Inhibition of human AML stem cell engraftment in severely immunodeficient NOG mice by CTL-2A12. (A) Specific lysis by CTL-2A12 of primary leukemia cells. A standard 4-hour 51Cr release assay was conducted at the indicated E/T ratios. The CD34+ fraction of 3 primary AML cells positive for HLA-B*4403 and the ACC-6+ allele by genotyping (AML-1, -2 and -3; the expression level of HMSD was 47%, 28%, and 24% of that in the recipient B-LCL, respectively) and 1 HLA-B*4403+, ACC-6 allele-negative (AML-4) were tested. FAB denotes French-American-British classification. (B) Representative flow cytometric profiles of peripheral blood and BM cells from AML-inoculated NOG mice for the expression of human CD45 and CD34. Peripheral blood and BM cells were obtained 5 weeks after inoculation from mice receiving 7.0 × 106 AML-2 CD34+ cells (negative for ACC-2D mHA) that had been incubated with either CTL-2A12 (top), control CTL-3B5 (middle; HLA-B*4403-restricted, ACC-2D mHA-specific CTL), or culture medium alone (bottom) at a T-cell/AML cell ratio of 5:1. (C) Summary of results from engraftment experiments. Mean (± SD) percentage of CD45 and CD34 double-positive cells of 3 mice in each group at 5 weeks after inoculation and the P values examined by 1-way ANOVA test are shown. Asterisk indicates that CD45 and CD34 double-positive cells were not detectable in NOG mice inoculated with AML-2 cells preincubated with CTL-2A12.