Expression of irf7 in zebrafish larvae. irf7 expression was detected with whole‐mount in situ hybridization at 48 hpf (a–c) and 72 hpf (d–f), respectively. The irf7 mRNA was expressed in the otic vesicle and lateral line (indicated by red arrowhead)

irf7 knockdown zebrafish embryos exhibit severe defects in hair cell (HC) development. (a) Phenotypes of control and irf7‐specific morpholino‐injected Tg(Brn3c:GFP) zebrafish larvae at 72 hpf. (b) Fluorescent imaging of green fluorescent protein (GFP)‐labeled HCs indicates the HC clusters on the lateral line of zebrafish larvae at 72 hpf. (c) Quantification of the number of HC clusters in control and irf7‐specific morpholino‐injected Tg(Brn3c:GFP) zebrafish embryos at 72 hpf. (d) Comparison of the phenotypes of crista HCs (blue dotted circles) in control, irf7‐specific morpholino‐injected and irf7‐specific morpholino & mRNA‐coinjected zebrafish embryos. (e) Quantification of the number of crista HCs in control, irf7‐specific morpholino‐injected and irf7‐specific morpholino & mRNA‐coinjected zebrafish embryos. Error bars indicate standard deviation. ***, P < 0.001

Apoptotic analysis of hair cells (HCs) in the neuromasts of control and irf7‐knockdown embryos. DAPI, green fluorescent protein (GFP) and TUNEL (TMR red) were used to label the live cell nuclei, HCs and apoptotic HCs, respectively

Significant differentially expressed genes (DEGs) regulated by irf7. (a) Number of DEGs upon knockdown of irf7. Among these DEGs, 18 genes are annotated to hair cell (HC) and posterior lateral line (PLL) neuromasts development. (b) Comparison of relative gene expression of the annotated 18 genes between irf7‐morphants and control. (c) atp1b2b mRNA injection rescues crista HC defects induced by irf7‐knockdown. ***, P < 0.001; ****, P < 0.0001

Working model of the Irf7 and Atp1b2b in zebrafish hair cells. Irf7, as a transcription factor, can positively regulate the Atp1b2b, which was a component of the Na⁺, K⁺‐ATPase