aro and E. coli infection could elicit AMA production, but that E. coli was the more potent stimulus. Next we examined the livers of N. aro- and E. coli-infected mice by histological and immunohistochemical staining. Although AMA were detectable as early as 4 weeks after bacterium infection, significant pathological changes in liver were not detected before 19 weeks after either N. aro or E. coli inoculation. However, by 26 weeks following infection, striking portal inflammation accompanied by granuloma formation was present in livers of both N. aro- and E. coli-infected mice, selleck chemical but not in the uninfected control group. Significant
biliary cell damage was also detected in both E. coli- and N. aro-infected mice (Fig. 3). To further determine the extent of bile duct Proteases inhibitor damage, we performed immunohistochemical staining
for CK19 to visualize biliary epithelial cells among lymphoid aggregation. As shown in Fig. 4, varying degrees of biliary cell damage were found in either E. coli- or N. aro-infected mice, but not in the control mice. In both infected groups, while some bile ducts are nearly intact with mild lymphoid aggregation (blue arrows), in some portal tracts the biliary epithelial cells were completely obliterated (red arrows). These results indicate that E. coli infection is sufficient to induce cholangitis in the biliary disease-prone NOD.B6-Idd10/Idd18 mice. We have previously used an antigen-presenting cell (APC)-free assay to identify microbes that have antigens for NK T cells [38, 39]. In this assay, microwells are coated with soluble mouse CD1d molecules and incubated either with antigen Sulfite dehydrogenase preparations or total bacterial sonicates. The plates are then cultured with NK T cell hybridomas and interleukin (IL)-2 release, which provides a bioassay for T cell antigen receptor engagement, was quantitated. As can be seen in Fig. 5, sonicates of S. yanoikuyae, which are known to have glycosphingolipid antigens for NK T cells , produced IL-2 release from several NK T cell hybridomas.
By contrast, E. coli sonicates, which do not have such antigens, did not produce hybridoma IL-2 release. Although related to Sphingomonas spp., N. aro sonicates also did not produce IL-2 secretion by NK T cells. Therefore, it is unlikely that N. aro has significant quantities of a glycolipid antigen capable of activating NK T cells. Our data also indicate that exposure to N. aro does not induce cholangitis by a unique NK T activating mechanism and we suggest that previous data were probably secondary to molecular mimicry. The challenge for researchers would be to identify genetically at-risk hosts and determine the extent of other secondary factors that may also contribute, perhaps concurrently with microbial infections, to the aetiology of PBC.