We iso lated the 514 RNAs in the WT flies that are expressed at very high levels in day 0 and day 1 but decreased signifi cantly thereafter. We then organized and presented these RNAs as a heatmap for both the WT and Dis3KD flies over our time course. We find two distinct effects of Dis3KD on these early RNAs. First, greater than 50% of the early expressed RNAs were robustly downregulated in Dis3KD flies in days 0 and 1. Second, those RNAs that showed similar expression between the WT and Dis3KD flies in days 0 and 1 persisted at high Inhibitors,Modulators,Libraries expression at day 2 only in the Dis3KD flies. We also find a striking effect when comparing these early expressed transcripts on day 4, one third of the transcripts that are highly upregulated in the WT are highly downregulated in the Dis3KD flies.
Together, these data provide strong evidence for Dis3 transcriptomic regulation in the embryo, at embryonic larval transition, and at the larval Inhibitors,Modulators,Libraries pupal transition. To further examine confirm our RNA seq data, we selected early expressed RNAs from our data set for graphical analysis. Two of these, hunchback and Kr��ppel, encode DNA binding proteins that are known to be present in the early embryo. The third RNA is annotated but has no known function, CG12011. In WT flies, these transcripts ex press at the first 2 time points. In Dis3KD flies, these three RNAs are substantially reduced at these early time points. To independently validate the Entinostat early expression of these RNAs and the Dis3KD effects seen by RNA seq, we performed qRT PCR with actin as a loading control.
The general trends are largely similar, with Inhibitors,Modulators,Libraries RNAs detected at early time points and Dis3KD eliciting their reduction. We suspect the differences between qRT PCR Inhibitors,Modulators,Libraries and RNA seq arise from the nature of RNA preparation and from the manner and efficiency of se quence detection and amplification. Finally, we verified that the changes in hunchback, Kr��ppel, and CG12011 mRNA levels were not observed in the da Gal4 early embryo. Analysis of exosome subunits expression during Drosophila development Given the established role of Dis3 in the RNA processing exosome��and given that the exosome has vital roles in numerous RNA metabolic pathways��we considered the possibility that the Dis3KD changes in the developmen tal transcriptome might arise from perturbation of exo some subunit RNA expression.
To test this hypothesis, we isolated and graphically analysed the RNA seq determined expression of Rrp6 and core exosome subu nits. While Dis3KD elicits a significant knockdown of Rrp6 RNA levels at day 0 and 1, there is no measurable effect at later developmen tal time points. We see a similar pattern of Dis3KD mediated effects on RNase PH and S1 subunits as well, with a few subunit RNAs showing decrease levels at the day 4 time point.