Fically as oral antigens can now be considered as a strategy to track T cells primed by gut luminal antigens. This new Title Loaded From File perspective on the DSS-induced colitis model will allow insight into the inflammatory processes needed to initiate the development of Title Loaded From File antigen-specific T cells during acute gastrointestinal inflammation 1480666 and their role in disease chronicity.AcknowledgementsWe would like to thank Mr Gerard Hofman for his help with several animal procedures and our colleagues for their insightful input.Author ContributionsConceived and designed the experiments: MEM ADK. Performed the experiments: MEM BZ LH MvR HJGvdK PJK. Analyzed the data: MEM LH PJK MvR ADK GF JG. Wrote the manuscript: MEM PJK GF ADK JG.Antigen-Specific T Cell Development during ColitisFigure 6. OVA-directed, CD4+ Foxp3-T cells are detected only in mice treated with DSS and OVA. Both mLN and spleen cell suspensions were prepared 14 days after the start of the DSS and OVA treatment for all groups. Cells were stimulated with OVA, and CD69 expression was measured using flow cytometry. A) Representative FACS dot plots of the CD69 expression in CD4+ Foxp3- (Tconv) and CD4+ Foxp3+ (Treg) T cells in the spleen. Percentages shown are the CD69+ cells in the specific gated Tconv or Treg populations. B) The mean percentage CD69 expression was calculated for Tconv and Treg in the spleen cells of each group. C) Representative FACS plots of the CD69 expression in Tconv and Treg cells in the mLN. D) The mean percentage CD69 1315463 expression was calculated for Tconv and Treg cells in the mLN. Results are expressed as mean + SEM, N = 6-9 per group. *** P < 0.001; **** P < 0.0001.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during Colitis
Rifaximin is a semi-synthetic, poorly-absorbed (,0.4 ) rifamycin derivative used to treat travelers’ diarrhea due to bacterial enteropathogens and hepatic encephalopathy (HE) [1,2,3,4,5,6]. Rifaximin also has been used for treatment of irritable bowel syndrome, small bowel bacterial overgrowth, pouchitis, and fulminant ulcerative colitis [2,7,8,9,10,11]. The mechanisms by which rifaximin confers its broad range of intestinal effects remain largely unknown [12]. Rifaximin was first approved for use in Italy in 1987. In contrast to conventional antibiotics that have broad antimicrobial effects dramatically altering body flora rifaximin acts primarily in the gut [13]. We previously demonstrated that pretreatment of the HEp-2 epithelial cell line with rifaximin significantly reduced the ability of enteroaggregative Escherichia coli (EAEC) to adhere to either the epithelial cells or glass slides compared to untreated cells or cells treated with the related antibiotic rifampin [14]. In addition, epithelial cells pretreated with rifaximin had fewer detectable proinflammatory cytokines present in the supernatant compared to untreated controls. Finally, rifaximin pretreatment of HEp-2 cells reduced Bacillus anthracis internalization into lung epithelial cells (A549) but had no effect on Shigella sonnei internalization into cervical epithelial (HeLa) cells. These data suggested that rifaximininduced changes to supernatant cytokine profiles and interfered with the cellular process utilized by some pathogens (EAEC and B. anthracis) but not others (S. sonnei) that use a type III secretory system to gain access to the intracellular compartment [14]. By analyzing and comparing epithelial cell protein expression profiles following treatment with or w.Fically as oral antigens can now be considered as a strategy to track T cells primed by gut luminal antigens. This new perspective on the DSS-induced colitis model will allow insight into the inflammatory processes needed to initiate the development of antigen-specific T cells during acute gastrointestinal inflammation 1480666 and their role in disease chronicity.AcknowledgementsWe would like to thank Mr Gerard Hofman for his help with several animal procedures and our colleagues for their insightful input.Author ContributionsConceived and designed the experiments: MEM ADK. Performed the experiments: MEM BZ LH MvR HJGvdK PJK. Analyzed the data: MEM LH PJK MvR ADK GF JG. Wrote the manuscript: MEM PJK GF ADK JG.Antigen-Specific T Cell Development during ColitisFigure 6. OVA-directed, CD4+ Foxp3-T cells are detected only in mice treated with DSS and OVA. Both mLN and spleen cell suspensions were prepared 14 days after the start of the DSS and OVA treatment for all groups. Cells were stimulated with OVA, and CD69 expression was measured using flow cytometry. A) Representative FACS dot plots of the CD69 expression in CD4+ Foxp3- (Tconv) and CD4+ Foxp3+ (Treg) T cells in the spleen. Percentages shown are the CD69+ cells in the specific gated Tconv or Treg populations. B) The mean percentage CD69 expression was calculated for Tconv and Treg in the spleen cells of each group. C) Representative FACS plots of the CD69 expression in Tconv and Treg cells in the mLN. D) The mean percentage CD69 1315463 expression was calculated for Tconv and Treg cells in the mLN. Results are expressed as mean + SEM, N = 6-9 per group. *** P < 0.001; **** P < 0.0001.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during Colitis
Rifaximin is a semi-synthetic, poorly-absorbed (,0.4 ) rifamycin derivative used to treat travelers’ diarrhea due to bacterial enteropathogens and hepatic encephalopathy (HE) [1,2,3,4,5,6]. Rifaximin also has been used for treatment of irritable bowel syndrome, small bowel bacterial overgrowth, pouchitis, and fulminant ulcerative colitis [2,7,8,9,10,11]. The mechanisms by which rifaximin confers its broad range of intestinal effects remain largely unknown [12]. Rifaximin was first approved for use in Italy in 1987. In contrast to conventional antibiotics that have broad antimicrobial effects dramatically altering body flora rifaximin acts primarily in the gut [13]. We previously demonstrated that pretreatment of the HEp-2 epithelial cell line with rifaximin significantly reduced the ability of enteroaggregative Escherichia coli (EAEC) to adhere to either the epithelial cells or glass slides compared to untreated cells or cells treated with the related antibiotic rifampin [14]. In addition, epithelial cells pretreated with rifaximin had fewer detectable proinflammatory cytokines present in the supernatant compared to untreated controls. Finally, rifaximin pretreatment of HEp-2 cells reduced Bacillus anthracis internalization into lung epithelial cells (A549) but had no effect on Shigella sonnei internalization into cervical epithelial (HeLa) cells. These data suggested that rifaximininduced changes to supernatant cytokine profiles and interfered with the cellular process utilized by some pathogens (EAEC and B. anthracis) but not others (S. sonnei) that use a type III secretory system to gain access to the intracellular compartment [14]. By analyzing and comparing epithelial cell protein expression profiles following treatment with or w.