Figure 5
Figure 5. The enhanced in vivo antitumor efficacy of in vitro programmed TEM cells is dependent on IFN-γ production but independent of T-cell responsiveness to IFN-γ. WT mice bearing 10 days established B16 melanoma were sublethally irradiated and left untreated as controls (×) or received unprogrammed pmel TEM cells (●), or pmel TEM (□) cells, pmel-Ifng−/− TEM cells (■), or pmel-Ifngr1−/− TEM cells (♦) programmed in vitro with anti-CD3/anti-CD28 for 24 hours before transfer. For mice receiving programmed pmel TEM, pmel-Ifng−/− TEM cells, or pmel-Ifngr1−/− TEM cells, cultures were started with 2 × 106 cells per recipient mouse, and the total number of cells present at 24 hours were transferred. Mice treated with nonprogrammed pmel TEM cells received 2 × 106 cells. All treated mice received rhIL-2 (36 μg/dose × 6 doses). Results from different representative experiments are presented as the mean measurements from 5 mice per group (± SEM).

The enhanced in vivo antitumor efficacy of in vitro programmed TEM cells is dependent on IFN-γ production but independent of T-cell responsiveness to IFN-γ. WT mice bearing 10 days established B16 melanoma were sublethally irradiated and left untreated as controls (×) or received unprogrammed pmel TEM cells (●), or pmel TEM (□) cells, pmel-Ifng−/− TEM cells (■), or pmel-Ifngr1−/− TEM cells (♦) programmed in vitro with anti-CD3/anti-CD28 for 24 hours before transfer. For mice receiving programmed pmel TEM, pmel-Ifng−/− TEM cells, or pmel-Ifngr1−/− TEM cells, cultures were started with 2 × 106 cells per recipient mouse, and the total number of cells present at 24 hours were transferred. Mice treated with nonprogrammed pmel TEM cells received 2 × 106 cells. All treated mice received rhIL-2 (36 μg/dose × 6 doses). Results from different representative experiments are presented as the mean measurements from 5 mice per group (± SEM).

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