Fig. 4.
Fig. 4. Proliferation and differentiation of purified CD34+ cells cultured in the presence of MIP-1α, IL-3, IL-6, IL-11, FL, SCF, and MGDF was evaluated by means of two-color staining with PE-labeled anti-CD34 (vertical axis) and FITC-labeled anti-CD61 (horizontal axis) antibodies. The first panel represents a control obtained with irrelevant antibodies, and the percentage of positive cells per each quadrant is indicated. The flow cytometry analysis shows the presence of a small subset of CD34+ cells that are also CD61+ among cells seeded on day 0. The number of CD34+/CD61+ cells increased on day 5, and expansion peaked on day 7. Cells expressing the CD34+ phenotype were still present during the first week of culture. Conversely, on day 12 most of the CD34+ cells were already differentiated, and 39% of the cells acquired the CD34−/CD61+ phenotype. The results of one representative experiment of five are shown.

Proliferation and differentiation of purified CD34+ cells cultured in the presence of MIP-1α, IL-3, IL-6, IL-11, FL, SCF, and MGDF was evaluated by means of two-color staining with PE-labeled anti-CD34 (vertical axis) and FITC-labeled anti-CD61 (horizontal axis) antibodies. The first panel represents a control obtained with irrelevant antibodies, and the percentage of positive cells per each quadrant is indicated. The flow cytometry analysis shows the presence of a small subset of CD34+ cells that are also CD61+ among cells seeded on day 0. The number of CD34+/CD61+ cells increased on day 5, and expansion peaked on day 7. Cells expressing the CD34+ phenotype were still present during the first week of culture. Conversely, on day 12 most of the CD34+ cells were already differentiated, and 39% of the cells acquired the CD34/CD61+ phenotype. The results of one representative experiment of five are shown.

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