Acetylcholine contributes to control the physiological inflammatory response during the peri-implantation period

Background: Maternal antigen-presenting cells attracted to the pregnant uterus interact with trophoblast cells and modulate their functional profile to favour immunosuppressant responses. Non-neuronal cholinergic system is expressed in human cytotrophoblast cells and in immune cells with homeostatic...

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Autor principal: Paparini, D.
Otros Autores: Gori, S., Grasso, E., Scordo, W., Calo, G., Pérez Leirós, C., Ramhorst, R., Salamone, G.
Formato: Capítulo de libro
Lenguaje:Inglés
Publicado: Blackwell Publishing Ltd 2015
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Acceso en línea:Registro en Scopus
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024 7 |2 cas  |a acetylcholine, 51-84-3, 60-31-1, 66-23-9; atropine, 51-55-8, 55-48-1; macrophage inflammatory protein 1alpha, 155075-84-6; neostigmine, 114-80-7, 588-17-0, 59-99-4, 8048-84-8; Acetylcholine 
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100 1 |a Paparini, D. 
245 1 0 |a Acetylcholine contributes to control the physiological inflammatory response during the peri-implantation period 
260 |b Blackwell Publishing Ltd  |c 2015 
270 1 0 |m Ramhorst, R.; Laboratory of Immunopharmacology, School of Sciences, University of Buenos Aires, Ciudad Universitaria, Pabellon 2 Piso 4., Argentina 
506 |2 openaire  |e Política editorial 
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520 3 |a Background: Maternal antigen-presenting cells attracted to the pregnant uterus interact with trophoblast cells and modulate their functional profile to favour immunosuppressant responses. Non-neuronal cholinergic system is expressed in human cytotrophoblast cells and in immune cells with homeostatic regulatory functions. Aim: The aim of this work was to evaluate whether non-neuronal acetylcholine conditions maternal monocyte and DC migration and activation profiles. Methods: We used an in vitro model resembling maternal-placental interface represented by the co-culture of human trophoblast cells (Swan-71 cell line) and monocytes or DC. Results: When cytotrophoblast cells were treated with neostigmine (Neo) to concentrate endogenous acetylcholine levels, monocyte migration was increased. In parallel, high levels of IL-10 and decreased levels of TNF-α were observed upon interaction of maternal monocytes with trophoblast cells. This effect was synergized by Neo and was prevented by atropine, a muscarinic acetylcholine receptor antagonist. Similarly, trophoblast cells increased the migration of DC independently of Neo treatment; however, enhanced IL-10 and MCP-1 synthesis in trophoblast-DC co-cultures with no changes in TNF-α and IL-6 was observed. In fact, there were no changes in HLA-DR, CD86 or CD83 expression. Finally, trophoblast cells treated with Neo increased the expression of two antigen-presenting cells attracting chemokines, MCP-1, MIP-1α and RANTES through muscarinic receptors, and it was prevented by atropine. Conclusions: Our present results support a novel role of acetylcholine synthesized by trophoblast cells to modulate antigen-presenting cell migration and activation favouring an immunosuppressant profile that contributes to immune homeostasis maintenance at the maternal-foetal interface. © 2015 Scandinavian Physiological Society. Published by John Wiley & Sons Ltd.  |l eng 
593 |a Departamento de Química Biológica, Facultad de Ciencias Exactas y Naturales, IQUIBICEN-CONICET, Universidad de Buenos Aires, Buenos Aires, Argentina 
593 |a Instituto de Medicina Experimental-IMEX-CONICET, Academia Nacional de Medicina, Buenos Aires, Argentina 
593 |a Servicio de Medicina Transfusional, Hospital Italiano de Buenos Aires, Buenos Aires, Argentina 
690 1 0 |a DENDRITIC CELLS 
690 1 0 |a MONOCYTES 
690 1 0 |a NON-NEURONAL ACETYLCHOLINE 
690 1 0 |a TROPHOBLAST CELLS 
690 1 0 |a ACETYLCHOLINE 
690 1 0 |a ATROPINE 
690 1 0 |a CD83 ANTIGEN 
690 1 0 |a CD86 ANTIGEN 
690 1 0 |a HLA DR ANTIGEN 
690 1 0 |a INTERLEUKIN 10 
690 1 0 |a INTERLEUKIN 6 
690 1 0 |a MACROPHAGE INFLAMMATORY PROTEIN 1ALPHA 
690 1 0 |a MONOCYTE CHEMOTACTIC PROTEIN 1 
690 1 0 |a MUSCARINIC RECEPTOR 
690 1 0 |a NEOSTIGMINE 
690 1 0 |a RANTES 
690 1 0 |a TUMOR NECROSIS FACTOR ALPHA 
690 1 0 |a ACETYLCHOLINE 
690 1 0 |a ANTIGEN PRESENTING CELL 
690 1 0 |a ARTICLE 
690 1 0 |a CELL INTERACTION 
690 1 0 |a COCULTURE 
690 1 0 |a CONTROLLED STUDY 
690 1 0 |a CYTOKINE PRODUCTION 
690 1 0 |a CYTOTROPHOBLAST 
690 1 0 |a DENDRITIC CELL 
690 1 0 |a FEMALE 
690 1 0 |a HUMAN 
690 1 0 |a HUMAN CELL 
690 1 0 |a IMMUNOMODULATION 
690 1 0 |a IN VITRO STUDY 
690 1 0 |a INFLAMMATION 
690 1 0 |a LEUKOCYTE ACTIVATION 
690 1 0 |a LEUKOCYTE MIGRATION 
690 1 0 |a MONOCYTE 
690 1 0 |a NIDATION 
690 1 0 |a PRIORITY JOURNAL 
690 1 0 |a PROTEIN EXPRESSION 
690 1 0 |a PROTEIN SYNTHESIS 
690 1 0 |a SWAN 71 CELL LINE 
690 1 0 |a TROPHOBLAST 
690 1 0 |a CELL SEPARATION 
690 1 0 |a CYTOLOGY 
690 1 0 |a IMMUNOLOGY 
690 1 0 |a INFLAMMATION 
690 1 0 |a METABOLISM 
690 1 0 |a NIDATION 
690 1 0 |a PREGNANCY 
690 1 0 |a PROCEDURES 
690 1 0 |a TROPHOBLAST 
690 1 0 |a ACETYLCHOLINE 
690 1 0 |a CELL SEPARATION 
690 1 0 |a COCULTURE TECHNIQUES 
690 1 0 |a EMBRYO IMPLANTATION 
690 1 0 |a FEMALE 
690 1 0 |a HUMANS 
690 1 0 |a INFLAMMATION 
690 1 0 |a PREGNANCY 
690 1 0 |a TROPHOBLASTS 
650 1 7 |2 spines  |a PLACENTA 
650 1 7 |2 spines  |a PLACENTA 
700 1 |a Gori, S. 
700 1 |a Grasso, E. 
700 1 |a Scordo, W. 
700 1 |a Calo, G. 
700 1 |a Pérez Leirós, C. 
700 1 |a Ramhorst, R. 
700 1 |a Salamone, G. 
773 0 |d Blackwell Publishing Ltd, 2015  |g v. 214  |h pp. 237-247  |k n. 2  |p Acta Physiol.  |x 17481708  |w (AR-BaUEN)CENRE-3545  |t Acta Physiologica 
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