Eeks of infection) since borrelial DNA was detected exclusively in all of the joint samples of dbpAB/dbpAB infected mice, while all other tissues were PCR negative. On the other hand, we could not culture dbpAB/dbpAB (or dbpAB) bacteria after ceftriaxone buy TSA treatment from any of the tested samples, not even in the case of anti-TNF-alpha treatment induced immunosuppression. The rationale for using anti-TNF-alpha immunosuppression in two groups of antibiotic treated mice was that we have previously shown that B. burgdorferi infected C3H/HeN mice treated with ceftriaxone once a day for five days became B. burgdorferi culture positive after anti-TNF-alpha treatment [8]. However, in the present study with two daily doses of ceftriaxone, anti-TNF-alpha treatment did not reactivate the infection. Thus, when the antibiotic treatment is frequent enough DNA positivity of the joint tissue samples of dbpAB/dbpAB infected mice rather suggests persistence of noncultivable borrelial remnants than an on-going infection. On the other hand, the persistence of antigenic remnants is supported by the similarly increased antibody levels against the whole B. burgdorferi antigen at 15 weeks of infection in treated (two or six weeks) and non-treated mice.PLOS ONE | DOI:10.1371/journal.pone.0121512 March 27,14 /DbpA and B Promote Arthritis and Post-Treatment Persistence in MiceBockenstedt and co-workers have elegantly shown that immunogenic antigens persist in mouse patellae after antibiotic treatment in a murine LB model [9]. They prepared homogenates from patellae of infected and antibiotic treated mice, and used the extract to immunize na e mice. Finally, they showed that in the sera of the immunized mice there were antibodies that recognized B. burgdorferi proteins on Western blot. From this, they draw the conclusion that there are persisting borrelial antigens in the joints of the antibiotic treated mice. Inspired by this, we also tried to demonstrate the presence of immunogenic B. burgdorferi antigens in the PCR positive tibiotarsal joints of infected and untreated, or infected and ceftriaxone treated (at two weeks) mice (Salo et al, unpublished results). Tibiotarsal joint samples were homogenized and proteins extracted using a commercial protein extraction kit. Na e C3H mice were immunized using a mixture of the protein extract (100 g) and an adjuvant (TiterMax1 Gold Adjuvant, Sigma-Aldrich). The mice were booster immunized two weeks later with 50 g of the extract. Sera were collected two weeks after the second immunization and used to probe B. burgdorferi lysate on Western blots. One to four bands were detected in the Western blot analysis using any of the post-immunization sera, while, however, none of them appeared to be B. burgdorferi specific, since all of the bands were also detected on a blot that was probed with the serum of the adjuvant only immunized animal. The reason for the discrepant results of our experiments v. the results of Bockenstedt and others’ is unclear. However, the mouse strain used by us was different, and we did not prepare the patellae of the mice, but instead used extracts of the whole tibiotarsal joints in the mice. Thus, this experiment did not clarify the nature of the persisting material in the mouse joints, and therefore the data of the experiment are not shown. In conclusion, the results of the present paper show that both Vorapaxar supplier decorin binding proteins A and B of B. burgdorferi are needed for early and prominent arthritis develo.Eeks of infection) since borrelial DNA was detected exclusively in all of the joint samples of dbpAB/dbpAB infected mice, while all other tissues were PCR negative. On the other hand, we could not culture dbpAB/dbpAB (or dbpAB) bacteria after ceftriaxone treatment from any of the tested samples, not even in the case of anti-TNF-alpha treatment induced immunosuppression. The rationale for using anti-TNF-alpha immunosuppression in two groups of antibiotic treated mice was that we have previously shown that B. burgdorferi infected C3H/HeN mice treated with ceftriaxone once a day for five days became B. burgdorferi culture positive after anti-TNF-alpha treatment [8]. However, in the present study with two daily doses of ceftriaxone, anti-TNF-alpha treatment did not reactivate the infection. Thus, when the antibiotic treatment is frequent enough DNA positivity of the joint tissue samples of dbpAB/dbpAB infected mice rather suggests persistence of noncultivable borrelial remnants than an on-going infection. On the other hand, the persistence of antigenic remnants is supported by the similarly increased antibody levels against the whole B. burgdorferi antigen at 15 weeks of infection in treated (two or six weeks) and non-treated mice.PLOS ONE | DOI:10.1371/journal.pone.0121512 March 27,14 /DbpA and B Promote Arthritis and Post-Treatment Persistence in MiceBockenstedt and co-workers have elegantly shown that immunogenic antigens persist in mouse patellae after antibiotic treatment in a murine LB model [9]. They prepared homogenates from patellae of infected and antibiotic treated mice, and used the extract to immunize na e mice. Finally, they showed that in the sera of the immunized mice there were antibodies that recognized B. burgdorferi proteins on Western blot. From this, they draw the conclusion that there are persisting borrelial antigens in the joints of the antibiotic treated mice. Inspired by this, we also tried to demonstrate the presence of immunogenic B. burgdorferi antigens in the PCR positive tibiotarsal joints of infected and untreated, or infected and ceftriaxone treated (at two weeks) mice (Salo et al, unpublished results). Tibiotarsal joint samples were homogenized and proteins extracted using a commercial protein extraction kit. Na e C3H mice were immunized using a mixture of the protein extract (100 g) and an adjuvant (TiterMax1 Gold Adjuvant, Sigma-Aldrich). The mice were booster immunized two weeks later with 50 g of the extract. Sera were collected two weeks after the second immunization and used to probe B. burgdorferi lysate on Western blots. One to four bands were detected in the Western blot analysis using any of the post-immunization sera, while, however, none of them appeared to be B. burgdorferi specific, since all of the bands were also detected on a blot that was probed with the serum of the adjuvant only immunized animal. The reason for the discrepant results of our experiments v. the results of Bockenstedt and others’ is unclear. However, the mouse strain used by us was different, and we did not prepare the patellae of the mice, but instead used extracts of the whole tibiotarsal joints in the mice. Thus, this experiment did not clarify the nature of the persisting material in the mouse joints, and therefore the data of the experiment are not shown. In conclusion, the results of the present paper show that both decorin binding proteins A and B of B. burgdorferi are needed for early and prominent arthritis develo.