Figure 3
Figure 3. Kinetics of CLPF-driven T cell reconstitution. (A) Kinetic analyses of B-cell (squares) and T-cell (diamonds) reconstitution of spleen (left panel) and blood (right panel) of sublethally irradiated mice that received transplants of 103 CLPF (black) or Flk2− fraction cells (white). Results shown are mean values of 3 to 5 animals analyzed per time point. For blood analysis, the same animals were bled periodically for 10 weeks. (B) FACS plots illustrating the CD4/CD8 profile of host (top row) and CLPF derived donor cells (bottom row) as well as reconstitution with thymic B cells (B220+), γδ T cells, and NK cells showing the lymphoid potential of CLPFs. (C) FACS plots illustrating the T-lineage development of intravenously injected CLPF in the thymus, from 1 to 5 weeks. Detailed analysis of CD4/CD8 development (top row), and within the CD4/CD8 double negative fraction, CD44 and CD25 development (middle row) or CD25 and c-Kit development (bottom row), after previously gating on lineage negative cells. Shown are representative FACS plots from 3 mice that received transplants per time point. (D) Thymic reconstitution 6 days after intrathymic (i.t.) injection transfer of 103 CLPF into congenic unirradiated mice. Events shown are gated on lineage negative donor-derived cells. FACS analysis reveals generation of c-Kithi DN1 (CD25−c-Kit+) and c-Kithi DN2(CD25+c-Kit+) directly derived from CLPF. Numbers on plots are percentages of gated cells.

Kinetics of CLPF-driven T cell reconstitution. (A) Kinetic analyses of B-cell (squares) and T-cell (diamonds) reconstitution of spleen (left panel) and blood (right panel) of sublethally irradiated mice that received transplants of 103 CLPF (black) or Flk2 fraction cells (white). Results shown are mean values of 3 to 5 animals analyzed per time point. For blood analysis, the same animals were bled periodically for 10 weeks. (B) FACS plots illustrating the CD4/CD8 profile of host (top row) and CLPF derived donor cells (bottom row) as well as reconstitution with thymic B cells (B220+), γδ T cells, and NK cells showing the lymphoid potential of CLPFs. (C) FACS plots illustrating the T-lineage development of intravenously injected CLPF in the thymus, from 1 to 5 weeks. Detailed analysis of CD4/CD8 development (top row), and within the CD4/CD8 double negative fraction, CD44 and CD25 development (middle row) or CD25 and c-Kit development (bottom row), after previously gating on lineage negative cells. Shown are representative FACS plots from 3 mice that received transplants per time point. (D) Thymic reconstitution 6 days after intrathymic (i.t.) injection transfer of 103 CLPF into congenic unirradiated mice. Events shown are gated on lineage negative donor-derived cells. FACS analysis reveals generation of c-Kithi DN1 (CD25c-Kit+) and c-Kithi DN2(CD25+c-Kit+) directly derived from CLPF. Numbers on plots are percentages of gated cells.

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