Figure 3
Figure 3. SR-A–mediated maturation of fucoidan-stimulated blood DCs. (A) iMDDCs (106) were left untreated (Untreated) or transfected with DharmaFECT alone (Shock), 200 nM siRNA of SR-A (SR-A siRNA), or 200 nM nontargeting siRNA (Non-siRNA) for 24 hours. Next, the cells were harvested and incubated with Alexa Fluor 488–conjugated anti–SR-A Ab for 30 minutes at 4°C and then analyzed by fluorescence-activated cell sorter. (Bottom panel) The expression of SR-A proteins in siRNA-transfected iMDDCs was then measured by Western blot. (B) iMDDCs were treated and harvested as in panel A. Control (Non-siRNA) and SR-A–deficient iMDDCs were then stimulated with the indicated concentrations of fucoidan or LPS for 24 hours, after which the expression level of CD83 was measured by flow cytometry. *P < .01 compared with Non-siRNA. (C) PBDCs were pretreated with control IgG or anti–SR-A Ab (5 μg) for 1 hour and further cultured in the presence or absence of fucoidan. After 24 hours, CD11chighCD123low and CD11clowCD123high cells were gated and examined for CD83 expression. (Top panel) The expression levels of CD123, CD11c, and CD83 on freshly isolated PBDCs. (D) CD11c+ mDCs were purified using a cell sorter as in Figure 2B and then treated with control IgG or anti–SR-A Ab for 24 hours. The results shown represent the mean ± SD of 3 independent experiments.

SR-A–mediated maturation of fucoidan-stimulated blood DCs. (A) iMDDCs (106) were left untreated (Untreated) or transfected with DharmaFECT alone (Shock), 200 nM siRNA of SR-A (SR-A siRNA), or 200 nM nontargeting siRNA (Non-siRNA) for 24 hours. Next, the cells were harvested and incubated with Alexa Fluor 488–conjugated anti–SR-A Ab for 30 minutes at 4°C and then analyzed by fluorescence-activated cell sorter. (Bottom panel) The expression of SR-A proteins in siRNA-transfected iMDDCs was then measured by Western blot. (B) iMDDCs were treated and harvested as in panel A. Control (Non-siRNA) and SR-A–deficient iMDDCs were then stimulated with the indicated concentrations of fucoidan or LPS for 24 hours, after which the expression level of CD83 was measured by flow cytometry. *P < .01 compared with Non-siRNA. (C) PBDCs were pretreated with control IgG or anti–SR-A Ab (5 μg) for 1 hour and further cultured in the presence or absence of fucoidan. After 24 hours, CD11chighCD123low and CD11clowCD123high cells were gated and examined for CD83 expression. (Top panel) The expression levels of CD123, CD11c, and CD83 on freshly isolated PBDCs. (D) CD11c+ mDCs were purified using a cell sorter as in Figure 2B and then treated with control IgG or anti–SR-A Ab for 24 hours. The results shown represent the mean ± SD of 3 independent experiments.

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