(A) Schematic of OT-I memory mouse generation (top) and subsequent stimulation assays (bottom). OT-I Tnaive cells were transferred and expanded with VSV-OVA, then aged to stable memory contraction; after, T cells were enriched from VSV-OVA expanded OT-I memory animals and stimulated with media alone (mock), IL-12, IL-15, and IL-18 in combination (IL-12/15/18; each at 100 ng/mL), or anti-CD3/CD28 microbeads (TCR) at an approximately 1:1 bead/cell ratio. (B and C) expression of (B) PD-1, (C) TOX, and (D) TCF1 within stimulated OT-I Tmem cells throughout experiment time course. TOX MedFI fold change in C was calculated against average TOX MedFI from mock stimulations in a subset-specific, batch-specific, and time point–specific manner. In B and C, bar chart symbols represent 1 animal at a unique time point/condition and are connected by animal identity, with bar indicating mean; the indicated statistical significances in B and C were calculated using paired t tests. In B–D, symbols in line plots comparing stimulation conditions represent the mean across all animals for a specific time point/condition ± SD; the indicated statistical significances were calculated using Mann-Whitney U tests. Results from n = 14 mice across 7 experiments are shown in B and C. Results from n = 9 mice across 2 experiments are shown in D. TOX, thymocyte selection–associated high-mobility group box; Tmem, memory T cells; Tnaive, naive T cells; VSV-OVA, OVA-expressing vesicular stomatitis virus; PD-1, programmed cell death protein 1; MedFI, median fluorescence intensity.