The mLN were shown to induce a prominent Th2 immune response by producing IL-4 and TGF-β, whereas pLN produced a stronger Th1 response via cytokines such as IFN-γ 22. LNtx from Ag-tolerant mice were removed and mRNA was isolated to determine the expression pattern of Th1 and Th2 cytokines. mRNA expression of IFN-γ (Fig. 5A) or IL-12 (data not shown), as examples for Th1 responses, was found in OVA-treated and untreated mLNtx-transplanted animals on a marginal expression
level, Topoisomerase inhibitor whereas OVA-treated pLNtx mice showed increased frequency compared to mLNtx. The expression of Th2-specific cytokine mRNA, including IL-4, was detected to be higher in mLNtx compared to pLNtx in Ag-tolerant mice (Fig. 5A) as well as in control mLNtx and pLNtx animals (data not shown). Furthermore, cytokines were shown to manipulate B-cell class switching from IgM to other Ig isotypes. Therefore, the serum of Ag-tolerant transplanted mice for Ig subclasses was analyzed and in pLNtx high levels of λ light chain Ab were found in the serum, whereas in mLNtx or mLN control no Ab production was detectable (Fig. 5B). In addition, in Ag-tolerant pLNtx mice increased mRNA levels of the B-cell-activating factor (BAFF) were seen compared to mLNtx Ag-tolerant (Fig. 5C)
and also to pLNtx-control mice (data not shown). These results suggest an Ig class switch and thereby Selleck Galunisertib a production of one specific Ab clone in pLNtx animals. Furthermore, increased IgG3
were found in pLNtx Ag-tolerant mice compared to mLNtx (Fig. 5B). Analyzing the serum for OVA-specific Ab, high amounts of Ag-specific IgG3 Ab were verifiable only in pLNtx animals (Fig. 5D). Nevertheless, these data showed that within pLNtx an antibody induction after tolerance induction took place. By contrast, the mLNtx followed normal tolerance induction including Treg activation. Taken together, these data over suggested a dominant role of B cells in the induction of tolerance induced by pLN. To examine these findings adoptive transfer experiments were performed. Therefore, CD4+ and IgG+ cells were isolated from untreated LN as control, pLN-pt as well as mLN-ot animals after tolerance induction. These isolated cells were injected into wt mice and 20 days later the DTH response was measured. Animals with IgG+ cells of pLN-pt mice showed a high reduction in the DTH response compared to the control and mLN-ot IgG group (Fig. 6). However, mice that received CD4+ cells of untreated control LN were not able to induce tolerance, whereas mice that contained CD4+ cells of mLN-ot showed a reduced DTH response (Fig. 6). Furthermore, the reduction of the DTH response was less pronounced in mice with CD4+ cells transferred from pLN-pt mice (Fig. 6). Therefore, these adoptive transfer experiments showed the ability of pLN to induce tolerance systemically, not only by Treg activation but predominantly by B-cell class switch and Ab production.