Sepsis-induced antigen-specific CD4+ T-cell dysfunction is corrected by anti-GITR treatment. DO11.10 mice were administered 300 μg anti-GITR or control antibody and were immunized 30 minutes later with Ova323-339 in alum at the time of cecal ligation and puncture or sham surgery. Five days later, lymph node cells were harvested and 2.5 × 104 CD4+ cells were cultured with 2.5 × 105 irradiated APCs with Ova peptide for 72 hours. (A) Proliferation of CD4+ T cells was measured as the incorporation of 3H-thymidine during the last 18 hours of culture. Media was harvested at the time of 3H-thymidine addition to assess cytokine production. (B) IL-2, (C) IFN-γ, (D) IL-4, and (E) IL-10 concentrations were assessed by Luminex multiplex analysis. (F) Representative examples of flow plots demonstrating the expansion of DO11.10 T cells (KJI-26+CD4+) from lymph nodes of Balb/c mice that were injected intravenously with 5 × 106 DO11.10 CD4+ T cells 3 days before sham (left), CLP with control antibody (middle), or CLP with anti-GITR antibody (right) treatment at the time of immunization with Ova323-337 peptide in alum. (G) The calculated percentage of living (Sytox Blue−), nondebris DO11.10 T cells (KJI26+CD4+) expanded in the peripheral lymph nodes of the Balb/c mice. (H) The calculated total number of live (Sytox Blue−), nondebris DO11.10 T cells using cell counts obtained with a hemacytometer. P values indicate differences between groups after post hoc analysis using the Fisher LSD method.