Micromass cultures were infected with RCASBP(A) alone (control) or containing either wild-type ACVR1, a constitutively active caACVR1 Q207D construct, or the R206H ACVR1 mutation either alone or together with RCASBP(B) expressing Noggin (NOG). (A) Micromass cultures were stained with Alcian blue to visualize early chondrogenic differentiation by extracellular matrix accumulation after 7 days. (B) Quantification of Alcian blue incorporation into the extracellular matrix is shown. Significant differences: wtACVR1 vs. caACVR1***; wtACVR1+NOG vs. caACVR1+NOG***; wtACVR1 vs. R206H***; wtACVR1+NOG vs. R206H+NOG***. (C) ALP-stained micromass cultures visualize prehypertrophic differentiation after 9 days in culture. Scale bars in A and C: 2 mm. (D) Quantification of ALP staining by histomorphometric analysis (ALP activity quantified as pixel² × 10,000) is shown. Significant differences: wtACVR1 vs. caACVR1***; wtACVR1+NOG vs. caACVR1+NOG***; wtACVR1 vs. R206H (NS); wtACVR1+NOG vs. R206H+NOG**. (E) Relative expression of marker genes for chondrogenic differentiation by qRT-PCR of cDNA from 8-day micromass cultures. Amplification was normalized to the expression of 28S rRNA. For quantification in B and D, significant differences in comparison to wtACVR1 or wtACVR1+NOG are indicated. Graphs in B and D show mean ± SEM of quadruplicate samples from 1 of 3 representative experiments. Horizontal lines represent significant differences at *P < 0.05; **P < 0.01; ***P < 0.001. Data in E, shown as mean ± SEM, are representative results from 2 independent cDNA syntheses and qRT-PCR.