Figure 3
Figure 3. Wnt4 has a direct effect on ETP and DN2 expansion. (A) Analysis of homing to the Wnt4-deficient and -sufficient adult thymus. The number and relative contribution of donor-derived (CD45.1+) Lin− cells was determined 36 hours after injection. The histograms represent mean ± SEM from 7 mice per group. (B) Expression of chemokines and P-selectin in the Wnt4-deficient and -sufficient adult thymus. The histograms represent mean ± SEM from 4 to 5 mice per group. (C) Analysis of T-cell development in culture in the presence of GFP+ OP9-DW4 or OP9-DL1 stromal cells. GFP− cells were analyzed by flow cytometry at indicated times and are expressed as number of cells/ETP seeded on day 0. The histogram represents mean ± SEM from a total of 8 replicates from 3 independent experiments. (D) Analysis of T-cell differentiation as defined by cKit and CD25 staining on day 5. The histogram on the left represents ETP and DN2 frequencies among GFP− cells. The histogram in the middle represents the number of cells with ETP and DN2 phenotype on d5 per ETP seeded (mean ± SEM; n = 8 for wild type, n = 5 for Tcf7−/−). Representative flow cytometry data gated on GFP− cells are shown on the right. (E) Expression of selected genes associated with DN2-DN3 progression and early T-cell development. Histogram represents the relative mRNA levels from sorted GFP− lymphocytes after 2 or 5 days of coculture (ratio OP9-DW4/OP9-DL1 from paired experiments; mean ± SEM; n = 3; *P < .05, **P < .01, ***P < .005).

Wnt4 has a direct effect on ETP and DN2 expansion. (A) Analysis of homing to the Wnt4-deficient and -sufficient adult thymus. The number and relative contribution of donor-derived (CD45.1+) Lin cells was determined 36 hours after injection. The histograms represent mean ± SEM from 7 mice per group. (B) Expression of chemokines and P-selectin in the Wnt4-deficient and -sufficient adult thymus. The histograms represent mean ± SEM from 4 to 5 mice per group. (C) Analysis of T-cell development in culture in the presence of GFP+ OP9-DW4 or OP9-DL1 stromal cells. GFP cells were analyzed by flow cytometry at indicated times and are expressed as number of cells/ETP seeded on day 0. The histogram represents mean ± SEM from a total of 8 replicates from 3 independent experiments. (D) Analysis of T-cell differentiation as defined by cKit and CD25 staining on day 5. The histogram on the left represents ETP and DN2 frequencies among GFP cells. The histogram in the middle represents the number of cells with ETP and DN2 phenotype on d5 per ETP seeded (mean ± SEM; n = 8 for wild type, n = 5 for Tcf7−/−). Representative flow cytometry data gated on GFP cells are shown on the right. (E) Expression of selected genes associated with DN2-DN3 progression and early T-cell development. Histogram represents the relative mRNA levels from sorted GFP lymphocytes after 2 or 5 days of coculture (ratio OP9-DW4/OP9-DL1 from paired experiments; mean ± SEM; n = 3; *P < .05, **P < .01, ***P < .005).

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