Figure 1
Figure 1. Activation of CD27− B cells with CpG DNA is a function of cell-cell contact conditions. CD27− and CD27+ B cells were labeled with CFSE and activated with CpG DNA2006. After 4 days, proliferation was analyzed by flow cytometry. Activation and proliferation of CD27− naive B cells required an increase in cell density to 1 × 105 cells per well for maximal proliferation to occur. In contrast, CD27+ B cells proliferated following CpG DNA at all cell concentrations and densities, although higher cell densities led to an increase in proliferation. IL-10 improved proliferation of both CD27+ and CD27− cells, while the combination of IL-2, IL-10, and IL-15 and cell-cell contact gave maximal proliferation. Results are representative of 15 independent experiments from 9 different blood donors.

Activation of CD27 B cells with CpG DNA is a function of cell-cell contact conditions. CD27 and CD27+ B cells were labeled with CFSE and activated with CpG DNA2006. After 4 days, proliferation was analyzed by flow cytometry. Activation and proliferation of CD27 naive B cells required an increase in cell density to 1 × 105 cells per well for maximal proliferation to occur. In contrast, CD27+ B cells proliferated following CpG DNA at all cell concentrations and densities, although higher cell densities led to an increase in proliferation. IL-10 improved proliferation of both CD27+ and CD27 cells, while the combination of IL-2, IL-10, and IL-15 and cell-cell contact gave maximal proliferation. Results are representative of 15 independent experiments from 9 different blood donors.

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