(A) Confocal images of cryostat 10 μm–thick slice of a WT D20 CO. The arrow points to dense vertical columns of SOX2/Ki67⁺ cells, including a fluid-filled luminal compartment with an apical layer of progenitors (double asterisk and arrowheads in the inset). Scale bar 75 μm; inset in A: scale bar 35 μm. (B) Whole-mount immunolabeling of D20 control and MCT8-deficient COs. Scale bar 500 μm. (C) Representative circular rosette-like substructures (nuclear staining DAPI in blue). ** indicates areas of undifferentiated tissue; scale bar 150 μm. (D and E) Quantitation of the diameter of the cortical rosettes and number of layers formed by SOX2⁺ cells. Scale bar 150 μm; inset in D: scale bar 50 μm. Note how both parameters are reduced in MCT8-deficient COs when compared with controls. Values are mean ± SD of 4 COs per line (5–6 rosettes per CO). (F) Staining for phospho-histone H3 (PH3; red) and phospho-Vimentin (green) to mark neural precursor cells in mitosis, which primarily divide at the apical surface. Arrows in F and in the insets mark apical surface horizontal (0–30 degrees) and vertical (60–90 degrees) divisions. Scale bar 10 μm; insets in F: scale bar 5 μm. (G) Quantitation of neural precursors’ division orientation from 4 COs per line. (H) Whole-mount immunolabeling of D20 COs, Tuj1 staining in green, nuclear staining DAPI (blue) showing evenly distributed postmitotic neurons. Scale bar 100 μm; and insets in H: scale bar 150 μm. (I) Quantitation of the mRNA levels of the indicated genes in D20 control and MCT8-deficient COs. Note how the expression of genes involved in neurogenesis and neuronal differentiation is reduced in MCT8-deficient when compared with control COs. n = 5–6 RNA samples, each of them consisting of 4 pooled COs from either WT or MCT8-deficient COs; 1-way ANOVA and Tukey test were used for multiple comparisons; *P < 0.05, **P < 0.01, ***P < 0.001.