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Clinical and Developmental Immunology
Volume 2012 (2012), Article ID 208054, 16 pages
Phenotypical and Functional Analysis of Intraepithelial Lymphocytes from Small Intestine of Mice in Oral Tolerance
1Department of Genetics, Evolution and Bioagents, Institute of Biology, University of Campinas (UNICAMP), Rua Monteiro Lobato of 255, CP 6109, 13083-970 Campinas, SP, Brazil
2Department of Histology and Embryology, Institute of Biology, University of Campinas (UNICAMP), CP 6109, 13083-970 Campinas, SP, Brazil
Received 18 May 2011; Accepted 14 September 2011
Academic Editor: Ana Maria Caetano Faria
Copyright © 2012 Maristela Ruberti et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
In this work, we evaluated the effects of administration of OVA on phenotype and function of intraepithelial lymphocytes (IELs) from small intestine of transgenic (TGN) DO11.10 and wild-type BALB/c mice. While the small intestines from BALB/c presented a well preserved structure, those from TGN showed an inflamed aspect. The ingestion of OVA induced a reduction in the number of IELs in small intestines of TGN, but it did not change the frequencies of CD8+ and CD4+ T-cell subsets. Administration of OVA via oral + ip increased the frequency of CD103+ cells in CD4+ T-cell subset in IELs of both BALB/c and TGN mice and elevated its expression in CD8β+ T-cell subset in IELs of TGN. The frequency of Foxp3+ cells increased in all subsets in IELs of BALB/c treated with OVA; in IELs of TGN, it increased only in CD25+ subset. IELs from BALB/c tolerant mice had lower expression of all cytokines studied, whereas those from TGN showed high expression of inflammatory cytokines, especially of IFN-γ, TGF-β, and TNF-α. Overall, our results suggest that the inability of TGN to become tolerant may be related to disorganization and altered proportions of inflammatory/regulatory T cells in its intestinal mucosa.
Oral tolerance has long been recognized as a physiological mechanism of immune unresponsiveness to dietary antigens (Ags) and indigenous bacterial Ags that maintains tissue integrity by preventing harmful delayed type hypersensitivity responses in the intestine . Three mechanisms were postulated to mediate oral tolerance: clonal deletion, anergy, and active immune suppression. Lower doses of Ag have favored active suppression, and this mechanism is mediated through regulatory cytokines such as TGF-β, IL-10, and IL-4 . T cells producing these regulatory cytokines may downregulate autoreactive T cells in an antigen nonspecific way [2, 3], whereas higher doses favor anergy and T-cell depletion . More recent results show that an activation of T cells is necessary before establishing oral tolerance , while enhanced antibacterial immunity can be achieved with concomitant generation of oral tolerance followed by oral administration of soluble antigen such as ovalbumin (OVA) .
The immunological consequences of oral administration of antigen ultimately depend on how antigen is taken up and presented to T cells by dendritic cells . Despite of the initiation of oral tolerance remains to be cleared, it seems to involve the active participation of the all gut-associated lymphoid tissue (GALT) . Intraepithelial lymphocytes (IELs) play an important role in the maintenance of mucosal homeostasis by regulating mucosal innate and acquired immunity . The populations of IELs exhibit unique characteristics, perform functions not fully elucidated, and differ widely from their systemic counterparts . IELs in mice and humans include large numbers of cells expressing T-cells receptor (TCRs) αβ and γδ . The majority of IELs are CD8+ cells that express a CD8αα homodimer. Among IELs subsets, it can still be found some CD4−CD8−double negative cells, CD4+CD8+ double positive cells and a few CD4+CD8αα+ cells [8, 10]. Nearly all CD8+ IELs expressed CD69 and had lytic activity .
Preliminary results of our group have shown that DO11.10 mice, that bear transgenic anti-OVA TCR, are not susceptible to oral tolerance with OVA . In the present work, we investigated the immune response that takes place in intestinal mucosa during the consumption of OVA in both BALB/c and DO11.10 mice. Since the majority of studies with oral tolerance induction and mucosal immune response have only evaluated the role of CD4+αβ T cells [13–15], we analyzed all subsets of IELs of these mice in the context of oral tolerance and immune response to OVA.
2. Material and Methods
Breeder pairs of TCR OVA-specific transgenic mice (clone DO11.10)  and BALB/c mice were supplied by CEMIB (Centro Multinstitucional de Investigacões Biológicas), UNICAMP. Mice were maintained under specific pathogen-free condition and were provided with autoclaved food and water. The study was approved by the Ethics Commitee for Animal Experimentation of University of Campinas (Protocol no. 736-2).
2.2. Tolerance Induction and Immunizations
Oral tolerance to OVA was induced in 8 weeks old mice as described elsewhere . Briefly, Mice were fed with 4 mg/mL OVA solution (Rhoster Indústria e Comércio, Ltda., Vargem Grande Paulista, SP, Brazil) for seven consecutive days. The mice in the control group received protein-free water. Seven days after the interruption of oral treatment, half of this group of mice was challenged with of 10 μg OVA (Sigma Chemical Co., St. Louis,MO, USA) plus 1 mg Al(OH)3 by intraperitoneal (ip) route. After 14 days, mice were boosted with 10 μg OVA in saline solution via ip. In control group, half of the animals were also challenged with the ip doses of OVA. Seven days after the last ip dose, all mice were bled for serum separation, and then euthanized in a CO2 chamber.
2.3. Cell Isolation and Purification
Intraepithelial lymphocytes were isolated from the small intestine of BALB/c and DO11.10 mice, according to Montufar-Solis and Klein . Briefly, small intestine tissues were removed, and Peyer’s patches were dissected out. Tissues were flushed of fecal material, opened longitudinally, and cut into 3 to 4 mm pieces in RPMI 1640 (Sigma-Aldrich) supplemented with FCS (10% v/v) (Nutricell, Campinas, SP, Brazil), gentamicin 20 μg/mL (GE Healthcare Biosciences, Pittsburgh, PA, USA). Tissue fragments were rinsed several times in Ca2−/Mg2− free PBS, transferred to Ca2−/Mg2− free PBS containing 5 mM EDTA (Sigma-Aldrich) and 2 mM DTT (Calbiochem; Cleveland’s reagent; Merck KGaA, Darmstadt, Germany) and shaken (bath Dubnoff-Marconi, Piracicaba, SP, Brazil) at 37°C for 30 min. Cell suspensions were filtered through 20-mL syringe barrels containing wetted nylon wool, centrifuged, suspended in 3 mL of 40% isotonic Percoll (Amersham and Sigma-Aldrich), layered on top of 70% isotonic Percoll (4 mL), and centrifuged for 30 min at 400 xg. IELs were recovered from the Percoll interface and washed by centrifugation in supplemented RPMI-1640, viability and cell numbers were measured by exclusion of Trypan blue dye and counting in a hemocytometer. IELs from BALB/c mice were further purified by immunomagnetic separation, using beads conjugated with mAb anti-CD90 (Thy-1.2) on MS columns, as recommended by the manufacturer (Midi Macs, Miltenyi Biotec, Bergisch-GladBach, Germany).
2.4. Phenotypic Analysis by Flow Cytometry
Single-cell suspensions from small intestine were suspending in PBS/0,01% BSA (Sigma) w/v supplemented with 0,1% sodium azide. Cells were first incubated with anti-CD16/32 (culture supernatants of clone 2.4G2) for 45 min to block Fc-mediated antibody binding. Then, cells were incubated with relevant mAb for 30 min at 4°C, washed with PBS/2% FCS, and fixed 9 with PBS/1% formaldehyde (Merck Darmstadt, Germany). Three- or four-color flow cytometry acquisition was performed on FACSAria (BD Bioscience, San Jose, CA, USA). A total of 30.000 events were acquired in each analysis. The following antibodies purchased from BDPharMingen were used for flow cytometry: anti-CD3 (clone 145-2C11)-PerCP Cy5.5 or FITC; anti-CD4 (clone GK1.5)-FITC, PE or PE-Cy7; anti-CD4 (clone RM4-5)-PE-Cy7; anti-CD8α (clone 53-6.7)-FITC or PE; anti-CD8β (clone 53-5.8)-FITC; anti-TCRβ (clone H57-597)-PE; anti-TCRγδ (clone GL3)-FITC or PE; anti-CD152 (CTLA-4) (clone UC10-4F10-11)-PE; anti-CD25 (clone 7D4)-FITC or PE; anti-CD103 (α IEL) (clone M290)-PE; anti-OVA TCR (clone KJ1-26)-PE. Anti-Foxp 3 (clone FJK-16 s)-PE or FITC were purchased from eBioscience (San Diego, CA, USA). Data were analyzed by the software FCS express V3. Respective isotype controls were included for each cell surface stain to exclude nonspecific binding and to determine the optimal setting fluorescence quadrants (BD Bioscience, San Jose, CA, USA). Data were analyzed by the software FCS express V3 (De Novo Software, Los Angeles, CA, USA).
2.5. Histological and Immunohistochemical Staining
For histological analysis, pieces from small intestine were fixed in 4% paraformaldehyde buffered solution (Sigma) and washed with PBS/1% Glycine (J.T. Baker, Mallinckrodt Baker, Phillipsburg, NJ, USA), and 5 μm paraffin-embedded sections were stained with hematoxylin and eosin (Sigma). Slides were observed in an optical microscope (Eclipse E-800 Microscope, NIKON; Tokyo, Japan) and analyzed using the software Proplus image. For immunofluorescence analysis, sections of small intestine were dehydrated, frozen in OCT-embedding compound (Leica) on dry ice, and stored at −70°C. Tissue sections (5 μm) were cut with a cryostat (Microm HM 505 E) and transferred to silane-coated microscope slides. Cryosections were brought to room temperature, fixed with acetone (Merck) for 10 min at 4°C, and blocked with PBS containing 1% of BSA (type V, INLAB, SP, Brazil) for 30 min. After washing with PBS, they were incubated with anti-CD3 FITC-labelled (clone 145-2C11 homemade) for 3 h, washed, and incubated with TRITC-phalloidin (Sigma) for 30 min. All incubations were made at room temperature. Vectashield-mounted slides (Vector Laboratories) were visualized by optical microscopy.
2.6. Quantitative Real-Time Polymerase Chain Reaction (PCR)
Total RNA was extracted from mouse IELs using PureLink Micro-to-Midi Total RNA Purification System (Invitrogen, SP, Brazil,) according to the manufacturer’s instructions. The cDNA was made using SuperScript III First-Strand Synthesis Supermix (Invitrogen) with random primers (Invitrogen) and analyzed for IL-2, IL-4, IL-10, IL-6, IL-17, IFN-γ, TGF-β, and TNF-α gene expression by real-time PCR assay using an 7500 Fast Real-Time PCR (Applied Biosystems, Foster City, CA) according to the manufacturer’s instructions; 18S ribosomal RNA (rRNA) was used as an internal control. All mouse primer and probe sets used were predesigned TaqMan Gene Expression Assays (Applied Biosystems). PCRs were performed in four replicates with a 2x TaqMan Mastermix (Applied Biosystems). Relative expression of mRNA species was calculated using the comparative 2 threshold cycle (ΔCT) method .
2.7. Statical Analysis
The statistical analysis was performed using GraphPad Prism 4 (GraphPad Software, CA, USA). The statistical significance of differences between control and experimental groups were determined by one-way and two-way ANOVA, followed by multiple comparison Bonferroni’s test. The results were expressed as mean ± SEM. Values were considered significant at . Supplemental data include two figures (see supplementary material available online at http://dx.doi.org/10.1155/2012/208054).
3.1. Histological Analysis and Distribution of IELs in Small Intestines of Mice DO11.10 and BALB/c
As depicted in Figure 1(a), the small intestine histoarchitecture of both naïve DO11.10 and BALB/c strains were preserved; however, it was found reduced tunica muscular thickness of DO11.10 when compared with BALB/c mice. Discrete but well-defined histological changes were observed in the lamina propria (LP) of intestinal villi of the transgenic mice after feeding with OVA, mainly in those challenged with OVA by ip route, with a loose connective tissue rupture and mild edema of lamina propria of villous projections in DO11.10 mice. BALB/c mice treated with OVA did not present any of those alterations. The total number of IELs isolated from the small intestine of DO11.10 mice of all experimental groups was always lower than those from BALB/c and markedly dropped upon OVA treatments (Table 1). As illustrated in Figure 1(b), the incidence of CD3 positive cells decreased substantially in the villi of TGN mice but not in the BALB/c. Cytometry analyses of IELs isolated from TGN showed that the clonotype anti-OVA TCR cells (KJ1-26 positive cells) decreased significantly from 65% to less than 20% after oral and ip administration of OVA (Figures 1(c) and 1(d)).
3.2. Analysis of Subsets of IELs after the Induction of Tolerance or Immunization
IELs from BALB/c and D011.10 mice treated with OVA by oral and/or ip route were stained with anti-CD3, anti-CD8α, anti-CD8β, anti-CD4 and analyzed by three-color flow cytometry (Figure 2). As shown in Figure 2(a), the frequency of CD3+ cells in the small intestine of BALB/c and DO11.10 mice was not changed by different treatments with OVA. No significant alteration was observed in the frequency of IEL subsets (CD8αα, CD8αβ, CD4/CD8α, CD4) upon treatments with OVA (Figure 2(c)).
The effects of administration of OVA on the distribution of phenotypic markers CD103 and CD25 were assessed in subsets CD4, CD8α, and CD8β of IELs isolated from BALB/c(Supplemental Figure 1, Panel A-D) and DO11.10 mice(Supplemental Figure 1, Panel (E-H)), as well as the frequencies of αβ+ and γδ+ T cells in these subsets (Supplemental Figure 2). Frequency and expression of CD103+ cells in subsets of IELs of BALB/c and DO11.10 mice are illustrated in histograms of (Figures 3(a) and 3(b), resp.). Significant increase of CD4+ CD103+ subset of IELs was observed following treatments with OVA by oral + ip routes, in both BALB/c and DO11.10 mice, whereas no antigen-dependent alteration was observed in the frequency of CD8αα and CD8αβ IELs expressing CD103 (Figure 3(c)). However, the expression of CD103 was significantly augmented in subpopulation of CD8αα+ and CD8αβ+ IELs when BALB/c mice were fed with OVA, as well as in CD8αα+ cells in ip immunized mice. Conversely, in DO11.10 mice, this marker was significantly reduced in CD8αα+ cells upon immunization with OVA by ip route (Figure 3(c)).
Frequency and expression of CD25+ cells in subsets of IELs of mice BALB/c and DO11.10 are illustrated in histograms of (Figures 4 (a) and 4(b) resp.). No antigen-dependent alteration was observed in the frequency of IELs expressing this marker in both DO11.10 and BALB/c mice, except in CD8β+ subset of IELs in which this marker was upregulated by treatments with OVA by oral route (Figure 4(c)).
3.3. Evaluation of Foxp3 Expression in IELs after Administration of OVA
To assess possible changes in the frequency of regulatory T cells after oral and/or ip administration of OVA, IELs from BALB/c and DO11.10 mice were stained with anti-Foxp3 and analyzed by flow cytometry in CD4+, CD8αα+, CD8αβ+, and CD25+ subsets. As shown in Figures 5(a) and 5(c), we observed that oral administration of OVA to BALB/c mice resulted in elevation of the frequency of Foxp3+ cells in CD4+ and CD8αβ+ subsets. Following parenteral administration of OVA, the frequency of cells Foxp3+ in IELs of BALB/c mice was more elevated in the CD8αα+, CD8αβ+, and CD25+ subsets. On the other hand, only the oral + ip treatment of DO11.10 mice increased the frequency of Foxp3+ cells in the CD25+ subset (Figures 5(b) and 5(c)).
3.4. Effect of Treatments with OVA on Cytokine mRNA Expression in IELs of BALB/c and DO11.10 Mice
In addition to phenotypic analysis, expression of pro-(IL-2, IFN-γ, IL-6, IL-17, and TNF-α) and anti-inflammatory (IL-10, IL-4, and TGF-β) cytokines has been assessed by real-time PCR from extracts of IELs of the small intestine of BALB/c and DO11.10 mice treated with OVA. The results are summarized in Figure 6. It is possible to notice that IELs from OVA-treated mice of both strains present opposite profiles in relation to the gene expression of most cytokines examined. IELs from tolerant BALB/c mice (oral and oral + ip groups) showed a diminished expression of mRNA for cytokines IL-10, IL-2, IFN-γ, TGF-β, and TNF-α in comparison to those from mice immunized by ip route. IELs from DO11.10 mice treated with OVA by oral + ip and ip routes showed an elevated expression of IL-6, IL17, TNF-α, and TGF-β, although differences were not significant in comparison with the oral group. IELs from DO11.10 mice that received OVA by oral + ip, however, showed a mRNA expression for TNF-α, IFN-γ, and TGF-β significantly more elevated than IELs from BALB/c mice of the same group.
Failure in the induction of oral tolerance seems to be associated with modifications in the gastrointestinal mucosa permeability and, especially, with the immunoregulation that occurs in this environment [19, 20]. Results obtained previously in our laboratory showed that transgenic DO11.10 and BALB/c mice differ in their immune response to oral OVA. While DO11.10 mice develop a specific humoral immune response after the ingestion of native ovalbumin, the BALB/c mice become tolerant to OVA. The transgenic mice fed with ovalbumin produced an immune response that is a mixed of TH1/TH2, with prevalence of a TH1 pattern . In this work, we observed that even before the oral treatment with OVA, the DO11.10 mice have showed morphological modifications in the intestinal epithelium villi and of the muscular layer in the intestinal tissue. Our results showed a deepening of changes in the epithelium of small intestine in DO11.10 mice treated with OVA, which are consistent to an inflammatory process. These changes have not been observed in the intestinal epithelium of BALB/c mice, which have been presented a good preservation of the villi. A chronic inflammatory process, with lymphocytic infiltration in the lamina propria and increased number of IELs in the epithelium has been shown in double-transgenic mice that express the haemagglutinin from influenza virus A (HA) and TCR HA-specific. The inflammatory reaction, however, is kept under control by the generation of regulatory T cells .
Deletion of self-reactive lymphocytes constitutes one of main mechanisms of peripheral tolerance induction and probably of oral tolerance induction [21, 22]. Conversely, intestinal inflammation has been correlated with failure in the induction of apoptosis in lymphocytes present in the mucosa . The initial hypothesis of our study was that resistance to the induction of oral tolerance in DO11.10 might be due to failure in the deletion of OVA-specific lymphocytes in the intestinal mucosa after ingestion of the antigen. Indeed, treatment with OVA by oral and/or ip routes resulted in reduction of IELs in the DO11.10 mice. Besides that, a remarkable reduction in OVA-specific cells (KJ1-26) was observed in small intestine of DO11.10 mice treated with OVA. Previous work has shown that the administration of OVA results in marked reduction of mature lymphocytes KJ1-26+ in the blood and peripheral lymphoid organs . However, a substantial portion of the IELs and lymphocytes from LP from the DO11.10 mice carries a second nonclonotypical TCR, probably due to the incomplete allelic exclusion of the endogenous TCRα during the rearrangement process in the thymus [21, 24]. Part of the alternative TCR seems to be specific to antigens from the intestinal environment as DO11.10/SCID or DO11.10/RAG2−/− mice do not exhibit reactivity to antigens from the intestinal microbiota [25, 26]. Thus, a possible explanation for the escape of DO11.10 from oral tolerance in spite of the occurrence of TCR OVA-specific cells deletion would be the activation of T cells bearing alternative TCR, that would result in local inflammatory response, with activation of nontransgenic IELs carrying TCR to other than OVA epitopes.
The IELs have phenotype similar to either effector or effector memory of cells that are present in other peripheral lymphoid organs , presenting a high expression of the CD103 marker (αEB7), an α-integrin responsible for the retention of IELs in the intestinal epithelium . This molecule has been associated to the immuneregulation in the mucosa as it is expressed by regulatory T lymphocytes [29, 30] as well as by dendritic cells involved in the generation of regulatory T cells [31, 32]. IELs from small intestine of the BALB/c mice treated with OVA orally and/or parenteral have shown marked increase in the expression of CD103, in all populations studied: TCD4, TCD8α, and TCD8β. Furthermore, IELs from orally treated DO11.10 mice have shown no changes in the expression of CD103 in any cell subset. In contrast, TGN immunized intraperitoneally with OVA showed an accentuated reduction in the expression of CD103 in these cells.
Several populations of regulatory cells have been described in oral tolerance, including IL-10 producer cells termed Tr1, TGF-β producing cells called Th3 and TCD4+/CD25+, and its relative importance in the establishment of oral tolerance is still under investigation [1, 20]. Some of these studies have emphasized the role of the CD8αα IELs in the immunoregulation that occurs in the intestinal mucosa [33, 34]. In this work, we did not observe changes in the frequency of this subset of IELs in either BALB/c or DO11.10 mice immunized orally or parenterally with OVA.
There is a consensus in the literature that the oral tolerance is related to the induction of antigen-specific regulatory T cells either by direct or cross-presentation of antigens from the enterocytes [20, 21, 34]. Our results have shown that the ingestion of OVA led to an increase in the frequency of TCD4+/Foxp3+, TCD8α+/Foxp3+, TCD8β+/Foxp3+, and TCD25+/Foxp3+ amongst the IELs of BALB/c mice, thus indicating that the establishment of tolerance in wild-type mouse are associated with the increase of regulatory T cells. The frequency of TCD25+/Foxp3+ cells has also increased in the IELs from TGN treated with OVA by oral + ip routes. However, this increase has not been sufficient to inhibit the inflammation that has settled in the small intestinal mucosa of the TGN after treatment with the protein.
TCD8+ cells also play an important role in the homeostatic maintenance of the intestinal epithelium. In this regard, TCD8αβ suppressor cells have been correlated with the establishment of antigen specific oral tolerance [30, 35, 36]. Although the ingestion of OVA leads to an increase in the frequency of Foxp3+ cells in all populations of IEL from both BALB/c and DO11.10 mice, our results showed that it is in the TCD8β+ population of IELs that occurs the highest frequency of cells carrying this suppression marker.
Due to the exposure of mucosal epithelium to a huge amount of strange antigens, the cytokines IFN-γ and interleukin-(IL-)4 are produced spontaneously under physiological conditions by IELs . In our study, we observed that the expression of IL-2, IL-10, IFN-γ, TGF-β, and TNF-α mRNA was smaller in IELS from BALB/c mice fed OVA and then challenged by ip route than in those that received OVA only by ip route; the levels of IL-17 and IL-6 mRNA were also reduced, but not significantly, in IELs from BALB/c mice. Instead, IELS from transgenic mice of the oral + ip group showed levels of IL-6, IFN-γ, TGF-β, and TNF-α mRNA similar to or higher than the animals immunized only by ip route.
The cytokines IL-10 and TGF-β were always related to anti-inflammatory reactions [1, 20]. More recently, however, these cytokines have been associated with inflammatory reactions by activating the process of differentiation of Th17 cells [38, 39]. TCD4+ cells that secrete IL-17, Th17 cells, are pathogenic in autoimmune diseases, and their development and expansion is driven by the cytokines IL-6, TGF-beta, IL-21, IL-1, and IL-23 [39, 40]. Recent studies have revealed a considerable number of IL-17-producing cells amongst the TCD4+ cells in the intestinal mucosa . Although these cells are important to establish a protective immune response against intestinal bacteria, they can also be responsible for inducing inflammatory response and the development of immunological disorders in the presence of IL-6 and/or IL-23 at mucosal sites [41, 42]. Despite the natural occurrence of higher expression of IL-6, TGF-β, and TNF-α mRNA in the DO11.10 IELS than in those of BALB/c mice, there was no significant change in IL-17 mRNA after administration of OVA orally and/or ip in both BALB/c and DO11.10 mice.
Th1-mediated immune responses are considered to be the primary mediators of most autoimmune and chronic inflammatory diseases. Th17, however, has emerged as a key protagonist in a number of inflammatory diseases. It has been shown that CD8+ Treg cells can suppress both Th1 and Th17 responses, being capable of mediating oral tolerance to OVA independently of their CD4+ counterparts in a normal immune system . In the present work, the increase in the frequency of CD8αβ+Foxp3+ cells among IELS of BALB/c mice after ingestion of OVA could explain the absence or reduced expression of IL-6, TGF-β, TNF-α, and IFN-γ.
Recent studies have shown that inflammatory bowel diseases (IBD) such as ulcerative colitis and Crohn’s disease may be related to the loss of tolerance to self-antigens or normal flora . Our results indicate that the structural disorder observed in epithelium of intestinal villi of transgenic mice would be a consequence of the preferential expression of pro-inflammatory cytokines by their IELs, in the absence of an efficient immunoregulation. This inflammatory state in intestinal environment may contribute to the impairment of oral tolerance to OVA in DO11.10 mice.
Taken together, the results of this study indicate that exposure to OVA orally causes IELs of the small intestine of TGN mice assume inflammatory characteristics, whereas in BALB/c antigen intake leads to the development of IELs with characteristics of regulatory cells. Thus, we speculate that the establishment of oral tolerance in transgenic mice is severely impaired by changes in the amounts and arrangements of T cells during the development of intestinal tissues that compromise the cellular interactions involved in the processes of mucosal immunity.
|GALT:||Gut-associated lymphoid tissue|
|IBD:||Inflammatory bowel disease|
|IELs:||Intestinal epithelial cells|
|MLN:||Mesenteric lymph node|
|TGF-β:||Transforming growth factor-β|
This work was supported by Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP no. 2005/51520-8); Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq no. 474074/2004-8); Fundo de Apoio ao Ensino, à Pesquisa e à Extensão da UNICAMP (FAEPEX no. 86256).
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