DC cytokine profile after culture with live or apoptotic B16 cells.

<p>DC were cultured alone (DC) or with live (zVAD treated) or apoptotic (γ-irradiated) B16 cells for 24 h and stimulated or not with LPS and IFNγ. As controls, B16 zVAD and B16γ cells were also cultured alone. DC were then assessed for their ability to produce IL-12p70 (A) or IL-10 (B) by ELISA. In the upper panels, data from one out of three independent experiments are shown. In the bottom panels, for LPS and IFNγ stimulation, relative IL-12p70 and IL-10 productions are expressed as a percentage of the cytokine production obtained for DC alone. Mean percentage values±SEM are shown. The significance of differences between series of results was assessed using a paired t test (n = 3, 3 independent experiments).</p

More native antigen in live than in apoptotic donor cells: improved antigen crosspresentation by DC.

<p>A, B, 30.10⁶ live (zVAD treated) or apoptotic (γ-irradiated) B16 cells (A) or L-OVA cells (B) were lysed for protein extraction. Lysates from B16 cells were analysed using anti-gp100, anti-TRP2 and anti-actin antibodies (A). Lysates from L-OVA cells were analysed using anti-OVA and anti-actin antibodies antibodies (B). Anti-actin antibodies were used as controls. C, DC were cultured with different numbers of live (filled triangle) or apoptotic (open triangle) L-OVA cells or live L cells (filled square). DC were then purified by magnetic sorting using anti-CD11c microbeads and cultured with B3Z-T cells hybridoma cells for 18 h. Activation after recognition of the SIINFEKL-K^b complex was detected by optical density measurement at 560 nm after addition of the CPRG substrate. The significance of differences between series of results was assessed using a two-tailed unpaired t test. **p<0.01, *p<0,05, n.s. not significant. Mean ± SEM, representative of two independent experiments.</p

DC maturation after culture with live or apoptotic B16 cells.

<p>DC were cultured with live (zVAD treated) or apoptotic (γ-irradiated) B16 cells for 24 h in the presence of culture medium or LPS and IFNγ. The expression of maturation molecules was then tested by flow cytometry. One representative experiment out of three independent experiments is shown.</p