(A) Representation of the Mastl(lox) and Mastl(Δ) alleles used in this study. A Pf4-Cre transgene was used to generate megakaryocyte-specific Mastl-null mice. (B) Generation of the Mastl(E166D) [Mastl(ED)] allele. The frt-neo_resistance-frt cassette was removed after crossing with Flp-expressing mice. In A and B, White and orange triangles represent lox or frt sequences, respectively. (C) Expression of Mastl in CD41⁺ bone marrow cells from mice of the indicated Mastl genotypes. Lysates from NIH3T3 cells were used as a control. Representative image from 2 independent experiments. See complete unedited blots in the supplemental material. (D) Platelet levels in 12-week-old male (blue) or female (pink) mice with the indicated genotypes. Blue line indicates a concentration of 800 × 10⁶ platelets/ml as a reference. (E) Percentage of mice with fewer than 800 × 10⁶ platelets/ml (using mice from panel D). Male and female mice are represented by separate bars (right). (F) Levels of TPO in peripheral blood from the indicated mice. Cdc20-deficient mice, which display severe thrombocytopenia (33), were used as a control (n ≥4 mice per genotype). (G) Representative micrographs of bone marrow from mice of the indicated genotypes. Images represent more than 3 mice per genotype analyzed. Scale bars: 50 μm. Plot shows quantification of the VWF signal in more than 100 megakaryocytes per genotype. Data are shown as the mean. (H) Quantification of CD41⁺ and CD42⁺ cells in bone marrow cells from mice of the indicated genotypes. (I) Quantification of the ploidy in CD41⁺CD42⁺ double-positive bone marrow cells from mice of the indicated genotypes. No significant differences were observed among the different genotypes (n = 3 per genotype; data are shown as the mean). *P < 0.05, **P < 0.01, and ***P < 0.001; Student’s t test with Welch’s correction (D, F, G, and I) and 1-way ANOVA (E).