Your search keyword '"Cartenì, M."' showing total 3 results

1. Antiapoptotic Seminal Vesicle Protein IV Induces Histamine Release from Human FcεRI+ Cells

Author

Gianni Marone, Salvatore Metafora, Amato de Paulis, Massimo Triggiani, Nella Prevete, Gianpietro Ravagnan, Salvatore De Maria, Maria Cartenì, Raffaele Ragone, Francesca Rossi, Vittoria Metafora, Prevete, Nella, Rossi, FRANCESCA WANDA, Triggiani, M, Marone, Gianni, DE PAULIS, Amato, Metafora, V, De Maria, S, Cartenì, M, Ragone, R, Ravagnan, G, Metafora, S., Rossi, F. W., Triggiani, Massimo, Metafora, V., De Maria, S., Carteni, M., Ragone, R., and Ravagnan, G.

Subjects

Protein SV-IV, Mast cells, Basophils, FcεRI receptor, Histamine, Degranulation, Blastocyst implantation, Immunology, Basophil, Biology, Seminal Vesicle Secretory Proteins, Histamine Release, Cell Line, chemistry.chemical_compound, Seminal vesicle, Immune Tolerance, medicine, Animals, Humans, Immunology and Allergy, Mast Cells, Receptor, Lung, Receptors, IgE, Drug Synergism, General Medicine, Mast cell, Antibodies, Anti-Idiotypic, Rats, medicine.anatomical_structure, Secretory protein, chemistry, Cell culture, Calcium, Apoptosis Regulatory Proteins

Abstract

Background: Seminal vesicle protein number 4 (SV-IV) is a small, basic, multifunctional, intrinsically disordered secretory protein synthesized in large amounts by rat seminal vesicle epithelium under androgen transcriptional control. SV-IV-immunorelated proteins occur in other rat tissues and in humans. Methods: The in vitro effect of SV-IV on human FcΕRI+ cells was investigated by standard immunologic, biochemical and molecular biology procedures. Results: SV-IV-induced histamine release from human basophils and lung mast cells without any influence on leukotriene C4 release and cell migration. The histamine release rate was slower compared with that induced by anti-IgE, the temperature dependence of the event being similar. SV-IV-induced histamine release was Ca2+-dependent, suggesting a physiological interaction of the protein with FcΕRI+ cells. SV-IV and anti-IgE acted synergistically on the histamine release. SV-IV did not induce de novo synthesis of cytokines and growth factors (transforming growth factor-β1, interleukin-10, interleukin-13, tumor necrosis factor-α, vascular endothelial growth factor A) in FcΕRI+ cells. Conclusions: SV-IV protein induces in human FcΕRI+ cells the release of histamine, a proinflammatory, antiapoptotic and immunosuppressive biogenic amine. These data: (1) are consistent with the antiapoptotic and immunosuppressive properties of SV-IV; (2) confirm a regulatory feature of SV-IV on mammal inflammatory reactivity by either inhibiting the arachidonate cascade pathway or stimulating proinflammatory cytokine release from lymphocyte/monocytes and histamine from FcΕRI+ cells; (3) raise the possibility of a protective role of SV-IV on implanting hemiallogenic blastocysts against maternal reactive oxygen species and immunological attacks at the uterine implantation site.

Published

2009

2. Antiapoptotic seminal vesicle protein IV induces histamine release from human FcepsilonRI+ cells.

Author

Prevete N, Rossi FW, Triggiani M, Marone G, de Paulis A, Metafora V, De Maria S, Cartenì M, Ragone R, Ravagnan G, and Metafora S

Subjects

Animals, Antibodies, Anti-Idiotypic pharmacology, Basophils immunology, Basophils metabolism, Basophils pathology, Calcium metabolism, Cell Line, Drug Synergism, Histamine Release immunology, Humans, Immune Tolerance, Lung pathology, Mast Cells immunology, Mast Cells metabolism, Mast Cells pathology, Rats, Apoptosis Regulatory Proteins pharmacology, Basophils drug effects, Histamine Release drug effects, Mast Cells drug effects, Receptors, IgE metabolism, Seminal Vesicle Secretory Proteins pharmacology

Abstract

Background: Seminal vesicle protein number 4 (SV-IV) is a small, basic, multifunctional, intrinsically disordered secretory protein synthesized in large amounts by rat seminal vesicle epithelium under androgen transcriptional control. SV-IV-immunorelated proteins occur in other rat tissues and in humans., Methods: The in vitro effect of SV-IV on human FcepsilonRI+ cells was investigated by standard immunologic, biochemical and molecular biology procedures., Results: SV-IV-induced histamine release from human basophils and lung mast cells without any influence on leukotriene C(4) release and cell migration. The histamine release rate was slower compared with that induced by anti-IgE, the temperature dependence of the event being similar. SV-IV-induced histamine release was Ca2+-dependent, suggesting a physiological interaction of the protein with FcepsilonRI+ cells. SV-IV and anti-IgE acted synergistically on the histamine release. SV-IV did not induce de novo synthesis of cytokines and growth factors (transforming growth factor-beta(1), interleukin-10, interleukin-13, tumor necrosis factor-alpha, vascular endothelial growth factor A) in FcepsilonRI+ cells., Conclusions: SV-IV protein induces in human FcepsilonRI+ cells the release of histamine, a proinflammatory, antiapoptotic and immunosuppressive biogenic amine. These data: (1) are consistent with the antiapoptotic and immunosuppressive properties of SV-IV; (2) confirm a regulatory feature of SV-IV on mammal inflammatory reactivity by either inhibiting the arachidonate cascade pathway or stimulating proinflammatory cytokine release from lymphocyte/monocytes and histamine from FcepsilonRI+ cells; (3) raise the possibility of a protective role of SV-IV on implanting hemiallogenic blastocysts against maternal reactive oxygen species and immunological attacks at the uterine implantation site., (2009 S. Karger AG, Basel.)

Published

2010

3. Differential mucosal IL-17 expression in two gliadin-induced disorders: gluten sensitivity and the autoimmune enteropathy celiac disease.

Author

Sapone A, Lammers KM, Mazzarella G, Mikhailenko I, Cartenì M, Casolaro V, and Fasano A

Subjects

Adult, CD3 Complex metabolism, Female, Gliadin administration & dosage, Gliadin immunology, Glutens administration & dosage, Glutens immunology, Humans, Interleukin-17 genetics, Intestinal Mucosa immunology, Intestinal Mucosa metabolism, Male, Receptors, Antigen, T-Cell, gamma-delta metabolism, Receptors, CCR6 metabolism, T-Lymphocytes immunology, Celiac Disease immunology, Celiac Disease metabolism, Celiac Disease physiopathology, Gastrointestinal Diseases immunology, Gastrointestinal Diseases metabolism, Gastrointestinal Diseases physiopathology, Gliadin adverse effects, Glutens adverse effects, Interleukin-17 metabolism, Intestine, Small metabolism

Abstract

Background: The immune-mediated enteropathy, celiac disease (CD), and gluten sensitivity (GS) are two distinct clinical conditions that are both triggered by the ingestion of wheat gliadin. CD, but not GS, is associated with and possibly mediated by an autoimmune process. Recent studies show that gliadin may induce the activation of IL-17-producing T cells and that IL-17 expression in the CD mucosa correlates with gluten intake., Methods: The small-intestinal mucosa of patients with CD and GS and dyspeptic controls was analyzed for expression of IL-17A mRNA by quantitative RT-PCR. The number of CD3+ and TCR-gammadelta lymphocytes and the proportion of CD3+ cells coexpressing the Th17 marker CCR6 were examined by in situ small-intestinal immunohistochemistry., Results: Mucosal expression of IL-17A was significantly increased in CD but not in GS patients, compared to controls. This difference was due to enhanced IL-17A levels in >50% of CD patients, with the remainder expressing levels similar to GS patients or controls, and was paralleled by a trend toward increased proportions of CD3+CCR6+ cells in intestinal mucosal specimens from these subjects., Conclusion: We conclude that GS, albeit gluten-induced, is different from CD not only with respect to the genetic makeup and clinical and functional parameters, but also with respect to the nature of the immune response. Our findings also suggest that two subgroups of CD, IL-17-dependent and IL-17-independent, may be identified based on differential mucosal expression of this cytokine., (Copyright 2009 S. Karger AG, Basel.)

Published

2010