Fig. 3.
Fig. 3. Cell tracking in vitro of cultured bone marrow G0CD34+ cells using the membrane dye PKH2. G0CD34+ cells were isolated, stained with PKH2, and cultured in IMDM containing 10% FCS in the presence of SCF, IL-3, and IL-6 for 7 days. A sample fixed in 1% paraformaldehyde on day 0 (A) was used to identify the fluorescence intensity corresponding to freshly stained cells. On day 7, cells were harvested and stained with either a PE-conjugated isotype control monoclonal antibody (B) or PE-conjugated CD34 (C). Samples were analyzed for PKH2 (X axis) and PE (Y axis) fluorescence to estimate the fraction of CD34+ cells remaining as CNR cells. As can be seen in C, 83% of cultured cells remained CD34+, and 16% could be identified as CNR cells.

Cell tracking in vitro of cultured bone marrow G0CD34+ cells using the membrane dye PKH2. G0CD34+ cells were isolated, stained with PKH2, and cultured in IMDM containing 10% FCS in the presence of SCF, IL-3, and IL-6 for 7 days. A sample fixed in 1% paraformaldehyde on day 0 (A) was used to identify the fluorescence intensity corresponding to freshly stained cells. On day 7, cells were harvested and stained with either a PE-conjugated isotype control monoclonal antibody (B) or PE-conjugated CD34 (C). Samples were analyzed for PKH2 (X axis) and PE (Y axis) fluorescence to estimate the fraction of CD34+ cells remaining as CNR cells. As can be seen in C, 83% of cultured cells remained CD34+, and 16% could be identified as CNR cells.

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