![Figure 3. Phenotype of CD4+CD25high T cells from patients with cGVHD. (A) Representative histogram plots are shown of flow sorted CD4+CD25high T cells (thick solid line) and CD4+CD25- T cells (thin solid line), which were fixed, permeabilized, and stained with PE-conjugated anti-CTLA-4 or isotype control (thin dotted line) in a patient with (left) or without (right) cGVHD. Mean cell fluorescence is shown as the figure to the top right of each histogram (n = 6 cGVHD; n = 5 no GVHD). (B) CD40L mean cellular fluorescence (± SEM) shown for both CD4+CD25high cells (▪) and CD4+CD25- cells (□) in patients with or without cGVHD and healthy volunteers. (C) CD62L expression of CD4+CD25high T cells expressed as mean cellular fluorescence (± SEM). Significant differences indicated below the histograms (cGVHD n = 10; no GVHD n = 8; healthy volunteers n = 5). (D) Results of add-back experiments in a representative patient with cGVHD (top, n = 8) and a healthy volunteer (bottom, n = 3); 1 × 104 flow-sorted CD4+CD25high (25+) and 1 × 104 CD4+CD25- T cells (25-), alone or in coculture (1:1 ratio of 25+ or 25- cells, total 2 × 104 cells/well, denoted as 25-/- or 25+/-), were stimulated with PHA (2 μg/mL) in the presence of 1 × 104/well irradiated autologous accessory cells (ACs). Proliferations at 72 hours by [H3]-thymidine incorporation are shown in the left panels and IFN-γ production by cytokine ELISA in the right panels. These experiments were also performed with the addition of neutralizing antibody to IL-10 (α-IL10). Similar results were observed in patients without GVHD (n = 6). (E) CD4+CD25- cells were stimulated as above in coculture with different numbers of CD4+CD25high T cells derived from a patient with cGVHD and a control. Percentage inhibition of proliferation at 72 hours is shown. (F) Autologous CD4+ T cells were stimulated with immobilized anti-CD3 monoclonal antibody (1 μg/mL) in the presence or absence of CD4+CD25high T cell clones at a 1:1 ratio and at 72 hours, proliferation was measured as above. Mean proliferations (± SEM) of individual clones derived from one patient are shown. (G) IL-10 was added to PHA-stimulated CD4+ cells in the presence of irradiated autologous ACs and in the presence or absence of neutralizing antibody to IL-10. Percentage inhibition of proliferation at 72 hours is shown.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/103/6/10.1182_blood-2003-06-2073/6/zh80060458440003.jpeg?Expires=1724192041&Signature=bUXr9Gn34XUkHrIWFH6Fmu-Ojy91UD6YvwiIszc-7tYvY4wNZPxbe757vmi0O5zG7WBBwTC0sXiGVKFdgk9si4WKtSf~U6xjK5NkqHTun7neNsk4MYmOTqjZdduF6bVgxv6gcr3K0B3aNgsVPP0y0VKkht1ckMEk806gqpJfiVAFh8RTtw2R-o6ijbORWKMbHtssmtXufbpVIhBzVbwzRjTU7L7C~mjpiZJ4U0T7HrsthC8sctERfdVzxLTCzB8A~1RvwBhAm5-9-5vH0cpXEVevqxe7vlHi-hUV9EYHIN7FZc1yewWaZaJ~CsWp3jDvvzFndoGNmMT8ZOpVdROTzg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Phenotype of CD4+CD25high T cells from patients with cGVHD. (A) Representative histogram plots are shown of flow sorted CD4+CD25high T cells (thick solid line) and CD4+CD25- T cells (thin solid line), which were fixed, permeabilized, and stained with PE-conjugated anti-CTLA-4 or isotype control (thin dotted line) in a patient with (left) or without (right) cGVHD. Mean cell fluorescence is shown as the figure to the top right of each histogram (n = 6 cGVHD; n = 5 no GVHD). (B) CD40L mean cellular fluorescence (± SEM) shown for both CD4+CD25high cells (▪) and CD4+CD25- cells (□) in patients with or without cGVHD and healthy volunteers. (C) CD62L expression of CD4+CD25high T cells expressed as mean cellular fluorescence (± SEM). Significant differences indicated below the histograms (cGVHD n = 10; no GVHD n = 8; healthy volunteers n = 5). (D) Results of add-back experiments in a representative patient with cGVHD (top, n = 8) and a healthy volunteer (bottom, n = 3); 1 × 104 flow-sorted CD4+CD25high (25+) and 1 × 104 CD4+CD25- T cells (25-), alone or in coculture (1:1 ratio of 25+ or 25- cells, total 2 × 104 cells/well, denoted as 25-/- or 25+/-), were stimulated with PHA (2 μg/mL) in the presence of 1 × 104/well irradiated autologous accessory cells (ACs). Proliferations at 72 hours by [H3]-thymidine incorporation are shown in the left panels and IFN-γ production by cytokine ELISA in the right panels. These experiments were also performed with the addition of neutralizing antibody to IL-10 (α-IL10). Similar results were observed in patients without GVHD (n = 6). (E) CD4+CD25- cells were stimulated as above in coculture with different numbers of CD4+CD25high T cells derived from a patient with cGVHD and a control. Percentage inhibition of proliferation at 72 hours is shown. (F) Autologous CD4+ T cells were stimulated with immobilized anti-CD3 monoclonal antibody (1 μg/mL) in the presence or absence of CD4+CD25high T cell clones at a 1:1 ratio and at 72 hours, proliferation was measured as above. Mean proliferations (± SEM) of individual clones derived from one patient are shown. (G) IL-10 was added to PHA-stimulated CD4+ cells in the presence of irradiated autologous ACs and in the presence or absence of neutralizing antibody to IL-10. Percentage inhibition of proliferation at 72 hours is shown.
