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Qi Shen, Shawn C. Little, Meiqi Xu, Julia Haupt, Cindy Ast, Takenobu Katagiri, Stefan Mundlos, Petra Seemann, Frederick S. Kaplan, Mary C. Mullins, Eileen M. Shore
Published in Volume 119, Issue 11
J Clin Invest. 2009; 119(11):3462–3472 doi:10.1172/JCI37412
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Figure 3
Overexpression of R206H ACVR1 in zebrafish embryos causes strong ventralization by enhancing BMP signaling.

Embryos from crosses between alk8+/– heterozygotes were injected with wild-type or mutant (R206H) ACVR1 mRNA, grouped by phenotype, then genotyped for the alk8 mutation. Compared with wild-type embryos (A), uninjected alk8–/– embryos are weakly (class 2; C2) dorsalized (B), with loss of the ventral fin fold (arrowheads). Wild-type ACVR1 mRNA (6–60 pg) at the 1-cell stage fully (as in A) or partially rescued the mutant phenotype (C1 dorsalized; C). (AC) Embryos at 1 day after fertilization. Right panels show posterior of same embryos at 2 days after fertilization. (D and E) Injection of 50 pg mutant ACVR1 mRNA strongly (D) or severely (E) ventralized alk8–/– embryos. Scale bars: 0.2 mm. (F) Phenotype quantification of injected alk8–/– embryos (WT ACVR1, n = 43; R206H, n = 15). (GL) In situ hybridization of wild-type embryos injected with wild-type (GI) or mutant ACVR1 (JL) to detect ventral markers eve1 (G, n = 12/12; J, n = 10/13; onset of gastrulation) and gata2 (H, n = 14/14; K, n = 15/19; mid-gastrulation) or dorsal marker foxb1.2 (I, n = 12/12; L, n = 6/13, 7/13 showed no expression; mid-gastrulation). Animal pole views with dorsal at right. Arrowheads delineate the dorsal-ventral expression domains. Scale bars: 0.2 mm. (M) Total mid-gastrulation stage protein from wild-type zebrafish embryos injected with wild-type or mutant ACVR1 mRNA was immunoblotted to detect phospho-Smad1/5. Increased Smad1/5 phosphorylation was observed even at a low dose (6 pg) of mutant ACVR1. β-Actin was detected as a loading control.