Figure 5.
SR1 CD7+ cells are capable of peripheral reconstitution in vivo. (A) Thymuses were harvested 10 to 12 weeks postinjection of SR1 CD7+ cells, and the percentage of live CD45+ cells and CD4 and CD8 are shown (n = 4). (B) Representative flow cytometric plots of CD3 expression on circulating human CD45+ cells harvested from the spleen of mice 10 to 12 weeks after injection of CD7+ cells (n = 6). Representative flow cytometric plots for intracellular IL-2, interferon-γ (IFN-γ), and tumor necrosis factor-α (TNF-α) upon in vitro stimulation. Human CD45+CD3+ cells were harvested from the spleen of mice 10 to 12 weeks postinjection of SR1 CD7+ cells, and stimulated for 6 hours with phorbol 12-myristate 13-acetate (PMA)/ionomycin (C) or 72 hours with CD3/CD28 (D). Percentage of cytokine-expressing cells is shown as a proportion of total human CD45+ cells within the thymus for individual mice. Results are from 3 independent experiments, with error bars corresponding to standard error of the mean.

SR1 CD7+ cells are capable of peripheral reconstitution in vivo. (A) Thymuses were harvested 10 to 12 weeks postinjection of SR1 CD7+ cells, and the percentage of live CD45+ cells and CD4 and CD8 are shown (n = 4). (B) Representative flow cytometric plots of CD3 expression on circulating human CD45+ cells harvested from the spleen of mice 10 to 12 weeks after injection of CD7+ cells (n = 6). Representative flow cytometric plots for intracellular IL-2, interferon-γ (IFN-γ), and tumor necrosis factor-α (TNF-α) upon in vitro stimulation. Human CD45+CD3+ cells were harvested from the spleen of mice 10 to 12 weeks postinjection of SR1 CD7+ cells, and stimulated for 6 hours with phorbol 12-myristate 13-acetate (PMA)/ionomycin (C) or 72 hours with CD3/CD28 (D). Percentage of cytokine-expressing cells is shown as a proportion of total human CD45+ cells within the thymus for individual mice. Results are from 3 independent experiments, with error bars corresponding to standard error of the mean.

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