Figure 5.
Characterization of CTLs induced by stimulation with mature DCs cocultured with apoptotic MM cells. (A) CTLs induced by stimulations with DCs cocultured with apoptotic U266 bodies showed significantly higher cytotoxicity (*, P = .02) against U266 cells (▪) than against RPMI 8226 cells (□) or K562 cells (▦), assessed with 51Cr-release assay at indicated effector-to-target (E/T) ratios for 4 hours at 37°C. Spontaneous release of target cells was less than 15%. Results shown are mean ± SD of triplicate wells and representative of 3 experiments. (B) HLA restriction of CTLs was examined using target blocking 51Cr-release assay. CTLs stimulated with apoptotic U266 body–pulsed DCs were cocultured with 51Cr-labeled U266 after incubation with blocking antibody against HLA class I (□), HLA class II (▨), control antibody (▦), or without antibody (▪). Cytotoxicity was significantly inhibited by anti–HLA class I Abs (*, P = .02). Spontaneous release of target cells was less than 15%. Results shown are mean ± SD of triplicate wells and representative of 2 experiments. (C) Cell surface phenotype of CTLs was analyzed by flow cytometry using FITC- or PE-conjugated Abs against CD3, CD8, CD4, and CD56 (filled histogram). Percentages positive are calculated relative to an isotype-matched control Ab (open histogram).