2vu242/vu242 mutant (B) larvae. (E,F) Western blot analysis of p-RPS6 and LC3 demonstrates that ttis450;Tsc2vu242/vu242 compound mutants at 96 hpf contain higher levels of p-RPS6 than ttis450 mutants due to increased Tor activity, yet LC3II levels are comparable between the two genotypes (refer to right hand half of the Western blot, where the larvae were pre-treated with chloroquine). p-RPS6 and LC3II levels are not significantly different between WT and tsc2vu242/vu242 larvae in the presence of chloroquine. Actin was used as a loading control. The levels of LC3II were quantitated by densitometric analysis of three independent Western blots. Data are represented as mean +/ SD, *p<0.05.