Figure 1
De novo priming of CD8+ T cells with RNA-pulsed DCs. (A) Coexpression of HLA-A2 and tyrosinase proteins was detected by flow cytometry in DCs of an HLA-A2+ donor transfected with 24 μg tyrosinase ivt-RNA (left histograms) and DCs of an HLA-A2− donor transfected with 48 μg HLA-A2 and 24 μg tyrosinase ivt-RNA (right histograms). Stained samples are represented by filled curves and corresponding controls by empty curves. Data are representative of 9 independent experiments, demonstrating that all DCs used for T-cell priming coexpressed both proteins. (B) Columns represent the amount of IFN-γ (picograms per milliliter) secreted by a tyrosinase-independent HLA-A2 allo-reactive T-cell clone (JB4) and an HLA-A2–restricted tyrosinase peptide–specific T-cell clone (Tyr-F8) after coincubation with RNA-pulsed DCs, 10 hours after electroporation. IFN-γ was quantified in culture supernatants by ELISA. Mean values and mean deviations represent duplicates. n.d. indicates not detectable. (C) DCs of an HLA-A2− donor were transfected with HLA-A2 (48 μg) and tyrosinase (24 μg) or melan-A (48 μg) ivt-RNA alone and in combination and used for coincubation with the HLA-A2 allo-reactive CTL clone (JB4), 2 HLA-A2–restricted tyrosinase peptide–specific CTL clones (Tyr-F8 and IVS-B), and an HLA-A2–restricted melan-A peptide–specific CTL clone (A42) 10 hours after electroporation. IFN-γ was quantified in culture supernatants by ELISA and presented as picograms per milliliter. Mean values and mean deviations represent duplicates. n.d. indicates not detectable.

De novo priming of CD8+ T cells with RNA-pulsed DCs. (A) Coexpression of HLA-A2 and tyrosinase proteins was detected by flow cytometry in DCs of an HLA-A2+ donor transfected with 24 μg tyrosinase ivt-RNA (left histograms) and DCs of an HLA-A2 donor transfected with 48 μg HLA-A2 and 24 μg tyrosinase ivt-RNA (right histograms). Stained samples are represented by filled curves and corresponding controls by empty curves. Data are representative of 9 independent experiments, demonstrating that all DCs used for T-cell priming coexpressed both proteins. (B) Columns represent the amount of IFN-γ (picograms per milliliter) secreted by a tyrosinase-independent HLA-A2 allo-reactive T-cell clone (JB4) and an HLA-A2–restricted tyrosinase peptide–specific T-cell clone (Tyr-F8) after coincubation with RNA-pulsed DCs, 10 hours after electroporation. IFN-γ was quantified in culture supernatants by ELISA. Mean values and mean deviations represent duplicates. n.d. indicates not detectable. (C) DCs of an HLA-A2 donor were transfected with HLA-A2 (48 μg) and tyrosinase (24 μg) or melan-A (48 μg) ivt-RNA alone and in combination and used for coincubation with the HLA-A2 allo-reactive CTL clone (JB4), 2 HLA-A2–restricted tyrosinase peptide–specific CTL clones (Tyr-F8 and IVS-B), and an HLA-A2–restricted melan-A peptide–specific CTL clone (A42) 10 hours after electroporation. IFN-γ was quantified in culture supernatants by ELISA and presented as picograms per milliliter. Mean values and mean deviations represent duplicates. n.d. indicates not detectable.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal