![Figure 9. Transgenic Th1 cells are inhibited by CGS during antigen presentation: reversal by exogenous IL-2. CD4+ T cells were purified from transgenic mice expressing TCR specific for pigeon cytochrome c (PCC) in the context of I-Ek, and induced toward a Th1 phenotype by in vitro culture, as described in “Materials and methods.” Antigen-specific Th1 cells were injected intravenously (5 × 106 cells) into lethally irradiated hosts capable or not capable of PCC antigen presentation (B10.BR hosts [I-Ek] or C57BL/10 hosts [I-Eb], respectively). At the time of adoptive transfer, PCC antigen mixed with complete Freund adjuvant was administered (intraperitoneally). After transplantation, mice were injected daily (intraperitoneally) with either DMSO vehicle (VEH) or the adenosine A2A receptor agonist CGS (2 mg/kg per day). On day 8 after transplantation, spleens were harvested, and the absolute number of transgenic T cells was enumerated by flow cytometry using anti-Vβ3 and anti-Vα11 and total spleen cell counts (values are mean ± SEM of n = 7 to 8 per cohort). * Statistically significant difference. The 4 cohorts shown in panel A did not receive posttransplant IL-2, whereas the 4 cohorts shown in panel B received posttransplant IL-2 (50 000 IU twice a day, intraperitoneally).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/105/12/10.1182_blood-2004-04-1407/5/zh80120579850009.jpeg?Expires=1724271343&Signature=Mpe2WsqUcfaznrx-vPYyW7vYceqg8y6IkKBvQSW8p5ZDGz7N92XBmEc0TfPnAfiCvV6B0YyANoAXaWpdIWhzwT2iTmQasqFE1nw4iBhTWGXuNPqpRbzng2sdsUTRtnf-OpzXRgZw~HaEmnNNwQgE7dLjjGRK1ObrGPvIjyAAqWogb~L9OOUW4FxByyH~p9vTjnUdn07tHbqVvYJxGeFI9QXjNEsDQJTzWb15Dkkse4aM8B85Jx8xN9-FKnO-U5kiexpWHUYiDIAAQ8ptOYYTolim3fp5nRe-BwzeYg1NnP6ozob19pikDKj7IShxSDhhUkcH5bdldG9RnxmAA4AIIg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Transgenic Th1 cells are inhibited by CGS during antigen presentation: reversal by exogenous IL-2. CD4+ T cells were purified from transgenic mice expressing TCR specific for pigeon cytochrome c (PCC) in the context of I-Ek, and induced toward a Th1 phenotype by in vitro culture, as described in “Materials and methods.” Antigen-specific Th1 cells were injected intravenously (5 × 106 cells) into lethally irradiated hosts capable or not capable of PCC antigen presentation (B10.BR hosts [I-Ek] or C57BL/10 hosts [I-Eb], respectively). At the time of adoptive transfer, PCC antigen mixed with complete Freund adjuvant was administered (intraperitoneally). After transplantation, mice were injected daily (intraperitoneally) with either DMSO vehicle (VEH) or the adenosine A2A receptor agonist CGS (2 mg/kg per day). On day 8 after transplantation, spleens were harvested, and the absolute number of transgenic T cells was enumerated by flow cytometry using anti-Vβ3 and anti-Vα11 and total spleen cell counts (values are mean ± SEM of n = 7 to 8 per cohort). * Statistically significant difference. The 4 cohorts shown in panel A did not receive posttransplant IL-2, whereas the 4 cohorts shown in panel B received posttransplant IL-2 (50 000 IU twice a day, intraperitoneally).
