RÉSUMÉ
Gel-forming mucins secreted by conjunctival goblet cells have been implicated in the clearance of allergens, pathogens, and debris. However, their roles remain incompletely understood. Here we show that human and mouse conjunctival goblet cell mucins have Alcian blue-detectable sialic acids, but not sulfates in the steady state. Interestingly, Balb/c mouse strain lacks this sialylation due to a point mutation in a sialyltransferase gene, St6galnac1, which is responsible for sialyl-Tn synthesis. Introduction of intact St6galnac1 to Balb/c restores the sialylation of conjunctival goblet cell mucus. Sialylated mucus efficiently captures and encapsulates the allergen particles in an impenetrable layer, leading to the protection of mice from the development of allergic conjunctivitis. Expression of ST6GALNAC1 and sialyl-Tn is upregulated in humans under conditions with chronic stimuli. These results indicate that the sialylated glycans on the ocular mucins play an essential role in maintaining the conjunctival mucosa by protecting from the incoming foreign bodies such as allergen particles.
Sujet(s)
Cellules caliciformes , Mucines , Souris , Humains , Animaux , Cellules caliciformes/métabolisme , Mucines/génétique , Mucines/métabolisme , Conjonctive , Mucus/métabolisme , AllergènesRÉSUMÉ
In the present study, we evaluated the effects of kaempferol on bone marrow-derived mast cells (BMMCs). Kaempferol treatment significantly and dose-dependently inhibited IgE-induced degranulation, and cytokine production of BMMCs under the condition that cell viability was maintained. Kaempferol downregulated the surface expression levels of FcεRI on BMMCs, but the mRNA levels of FcεRIα, ß, and γ-chains were not changed by kaempferol treatment. Furthermore, the kaempferol-mediated downregulation of surface FcεRI on BMMCs was still observed when protein synthesis or protein transporter was inhibited. We also found that kaempferol inhibited both LPS- and IL-33-induced IL-6 production from BMMCs, without affecting the expression levels of their receptors, TLR4 and ST2. Although kaempferol treatment increased the protein amount of NF-E2-related factor 2 (NRF2)-a master transcription factor of antioxidant stress-in BMMCs, the inhibition of NRF2 did not alter the suppressive effect of kaempferol on degranulation. Finally, we found that kaempferol treatment increased the levels of mRNA and protein of a phosphatase SHIP1 in BMMCs. The kaempferol-induced upregulation of SHIP1 was also observed in peritoneal MCs. The knockdown of SHIP1 by siRNA significantly enhanced IgE-induced degranulation of BMMCs. A Western blotting analysis showed that IgE-induced phosphorylation of PLCγ was suppressed in kaempferol-treated BMMCs. These results indicate that kaempferol inhibited the IgE-induced activation of BMMCs by downregulating FcεRI and upregulating SHIP1, and the SHIP1 increase is involved in the suppression of various signaling-mediated stimulations of BMMCs, such as those associated with TLR4 and ST2.
Sujet(s)
Mastocytes , Récepteurs aux IgE , Dégranulation cellulaire , Immunoglobuline E/métabolisme , Protéine-1 analogue au récepteur de l'interleukin-1/métabolisme , Kaempférols/pharmacologie , Kaempférols/métabolisme , Mastocytes/métabolisme , Facteur-2 apparenté à NF-E2/génétique , Facteur-2 apparenté à NF-E2/métabolisme , Récepteurs aux IgE/génétique , Récepteurs aux IgE/métabolisme , ARN messager/métabolisme , Récepteur de type Toll-4/génétique , Récepteur de type Toll-4/métabolismeRÉSUMÉ
Rodent mast cells are classified into two major subsets, mucosal mast cells (MMCs) and connective tissue mast cells. MMCs arise from mast cell progenitors that are mobilized from the bone marrow to mucosal tissues in response to allergic inflammation or helminth infection. TGF-ß is known as an inducer of MMC differentiation in mucosal tissues, but we have previously found that Notch receptor-mediated signaling also leads to the differentiation. Here, we examined the relationship between Notch and TGF-ß signaling in MMC differentiation using mouse bone marrow-derived mast cells (BMMCs). We found that the coexistence of Notch and TGF-ß signaling markedly upregulates the expression of MMC markers, mouse mast cell protease (mMCP)-1, mMCP-2, and αE integrin/CD103, more than Notch or TGF-ß signaling alone, and that their signals act interdependently to induce these marker expressions. Notch and TGF-ß-mediated transcription of MMC marker genes were both dependent on the TGF-ß signaling transducer SMAD4. In addition, we also found that Notch signaling markedly upregulated mMCP-1 and mMCP-2 expression levels through epigenetic deregulation of the promoter regions of these genes, but did not affect the promoter of the CD103-encoding gene. Moreover, forced expression of the constitutively active Notch2 intracellular domain in BMMCs showed that Notch signaling promotes the nuclear localization of SMADs 3 and 4 and causes SMAD4-dependent gene transcription. These findings indicate that Notch and TGF-ß signaling play interdependent roles in inducing the differentiation and maturation of MMCs. These roles may contribute to the rapid expansion of the number of MMCs during allergic mucosal inflammation.
Sujet(s)
Mastocytes , Facteur de croissance transformant bêta , Animaux , Expression des gènes , Inflammation/métabolisme , Mastocytes/métabolisme , Souris , Muqueuse , Facteur de croissance transformant bêta/métabolismeRÉSUMÉ
NLRP3 inflammasomes play crucial roles in the initiation of host defense by converting pro-Caspase-1 to mature Caspase-1, which in turn processes immature IL-1ß and IL-18 into their biologically active forms. Although NLRP3 expression is restricted to monocytic lineages such as monocytes, macrophages, and dendritic cells, the mechanisms determining the lineage-specific expression of NLRP3 remain largely unknown. In this study, we investigated the transcription factors involved in cell-type-specific transcription of NLRP3. We found that a distal, rather than a proximal, promoter of human NLRP3 was predominantly used in the human monocytic cell lines and macrophages. Reporter analysis showed that an Ets/IRF composite element (EICE) at -309/-300 and an Ets motif at +5/+8 were critical for transcriptional activity of the distal promoter. Electrophoretic mobility shift assays and chromatin immunoprecipitation assays demonstrated that two transcription factors, PU.1 and IRF8, both of which play essential roles in development and gene expression of the monocytic lineage, were bound to the EICE site, whereas PU.1 alone was bound to the Ets site. Knockdown of PU.1 and/or IRF8 mediated by small interfering RNA downregulated expression of NLRP3 and related molecules and markedly diminished the LPS-induced release of IL-1ß in THP-1, suggesting that activity of the NLRP3 inflammasome was suppressed by knockdown of PU.1 and IRF8. Taken together, these results indicate that PU.1 and IRF8 are involved in the monocytic lineage-specific expression of NLRP3 by binding to regulatory elements within its promoter and that PU.1 and IRF8 are potential targets for regulating the activity of the NLRP3 inflammasome.
Sujet(s)
Inflammasomes/génétique , Facteurs de régulation d'interféron/métabolisme , Macrophages/immunologie , Protéine-3 de la famille des NLR contenant un domaine pyrine/génétique , Protéines proto-oncogènes/métabolisme , Transactivateurs/métabolisme , Animaux , Régulation de l'expression des gènes/immunologie , Techniques de knock-down de gènes , Humains , Inflammasomes/immunologie , Inflammasomes/métabolisme , Facteurs de régulation d'interféron/génétique , Macrophages/métabolisme , Souris , Protéine-3 de la famille des NLR contenant un domaine pyrine/métabolisme , Régions promotrices (génétique) , Protéines proto-oncogènes/génétique , Spécificité d'espèce , Cellules THP-1 , Transactivateurs/génétique , Cellules U937RÉSUMÉ
IL-33-activated group 2 innate lymphoid cells critically contribute to protease allergen-induced airway inflammation models. However, IL-33 is dispensable for a subcutaneous (s.c.) papain-induced skin inflammation model, suggesting distinct mechanisms between intranasal and s.c. sensitization. Here, we examined the role of IL-17A in the s.c. model. Papain-exposed skin produced IL-17A and an excess amount of a soluble decoy receptor for IL-33, with the latter being a possible reason for the independence of the s.c. model from IL-33. An IL-17A deficiency attenuated papain-induced skin eosinophilia and serum papain-specific IgE and IgG1 levels, whereas the s.c. administration of IL-17A with enzymatically inactive papain enhanced serum papain-specific IgE and IgG1 levels and T helper 2 development in draining lymph nodes in an IL-33-independent manner, suggesting IL-33-independent enhancement of papain-specific type 2 responses by IL-17A. The s.c. papain increased IL-17A+ γδ T cells in draining lymph nodes, approximately half of which were Vγ4+, as the majority of IL-17A+ cells, and increased Vγ5+ and Vγ4+ γδ T cells in the skin. Depletion of γδ TCR+ cells reduced T helper cytokine production in antigen-restimulated draining lymph node cells. These results suggest a novel role for IL-17A as an enhancer of skin eosinophilia and serum antigen-specific IgE production and for γδ T cells as an enhancer of T helper cell activation in the s.c. papain model.
Sujet(s)
Dermatite/immunologie , Éosinophilie/immunologie , Immunité innée , Interleukine-17/métabolisme , Interleukine-33/métabolisme , Papaïne/administration et posologie , Peau/anatomopathologie , Animaux , Dermatite/métabolisme , Dermatite/anatomopathologie , Éosinophilie/métabolisme , Éosinophilie/anatomopathologie , Humains , Injections sous-cutanées , Peau/immunologie , Peau/métabolismeRÉSUMÉ
BACKGROUND: Oral immunotherapy (OIT) aims to establish desensitization and sustained unresponsiveness (SU) in patients with food allergy by ingestion of gradually increasing doses of specific food allergens. However, little is known about the mechanisms by which OIT induces SU to specific allergens. OBJECTIVES: We investigated the role of Notch signaling, which controls cell fate decisions in many types of immune cells in the induction of SU by OIT treatment. METHODS: Two types of mouse models, ovalbumin-induced food allergy and OIT, were generated. To elucidate the role of Notch signaling in OIT-induced SU, mice were intraperitoneally injected with the Notch signaling inhibitor N-[(3,5-difluorophenyl)acetyl]-l-alanyl-2-phenylglycine-1,1-dimethylethyl ester during the OIT treatment period. RESULTS: Ovalbumin-sensitized mice were desensitized and also had SU induced by OIT treatment, whereas repeated challenges with ovalbumin caused the development of severe allergic reactions in ovalbumin-sensitized mice. Administration of N-[(3,5-difluorophenyl)acetyl]-l-alanyl-2-phenylglycine-1,1-dimethylethyl ester to mice during the OIT treatment period inhibited the establishment of SU to ovalbumin but did not affect the induction of desensitization. OIT induced a systemic expansion of IL-10-producing CD4+ T cells, including TH2 cells, and myeloid-derived suppressor cells (MDSCs), particularly the monocytic MDSC subpopulation. Inhibition of Notch signaling prevented the OIT-induced expansion of those cells. In vitro cultures of bone marrow cells showed that Notch signaling directly promoted the generation of monocytic MDSCs. In addition, the contribution of MDSCs to OIT-induced SU was confirmed by MDSC depletion with the anti-Gr1 antibody. CONCLUSION: Notch signaling contributes to the establishment of SU induced by OIT through systemic expansion of immunosuppressive cells, such as IL-10-producing CD4+ T cells and MDSCs.
Sujet(s)
Désensibilisation immunologique/méthodes , Hypersensibilité alimentaire/immunologie , Cellules myéloïdes suppressives/immunologie , Récepteurs Notch/métabolisme , Lymphocytes auxiliaires Th2/immunologie , Administration par voie orale , Allergènes/immunologie , Animaux , Cellules cultivées , Modèles animaux de maladie humaine , Femelle , Hypersensibilité alimentaire/thérapie , Humains , Tolérance immunitaire , Interleukine-10/métabolisme , Souris , Souris de lignée BALB C , Ovalbumine/immunologie , Transduction du signalRÉSUMÉ
C-C chemokine receptor type 7 (CCR7) is essential for migration of dendritic cells (DCs) to draining lymph nodes. PU.1/Spi1 is a transcription factor playing a critical role in the gene regulation of DCs. PU.1 knockdown decreased the expression of CCR7 in bone marrow-derived DCs and subsequently attenuated migration in vitro and in vivo. Reporter assays, EMSA, and chromatin immunoprecipitation assays revealed that PU.1 binds to the most proximal Ets motif of the Ccr7 promoter, which is involved in transcriptional activation. The CCR7 expression level, which was higher in the programmed cell death 1 ligand 2 (PD-L2)+ population than in the PD-L2- population and was markedly suppressed by TGF-ß treatment, coincided with the binding level of PU.1 to the Ccr7 promoter. The PU.1 binding level in CCR7high mesenteric lymph nodes DCs was higher than in other DC subtypes. The involvement of PU.1 in the expression of the CCR7 gene was also observed in human DCs. We conclude that PU.1 plays a pivotal role in DC migration by transactivating the CCR7 gene via the Ets motif in the promoter in both humans and mice.-Yashiro, T., Takeuchi, H., Nakamura, S., Tanabe, A., Hara, M., Uchida, K., Okumura, K., Kasakura, K., Nishiyama, C. PU.1 plays a pivotal role in dendritic cell migration from the periphery to secondary lymphoid organs via regulating CCR7 expression.
Sujet(s)
Mouvement cellulaire/génétique , Cellules dendritiques/physiologie , Noeuds lymphatiques/physiologie , Tissu lymphoïde/physiologie , Protéines proto-oncogènes/génétique , Récepteurs CCR7/génétique , Transactivateurs/génétique , Animaux , Lignée cellulaire , Femelle , Régulation de l'expression des gènes/génétique , Humains , Souris , Souris de lignée BALB C , Souris de lignée C57BL , Régions promotrices (génétique)/génétique , Activation de la transcription/génétiqueSujet(s)
Immunité acquise/effets des médicaments et des substances chimiques , Allergènes/immunologie , Inhibiteurs des cyclooxygénases/pharmacologie , Immunité innée/effets des médicaments et des substances chimiques , Interleukine-13/immunologie , Peptide hydrolases/immunologie , Prostaglandin-endoperoxide synthases/métabolisme , Animaux , Asthme/traitement médicamenteux , Asthme/immunologie , Asthme/métabolisme , Asthme/anatomopathologie , Cytokines/métabolisme , Modèles animaux de maladie humaine , Souris , Sous-populations de lymphocytes T/effets des médicaments et des substances chimiques , Sous-populations de lymphocytes T/immunologie , Sous-populations de lymphocytes T/métabolismeRÉSUMÉ
NR4A3/NOR1 belongs to the NR4A subfamily of the nuclear hormone receptor superfamily, which is activated in a ligand-independent manner. To examine the role of NR4A3 in gene expression of dendritic cells (DCs), we introduced NR4A3 small interfering RNA (siRNA) into bone marrow-derived DCs and determined the expression levels of mRNA and proteins of cytokines, cell surface molecules, NF-κB signaling-related proteins, and transcription factors. The expression level of NR4A3 was markedly upregulated by TLR-mediated stimulation in DCs. NR4A3 knockdown significantly suppressed LPS, CpG, or poly(I:C)-mediated upregulation of CD80, CD86, IL-10, IL-6, and IL-12. Proliferation and IL-2 production levels of T cells cocultured with NR4A3 knocked-down DCs were significantly lower than that of T cells cocultured with control DCs. Furthermore, the expression of IKKß, IRF4, and IRF8 was significantly decreased in NR4A3 siRNA-introduced bone marrow-derived DCs. The knockdown experiments using siRNAs for IKKß, IRF4, and/or IRF8 indicated that LPS-induced upregulation of IL-10 and IL-6 was reduced in IKKß knocked-down cells, and that the upregulation of IL-12 was suppressed by the knockdown of IRF4 and IRF8. Taken together, these results indicate that NR4A3 is involved in TLR-mediated activation and gene expression of DCs.
Sujet(s)
Différenciation cellulaire , Protéines de liaison à l'ADN/métabolisme , Cellules dendritiques/immunologie , Activation des lymphocytes , Protéines de tissu nerveux/métabolisme , Récepteurs aux stéroïdes/métabolisme , Récepteurs des hormones thyroïdiennes/métabolisme , Lymphocytes T/immunologie , Animaux , Présentation d'antigène , Prolifération cellulaire , Cellules cultivées , Techniques de coculture , Protéines de liaison à l'ADN/génétique , Lipopolysaccharides/immunologie , Souris , Souris de lignée BALB C , Souris de lignée C57BL , Facteur de transcription NF-kappa B/métabolisme , Protéines de tissu nerveux/génétique , Petit ARN interférent/génétique , Récepteurs aux stéroïdes/génétique , Récepteurs des hormones thyroïdiennes/génétique , Transduction du signal , Récepteurs de type Toll/immunologieRÉSUMÉ
BACKGROUND: Interleukin-33 (IL-33) is an alarmin cytokine that binds to the interleukin 1 receptor-like 1 protein ST2. Clock is a key circadian gene that is essential for endogenous clockworks in mammals. This study investigated whether Clock temporally regulated IL-33-mediated responses in mast cells. METHODS: The kinetics of IL-33-mediated IL-6, IL-13, and TNF-α productions were compared between bone marrow-derived mast cells (BMMCs) from wild-type and Clock-mutated mice (ClockΔ19/Δ19 mice). The kinetics of the neutrophil influx into the peritoneal cavity or expression of IL-13 and Gob-5 in the lung in response to IL-33 were compared between wild-type and ClockΔ19/Δ19 mice. We also examined the kinetics of ST2 expression in mast cells and its association with Clock expression. RESULTS: There was a time-of-day-dependent variation in IL-33-mediated IL-6, IL-13, and TNF-α production in wild-type BMMCs, which was absent in Clock-mutated BMMCs. IL-33-induced neutrophil infiltration into the peritoneal cavity also showed a time-of-day-dependent variation in wild-type mice, which was absent in ClockΔ19/Δ19 mice. Furthermore, IL-33-induced IL-13 and Gob-5 expression in the lung exhibited a time-of-day-dependent variation in wild-type mice. These temporal variations in IL-33-mediated mast cell responses were associated with temporal variations of ST2 expression in mast cells. In addition, CLOCK bound to the promoter region of ST2 and Clock deletion resulted in down-regulation of ST2 expression in mast cells. CONCLUSIONS: CLOCK temporally gates mast cell responses to IL-33 via regulation of ST2 expression. Our findings provide novel insights into IL-33/mast cell-associated physiology and pathologies.
Sujet(s)
Protéines CLOCK/génétique , Protéines CLOCK/métabolisme , Protéine-1 analogue au récepteur de l'interleukin-1/métabolisme , Interleukine-33/métabolisme , Mastocytes/immunologie , Mastocytes/métabolisme , Animaux , Granulocytes basophiles/effets des médicaments et des substances chimiques , Granulocytes basophiles/immunologie , Granulocytes basophiles/métabolisme , Cytokines/métabolisme , Régulation de l'expression des gènes , Protéine-1 analogue au récepteur de l'interleukin-1/génétique , Interleukine-33/pharmacologie , Mâle , Mastocytes/effets des médicaments et des substances chimiques , Souris , Souris knockout , Souris transgéniques , Granulocytes neutrophiles/effets des médicaments et des substances chimiques , Granulocytes neutrophiles/immunologie , Granulocytes neutrophiles/métabolisme , PhotopériodeRÉSUMÉ
PU.1 is a hematopoietic cell-specific transcription factor belonging to the Ets family, which plays an important role in the development of dendritic cells (DCs). CD11c (encoded by Itgax) is well established as a characteristic marker of hematopoietic lineages including DCs. In the present study, we analyzed the role of PU.1 (encoded by Spi-1) in the expression of CD11c. When small interfering RNA (siRNA) for Spi-1 was introduced into bone marrow-derived DCs (BMDCs), the mRNA level and cell surface expression of CD11c were dramatically reduced. Using reporter assays, the TTCC sequence at -56/-53 was identified to be critical for PU.1-mediated activation of the promoter. An EMSA showed that PU.1 directly bound to this region. ChIP assays demonstrated that a significant amount of PU.1 bound to this region on chromosomal DNA in BMDCs, which was decreased in LPS-stimulated BMDCs in accordance with the reduced levels of mRNAs of Itgax and Spi-1, and the histone acetylation degree. Enforced expression of exogenous PU.1 induced the expression of the CD11c protein on the cell surface of mast cells, whereas control transfectants rarely expressed CD11c. Quantitative RT-PCR also showed that the expression of a transcription factor Irf4, which is a partner molecule of PU.1, was reduced in PU.1-knocked down BMDCs. IRF4 transactivated the Itgax gene in a synergistic manner with PU.1. Taken together, these results indicate that PU.1 functions as a positive regulator of CD11c gene expression by directly binding to the Itgax promoter and through transactivation of the Irf4 gene.
Sujet(s)
Antigènes CD11c/métabolisme , Cellules dendritiques/physiologie , Hématopoïèse , Facteurs de régulation d'interféron/métabolisme , Protéines proto-oncogènes/métabolisme , Transactivateurs/métabolisme , Acétylation , Animaux , Antigènes CD11c/génétique , Cellules cultivées , Protéines de liaison à l'ADN/génétique , Régulation de l'expression des gènes , Hématopoïèse/génétique , Histone/métabolisme , Facteurs de régulation d'interféron/génétique , Souris , Souris de lignée BALB C , Spécificité d'organe , Régions promotrices (génétique)/génétique , Protéines proto-oncogènes/génétique , Petit ARN interférent/génétique , Transactivateurs/génétique , Activation de la transcriptionRÉSUMÉ
BACKGROUND: Mucosal mast cells (MMCs) play a central role in the development of symptoms associated with IgE-mediated food allergy. Recently, Notch2-mediated signaling was shown to be involved in proper MMC distribution in the intestinal tract. OBJECTIVE: This study aimed to clarify the mechanism by which Notch signaling regulates MMC distribution in the intestinal mucosa. Furthermore, pharmacologic inhibition of Notch signaling was evaluated as a treatment for symptoms associated with experimental food allergy. METHODS: Bone marrow-derived mast cells generated from mice were cultured with Notch ligands, and then expression of genes associated with MMCs was measured in the cells. In addition, the effect of an inhibitor of Notch signaling on food antigen-induced allergic reactions was examined in a mouse model of food allergy. RESULTS: Notch signaling induced MMC differentiation through upregulation of expression of genes characteristic of MMCs in the presence of IL-3. Some lamina propria cells isolated from the mouse small intestine expressed Notch ligands and were able to upregulate MMC markers in bone marrow-derived mast cells through Notch signaling. In a mouse model of food allergy, administration of a Notch signaling inhibitor led to suppression of food antigen-induced hyperplasia of intestinal MMCs, resulting in alleviation of allergic diarrhea and systemic anaphylaxis. CONCLUSION: Notch signaling contributes to differentiation and accumulation of MMCs in the intestinal mucosa. Thus inhibition of Notch signaling alleviates symptoms associated with experimental food allergy. These results raise the possibility that Notch signaling in mast cells is a novel target for therapy in patients with food allergy.
Sujet(s)
Hypersensibilité alimentaire/immunologie , Muqueuse intestinale/immunologie , Mastocytes/immunologie , Récepteurs Notch/antagonistes et inhibiteurs , Allergènes/immunologie , Animaux , Cytokines/immunologie , Dipeptides/pharmacologie , Dipeptides/usage thérapeutique , Femelle , Hypersensibilité alimentaire/traitement médicamenteux , Hypersensibilité alimentaire/anatomopathologie , Hyperplasie/traitement médicamenteux , Hyperplasie/immunologie , Hyperplasie/anatomopathologie , Intestin grêle/cytologie , Mastocytes/anatomopathologie , Souris de lignée BALB C , Ovalbumine/immunologie , Récepteurs Notch/immunologie , Transduction du signal/effets des médicaments et des substances chimiquesRÉSUMÉ
PU.1 is a hematopoietic lineage-specific transcription factor belonging to the Ets family. We investigated the role of PU.1 in the expression of OX40L in dendritic cells (DCs), because the regulatory mechanism of cell type-specific expression of OX40L, which is mainly restricted to antigen-presenting cells, is largely unknown despite the critical involvement in Th2 and Tfh development. PU.1 knockdown decreased the expression of OX40L in mouse DCs. Chromatin immunoprecipitation (ChIP) assays demonstrated that PU.1 constitutively bound to the proximal region of the OX40L promoter. Reporter assays and electrophoretic mobility shift assays revealed that PU.1 transactivated the OX40L promoter through direct binding to the most-proximal Ets motif. We found that this Ets motif is conserved between mouse and human, and that PU.1 bound to the human OX40L promoter in ChIP assay using human monocyte-derived DCs. ChIP assays based on ChIP-seq datasets revealed that PU.1 binds to several sites distant from the transcription start site on the OX40L gene in addition to the most-proximal site in mouse DCs. In the present study, the structure of the OX40L promoter regulated by PU.1 is determined. It is also suggested that PU.1 is involved in mouse OX40L expression via multiple binding sites on the gene.
Sujet(s)
Cellules dendritiques/physiologie , Glycoprotéines membranaires/génétique , Régions promotrices (génétique) , Protéines proto-oncogènes/métabolisme , Transactivateurs/métabolisme , Facteurs de nécrose tumorale/génétique , Animaux , Femelle , Régulation de l'expression des gènes , Techniques de knock-down de gènes , Cellules HEK293 , Humains , Glycoprotéines membranaires/métabolisme , Souris de lignée BALB C , Souris de lignée C57BL , Motifs nucléotidiques , Ligand de OX40/génétique , Ligand de OX40/métabolisme , Protéines proto-oncogènes/génétique , Transactivateurs/génétique , Site d'initiation de la transcription , Activation de la transcription , Facteurs de nécrose tumorale/métabolismeRÉSUMÉ
The cofactor CIITA is a master regulator of MHC class II expression and several transcription factors regulating the cell type-specific expression of CIITA have been identified. Although the MHC class II expression in plasmacytoid dendritic cells (pDCs) is also mediated by CIITA, the transcription factors involved in the CIITA expression in pDCs are largely unknown. In the present study, we analyzed the role of a hematopoietic lineage-specific transcription factor, PU.1, in CIITA transcription in pDCs. The introduction of PU.1 siRNA into mouse pDCs and a human pDC cell line, CAL-1, reduced the mRNA levels of MHC class II and CIITA. When the binding of PU.1 to the 3rd promoter of CIITA (pIII) in CAL-1 and mouse pDCs was analyzed by a chromatin immunoprecipitation assay, a significant amount of PU.1 binding to the pIII was detected, which was definitely decreased in PU.1 siRNA-transfected cells. Reporter assays showed that PU.1 knockdown reduced the pIII promoter activity and that three Ets-motifs in the human pIII promoter were candidates of cis-enhancing elements. By electrophoretic mobility shift assays, it was confirmed that two Ets-motifs, GGAA (-181/-178) and AGAA (-114/-111), among three candidates, were directly bound with PU.1. When mouse pDCs and CAL-1 cells were stimulated by GM-CSF, mRNA levels of PU.1, pIII-driven CIITA, total CIITA, MHC class II, and the amount of PU.1 binding to pIII were significantly increased. The GM-CSF-mediated up-regulation of these mRNAs was canceled in PU.1 siRNA-introduced cells. Taking these results together, we conclude that PU.1 transactivates the pIII through direct binding to Ets-motifs in the promoter in pDCs.
Sujet(s)
Cellules dendritiques/immunologie , Antigènes d'histocompatibilité de classe II/immunologie , Protéines nucléaires/génétique , Protéines proto-oncogènes/physiologie , Transactivateurs/génétique , Transactivateurs/physiologie , Transcription génétique , Animaux , Lignée cellulaire , Techniques de knock-down de gènes , Humains , Souris , Souris de lignée BALB C , Régions promotrices (génétique) , Liaison aux protéines , Protéines proto-oncogènes/génétique , Petit ARN interférent/génétiqueRÉSUMÉ
Allergen sources such as mites, insects, fungi, and pollen contain proteases. Airway exposure to proteases induces allergic airway inflammation and IgE/IgG1 responses via IL-33-dependent mechanisms in mice. We examined the epicutaneous sensitization of mice to a model protease allergen, papain; the effects of tape stripping, which induces epidermal barrier dysfunction; and the atopic march upon a subsequent airway challenge. Papain painting on ear skin and tape stripping cooperatively promoted dermatitis, the skin gene expression of proinflammatory cytokines and growth factors, up-regulation of serum total IgE, and papain-specific IgE/IgG1 induction. Epicutaneous sensitization induced T helper (Th) 2 cells and Th17 differentiation in draining lymph nodes. Ovalbumin and protease inhibitor-treated papain induced no or weak responses, whereas the co-administration of ovalbumin and papain promoted ovalbumin-specific IgE/IgG1 induction. Wild-type and IL-33-deficient mice showed similar responses in the epicutaneous sensitization phase. The subsequent airway papain challenge induced airway eosinophilia and maintained high papain-specific IgE levels in an IL-33-dependent manner. These results suggest that allergen source-derived protease activity and mechanical barrier damage such as that caused by scratching cooperatively promote epicutaneous sensitization and skin inflammation and that IL-33 is dispensable for epicutaneous sensitization but is crucial in the atopic march upon a subsequent airway low-dose encounter with protease allergens.
Sujet(s)
Allergènes/immunologie , Dermatite/immunologie , Hypersensibilité/immunologie , Peau/immunologie , Peau/traumatismes , Animaux , Différenciation cellulaire , Cytokines/métabolisme , Test ELISA , Femelle , Immunoglobuline E/immunologie , Immunoglobuline G/immunologie , Inflammation , Interleukine-33/génétique , Interleukine-33/immunologie , Souris , Souris de lignée C57BL , Ovalbumine , Papaïne/immunologie , Inhibiteurs de protéases/composition chimique , Réaction de polymérisation en chaine en temps réel , Peau/effets des médicaments et des substances chimiques , Contrainte mécanique , Cellules Th17/cytologie , Lymphocytes auxiliaires Th2/cytologie , Plaies et blessures/métabolismeRÉSUMÉ
Protease activity of papain, a plant-derived occupational allergen homologous to mite major allergens, is essential to IgE/IgG1 production and lung eosinophilia induced by intranasal papain administration in mice, and IL-33 contributes to these responses. In this work, we investigate skin and Ab responses induced by s.c. papain administration into ear lobes and responses induced by subsequent airway challenge with papain. Subcutaneous papain injection induced swelling associated with increased epidermal thickness, dermal inflammation, serum IgE/IgG1 responses, and Th2 cytokine production in draining lymph node cells restimulated in vitro. These responses were markedly less upon s.c. administration of protease inhibitor-treated papain. Results obtained by using mast cell-deficient mice and reconstitution of tissue mast cells suggested the contribution of mast cells to papain-specific IgE/IgG1 responses and eosinophil infiltration. The responses were equivalent between wild-type and IL-33(-/-) mice. After the subsequent airway challenge, the s.c. presensitized wild-type mice showed more severe lung eosinophilia than those without the presensitization. The presensitized IL-33(-/-) mice showed modest lung eosinophilia, which was absent without the presensitization, but its severity and IgE boost by the airway challenge were markedly less than the presensitized wild-type mice, in which protease activity of inhaled papain contributed to the responses. The results suggest that mechanisms for the protease-dependent sensitization differ between skin and airway and that cooperation of mast cell-dependent, IL-33-independent initial sensitization via skin and protease-induced, IL-33-mediated mechanism in re-exposure via airway to protease allergens maximizes the magnitude of the transition from skin inflammation to asthma in natural history of progression of allergic diseases.
Sujet(s)
Allergènes/administration et posologie , Allergènes/immunologie , Hypersensibilité/immunologie , Interleukine-33/immunologie , Mastocytes/immunologie , Absorption nasale , Peptide hydrolases/immunologie , Absorption sous-cutanée , Animaux , Asthme , Hyperréactivité bronchique/immunologie , Hyperréactivité bronchique/anatomopathologie , Granulocytes éosinophiles/immunologie , Hypersensibilité/anatomopathologie , Immunoglobuline E/sang , Immunoglobuline G/sang , Inflammation , Interleukine-33/déficit , Poumon/immunologie , Souris , Papaïne/administration et posologie , Papaïne/immunologie , Peptide hydrolases/administration et posologie , Poumon éosinophile/immunologie , Poumon éosinophile/anatomopathologie , Peau/immunologie , Peau/anatomopathologie , Lymphocytes auxiliaires Th2/immunologieRÉSUMÉ
BACKGROUND: Patients with house dust mite (HDM) allergy or Ascariasis produce serum IgE specific to the antigens of HDM or nematode Ascaris, respectively. Although human IgE cross-reactivity has been reported between HDM and Ascaris antigens, it remains unclear whether it contributes to the pathogenesis of allergic diseases. We herein investigated the induction of cross-reactive antibodies and T cells in mice and effects of airway exposure to HDM antigens after preimmunization with Ascaris antigens. METHODS: Mice were intraperitoneally immunized with HDM or Ascaris antigens with Alum, followed by the intranasal administration of HDM antigens. Serum antigen-specific IgE and IgG were measured by ELISA. Cytokine release in splenocytes from Ascaris-immunized mice upon in vitro restimulation with HDM antigens were measured by ELISA. RESULTS: Immunization with Ascaris or HDM antigens induced cross-reactive IgG1. Splenocytes from Ascaris-immunized mice released IL-5 and IL-13 in response to the restimulation with HDM antigens. Subsequent airway exposure to HDM antigens promoted the induction of HDM-specific IgE and upregulation of HDM-specific IgG1 in Ascaris-immunized mice, whereas these responses were not detected or smaller without the Ascaris presensitization. CONCLUSIONS: We demonstrated that the immunization of naïve mice with Ascaris antigens induced production of antibodies and differentiation of Th2 cells, which were cross-reactive to HDM antigens, and accelerated induction of serum HDM-specific IgE upon subsequent airway exposure to HDM antigens in mice. These results suggest that sensitization to HDM towards IgE-mediated allergic diseases is faster in individuals with a previous history of Ascaris infection than in those without presensitization to Ascaris.
Sujet(s)
Antigènes de Dermatophagoides/immunologie , Antigènes d'helminthe/immunologie , Ascaris/immunologie , Hypersensibilité/immunologie , Immunisation , Immunoglobuline E/immunologie , Animaux , Modèles animaux de maladie humaine , Test ELISA , Femelle , Hypersensibilité/sang , Immunoglobuline E/sang , Immunoglobuline G/sang , Immunoglobuline G/immunologie , Souris , Rate/cytologie , Rate/immunologie , Spécificité antigénique des récepteurs des lymphocytes T/immunologieRÉSUMÉ
FcεRI, which is composed of α, ß, and γ subunits, plays an important role in IgE-mediated allergic responses. TGF-ß1 has been reported to suppress FcεRI and stem cell factor receptor c-Kit expression on mast cell surfaces and to suppress mast cell activation induced by cross-linking of FcεRI. However, the molecular mechanism by which these expressions and activation are suppressed by TGF-ß1 remains unclear. In this study, we found that the expression of Ets homologous factor (Ehf), a member of the Ets family transcriptional factors, is upregulated by TGF-ß/Smad signaling in mouse bone marrow-derived mast cells (BMMCs). Forced expression of Ehf in BMMCs repressed the transcription of genes encoding FcεRIα, FcεRIß, and c-Kit, resulting in a reduction in cell surface FcεRI and c-Kit expression. Additionally, forced expression of Ehf suppressed FcεRI-mediated degranulation and cytokine production. Ehf inhibited the promoter activity of genes encoding FcεRIα, FcεRIß, and c-Kit by binding to these gene promoters. Furthermore, the mRNA levels of Gata1, Gata2, and Stat5b were lower in BMMCs stably expressing Ehf compared with control cells. Because GATA-1 and GATA-2 are positive regulators of FcεRI and c-Kit expression, decreased expression of GATAs may be also involved in the reduction of FcεRI and c-Kit expression. Decreased expression of Stat5 may contribute to the suppression of cytokine production by BMMCs. In part, mast cell response to TGF-ß1 was mimicked by forced expression of Ehf, suggesting that TGF-ß1 suppresses FcεRI and c-Kit expression and suppresses FcεRI-mediated activation through upregulation of Ehf.
Sujet(s)
Protéines proto-oncogènes c-kit/biosynthèse , Récepteurs aux IgE/immunologie , Facteurs de transcription/immunologie , Facteur de croissance transformant bêta-1/métabolisme , Animaux , Cellules de la moelle osseuse , Dégranulation cellulaire/immunologie , Cellules cultivées , Cytokines/biosynthèse , Facteur de transcription GATA-1/biosynthèse , Facteur de transcription GATA-1/génétique , Facteur de transcription GATA-2/biosynthèse , Facteur de transcription GATA-2/génétique , Immunoglobuline E/immunologie , Mastocytes/immunologie , Souris , Souris de lignée BALB C , Régions promotrices (génétique)/génétique , Protéines proto-oncogènes c-kit/génétique , Interférence par ARN , ARN messager/métabolisme , Petit ARN interférent , Récepteurs aux IgE/biosynthèse , Facteur de transcription STAT-5/biosynthèse , Facteur de transcription STAT-5/génétique , Transduction du signal/immunologie , Protéines Smad/métabolisme , Facteurs de transcription/biosynthèse , Transcription génétique/génétique , Activation de la transcriptionRÉSUMÉ
BACKGROUND: The transcription factors NFATc1 and PU.1 play important roles in osteoclast development. NFATc1 and PU.1 transactivate osteoclast-specific gene expression and a deficiency in NFATc1 or PU.1 genes causes osteopetrosis due to an insufficient development of osteoclasts. However, the existence of cross-regulation between NFATc1 and PU.1 is largely unknown. In the present study, the role of PU.1 in NFATc1 expression was investigated. METHODS: Osteoclasts were generated from mouse bone marrow cells. PU.1 knockdown was performed with siRNA introduction. The mRNA levels in siRNA-introduced cells were determined by quantitative RT-PCR. The involvement of PU.1 in the NFATc1 promoter was analyzed by using a chromatin immunoprecipitation (ChIP) assay and a reporter assay. Retrovirus vector was used for enforced expression of PU.1. RESULTS: Introduction of PU.1 siRNA into bone marrow-derived osteoclasts resulted in a decrease in NFATc1 mRNA level. A ChIP assay showed that PU.1 bound to the NFATc1 promoter in osteoclasts. NFATc1 promoter activity was reduced in PU.1 knockdown cells as assessed by a reporter assay. PU.1 siRNA introduction also downregulated the expression of osteoclast-specific genes and tartrate resistant acid phosphatase (TRAP) activity. Enforced expression of PU.1 using a retrovirus vector increased NFATc1 expression and TRAP activity. When NFATc1 expression was knocked down by using siRNA, the induction of osteoclast-specific genes and TRAP-positive cells was suppressed without affecting the expression level of PU.1. CONCLUSIONS: These results indicate that PU.1 is involved in osteoclast development by transactivating NFATc1 expression via direct binding to the NFATc1 promoter.