Figure 7
Figure 7. Inhibition of Treg function in the presence of PEG-ADA. (A) Percentage of CD25+FoxP3+ Tregs in ADA−/− rescued with PEG-ADA (n = 20), lentiviral GT (n = 8), and BMT (n = 11) compared with ADA+/+ mice (n = 23). Data are mean ± SEM. ***P = .0001. *P = .05. N.S. indicates not significant. (B) Absolute numbers of Tregs. Data are mean ± SEM. (C) Suppressive function versus ADA+/+ effector cells of ADA+/+ (n = 11) and ADA−/− (n = 8) Tregs compared with Tregs from ADA−/− mice treated with BMT (n = 3), GT (n = 3), and PEG-ADA after 10 (n = 3), 14 (n = 3), and 18 (n = 7) weeks. Data are interexperimental mean ± SD. ***P < .0005. **P < .005. *P < .05. (D) Summarized MFI of CD39 and CD73 gated on CD4+CD25+FoxP3+ cells from ADA+/+ (n = 6) mice compared with ADA−/− mice treated with PEG-ADA for 18 weeks (n = 4). (E) Representative histogram plots for CD39 and CD73 on CD4+CD25+FoxP3+ splenocytes from ADA+/+ and ADA−/− mice treated with PEG-ADA for 18 weeks. Isotype-identical monoclonal antibodies served as controls (solid gray histogram). (F) Measurement of ATP consumption and AMP formation (left panel) as well as adenosine formation (right panel) by purified CD4+CD25+ Treg cells from PEG-ADA–treated ADA−/− (n = 4) and ADA+/+ mice (n = 3). Data are interexperimental mean ± SD. *P < .05. (G) Serum adenosine levels in PEG-ADA–treated ADA−/− (n = 4) and age-matched ADA+/+ mice (n = 4) at 10, 14, and 18 weeks of follow-up. Data are interexperimental mean ± SD. *P < .05. (H) Serum hypoxanthine levels in PEG-ADA–treated ADA−/− (n = 4) and age-matched ADA+/+ mice (n = 4) at 10, 14, and 18 weeks of follow-up. Data are interexperimental mean ± SD. **P < .005.

Inhibition of Treg function in the presence of PEG-ADA. (A) Percentage of CD25+FoxP3+ Tregs in ADA−/− rescued with PEG-ADA (n = 20), lentiviral GT (n = 8), and BMT (n = 11) compared with ADA+/+ mice (n = 23). Data are mean ± SEM. ***P = .0001. *P = .05. N.S. indicates not significant. (B) Absolute numbers of Tregs. Data are mean ± SEM. (C) Suppressive function versus ADA+/+ effector cells of ADA+/+ (n = 11) and ADA−/− (n = 8) Tregs compared with Tregs from ADA−/− mice treated with BMT (n = 3), GT (n = 3), and PEG-ADA after 10 (n = 3), 14 (n = 3), and 18 (n = 7) weeks. Data are interexperimental mean ± SD. ***P < .0005. **P < .005. *P < .05. (D) Summarized MFI of CD39 and CD73 gated on CD4+CD25+FoxP3+ cells from ADA+/+ (n = 6) mice compared with ADA−/− mice treated with PEG-ADA for 18 weeks (n = 4). (E) Representative histogram plots for CD39 and CD73 on CD4+CD25+FoxP3+ splenocytes from ADA+/+ and ADA−/− mice treated with PEG-ADA for 18 weeks. Isotype-identical monoclonal antibodies served as controls (solid gray histogram). (F) Measurement of ATP consumption and AMP formation (left panel) as well as adenosine formation (right panel) by purified CD4+CD25+ Treg cells from PEG-ADA–treated ADA−/− (n = 4) and ADA+/+ mice (n = 3). Data are interexperimental mean ± SD. *P < .05. (G) Serum adenosine levels in PEG-ADA–treated ADA−/− (n = 4) and age-matched ADA+/+ mice (n = 4) at 10, 14, and 18 weeks of follow-up. Data are interexperimental mean ± SD. *P < .05. (H) Serum hypoxanthine levels in PEG-ADA–treated ADA−/− (n = 4) and age-matched ADA+/+ mice (n = 4) at 10, 14, and 18 weeks of follow-up. Data are interexperimental mean ± SD. **P < .005.

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