![Figure 1. CD25 expression marks distinct subsets of cells in the CML LIC population. (A) Screening strategy for antigens differentially expressed on CML LSK cells. LSK cells were transduced with BCR-ABL retroviral vector and transplanted into recipient mice. Bone marrow cells were collected 10 to 12 days after transplantation, and staining patterns of candidate antigens in 3 types of cells (BCR-ABL+LSK, LKS−, and BCR-ABL−LSK) were analyzed by flow cytometry. (B) CD25+ cells in the 3 cell types in panel A (%) (means ± standard deviation [SD], n = 3). (C) Flow cytometric analysis of CD25 expression in normal bone marrow fractions, including LSK, GMP (Lin−c-Kit+Sca-1−CD34+FcγRII/III+), and CD4+ cells (orange histograms). Gray histograms indicate isotype control staining. Numbers indicate the CD25-positive fraction (means ± SD, n = 3). (D) Flow cytometric analysis of BCR-ABL+LSK cells from CML model mice costained with CD25 and FcεRIα. Giemsa-stained cytospin specimens of the 3 fractions (CD25+F+LSK, CD25+F−LSK, and CD25−F−LSK cells) are shown. Images were obtained and analyzed using a microscope (IX70; Olympus). UPlanApo 40×/0.85 objective lens (Olympus) and DP Controller (Olympus). (E) qPCR analysis of mast cell–related genes in the indicated fractions from CML model mice (means ± SD, n = 4). *P < .05; **P < .01.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/123/16/10.1182_blood-2013-07-517847/4/2540f1.jpeg?Expires=1735812138&Signature=2n9Nmo8hixq4NkKdK57z7~79cSl8IMNZN3DOhjVcCAdR42PJL4s54hKY1G2TQhNlRv~0cabJnWaoYgZtz2swLq1EmCiIvheZoIaF-hCJwrBFhui-EXgYaFdQNEmlU0df3d~T2s4b6cQR7ivoGG5vMvsKYLwpYNXJia0fmfIUVAifd8EV-gfa9zWYoeJ9G5S6vzc9-PSF8GXJIrAlWBcAMCEd3MH1CO9gklyXtfIa4DVOg8KHcrdPFMl7SIGqlHFanhp1aXnsFWO1cB6yjaeyvKxH3J707cEbYdL7oC-Gwwtdt6aILgaLr7A~fzHlN2VyzsxyJey2OE9J0DVZfWSv6w__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
CD25 expression marks distinct subsets of cells in the CML LIC population. (A) Screening strategy for antigens differentially expressed on CML LSK cells. LSK cells were transduced with BCR-ABL retroviral vector and transplanted into recipient mice. Bone marrow cells were collected 10 to 12 days after transplantation, and staining patterns of candidate antigens in 3 types of cells (BCR-ABL+LSK, LKS−, and BCR-ABL−LSK) were analyzed by flow cytometry. (B) CD25+ cells in the 3 cell types in panel A (%) (means ± standard deviation [SD], n = 3). (C) Flow cytometric analysis of CD25 expression in normal bone marrow fractions, including LSK, GMP (Lin−c-Kit+Sca-1−CD34+FcγRII/III+), and CD4+ cells (orange histograms). Gray histograms indicate isotype control staining. Numbers indicate the CD25-positive fraction (means ± SD, n = 3). (D) Flow cytometric analysis of BCR-ABL+LSK cells from CML model mice costained with CD25 and FcεRIα. Giemsa-stained cytospin specimens of the 3 fractions (CD25+F+LSK, CD25+F−LSK, and CD25−F−LSK cells) are shown. Images were obtained and analyzed using a microscope (IX70; Olympus). UPlanApo 40×/0.85 objective lens (Olympus) and DP Controller (Olympus). (E) qPCR analysis of mast cell–related genes in the indicated fractions from CML model mice (means ± SD, n = 4). *P < .05; **P < .01.
