Figure 4.
Induction of DC maturation and cytokines secretion by recombinant Hsp70L1 protein. (A) Phenotypic maturation of DCs induced by recombinant Hsp70L1 protein. DCs were treated with Hsp70L1, Hsp70, LPS, or His-CK for 48 hours then collected for FACS analysis of CD40, CD80, CD83, CD86, and HLA-DR expression. Gray histograms indicate autofluorescence; open thin line histograms, His-CK–treated DCs; and open thick line histograms, HSP- or LPS-treated DCs. (B) Functional DC maturation, assessed by MLR. DCs pretreated with the indicated stimuli, as described for panel A, were irradiated and used as stimulators, with T cells from a different donor as responders. T-cell proliferation was measured by thymidine incorporation. Experiments were repeated 3 times, and data are displayed as means ± SEM. (C) Cytokine production of DCs stimulated with recombinant Hsp70L1. DCs were cultured with Hsp70L1, Hsp70, His-CK, or LPS proteins in 3 formats; native protein (▪), native protein in the presence of 50 μg/mL PMB (▪), or denatured protein (100°C, 20 minutes) for 24 hours (□). The levels of IL-12p70, TNF-α, and IL-1β in supernatants were measured by ELISA. Data are displayed as mean cytokine concentration (pg/mL) ± SEM. P < .05 for IL-12p70 production between Hsp70L1 and human Hsp70.