Viability (%) of unpulsed-DC (UP-DC), KLH pulsed-DC (KLH-DC) and cryopreserved KLH pulsed-DC (C-KLH-DC) by 7-AAD staining. UP-DC, KLH-DC, and C-KLH-DC were stained with 7-AAD and analyzed by flow cytometry. Numbers in dot plots represent percentage of viable cells. This experiment was repeated three times with similar results.

Endocytic capacity of unpulsed-DC (UP-DC), KLH pulsed-DC (KLH-DC), cryopreserved KLH pulsed-DC (C-KLH-DC) and LPS pulsed-DC (LPS-DC). UP-DC, KLH-DC, C-KLH-DC and LPS-DC were incubated for 2 hours with fluorescein isothiocyanate-dextran at 37°c (thick line) or 4°C (thin line) and then analyzed by flow cytometry. Numbers in histogram plots designate percentage of positive cells and geometrical mean of fluorescence intensity of positive cells, respectively. This experiment was repeated three times with similar results.

Induction of tumor-specific IFNγ-secreting splenocytes by i.t. vaccination with unpulsed-DC (UP-DC), KLH pulsed-DC (KLH-DC) or cryopreserved KLH pulsed-DC (C-KLH-DC). Mice were inoculated s.c. with 2 × 10⁶ D5 tumor cells on day 0. UP-DC, KLH-DC or C-KLH-DC (1 × 10⁶) were administered i.t. on days 6, 11, 14 and 18. A control group received no treatment (i.t. PBS). Twenty one days after tumor inoculation, splenocytes from treated and control mice were incubated with specific (D5) or irrelevant (PAN 02) irradiated tumor cells in an IFNγ ELISPOT assay. Six spleens were harvested from each group and pooled together. Data are reported as the average number of tumor-specific spots per 1 × 10⁶ responders ± SE of triplicate samples after subtracting non-specific spots as detailed in the Materials and Methods section. *, P < 0.0001 versus PBS.

A. Phenotype of unpulsed-DC (UP-DC), KLH pulsed-DC (KLH-DC), cryopreserved KLH pulsed-DC (C-KLH-DC) and LPS pulsed-DC (LPS-DC). UP-DC, KLH-DC, C-KLH-DC and LPS-DC were stained using fluorochrome-conjugated monoclonal antibodies (mAbs) for MHC class I, MHC class II, CD80, CD86, CD40 and CD11c and analyzed by flow cytometry. Thin lines represent staining with matched isotype control mAbs, thick lines represent staining with the designated mAbs. Numbers in histogram plots designate percentage of positive cells and geometrical mean of fluorescence intensity of positive cells, respectively. B. Cytokine secretion by UP-DC, KLH-DC, C-KLH-DC and LPS-DC. Supernatants of DC cultures were analyzed for IL-12p70 and IL-10 content using ELISA. These experiments were repeated three times with similar results.

A. Allogeneic splenocyte stimulatory capacity of unpulsed-DC (UP-DC), KLH pulsed-DC (KLH-DC) and cryopreserved KLH pulsed-DC (C-KLH-DC). Allogeneic splenocytes (2 × 10⁵ per well), as responders, were incubated with or without increasing numbers of each type of DC as stimulators. Proliferation was measured after 5 days of co-culture using a WST-1-based assay as described in the Materials and Methods. Data are reported as the average absorbance ± SD of triplicate samples. * P < 0.001 versus UP-DC and KLH-DC. B. Cytokine release capacity of UP-DC, KLH-DC and C-KLH-DC upon induction of maturation. Supernatants of DC cultured in the presence of LPS were analyzed for IL-12p70 and IL-10 content using ELISA. * P < 0.05 versus UP-DC and KLH-DC. These experiments were repeated at least two times with similar results.

I.t. KLH pulsed-DC (KLH-DC) or cryopreserved KLH pulsed-DC (C-KLH-DC) vaccination is as effective as unpulsed-DC (UP-DC) vaccination in eliciting anti-tumor immune responses (A) and inhibiting D5 tumor growth (B, C). Mice were inoculated s.c. with 2 × 10⁶ D5 tumor cells on day 0. UP-DC, KLH-DC or C-KLH-DC (1 × 10⁶) were administered i.t. on days 6, 11, 14 and 18. Tumors were locally irradiated on days 7–11 (8.5 Gy×5). Control groups received either no treatment (i.t. PBS), i.t. UP-DC alone, i.t. KLH-DC alone, i.t. C-KLH-DC alone or radiotherapy (RT) alone. A. Induction of circulating tumor-reactive IFNγ-producing CD8⁺ and CD4⁺ cells by i.t. vaccination with UP-DC, KLH-DC or C-KLH-DC combined with radiotherapy. Fifteen days after tumor inoculation, peripheral blood mononuclear cells were collected from treated mice and incubated with irradiated D5 tumor cells. Intracellular IFNγ production along with cell surface expression of CD4 and CD8 were analyzed using flow cytometry. Specificity of staining was confirmed using isotype matched control monoclonal antibodies. Blood samples (100 µl) were drawn from 6 mice per group and pooled together in order to obtain sufficient numbers of cells for analysis. B. Tumor growth curves of individual mice are shown. Each group consisted of 6 mice. C. Data are reported as the average tumor size ± SE of six mice per group. All eight groups of mice in the left and right panel were treated simultaneously in a single experiment. Data are presented in two separate graphs to enhance clarity. *, P < 0.0001 versus PBS. **, P < 0.004 versus all mono-therapies. This experiment was repeated two times with similar results.