Chondrogenesis and osteogenesis defects in ncl?/? embryos. (A) qPCR revealed a significant downregulation of sox9a and col2a1 chondrogenesis markers in 36?hpf ncl?/? embryos compared with ncl+/+ embryos (n=10 per replicate). actb was used as a housekeeping control. (B,B?) Sox9a protein expression was significantly reduced in branchial arches 2-5 (white arrows) in ncl?/? embryos at 36?hpf (n=15). (C) qPCR of osteogenesis markers in 36?hpf ncl+/+ and ncl?/? embryos indicates significant upregulation in runx2a transcripts and downregulation in both col1a2 and col10a1 transcripts in ncl?/? embryos (n=10 per replicate). (D,D?) runx2a mRNA expression was significantly increased ncl?/? embryos at 3?dpf (n=15). Black arrows indicate expression of runx2a in the ceratohyal and otic vesicles. (E,E?) At 3?dpf, Runx2 protein expression was significantly increased in the palatoquadrate and the parasphenoid in ncl?/? embryos. (F) qPCR indicates a significant upregulation of the early osteoblast markers bglap and spp1 and downregulation of the late osteoblast marker sp7 in 36?hpf ncl?/? embryos compared with controls (n=10 per replicate). (G-H?) Alkaline phosphatase staining of ncl+/+ and ncl?/? embryos reveals reduced staining in the lower jaw (ventral view, black arrows) at 3?dpf (G,G?) and 5?dpf (H,H?) (n=15). All experiments were performed three times. cb, ceratobranchial. Scale bars: 200?µm (B,B?); 100?µm (D-E?,G,G?); 140?µm (H,H?). Data are represented as mean±s.d. ns, not significant; *P<0.05 (two-tailed, paired Student's t-test).
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