(A and B) Percentages of proliferating (PCNA⁺, A) or apoptotic (TUNEL⁺, B) YFP⁺ hybrids on the total amount of YFP⁺ hybrids in MNU-damaged Gfap-Cre retinas 24 hours after transplantation of untreated (HSPCs) or BIO-treated (BIO-HSPCs) HSPCs^R26Y. ***P < 0.0001, unpaired Student’s t test. (C) qPCR analysis of cell-cycle genes on FACS-sorted DiD⁺YFP⁺ hybrids harvested 24 hours after transplantation of untreated or BIO-treated HSPCs^R26Y in MNU-damaged Gfap-Cre retinas. Data are represented as mean ± SD of log₁₀ fold changes of gene expression in DiD⁺YFP⁺ hybrids with respect to DiD⁺YFP⁺ population-depleted retinas. n = 3. (D) Total YFP⁺ hybrids (green bars) that also incorporated BrdU (red bars) detected in MNU-damaged Gfap-Cre retinas 24 hours, 72 hours, and 1 week after transplantation of untreated or BIO-treated HSPCs^R26Y. **P < 0.001, 2-way ANOVA and Bonferroni’s post-test. Red and green lines show the statistical significance of green (YFP) or red (BrdU) bars. (E–G) Percentages of YFP⁺BrdU⁺ hybrids also positive for GS (E, Müller cells), OTX2 (F, photoreceptor progenitors), or recoverin (G, REC, mature photoreceptors) detected in MNU-damaged Gfap-Cre retinas 24 hours, 72 hours, and 1 week after transplantation of untreated or BIO-treated HSPCs^R26Y. (H–J) Representative immunostainings of double YFP⁺ (green)/BrdU⁺ (red) hybrids also positive for either GS (magenta in H, white arrowheads), OTX2 (magenta in I, yellow arrowheads), or recoverin (magenta in J, green arrowheads) stainings in MNU-damaged Gfap-Cre retinas 24 hours (H), 72 hours (I), and 1 week (J) after transplantation of BIO-treated HSPCs. Nuclei were counterstained with DAPI (blue). Images on the top show higher magnification and single channels of areas in the white squares. Scale bars: 20 μm. (A, B, and D–G) Values in graphs are represented as mean ± SD (n = 9).