Figure 1.
Figure 1. LSelhi, but not LSello, Tregs protect against GVHD-associated mortality and morbidity by interfering with the activation and expansion of GVHD effector T cells. Lethally irradiated B6 mice were infused with BALB/c BM. Cohorts received 5 × 106 BALB/c CD25-depleted effector T cells alone or with ex vivo activated and expanded BALB/c LSelhi or LSello Tregs at the indicated T/reg ratio. Experiments illustrated in panels C-E used a ratio of 1 T cell to 3 Tregs. (A) Survival is indicated (n = 8/group;*P = .008 compared to T cells). (B) Average weight in grams of mice from panel A is indicated. *Only one mouse survived after this time point. (C) Spleens were harvested and enumerated 6 days after transplantation. Use of BALB/c Thy1 congenics allowed Thy1.1+ effectors to be distinguished from Thy1.2+ Tregs. The average total number of effector CD4+ and CD8+ T cells per spleen is shown. Error bars indicate standard deviation (n = 4 separate pools of 2 spleens/pool for each group; *P < .05). Data for panels C-E were taken from one of 2 replicate experiments. (D) Splenocytes from panel C were phenotyped. Shown is LSel expression on gated GVHD effector thy1.1+ CD4+ and CD8+ T cells. Shown are data from one of 4 representative splenic pools per treatment group. Percentage of LSel+ cells is indicated in the top right quadrant. (E) Splenocytes from panels C and D were stimulated in vitro with irradiated host-type splenic stimulators. Shown are peak secondary antihost proliferative responses of 4 separate pools of 2 spleens/pool from GVHD control mice, LSelhi and LSello Treg-treated mice. Cultures consisted of 3 × 104 effector Thy1.1+ CD4+ T cells restimulated with 105 irradiated B6 splenocytes, plated in replicates of 6. Note that infused Tregs are not depleted from the culture.

LSelhi, but not LSello, Tregs protect against GVHD-associated mortality and morbidity by interfering with the activation and expansion of GVHD effector T cells. Lethally irradiated B6 mice were infused with BALB/c BM. Cohorts received 5 × 106 BALB/c CD25-depleted effector T cells alone or with ex vivo activated and expanded BALB/c LSelhi or LSello Tregs at the indicated T/reg ratio. Experiments illustrated in panels C-E used a ratio of 1 T cell to 3 Tregs. (A) Survival is indicated (n = 8/group;*P = .008 compared to T cells). (B) Average weight in grams of mice from panel A is indicated. *Only one mouse survived after this time point. (C) Spleens were harvested and enumerated 6 days after transplantation. Use of BALB/c Thy1 congenics allowed Thy1.1+ effectors to be distinguished from Thy1.2+ Tregs. The average total number of effector CD4+ and CD8+ T cells per spleen is shown. Error bars indicate standard deviation (n = 4 separate pools of 2 spleens/pool for each group; *P < .05). Data for panels C-E were taken from one of 2 replicate experiments. (D) Splenocytes from panel C were phenotyped. Shown is LSel expression on gated GVHD effector thy1.1+ CD4+ and CD8+ T cells. Shown are data from one of 4 representative splenic pools per treatment group. Percentage of LSel+ cells is indicated in the top right quadrant. (E) Splenocytes from panels C and D were stimulated in vitro with irradiated host-type splenic stimulators. Shown are peak secondary antihost proliferative responses of 4 separate pools of 2 spleens/pool from GVHD control mice, LSelhi and LSello Treg-treated mice. Cultures consisted of 3 × 104 effector Thy1.1+ CD4+ T cells restimulated with 105 irradiated B6 splenocytes, plated in replicates of 6. Note that infused Tregs are not depleted from the culture.

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