Figure 3
Figure 3. CD25highCD27pos Treg differentiation into CD27neg IL-17–producing cells and pass through into a Foxp3/IL-17 double-positive stage. Flow cytometry of sorted CD4posCD25highCD27posCD45RAneg (CD25highCD27pos) Tregs and CD4posCD25negCD27posCD45RAneg (CD25negCD27pos) Teffs that were stimulated with allogeneic PBMCs in the presence of both rIL-2 and rIL-15 and analyzed for cell division, IL-17 production, and Foxp3 and CD27 expression. To analyze IL-17 production, cells were restimulated with PMA plus ionomycin in the presence of Brefeldin A. (A) Density plots at the top show intracellular expression of IL-17 (y-axis) and Foxp3 (x-axis) at days 5, 7, and 8 after culture of CD25highCD27pos Tregs. Numbers at the top of the plots indicate the percentages of IL-17–producing cells. The lower density plots show CFSE content and costaining of Foxp3 of CFSE-labeled CD25highCD27pos Tregs at day 6 of the culture. (B) Summary plot showing percentage of IL-17– and Foxp3–expressing cells, such as analyzed under panel A, at day 8 of the cultures (data from 12 individual experiments, using 12 different blood donors). (C,D) Sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs were CFSE labeled and subsequently stimulated with allogeneic PBMCs and rIL-2 plus rIL-15. Plots show CFSE content (x-axis) and expression of CD27 (C) or IL-17 (D, y-axis) at day 8 of the culture. (E) Density plots show CD27 (x-axis) expression and intracellular IL-17 expression (y-axis). (F) Cytokine measurements of differentiated CD27pos and CD27neg cells obtained after differentiation of sorted peripheral CD25highCD27pos Tregs and CD25negCD27pos Teffs. CD25highCD27pos Tregs and CD25negCD27pos Teffs were sorted from peripheral blood, labeled with CFSE, and cultured in the presence of allogeneic stimulator PBMCs and rIL-2 plus rIL-15 for 10 days. At day 10, the resultant CD27pos and CD27neg cells in the divided CFSE-low cell population were isolated by cell sorting using flow cytometry. The sorted cell populations (20 × 103) were stimulated for 20 hours with PMA plus ionomycin; thereafter IL-17 concentrations were analyzed in the culture supernatants. Means plus or minus SD are shown for 3 independent experiment performed with cells obtained from different donors. Data are representative of 2 (A) or 3 or more (C-E) separate experiments conducted with cells obtained from different blood donors.

CD25highCD27pos Treg differentiation into CD27neg IL-17–producing cells and pass through into a Foxp3/IL-17 double-positive stage. Flow cytometry of sorted CD4posCD25highCD27posCD45RAneg (CD25highCD27pos) Tregs and CD4posCD25negCD27posCD45RAneg (CD25negCD27pos) Teffs that were stimulated with allogeneic PBMCs in the presence of both rIL-2 and rIL-15 and analyzed for cell division, IL-17 production, and Foxp3 and CD27 expression. To analyze IL-17 production, cells were restimulated with PMA plus ionomycin in the presence of Brefeldin A. (A) Density plots at the top show intracellular expression of IL-17 (y-axis) and Foxp3 (x-axis) at days 5, 7, and 8 after culture of CD25highCD27pos Tregs. Numbers at the top of the plots indicate the percentages of IL-17–producing cells. The lower density plots show CFSE content and costaining of Foxp3 of CFSE-labeled CD25highCD27pos Tregs at day 6 of the culture. (B) Summary plot showing percentage of IL-17– and Foxp3–expressing cells, such as analyzed under panel A, at day 8 of the cultures (data from 12 individual experiments, using 12 different blood donors). (C,D) Sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs were CFSE labeled and subsequently stimulated with allogeneic PBMCs and rIL-2 plus rIL-15. Plots show CFSE content (x-axis) and expression of CD27 (C) or IL-17 (D, y-axis) at day 8 of the culture. (E) Density plots show CD27 (x-axis) expression and intracellular IL-17 expression (y-axis). (F) Cytokine measurements of differentiated CD27pos and CD27neg cells obtained after differentiation of sorted peripheral CD25highCD27pos Tregs and CD25negCD27pos Teffs. CD25highCD27pos Tregs and CD25negCD27pos Teffs were sorted from peripheral blood, labeled with CFSE, and cultured in the presence of allogeneic stimulator PBMCs and rIL-2 plus rIL-15 for 10 days. At day 10, the resultant CD27pos and CD27neg cells in the divided CFSE-low cell population were isolated by cell sorting using flow cytometry. The sorted cell populations (20 × 103) were stimulated for 20 hours with PMA plus ionomycin; thereafter IL-17 concentrations were analyzed in the culture supernatants. Means plus or minus SD are shown for 3 independent experiment performed with cells obtained from different donors. Data are representative of 2 (A) or 3 or more (C-E) separate experiments conducted with cells obtained from different blood donors.

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