Fig. 4.
Fig. 4. In vivo differentiative capacity of SL-ICs analyzed by flow cytometry. / Cell surface marker analysis of a representative engrafted NOD/SCID mouse is shown. (A) Six weeks later, bone marrow cells from a NOD/SCID mouse implanted with 105 CD34++CD38−cells from patient No. 5 were analyzed by flow cytometry. Cells were stained with anti–CD45 mAb and the mouse isotype IgG1 control mAb. Viable cells were sorted according to their CD45 expression. (B) The CD45+ gated cells were stained with anti–CD34-FITC, anti–CD38-PE, and anti–CD19-PE mAbs, respectively. (C) Identical cell surface marker analysis was performed on the original blasts of patient No. 5.

In vivo differentiative capacity of SL-ICs analyzed by flow cytometry.

Cell surface marker analysis of a representative engrafted NOD/SCID mouse is shown. (A) Six weeks later, bone marrow cells from a NOD/SCID mouse implanted with 105 CD34++CD38cells from patient No. 5 were analyzed by flow cytometry. Cells were stained with anti–CD45 mAb and the mouse isotype IgG1 control mAb. Viable cells were sorted according to their CD45 expression. (B) The CD45+ gated cells were stained with anti–CD34-FITC, anti–CD38-PE, and anti–CD19-PE mAbs, respectively. (C) Identical cell surface marker analysis was performed on the original blasts of patient No. 5.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal