Figure 5
Figure 5. The cytokine signaling deficit in FL TILs is restricted to PD-1hiCD4+ T cells and includes TFH cells and non-TFH cells. FL LN specimens were cultured with or without IL-4 for 15 minutes and then assayed for IL-4–induced phosphorylation of p-STAT6 by combining CD3-, CD5-, CD4-, and PD-1-specific Abs with p-STAT6 Ab in the phospho-flow cytometric assay. (A) IL-4–induced p-STAT6 was determined in CD4+ TILs gated on different expression levels of PD-1. (B) Data are shown as mean FC ± SEM; FL, n = 7. (C) IL-4–induced p-STAT6 was determined in CD4+ FL TILs, based on expression of ICOS and CXCR5. Shown is 1 representative case, and (D) mean FC ± SEM; FL, n = 3. (E) IL-4–induced p-STAT6 was determined in CD4+ tonsil T cells, based on expression of ICOS and CXCR5. Mean FC ± SEM; tonsil, n = 3. Statistical difference between groups was determined by paired 2-tailed Student t test.

The cytokine signaling deficit in FL TILs is restricted to PD-1hiCD4+ T cells and includes TFH cells and non-TFH cells. FL LN specimens were cultured with or without IL-4 for 15 minutes and then assayed for IL-4–induced phosphorylation of p-STAT6 by combining CD3-, CD5-, CD4-, and PD-1-specific Abs with p-STAT6 Ab in the phospho-flow cytometric assay. (A) IL-4–induced p-STAT6 was determined in CD4+ TILs gated on different expression levels of PD-1. (B) Data are shown as mean FC ± SEM; FL, n = 7. (C) IL-4–induced p-STAT6 was determined in CD4+ FL TILs, based on expression of ICOS and CXCR5. Shown is 1 representative case, and (D) mean FC ± SEM; FL, n = 3. (E) IL-4–induced p-STAT6 was determined in CD4+ tonsil T cells, based on expression of ICOS and CXCR5. Mean FC ± SEM; tonsil, n = 3. Statistical difference between groups was determined by paired 2-tailed Student t test.

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