Fig. 5

Ddx41 regulates HSPC number via the cGAS-STING inflammatory pathway (A) Schematic of the cGAS-STING pathway knockdown experiments with HSPC quantification. (B) Flow cytometry plots of cd41:gfp+ HSPCs from ddx41 mutants injected with control morpholino (left), splice-blocking sting morpholino (middle), or translation-blocking (ATG) cgas morpholino (right) at 40 hpf. (C) Graph depicting the absolute number of cd41:gfp+ cells per embryo shown in (B). (D) Schematic of the STING knockdown and RNASEH1 overexpression experiment with HSPC quantification. (E) Flow cytometry plots of runx1:mcherry+ HSPCs from Tg(hsp70:M27RNASEH1-GFP)-negative (top left) and Tg(hsp70:M27RNASEH1-GFP)-positive (top right) uninjected ddx41 mutants versus Tg(hsp70:M27RNASEH1-GFP)-negative (bottom left) and Tg(hsp70:M27RNASEH1-GFP)-positive (bottom right) STING morpholino-injected ddx41 mutants at 40 hpf. (F) Graph depicting the number of runx1:mcherry+ HSPCs per embryo from (E). Graphs display means ± stds with p values calculated with a one-way ANOVA with Tukey’s multiple testing correction, ∗∗p < 0.01, ∗∗∗p < 0.001, ∗∗∗∗p < 0.0001, ns, not significant (p > 0.05). N = 3–6 replicates per experiment.