Figure 4.
ΔdblGATA mice have defective priming in EAE. WT and ΔdblGATA mice were immunized for EAE induction and euthanized on day 8 after immunization (n = 4-5 per group; 2 independent experiments). (A-C) Analysis of inguinal dLN cells are shown in panels A-C. (A) Total number of CD45+ cells per mouse in inguinal dLNs. (B) Number of CD45+CD11b+, CD45+CD11b+CD11c+, CD11b+Ly6ChiLy6Glo/−, and CD4+ cells. (C) Cells from dLNs were stimulated with 20 μg/mL PLP180-199, and proliferation of cells was measured by [3H]adenine incorporation. (D-E) Analysis of splenocytes. (D) Total number of cells in the spleens of mice with EAE. (E) [3H]adenine incorporation assay for PLP180-199–stimulated splenocytes showing the average proliferation per mouse. (F-K) Analysis of the CNS. (F) Number of CD45hi cells. (G) Number of CD45hiCD11b+, CD45hiCD11b+CD11c+, CD11b+Ly6ChiLy6Glo/−, and CD4+ cells. (H) Representative flow cytometry plots showing MHC-II expression in myeloid DCs present in the CNS of the EAE mice. Gated on CD45hiCD11c+CD11b+ cells. (I) Quantification of the frequency of MHC-IIhi and MHC-IIlo cells among CD45hiCD11b+CD11c+ cells. (J) Histograms normalized to the mode of data depicting MHC-II, CD80, and CD86 expression among CD45hiCD11b+CD11c+ cells. (K) Quantification of the median fluorescent intensity of MHC-II, CD80, and CD86 expression among CD45hiCD11b+CD11c+MHC-II+ cells. Error bars are SEM, and significance was calculated using unpaired Student t test.

ΔdblGATA mice have defective priming in EAE. WT and ΔdblGATA mice were immunized for EAE induction and euthanized on day 8 after immunization (n = 4-5 per group; 2 independent experiments). (A-C) Analysis of inguinal dLN cells are shown in panels A-C. (A) Total number of CD45+ cells per mouse in inguinal dLNs. (B) Number of CD45+CD11b+, CD45+CD11b+CD11c+, CD11b+Ly6ChiLy6Glo/−, and CD4+ cells. (C) Cells from dLNs were stimulated with 20 μg/mL PLP180-199, and proliferation of cells was measured by [3H]adenine incorporation. (D-E) Analysis of splenocytes. (D) Total number of cells in the spleens of mice with EAE. (E) [3H]adenine incorporation assay for PLP180-199–stimulated splenocytes showing the average proliferation per mouse. (F-K) Analysis of the CNS. (F) Number of CD45hi cells. (G) Number of CD45hiCD11b+, CD45hiCD11b+CD11c+, CD11b+Ly6ChiLy6Glo/−, and CD4+ cells. (H) Representative flow cytometry plots showing MHC-II expression in myeloid DCs present in the CNS of the EAE mice. Gated on CD45hiCD11c+CD11b+ cells. (I) Quantification of the frequency of MHC-IIhi and MHC-IIlo cells among CD45hiCD11b+CD11c+ cells. (J) Histograms normalized to the mode of data depicting MHC-II, CD80, and CD86 expression among CD45hiCD11b+CD11c+ cells. (K) Quantification of the median fluorescent intensity of MHC-II, CD80, and CD86 expression among CD45hiCD11b+CD11c+MHC-II+ cells. Error bars are SEM, and significance was calculated using unpaired Student t test.

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