Figure 2.
Figure 2. Expression of Runx1 in hematopoietic lineages analyzed by flow cytometry. (A) GFP expression was determined in hematopoietic cell subsets from wild-type (WT), Runx1-IRES-GFPk/+, and Runx1-IRES-GFPk/k mice. The mean fluorescence intensity (MFI) of GFP expression in Runx1-IRES-GFPk/+ and Runx1-IRES-GFPk/k cells is shown in each panel. GFP expression in CD19+ B cells is shown; other hematopoietic subsets from Runx1-IRES-GFPk/k mice likewise had an MFI approximately twice that of cells from Runx1-IRES-GFPk/+ mice in all lineages that expressed Runx1. (B) Bone marrow (BM) cell suspensions were prepared from Runx1-IRES-GFPk/k and wild-type mice, stained with either Ter-119, Mac 1 (CD11b), or GR-1, and analyzed for GFP expression by flow cytometry. In the analysis of Ter-119+ expression, the curve for Runx1-IRES-GFPk/k cells is superimposable with that of wild-type cells and is therefore not readily apparent. (C) GFP expression in lymph node T cells (CD3+) and B cells (CD19+) from wild-type and Runx1-IRES-GFPk/k mice was determined using flow cytometry. In panels B-C, the filled and open curves indicate GFP expression in wild-type and Runx1-IRES-GFPk/k cells, respectively. (D) Western blot analysis of FACS-purified CD3+ or CD19+ lymph node cells and Ter-119+ BM cells from Runx1-IRES-GFPk/k mice. The analyzed populations had more than 98% purity. Lysates from an equal number of cells for each group (6 × 106 cells) were analyzed, and the blot was probed with a rabbit polyclonal antibody that specifically recognizes Runx1. Determination of the relative level of Runx1 mRNA expression by real-time RT-PCR in these FACS-purified cell populations is indicated below the Western blot. The results were normalized relative to input cell number.

Expression of Runx1 in hematopoietic lineages analyzed by flow cytometry. (A) GFP expression was determined in hematopoietic cell subsets from wild-type (WT), Runx1-IRES-GFPk/+, and Runx1-IRES-GFPk/k mice. The mean fluorescence intensity (MFI) of GFP expression in Runx1-IRES-GFPk/+ and Runx1-IRES-GFPk/k cells is shown in each panel. GFP expression in CD19+ B cells is shown; other hematopoietic subsets from Runx1-IRES-GFPk/k mice likewise had an MFI approximately twice that of cells from Runx1-IRES-GFPk/+ mice in all lineages that expressed Runx1. (B) Bone marrow (BM) cell suspensions were prepared from Runx1-IRES-GFPk/k and wild-type mice, stained with either Ter-119, Mac 1 (CD11b), or GR-1, and analyzed for GFP expression by flow cytometry. In the analysis of Ter-119+ expression, the curve for Runx1-IRES-GFPk/k cells is superimposable with that of wild-type cells and is therefore not readily apparent. (C) GFP expression in lymph node T cells (CD3+) and B cells (CD19+) from wild-type and Runx1-IRES-GFPk/k mice was determined using flow cytometry. In panels B-C, the filled and open curves indicate GFP expression in wild-type and Runx1-IRES-GFPk/k cells, respectively. (D) Western blot analysis of FACS-purified CD3+ or CD19+ lymph node cells and Ter-119+ BM cells from Runx1-IRES-GFPk/k mice. The analyzed populations had more than 98% purity. Lysates from an equal number of cells for each group (6 × 106 cells) were analyzed, and the blot was probed with a rabbit polyclonal antibody that specifically recognizes Runx1. Determination of the relative level of Runx1 mRNA expression by real-time RT-PCR in these FACS-purified cell populations is indicated below the Western blot. The results were normalized relative to input cell number.

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