Kidneys of BALB/cJ WT and Pkd1^RC/RC mice were harvested at 1 and 6 months of age and analyzed by flow cytometry for expression of CTLA-4 on CD8⁺ T cells (CD45⁺TCRβ⁺CD8⁺; A and B), CD80 or CD86 on macrophages (CD45⁺CD19^–Ly6G^–CD64⁺; C and D), and CD80 or CD86 on epithelial cells (CD45^–EpCAM⁺APN⁺; E and F). (A, C, and E) Representative flow diagrams of 1-month-old BALB/cJ WT and Pkd1^RC/RC kidneys. (B, D, and F) Quantification of CTLA-4–positive CD8⁺ T cells (B), CD80/CD86–positive CD64⁺ macrophages (D), and CD80/CD86–positive epithelial cells (F) as percentage live and percentage parent population comparing WT (brown) with Pkd1^RC/RC (white). CTLA-4 or CD80/CD86 expression is significantly upregulated on the respective cell type in Pkd1^RC/RC versus WT. (G) Analysis of CD8⁺ T cells that express PD-1 (blue), CTLA-4 (green), PD-1 and CTLA-4 (yellow), or no immune checkpoint receptor (gray). (H) Analysis of macrophages/epithelial cells that express PD-L1 (blue), CD80/CD86 (green), PD-L1 and CD80/CD86 (yellow), or no immune checkpoint ligand (gray). Few cells coexpress both immune checkpoint proteins on the same cell, suggesting that treatment with antibodies against each immune checkpoint targets different cells. Supplemental Figure 4 contains quantification of CTLA-4 expression on CD4⁺ T cells and individual CD80 or CD86 expression on macrophages/epithelial cells. (B, D, and F) Box plot (25th to 75th percentile and median) with whiskers of 10th and 90th percentiles; single data points are depicted. (B, D, and F–H) Brown-Forsythe 1-way ANOVA with multiple-comparison follow-up by controlling for false discovery rate (Benjamini, Krieger, Yekutieli). Nonsignificant pairwise comparisons are not shown. (G and H) Comparisons are limited to cells expressing neither immune checkpoint protein. *P < 0.05, **P < 0.01. N = 4 BALB/cJ WT; N = 3 BALB/cJ Pkd1^RC/RC. Data points are male and female.