Figure 5.
Figure 5. Functional effects of CD8CXCR5+ICOS+T cells. Cell Trace–labeled purified B cells from lymphoma tissues were activated by anti-BCR and CpG and cocultured with autologous sorted T cells in presence of PHA and IL-2 for 5 days (n = 3). (A) Proliferation of B cells evaluated by DI in each condition. (B) Representative dot plots and histograms for percentages of IgD+CD38−, IgD+CD38+, and IgD−CD38+/− cells among viable B cells (top) and proliferation rate of IgD−CD38+/− B cells (bottom) after 5 days of coculture in each condition. (C) IgG production measured in supernatant at day 5 by ELISA. A 1-way ANOVA statistic test was done.

Functional effects of CD8CXCR5+ICOS+T cells. Cell Trace–labeled purified B cells from lymphoma tissues were activated by anti-BCR and CpG and cocultured with autologous sorted T cells in presence of PHA and IL-2 for 5 days (n = 3). (A) Proliferation of B cells evaluated by DI in each condition. (B) Representative dot plots and histograms for percentages of IgD+CD38, IgD+CD38+, and IgDCD38+/− cells among viable B cells (top) and proliferation rate of IgDCD38+/− B cells (bottom) after 5 days of coculture in each condition. (C) IgG production measured in supernatant at day 5 by ELISA. A 1-way ANOVA statistic test was done.

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