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. 2013 Sep 23;110(41):16486–16491. doi: 10.1073/pnas.1314819110

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Fig. 2. — Postnatal proliferation of cerebellar granule neuron precursors in Gpr37l1^+/+ and Gpr37l1^−/− male mice. (A) Immunofluorescence labeling of BrdU and Hoechst staining of EGL cells at P3, P5, and P7 in Gpr37l1^+/+ and Gpr37l1^−/− littermates. (B) Quantification of the average number of BrdU-positive cells normalized by the EGL length (mean ± SEM), *P < 0.05 ^+/+ vs. ^−/−; ^#P < 0.05 P3 vs. P5, P7 in Gpr37l1^+/+ mice; °P < 0.05 P7 vs. P3, P5 in Gpr37l1^−/− mice, unpaired t test. (C) Quantification of the average number of phosphohistone H3 (PH3)-positive and G2- or M-phase cells at P0, P3, P5, P10, and P15 in the EGL of Gpr37l1^+/+ and Gpr37l1^−/− littermates (mean ± SEM n = 3 per group), *P ≤ 0.05 ^+/+ vs. ^−/−, unpaired t test. (Lower) Representative images of anti-PH3 immunofluorescence labeling and nuclear Hoechst counterstaining of EGL cells in P10 Gpr37l1^+/+ pups, showing distinct PH3-positive cells in either early or late G2 phase and either early or late (mitotic division) M phase. (Scale bars in A and C, 10 μm.)