Ory CD4+ T cells (TEM, CD4+ CD62L-CD44-) in colon mononuclear cells and mLN cells collected from Acid Yellow 23 supplier healthy and DSS-treated mice. In the colon and the mLN, na e CD4+ T cells were the most abundant, comprising 30 -60 of the CD4+ T cells. During inflammation, na e T cells were significantly decreased in the mLN (P < 0.0001, Figure 1D). In healthy colons and mLNs, CD4+ TCM cells comprised 20 -40 of the population. DuringOral OVA does not change clinical parameters of DSSinduced colitisIn IBD patients, responses to orally administered antigens are measured in the peripheral blood mononuclear cells, 1-Antigen-Specific T Cell Development during ColitisFigure 1. During colitis, T cells accumulate in the inflamed regions of the colon. Mice were treated with DSS for 6 days and sacrificed on day 7. The mice displayed signs of colitis including (A) an increased Disease Activity Index (DAI) and (B) shortened colons. C) Immunohistochemical staining of CD3+ cells in colons obtained from both control (left panes) and DSS-treated (right panes) mice. Top panes are 200x (bar: 5 ) and bottom panes are 400x magnification (bar: 1 ). Increased CD3+ cells are observed in inflamed colons. D) Na e (CD4+ CD62L+ CD44-), central memory (TCM, CD4+ CD62L+ CD44+) and effector memory (TEM, CD4+ CD62L-CD44+) T cells were measured in the mLNs and colon mononuclear cell suspensions using flow cytometry. Results are expressed as mean + SEM, N = 4-6 mice per group. *** P < 0.001; **** P < 0.0001.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during ColitisFigure 2. Th17 cells are detected in 23148522 the spleen after colitis resolution. IFN and IL-17A (-)-Calyculin A site producing CD4+ T cells were detected in the spleens and mLNs, 14 days after the start of DSS using intracellular cytokine staining. A) Percentages depicted are the populations of cytokine expressing CD4+ cells within the total CD4+ population. Bars indicate the mean, N = 8 mice per group. ** P < 0.01. B) Representative FACS contour dot plots for spleen and mLN showing intracellular staining of IL-17A and IFN within the gated CD4+ T cell population. Percentages within CD4+ T cell population are shown.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during ColitisFigure 3. Oral antigens are presented in the draining lymph nodes of both healthy and DSS treated mice. A) OVA presentation in the gastrointestinal tract was visualized by the proliferation of adoptively transferred, CFSE labeled, OTII T cells. Representative FACS dot plots displaying OTII T cell proliferation within the mLNs of both healthy and DSS-treated mice after oral gavage of saline, "no antigen" or oral gavage with OVA, "ovalbumin". The loss of CFSE intensity is an indication of dividing T cells. B) Percent proliferated OTII cells found within isolated mLNs. C) Percent proliferated OTII cells in the non-local, axillary lymph nodes. Results for (B) and (C) are expressed as mean + SEM, N = 4 mice per group, pooled from two independent experiments. * P < 0.05; ** P < 0.01.doi: 10.1371/journal.pone.0069936.gweeks after the oral feeding of antigens [2]. To provide oral tracking antigens during DSS colitis, we administered OVA via the drinking water along with dissolved DSS for 6 days. The expectation was that oral OVA would not influence the clinical parameters. However, as oral tolerance induction against bystander antigens has been known to result in the amelioration of chronic inflammatory disease models in a phenomenon calle.Ory CD4+ T cells (TEM, CD4+ CD62L-CD44-) in colon mononuclear cells and mLN cells collected from healthy and DSS-treated mice. In the colon and the mLN, na e CD4+ T cells were the most abundant, comprising 30 -60 of the CD4+ T cells. During inflammation, na e T cells were significantly decreased in the mLN (P < 0.0001, Figure 1D). In healthy colons and mLNs, CD4+ TCM cells comprised 20 -40 of the population. DuringOral OVA does not change clinical parameters of DSSinduced colitisIn IBD patients, responses to orally administered antigens are measured in the peripheral blood mononuclear cells, 1-Antigen-Specific T Cell Development during ColitisFigure 1. During colitis, T cells accumulate in the inflamed regions of the colon. Mice were treated with DSS for 6 days and sacrificed on day 7. The mice displayed signs of colitis including (A) an increased Disease Activity Index (DAI) and (B) shortened colons. C) Immunohistochemical staining of CD3+ cells in colons obtained from both control (left panes) and DSS-treated (right panes) mice. Top panes are 200x (bar: 5 ) and bottom panes are 400x magnification (bar: 1 ). Increased CD3+ cells are observed in inflamed colons. D) Na e (CD4+ CD62L+ CD44-), central memory (TCM, CD4+ CD62L+ CD44+) and effector memory (TEM, CD4+ CD62L-CD44+) T cells were measured in the mLNs and colon mononuclear cell suspensions using flow cytometry. Results are expressed as mean + SEM, N = 4-6 mice per group. *** P < 0.001; **** P < 0.0001.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during ColitisFigure 2. Th17 cells are detected in 23148522 the spleen after colitis resolution. IFN and IL-17A producing CD4+ T cells were detected in the spleens and mLNs, 14 days after the start of DSS using intracellular cytokine staining. A) Percentages depicted are the populations of cytokine expressing CD4+ cells within the total CD4+ population. Bars indicate the mean, N = 8 mice per group. ** P < 0.01. B) Representative FACS contour dot plots for spleen and mLN showing intracellular staining of IL-17A and IFN within the gated CD4+ T cell population. Percentages within CD4+ T cell population are shown.doi: 10.1371/journal.pone.0069936.gAntigen-Specific T Cell Development during ColitisFigure 3. Oral antigens are presented in the draining lymph nodes of both healthy and DSS treated mice. A) OVA presentation in the gastrointestinal tract was visualized by the proliferation of adoptively transferred, CFSE labeled, OTII T cells. Representative FACS dot plots displaying OTII T cell proliferation within the mLNs of both healthy and DSS-treated mice after oral gavage of saline, "no antigen" or oral gavage with OVA, "ovalbumin". The loss of CFSE intensity is an indication of dividing T cells. B) Percent proliferated OTII cells found within isolated mLNs. C) Percent proliferated OTII cells in the non-local, axillary lymph nodes. Results for (B) and (C) are expressed as mean + SEM, N = 4 mice per group, pooled from two independent experiments. * P < 0.05; ** P < 0.01.doi: 10.1371/journal.pone.0069936.gweeks after the oral feeding of antigens [2]. To provide oral tracking antigens during DSS colitis, we administered OVA via the drinking water along with dissolved DSS for 6 days. The expectation was that oral OVA would not influence the clinical parameters. However, as oral tolerance induction against bystander antigens has been known to result in the amelioration of chronic inflammatory disease models in a phenomenon calle.
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