Figure 2
Figure 2. NIK-deficient T cells are defective in mediating EAE induction when adoptively transferred to Rag2−/− mice. (A,B) T cells isolated from NIK+/+ and NIK−/− mice were mixed with B cells derived from NIK+/+ mice and adoptively transferred into Rag2−/− mice. One day after the cell transfer, recipient mice were immunized with MOG35-55 peptide as described in Figure 1A. EAE incidence (A) and disease scores (B) were monitored daily. Mice transferred with NIK+/+ and NIK−/− donor T cells are indicated as filled circles and squares, respectively. (C) Rag2−/− mice were transferred with the indicated donor T cells together with wild-type B cells. MOG35-55-immunized mice were killed on day 14 or day 24. Splenic T cells were stimulated for 4 hours with PMA plus ionomycin and subjected to ICS and flow cytometry to determine the frequency of Th17 cells among CD4+CD44+ cells based on IL-17A production. Data are mean value of the indicated number of mice (each circle or square represents 1 individual mouse). (D) Rag2−/− mice were transferred with the indicated donor T cells together with wild-type B cells. After 14 or 24 days of MOG immunization, flow cytometry was performed to determine the frequency of CD4+CD45+ cells infiltrating to the brain and spinal cord. Data are mean value of the indicated number of mice. (E) MOG-immunized Rag2−/− recipients were killed on day 24 for isolating RNA from total CNS tissue. Real-time PCR was performed to determine the relative expression of the indicated genes as described in Figure 1F.

NIK-deficient T cells are defective in mediating EAE induction when adoptively transferred to Rag2−/− mice. (A,B) T cells isolated from NIK+/+ and NIK−/− mice were mixed with B cells derived from NIK+/+ mice and adoptively transferred into Rag2−/− mice. One day after the cell transfer, recipient mice were immunized with MOG35-55 peptide as described in Figure 1A. EAE incidence (A) and disease scores (B) were monitored daily. Mice transferred with NIK+/+ and NIK−/− donor T cells are indicated as filled circles and squares, respectively. (C) Rag2−/− mice were transferred with the indicated donor T cells together with wild-type B cells. MOG35-55-immunized mice were killed on day 14 or day 24. Splenic T cells were stimulated for 4 hours with PMA plus ionomycin and subjected to ICS and flow cytometry to determine the frequency of Th17 cells among CD4+CD44+ cells based on IL-17A production. Data are mean value of the indicated number of mice (each circle or square represents 1 individual mouse). (D) Rag2−/− mice were transferred with the indicated donor T cells together with wild-type B cells. After 14 or 24 days of MOG immunization, flow cytometry was performed to determine the frequency of CD4+CD45+ cells infiltrating to the brain and spinal cord. Data are mean value of the indicated number of mice. (E) MOG-immunized Rag2−/− recipients were killed on day 24 for isolating RNA from total CNS tissue. Real-time PCR was performed to determine the relative expression of the indicated genes as described in Figure 1F.

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