Figure 2
Figure 2. Impaired cutaneous DC migration in mDia1−/− mice. (A) The number of cutaneous DCs migrating from the skin to draining LNs. The numbers of FITC+ MHC class II+ total DCs (A) and FITC+ MHC class II+ Langerin+ DC and FITC+ MHC class II+ Langerin− DC subsets (B) in draining LNs of B6 (open bars) and mDia1−/− mice (shaded bars) were analyzed 72 hours after application of FITC to the footpad. Bars represent the mean ± SD from at least 3 mice per group. (C) Mobility of LCs to CCL21. Epidermal cell suspensions were applied to the upper chamber of a transwell with 3 μm (left panel) and 8 μm (right panel) pore size without coating for 3 hours. Percentages of MHC class II+ LCs that migrated from the upper chambers to the lower are shown. (D-E) Invasive movement of LCs to CCL21. Epidermal cell suspensions were applied to the upper chamber of a transwell coated with Matrigel for 3 hours (D) and 24 hours (E). The numbers of MHC class II+ cells in the lower chamber (left panels) or in the Matrigel (right panels) were counted with flow cytometry. Data are mean ± SD of 3 independent experiments. *P < .05 vs corresponding B6 mice. (F) TAXIScan assay. BMDCs chemotaxing under the CCL21 gradient were analyzed with TAXIScan. BMDCs from B6 and mDia1−/− mice were compared in terms of the velocity. Data are mean ± SD of 4 independent experiments. *P < .05 vs corresponding B6 mice.

Impaired cutaneous DC migration in mDia1−/− mice. (A) The number of cutaneous DCs migrating from the skin to draining LNs. The numbers of FITC+ MHC class II+ total DCs (A) and FITC+ MHC class II+ Langerin+ DC and FITC+ MHC class II+ Langerin DC subsets (B) in draining LNs of B6 (open bars) and mDia1−/− mice (shaded bars) were analyzed 72 hours after application of FITC to the footpad. Bars represent the mean ± SD from at least 3 mice per group. (C) Mobility of LCs to CCL21. Epidermal cell suspensions were applied to the upper chamber of a transwell with 3 μm (left panel) and 8 μm (right panel) pore size without coating for 3 hours. Percentages of MHC class II+ LCs that migrated from the upper chambers to the lower are shown. (D-E) Invasive movement of LCs to CCL21. Epidermal cell suspensions were applied to the upper chamber of a transwell coated with Matrigel for 3 hours (D) and 24 hours (E). The numbers of MHC class II+ cells in the lower chamber (left panels) or in the Matrigel (right panels) were counted with flow cytometry. Data are mean ± SD of 3 independent experiments. *P < .05 vs corresponding B6 mice. (F) TAXIScan assay. BMDCs chemotaxing under the CCL21 gradient were analyzed with TAXIScan. BMDCs from B6 and mDia1−/− mice were compared in terms of the velocity. Data are mean ± SD of 4 independent experiments. *P < .05 vs corresponding B6 mice.

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