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181	Ação de prostaglandinas tópicas na conjuntiva de coelhos. Aguiar, Evian Valli January 2019 (has links) Orientador: Eliane Chaves Jorge / Resumo: A utilização prolongada de colírios análogos de prostaglandinas (AP) no tratamento do glaucoma tem sido associada a alterações tóxicas e inflamatórias dos tecidos oculares. As causas destes efeitos adversos locais ainda não são bem conhecidas. Uma das hipóteses aventadas seria o efeito citotóxico dos conservantes dos colírios e outra o envolvimento das metaloproteinases, cuja expressão estaria relacionada às alterações estruturais induzidas pelo uso crônico dos AP. Objetivo: O objetivo deste estudo foi avaliar a conjuntiva de coelhos submetidos à tratamento ocular tópico com AP e solução conservante por meio de estudo histológico, morfométrico e imuno-histoquímico. Material e Métodos: Quarenta coelhos adultos sadios da raça Norfolk, de ambos os sexos, com peso entre 1500 e 2500g, foram divididos por sorteio em quatro grupos experimentais. Os olhos direitos dos animais foram tratados com uma gota diária de bimatoprosta 0,03%, travoprosta 0,004%, latanoprosta 0,005%, e solução conservante por 30 dias (20 animais) e 60 dias (20 animais). Todos os coelhos foram submetidos à avaliação clínica oftalmológica com documentação fotográfica. Após a eutanásia, os olhos foram enucleados e preparados para análise histológica, morfométrica e imuno-histoquímica com pesquisa de expressão de metaloproteinase 2 (MMP2). Resultados: Houve aumento de espessura epitelial e estromal em todos os grupos tratados, principalmente no grupo latanoprosta com 30 dias e bimatoprosta com 60 dias (p<0,001). A ... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Prolonged use of prostaglandin (PA) analog drops in the treatment of glaucoma has been associated with toxic and inflammatory changes in ocular tissues. The causes of these local adverse effects are not yet well known. One of the hypotheses proposed would be the cytotoxic effect of the preservatives of the eye drops and another the involvement of the metalloproteinases, whose expression would be related to the structural alterations induced by the chronic use of PA. Objective: The objective of this study was to evaluate the conjunctiva of rabbits submitted to topical ocular treatment with PA and preservative solution by histological, morphometric and immunohistochemical study. Material and Methods: Forty healthy adult Norfolk rabbits, weighing between 1500 and 2500g, were divided by lot into four experimental groups. The right eyes of animals were treated with a daily drop of 0.03% bimatoprost, 0.04% travoprost, 0.005% latanoprost, and placebo preservative solution for 30 days (20 animals) and 60 days (20 animals). All rabbits were submitted to clinical ophthalmological evaluation with photographic documentation. After euthanasia, the eyes were enucleated and prepared for histological, morphometric and immunohistochemical analysis with metalloproteinase 2 (MMP2) expression research. Results: There was an increase in epithelial and stromal thickness in all treated groups, mainly in the 30 day latanoprost group and 60 day bimatoprost group (p <0.001). Histological analysis with... (Complete abstract click electronic access below) / Mestre Conjuntiva. Coelho. Inflamação. análogos de prostaglandinas metaloproteinase 2 Imuno-histoquímica. conjunctiva rabbits inflammation prostaglandin analogs metalloproteinase 2 immunohistochemistry
182	Estudos de efeitos de uma metaloproteinase de veneno ofídico em células de músculo liso vascular: produção de fatores que modulam a migração e proliferação destas células e mecanismos e / Studies on the effects of an ophidian venom metalloproteinase in vascular smooth muscle cells: production of factors that modulate cell migration and proliferation and mechanisms involved Viana, Mariana do Nascimento 04 December 2018 (has links) As metaloproteinases, abundantes em venenos de serpentes da família Viperidae, apresentam homologia estrutural e funcional com as metaloproteinases de mamíferos (MMPs), cujos níveis estão elevados em doenças de natureza inflamatória, como a aterosclerose. A metaloproteinase BaP1, do veneno da serpente Bothrops asper, apresenta potente atividade inflamatória e constitui ferramenta científica importante para o estudo das ações das MMPs. Durante a aterosclerose, as células de músculo liso vascular (CMLVs) mudam do fenótipo contrátil para sintético, migram para a camada subendotelial do vaso, liberam mediadores inflamatórios e expressam MMPs. No entanto, o papel destas enzimas na resposta inflamatória das CMLVs e a potencial relação deste efeito com a migração das mesmas, não foi esclarecida. Neste estudo, investigou-se os efeitos da BaP1 em CMLVs, quanto à 1) indução da migração; 2) liberação de diferentes classes de mediadores inflamatórios e expressão de moléculas de adesão; 3) indução da mudança fenotípica das CMLVs; 4) expressão e participação de enzimas de síntese de prostaglandinas e de receptores de PGE2 na liberação deste eicosanoide; 5) participação de eicosanoides e da IL-1&#946 na migração e mudança de fenótipo das CMLVs. Os resultados obtidos, a partir dos ensaios de transwell e wound healing, mostraram que a BaP1(50nM) induziu a migração das CMLVs, após 48 h, mas não a proliferação celular, observada pelo ensaio de ciclo celular. Além disso, a metaloproteinase induziu aumento da liberação de PGE2 (1-48h), LTB4 (1-3h), IL-1&#946 (12-24h), MCP-1 (24-48h) e fractalcina (24-48h), mas não de PGI2 e nem TXA2, analisados por ensaios de EIA e multiplex. Ainda, a BaP1 aumentou a expressão proteica de COX-2 (1° h) e de PGESm-1 (4° h), analisada por Western blotting, e expressão gênica das sFLA2-IIA (30 min) e cFLA2-IVA (30 min), verificada por PCR em tempo real, sem alterar os níveis de COX-1, dos receptores EP1, EP2, EP3 e EP4, de ICAM-1 e VCAM-1 e da iFLA2. A intervenção farmacológica com os inibidores de COX-2 ou de FLA2 intracelulares reduziu a liberação de PGE2 induzida pela BaP1. Além disso, o pré-tratamento das células com o inibidor da FLAP e com os antagonistas do receptor de IL-1&#946 ou do receptor EP3 reduziu a migração celular induzida pela BaP1. Esta metaloproteinase também induziu a mudança de fenótipo contrátil para o sintético, das CMLVs, verificada pela diminuição da expressão de &#945-actina pelo ensaio de citometria de fluxo. A inibição da COX-2 e da FLAP não alterou este efeito. Este conjunto de dados demonstra a capacidade da BaP1 estimular diretamente as CMLVs para migração, liberação de mediadores inflamatórios e a expressão de COX-2, PGESm-1, sFLA2-IIA e cFLA2-IVA. A produção de PGE2 induzida pela BaP1 depende das FLA2s intracelulares, com ativação das vias da COX-1 e -2. A migração das CMLVs, induzida pela BaP1, depende da PGE2 via ativação do receptor EP3, do LTB4 e da IL-1&#946. Ainda, esta metaloproteinase estimula a mudança fenotípica das CMLVs para o estágio sintético, em que as CMLVs migram e proliferam. Os dados deste estudo, ao demonstrarem que as metaloproteinases contribuem para o desenvolvimento de eventos inflamatórios, em CMLVs, apontam um papel adicional desta classe de enzimas em doenças de natureza inflamatória, como a aterosclerose. / Metalloproteinases are abundant enzymes in Viperidae family snake venoms and exhibit structural and functional homology with mammalian matrix metalloproteinases (MMPs). The levels of these enzymes are incresead in inflammatory diseases, such as atherosclerosis. The BaP1 metalloproteinase from Bothrops asper snake venom presents potent inflammatory activity and constitutes important scientific tool for the study of the actions of MMPs. During atherosclerosis, vascular smooth muscle cells (VSMCs) switch their phenotype from a contractile to a synthetic state, migrate into the subendothelial vessel layer, release inflammatory mediators and express high levels of MMPs. However, the role of these enzymes in the inflammatory response of VSMCs and the potential relationship of this effect with cell migration have not been clarified. In this study, we investigated the effects of BaP1 on CMLVs with focus on: 1) induction of cell migration; 2) release of different classes of inflammatory mediators and protein expression of adhesion molecules; 3) induction of VSMCs phenotype switching; 4) expression and participation of prostaglandin synthesis enzymes and PGE2 receptors in the release of this eicosanoid; 5) participation of eicosanoids and IL-1&#946 in migration and phenotype switching of VSMCs. Results obtained from the transwell and wound healing assays showed that BaP1 (50nM) induced VSMCs migration after 48 h, but not cell proliferation, observed by the cell cycle assay. In addition, this metalloproteinase caused release of PGE2 (1-48h), LTB4 (1-3h), IL-1 (12-24h), MCP-1 (24-48h) and fractalkine (24-48h), but not PGI2 and TXA2, analyzed by EIA and multiplex assays. Furthermore, BaP1 increased protein expression of COX-2 (1 h) and PGESm-1 (4 h), analyzed by western blotting and gene expression of sFLA2-IIA (30 min) and cFLA2-IVA (30 min), evaluated by real-time PCR, without altering COX-1, EP1, EP2, EP3 and EP4, ICAM-1 and VCAM-1 and iFLA2 levels. Pharmacological intervention with COX-2 or intracellular FLA2 inhibitors reduced PGE2 release induced by BaP1. In addition, pretreatment of cells with either a FLAP inhibitor, or IL-1&#946 receptor, or EP3 receptor antagonist reduced cell migration induced by BaP1. This metalloproteinase also induced conversion of contractile VSMCs to an synthetic phenotype, as evidenced by decrease of -actin expression, analyzed by flow cytometry assay. Inhibition of COX-2 and FLAP did not alter this effect. Altogether, these data demonstrate the ability of BaP1 to directly stimulate VSMCs for migration, release of inflammatory mediators and expression of COX-2, PGESm-1, sFLA2-IIA and cFLA2-IVA. PGE2 production induced by BaP1 depends on the intracellular FLA2s, with activation of COX-1 and -2 pathways. VSMCs migration induced by BaP1 depends on PGE2 via EP3 receptor engagement, LTB4 and IL-1&#946. Furthermore, this metalloproteinase stimulates VSMCs phenotypic switching to a synthetic phenotype, in which these cells migrate and proliferate. These data demonstrate that metalloproteinases can contribute to the development of inflammatory events in VSMCs, evidencing an additional role of this class of enzymes in inflammatory diseases, such as atherosclerosis. Célula de músculo liso vascular Inflamação Inflammation Metalloproteinase Metaloproteinase Migração Migration Prostaglandin E2 Prostaglandina E2 Vascular smooth muscle cells
183	Efeitos das isoflavonas da soja (Glycine max) na síntese de fatores vasoativos derivados de células endoteliais humanas da linhagem ECV304 / Effects of soy isoflavones (Glycine max) in the synthesis of vasoactive factors derived from human endothelial cells line ECV304. Paulo, Michele 03 April 2008 (has links) As mulheres na fase reprodutiva apresentam menor incidência de doenças cardiovasculares (DCV), em relação aos homens de mesma idade. Porém, essa vantagem desaparece na pós-menopausa, sugerindo que os hormônios sexuais femininos exercem algum efeito cardioprotetor. Um dos mecanismos propostos para explicar essa proteção é o fato dos estrógenos promoverem a produção de importantes fatores vasoativos pelo endotélio vascular, entre eles o óxido nítrico e a prostaglandina I2. Com a diminuição da quantidade de estrógenos circulante, as mulheres na pós-menopausa, estão mais suscetíveis à disfunção endotelial e a doenças cardiovasculares. Estudos têm demonstrado que a terapia de reposição hormonal (TRH) utilizada por mulheres na pós-menopausa combate os sintomas deste período, melhora o quadro de disfunção endotelial e o perfil lipídico e aumenta a síntese de fatores vasoativos, que auxiliam na prevenção da DCV. Entretanto a TRH vem sendo questionada por grandes estudos como o WHI (Writing Group for the Women\'s Health Initiative Investigators) e o HERS (Heart and Estrogen/Progestin Replacement Study), que mostraram um risco aumentado de desenvolvimento de câncer de mama e endometrial em mulheres fazendo uso da TRH. Entre as terapias alternativas para combater os sintomas indesejáveis da menopausa e as implicações mórbidas que acompanham esse período, sem expor as pacientes aos efeitos colaterais da TRH, a literatura aponta os fitoestrógenos, principalmente os extraídos da soja (Glycine max). O objetivo geral deste estudo é avaliar a ação das isoflavonas da soja, que vem sendo utilizadas por mulheres na pós-menopausa, na produção de óxido nítrico, prostaglandina E2 e endotelina-1, por células endoteliais, utilizando um modelo \"in vitro\", células endoteliais da linhagem ECV304. / During their reproductive years, women have a lower incidence of coronary heart disease (CHD) compared to men of similar age. However, this advantage disappears in post-menopause, suggesting that female sex hormones exert some cardio protective effect. One of the mechanisms proposed to explain this protection is the fact that estrogens promote the production of important vasoative factors by vascular endothelium, including nitric oxide and prostaglandin I2. By decreasing circulating estrogen, women in post-menopause are more susceptible of endothelial dysfunction and cardiovascular diseases. Studies have shown that the hormone replacement therapy (HRT) used by post-menopausal women in combating the symptoms of this period, improve endothelial dysfunction and lipid profile and increases the synthesis of vasoative factors, which help in the prevention of CHD. Meanwhile the HRT has been questioned by two large trials, the WHI (Writing Group for the Women\'s Health Initiative Investigators) and HERS (Heart and Estrogen/Progestin Replacement Study), which showed an increased risk of developing breast cancer and endometrial cancer in women using HRT. Among the alternative therapies to combat the symptoms of menopause and undesirable morbid implications that accompany this period, without exposing the patients to the side effects of HRT, the literature suggests the phytoestrogens, especially those from the soybean (Glycine max). The aim of this study is to evaluate the effect of isoflavones from soy, which are used by women in post-menopause, in the production of nitric oxide, prostaglandin E2 and endothelin-1 by endothelial cells, using an \"in vitro\" model: human endothelial cell line ECV304. Células endoteliais Endothelial cell Isoflavonas da soja Nitric oxide Óxido Nítrico Prostaglandin and Endothelin-1. Prostaglandina e Endotelina-1. Soy isoflavones
184	Efeito do exercício de força em diferentes intensidades com volume total similar sobre a dor muscular de início tardio, marcadores de lesão muscular e perfil endócrino. / The effect of different resistance exercise intensities with similar total volume upon delayed on set muscle soreness, muscle damage markers and hormonal profile. Uchida, Marco Carlos 23 June 2008 (has links) Este estudo compara quatro diferentes intensidades com o volume total similar no exercício supino. Avaliou-se a dor muscular de início tardio (DMIT), atividade de creatina quinase (CK), as concentrações sangüíneas de interleucina (IL)-1<font face=\"symbol\">b, IL-6, fator de necrose tumoral-<font face=\"symbol\">a (TNF-<font face=\"symbol\">a), prostaglandina E2 (PGE2) e o perfil hormonal. A amostra foi composta de soldados do exército brasileiro, divididos em cinco grupos: 50%-1RM, 75%-1RM, 90%-1RM, 110%-1RM e o controle. A DMIT e a atividade plasmática de CK aumentaram significativamente (P<0,05) após a sessão de exercício. A concentração de PGE2 também teve aumento significativo (P<0,05) após a sessão (P<0,05). A concentração plasmática de cortisol após 1h do término do exercício aumentou apenas no grupo 75%-1RM (p < 0,05). Esses resultados sugerem que a intensidade no exercício supino não afeta a magnitude da DMIT, marcadores de lesão muscular, inflamação e na resposta hormonal geral, desde que haja a equalização do volume total, com exceção da concentração plasmática do cortisol, grupo 75%-1RM. / This study compared four different intensities with similar total volume of a bench press exercise for muscle soreness, creatine kinase (CK) activity, interleukin (IL)-1<font face=\"symbol\">b, IL-6, tumor necrosis factor-<font face=\"symbol\">a (TNF-<font face=\"symbol\">a), prostaglandin E2 (PGE2) and hormonal concentrations in the blood. Brazilian Army male soldiers were placed into five groups: 50%-1RM, 75%-1RM, 90%-1RM, and 110%-1RM, and control that did not perform the exercise. Muscle soreness and plasma CK activity increased significantly (p<0.05) after exercise. Serum PGE2 concentration also increased significantly (p<0.05) after exercise. After one hour post exercise cortisol increased in 75%-1RM group, with this response also exceeding the other intensities (p<0.05). These results suggest that the intensity of bench press exercise does not affect the magnitude of muscle soreness and blood markers of muscle damage, inflammation and largely similar hormonal responses, which may be attributed to the equalization of total volume, exception made for the 75%-1RM group for serum cortisol concentration. Bench press Cortisol Cortisol Creatina quinase Creatine kinase DMIT DOMS Prostaglandin E2 Prostaglandina E2 Supino Total volume Volume total
185	Atividade antiluteolítica no microambiente uterino durante o período crítico para o estabelecimento da gestação em bovinos / Antiluteolytic activity in the uterine microenvironment during the critic period to pregnancy establishment in bovines Marques, Vanessa Belentani 14 December 2006 (has links) A inibição da secreção pulsátil de prostaglandina F2alfa (PGF2α) uterina (atividade antiluteolítica) pela ação do interferon-tau (IFN-τ) trofoblástico, mantêm a secreção de progesterona pelo corpo lúteo, fundamental ao estabelecimento da gestação nas fêmeas bovinas. Supõe-se que essa atividade antiluteolítica esteja presente no microambiente uterino bovino, portanto objetivou-se estudá-la. Dada à inexistência de ensaios que meçam especificamente a atividade antiluteolítica propôs-se elaborar um ensaio biológico para tal. Observou-se que células BEND tratadas com forbol 12,13 dibutirato (PdBu) por 6 horas em cultivo sintetizam PGF2α e tal síntese é inibida na presença de interferon-tau recombinante bovino (rbIFN-τ). Em outro estudo definiu-se que 25 ng/mL de PdBu promove estímulo consistente à síntese de PGF2α. A partir da análise de regressão do percentual de inibição à síntese de PGF2α estimulada por PdBu, em função da concentração de interferon-tau recombinante (rbIFN-τ), calculou-se a concentração de rbIFN-τ que inibiu em 50% a síntese máxima de PGF2α (observada na presença apenas de PdBu). Definiu-se a atividade antiluteolítica como o recíproco da concentração proteica requerida para atingir esse percentual de inibição (50%), e que a solução com uma unidade antiluteolítica é aquela que com um micrograma exerça tal efeito. Caracterizou-se a utilização dessa isoforma como padrão do ensaio antiluteolítico e calculou-se a atividade antiluteolítica do mesmo, 9,61 x 10² UA/µg de proteína. Em estudo seguinte observou-se a modulação da síntese de PGF2α estimulada por PdBu, em função da concentração proteica de um pool de lavados uterinos ou meios condicionados por conceptos obtidos no décimo sétimo dia de gestação. Notou-se que para cada fluido testado há um intervalo de concentrações onde observa-se aumento linear na atividade antiluteolítica em função do acréscimo proteico. A partir da análise por regressão linear desse evento calculou-se a atividade antiluteolítica de cada amostra. Para o pool de lavados uterinos calculou-se 1,63 x 10-¹ UA/ µg de proteína, e para o pool de meios condicionados por conceptos 1,66 x 10² UA/µg de proteína. Estes estudos permitiram desenvolver uma metodologia para observar a atividade antiluteolítica em humores biológicos. Aplicando o ensaio antiluteolítico estudou-se a atividade antiluteolítica presente em lavados uterinos obtidos durante o período crítico de fêmeas bovinas prenhes ou cíclicas ( respectivamente, 56,2 e 33,9 UA/µg de proteina), notou-se que a atividade antiluteolítica foi maior no microambiente uterino de fêmeas gestantes. Tal resultado associado à potente atividade antiluteolítica observada para os meios condicionados por conceptos indicam a participação do IFN-τ secretado pelo concepto na modulação da síntese de PGF2α. Entretanto, observou-se atividade antiluteolítica nos lavados uterinos obtidos de fêmeas cíclicas, o que indica que a síntese de PGF2α estimulada por PdBu pode ser modulada por outras proteínas, além do IFN-τ. Sugere-se que a atividade antiluteolítica, observada através do ensaio biológico proposto, é resultante da atuação de fatores estimulatórios e inibitórios presentes nos humores biológicos. Conclui-se que a atividade antiluteolítica pode ser mensurada pelo ensaio biológico proposto, no entanto outros estudos devem ser conduzidos para correlacionar essa atividade com a atuação do IFN-τ. / The inhibition of pulsatile secretion of PGF2α mediated by interferon-tau (IFN) is fundamental on the maternal recognition of pregnancy, maintaining the progesterone secretion by corpus luteum. Therefore the measurement of interferon activity in the uterine microenvironment was studied. Due to a lack of assays those measure specific antiluteolytic capacities we suggest develop a biological assay for it. In this research we observed that BEND cells treated with PdBu synthesize PGF2α, wich is inhibited by the presence of recombinant bovine interferon-tau (rbIFN-τ). Following we defined 25ng/mL as PdBu (phorbol 12,13 dibutirate) stimulus at the PGF2α synthesis to be applied in this biological assay. Studies about the modulation of PdBu-stimulated PGF2α synthesis by the rbIFN-τ validate the use of this isoform as a reference, defining a standard-curve and allowing estimating the antiluteolytic activity of 9.61 x 10² antiluteolytic units per microgram (UA/µg) of protein. Further, we observed the modulation of PdBu-stimulated PGF2α synthesis exerted by a pool of uterine flushings or conceptus conditioned medium, and for each tested fluid, there is a range of concentrations where is observed an increasing rate on the inhibition of PGF2α synthesis. A restrict analysis on this concentrations range shows a linear behavior and allow calculate the antiluteolytic activity of each sample1.63 x 10-¹ UA/ µg of protein from a pool of uterine flushings, and 1.66 x 10² UA/µg from conceptus conditioned medium. These studies validated a method to observe the antiluteolytic activity from biological fluids. Using the antiluteolytic assay, we studied the antiluteolytic activity present in uterine flushings obtained during the critic period by pregnant or cyclic bovine females cíclicas (respectively 56,2 e 33,9 UA/µg of protein). We observed higher antiluteolytic activity from pregnant uterine microenvironment than in cyclic uterine microenvironment. This result linked with the high antiluteolytic activity observed to conceptus conditioned medium, suggest the participation of IFN-τ secreted by the conceptus in the PGF2α synthesis modulation. However, we observed the antiluteolytic activity in uterine flushing obtained by cyclic cows, suggesting that the PGF2α synthesis could be modulated by another proteins. We believe that the antiluteolytic activity, observed by the antiluteolytic assay, ensue the action of inhibitors or stimulators factors in the biological fluids. We conclude that the antiluteolytic assay could be measured by the proposed biological assay, nevertheless another studies must be done in order to correlate this activity with the interferon action. biological assay bovines bovinos ensaio biológico interferons interferons pregnancy recognition prostaglandin F2&alpha prostaglandina F2&alpha reconhecimento da gestação
186	O PAF como regulador endógeno do fenótipo e função das células dendríticas. / PAF as an endogenous modulator of Dendritic Cells phenotype and function. Marianna Mainardi Koga 16 October 2015 (has links) Neste trabalho nós mostramos que células dendríticas (DCs) de camundongos BALB/c expressam receptor para o PAF (Fator ativador de Plaquetas) e que sua ativação promove um fenótipo tolerogênico, associado à produção de IL10 e PGE2. O bloqueio do PAF-receptor por antagonistas aumentou a capacidade das DCs induzirem proliferação de linfócitos T. O antagonista WEB2170 potencializou a resposta imune in vivo a concentração de anticorpo IgG2a OVA-específico aumentou 30 vezes no grupo tratado; a concentração de IgG1 foi semelhante nos dois grupos. O bloqueio do PAFR em camundongos imunizados com OVA em adjuvante completo de Freund, aumentou a produção de IgG1 e IgG2a OVA-específicos. Em camundongos imunizados com OVA/alum o antagonista não alterou a produção de IgG1. Estes resultados indicam que a ativação do PAFR em DCs modula a sua função apresentadora de antígenos pela produção de IL10 e PGE2. O bloqueio do PAFR pode ser útil na ativação das DCs em protocolos de vacinação com DCs e/ou como co-adjuvante em protocolos de imunização. / In the present work we show that BALB/c mice dendritic cells (DCs) express the PAF (platelet-activating factor) receptor and that its activation promotes a tolerogenic phenotype via IL10 and PGE2 production. Blocking PAFR by selective antagonists markedly enhanced DCs ability to induce T cell proliferation. The antagonist WEB2170 potentiated the in vivo immune response the IgG2a OVA-specific levels were 30 fold increased in the treated group; IgG1 concentration was similar for both groups. The PAFR blockade in mice immunized with OVA in complete Freunds adjuvant enhanced both IgG1 and IgG2a OVA-specific antibody production. In OVA/alum immunized mice, the antagonist did not change IgG1 production. These results suggest that PAFR activation in DCs modulates their antigen-presenting function through IL10 and PGE2 production. Blocking PAFR may be useful to induce DCs activation in DCs-based vaccination protocols and/or as a co-adjuvant in immunization protocols. Células dendríticas Imunização Interleucina 10 Prostaglandina E2 Receptor do PAF Dendritic cells Immunization Interleukin 10 PAF receptor Prostaglandin E2
187	Manipulação farmacológica do ciclo estral em vacas Nelore: I - Efeito de doses de PGF2α sobre a luteólise nos dias 5 e 7 do ciclo estral. II - Efeito da substituição do GNRH pelo BE nos protocolos de 5 dias de implante de P4 sobre o tempo de aparecimento e distribuição do estro, na taxa de ovulação e na taxa de prenhez / Pharmacological manipulation of the estrous cycle in Nellore cows: I - Effect of doses of PGF2α for luteolysis on days 5 and 7 of the estrous cycle. II - Effect of replacement of GNRH by EB, in the 5Co-Synch program, at estrus detection and distribution, at ovulation rate and pregnancy rate Marcos Vinicius de Castro Ferraz Junior 02 July 2013 (has links) O objetivo do experimento I foi avaliar a luteólise causada por três doses de PGF2α (12,5; 25 e 50 mg de Dinoprost tometamina) nos dias 5 e 7 do ciclo estral. Foram utilizadas 339 vacas não lactantes da raça Nelore. Os animais foram divididos em dois grupos de acordo com a apresentação do estro, recebendo a dose de PGF2α nos dias 5 e 7 do ciclo estral. Cada grupo foi subdividido em três, que receberam os seguintes tratamentos de PGF2α (12,5 mg; 25 mg; 50 mg). Através da concentração de P4 foram estimadas as taxas de regressão luteal 1 e 0,5 (1 - animais com concentração de P4 abaixo de 1 ng/mL; 0,5 animais com concentração de P4 abaixo de 0,5 ng/mL). Não houve interação entre a dose de PGF2α e o dia do ciclo estral. A aplicação de PGF2α no dia 7 do ciclo estral apresentou maior taxa de regressão luteal 1 e 0,5 quando comparada com o dia 5 do ciclo estral (1 - 76,9 vs 37,0 % - P = 0,0001; 0,5 - 57,5 vs 21,7 %, P = 0,0001, respectivamente). A taxa de regressão luteal 1 aumentou de acordo com a dose de PGF2α administrada (12,5 mg 39,0 %; 25 mg 56,9 %; 50 mg 76,5 % P <0,0001). Quando a PGF2α foi administrada no dia 5 do ciclo estral a concentração média de P4 segui o padrão de luteólise parcial e foi dependente da dose de PGF2α. Quando a PGF2α foi aplicada no dia 7 do ciclo estral a concentração média de P4 caiu drasticamente de 0 para 24 h e não voltou a se elevar em 48 h. A concentração de P4 em 48 h após a aplicação de PGF2α foi menor na dose de 50 mg (0,51 ± 0,07 ng/mL). A taxa de luteólise foi menor no dia 5 do ciclo estral comparado com o dia 7 do ciclo estral. À medida que a dose de PGF2α foi aumentada, a porcentagem de regressão luteal se elevou. O objetivo do experimento II foi avaliar se a substituição das aplicações do GnRH por BE, ECP e eCG no protocolos de 5 dias de P4 causa dupla ovulação e se a utilização de 1 ou 2 mg de BE no início do protocolo influencia na taxa de ovulação dupla. Foram utilizadas 85 multíparas da raça Nelore. No dia 0 do protocolo, as vacas receberam um implante de P4 e a dose de BE segundo o tratamento pertencente (tratamento A 1 mg de BE, tratamento B 2 mg de BE). Cinco dias após, o dispositivo foi retirado e aplicou-se PGF2α, ECP eCG. Houve 5,9 % de dupla ovulação. O tratamento A causou menor porcentagem folículos maiores que 8 mm no dia 7 protocolo que o tratamento B (28,7 vs 50,6 P = 0,0460). Não houve diferença significativa na taxa de ovulação dupla, no diâmetro do folículo dominante no dia 5 e no dia 7 do protocolo e na taxa de crescimento folicular entre os tratamentos A e B. O protocolo de 5 dias de P4 com BE, ECP e eCG causou uma baixa taxa de dupla ovulação. O objetivo do experimento III foi comparar o aparecimento e a frequência de estro e a taxas de ovulação e gestação entre os protocolos de 5 dias de P4 + GnRH / GnRH e de 7 dias de P4 + BE / ECP + eCG em nulíparas, primíparas e multíparas. Foram utilizadas 411 fêmeas da raça Nelore (nulíparas - n = 198; primíparas - n = 80; multíparas - n = 133). No protocolo de 7 dias de P4, os animais receberam no dia 0 um implante de P4 e BE. No dia 7, o dispositivo foi retirado e aplicou-se PGF2α, ECP e eCG. No protocolo de 5 dias de P4, os animais receberam no dia 0 o implante de P4 e GnRH. No dia 5, o dispositivo foi retirado e aplicaram-se 2 doses de PGF2α com intervalo de 6 h entre as doses de PGF2. Os animais que não apresentaram estro até a hora da IA receberam 100 μg de GnRH no momento da IA. A taxa de prenhez utilizando o protocolo de 5 ou 7 dias de P4 variou de acordo com a categoria da fêmea (nulíparas - 41,0 vs 51,0 % - P = 0.1608; primíparas 25,6 vs 31,7 % - P = 0,5513; multíparas - 58,4 vs 32,8 % - P = 0,0041, respectivamente). A taxa de apresentação de estro no protocolo de 7 dias de P4 foi maior para todas as categorias de fêmeas quando comparado com o protocolo de 5 dias deP4. (nulíparas 95,8 vs 66,0 % - P <0,0001; primíparas 48,7 vs 0 %; multíparas - 76,9 vs 13,4 % - P <0,0001, respectivamente). A resposta ao protocolo de 5 dias com GnRH foi pior nas multíparas. / The objective of the experiment I was to evaluate the luteolysis caused by three doses of PGF2α (12.5, 25 and 50 mg of Dinoprost tometamina) when applied on the 5th and 7th days of the estrous cycle. Three hundred thirty-nine (339) nonlactating Nelore cows were used. The animals were divided into two groups according to the onset of estrus, and received the PGF2α dose on the 5th or 7th day of the estrous cycle. Each group was divided into three subgroups, which were submitted to the treatments of PGF2α with dose of 12.5 mg, 25 mg or 50 mg. Through the P4 concentration, the rates of 1 and 0.5 luteal regression were estimated (1 - animals with P4 concentration below 1 ng/mL and 0.5 - animals with P4 concentration below 0.5 ng/mL). There was no interaction between the PGF2α dose and the day of the estrous cycle. The PGF2α application on the 7th day of the estrous cycle had higher rates of the 1 and 0.5 luteal regression, when compared to the PGF2α application on the 5th day of the estrous cycle (1 - 76.9 vs 37.0 % - P = 0.0001; 0,5 - 57.5 vs 21.7 %, P = 0.0001, respectively). The rate of 1 luteal regression increased with the PGF2α dose (12.5 mg - 39.0 %; 25 mg - 56.9 %; 50 mg - 76.5 %, P < 0.0001). The average concentrations of P4, when the PGF2α was administered on the 5th day of the estrous cycle, follow the partial luteolysis standard that dependent on the PGF2α dose. When the PGF2α is applied on 7th day of the estrous cycle, the average concentration of P4 drops dramatically from 0 to 24 h and it do not rise again in 48 h. The P4 concentration is lower in the 50 mg (0.51 ± 0.07 ng/mL), 48 h after the PGF2α application. The luteolysis rate was low on the 5th day of the estrous cycle. The luteal regression percentage increased with increase of the PGF2α dose. The objective of the experiment II was to evaluate whether the replacement of the GnRH applications by BE, ECP and eCG in the 5-day protocols of P4 cause double ovulation and if the use of 1 or 2 mg of BE at the beginning of the protocol influences the double ovulation rate. Eighty-five (85) multiparous Nelore cows were used. On day 0 of the protocol, the cows received a P4 implant and a dose of BE that depending on the treatment to which the cows belong (Treatment A - 1 mg of BE, treatment B - 2 mg of BE). Five days later, the device was removed and the PGF2α, ECP and eCG were applied. In the experiment II, there was 6.5 % of double ovulation. There was no significant difference in the double ovulation rate, dominant follicle diameter on the 5th and 7th day of the protocols, and follicular growth rate between the treatments A and B. The 5-day protocol of P4 with BE, eCG and ECP caused a low rate of the double ovulation, and there was no difference between 1 or 2 mg of BE to synchronize the follicular development wave. The objective of the experiment III was to compare the onset and frequency of estrus and the ovulation and pregnancy rates among the protocols of 5 days of P4 with GnRH and 7 days of P4 with BE, ECP and eCG in nulliparous, primiparous and multiparous. Four hundred eleven (411) Nellore females were used (nulliparous - n = 198; primiparous - n = 80; multiparous - n = 133). In 7-day protocol of P4, the animals received an implant of P4 and BE on day 0. On day 7, the device was removed and the PGF2α, ECP and eCG were applied in the cows. In 5-day protocol of P4, the animals received implants of GnRH and P4 on the day 0. On day 5, the device was removed and two doses of PGF2α were applied with interval of 6 h. The animals that did not show estrus until the AI time received 100 mg of GnRH at this moment. The pregnancy rate varied according to the female category in both protocols (nulliparous - 41.0 vs 51.0 % - P = 0.1608; primiparous - 25.6 vs 31.7 % - P = 0.5513; multiparous - 58.4 vs 32.8 % - P = 0.0041, respectively). The rate estrus onset in the 5-day protocol of P4 with GnRH was lower for all female categories, when compared to the 7-day protocol (nulliparous - 95.8 vs 66.0 % - P <0.0001; primiparous 0 vs 48.7 %; multiparous - 76.9 vs 13.4 % - P <0.0001, respectively). The response in the 5-day protocol with GnRH was worse in multiparous cows. Ovulação dupla Progesterona Prostaglandina F2&#945 Sincronização da ovulação Double ovulation Ovulation synchronization Progesterone Prostaglandin F2&#945
188	THE ROLE OF PRO-INFLAMMATORY MEDIATORS IFNβ AND PROSTAGLANDIN E2 IN SUPPRESSION OF INNATE IMMUNITY TO LISTERIA MONOCYTOGENES Pitts, Michelle G. 01 January 2018 (has links) As a foodborne pathogen, Listeria monocytogenes (Lm) encounters many barriers to invasion and dissemination in the host that may change the nature of host response. Lm has been most commonly studied using intravenous (i.v.) inoculation, however, a method that delivers a bolus of bacteria directly to the bloodstream. Thus, little is known about what systemic and local mediators are triggered during the natural course of infection and how these may impact susceptibility. Our laboratory used foodborne transmission of Lm in mice to assess whether the method of transmission and the specific organ microenvironment could affect infection-induced secretion of type I interferon or prostaglandin E2. Type I interferon is a pro-inflammatory effector secreted in response to viruses that has been proposed to paradoxically down-regulate innate immunity to intracellular bacteria. In contrast to i.v. infection, type I interferon was not detrimental to the immune response when Lm were acquired orally. In fact, most of the anti-inflammatory effects of type I interferon in the spleen were attributable to i.v. but not foodborne infection. Importantly however, downregulation of the receptor for interferon gamma (IFNGR1), previously ascribed to the type I interferon response, was found to be a consequence of infection and unrelated to type I interferon. In the liver, robust recruitment and activation of neutrophils (PMN) is thought to be required for initiation of Lm immunity. Prostaglandin E2 (PGE2) is a lipid mediator most commonly associated with pain and fever that has also been demonstrated to have anti-inflammatory or tolerogenic effects. It is unknown, however, whether foodborne infection induces PGE2 in the liver and if PGE2 then down-regulates PMN activities. Recruitment of PMN to the liver following foodborne infection was robust in both susceptible and resistant animals. Bone marrow PMN from each killed Lm ex vivo with similar efficiency, thus suggesting that if PMN were dysfunctional during the course of natural infection, they were responding to cues in the microenvironment. Accordingly, significantly more PGE2 was made ex vivo by cells from the livers of susceptible animals than from resistant animals. When PGE2 was applied to naïve PMN prior to exposure to Lm, it consistently dampened the killing efficiency of these cells, suggesting that this lipid better known for its pro-inflammatory roles might have anti-inflammatory effects during Lm infection. Overall, these studies indicate that mediators produced as a result of infection may have very different roles dependent on route of inoculation, timing, and the specific organ examined. innate immunity neutrophil prostaglandin E2 type I interferon Listeria monocytogenes Bacteria Bacterial Infections and Mycoses
189	INVESTIGATION OF THE BIOTRANSFORMATION OF 4-(METHYLNITROSAMINO)-1-(3-PYRIDYL)-1-BUTANONE BY PROSTAGLANDIN H SYNTHASE AND CYTOCHROME P450 2F Fikree, Hana M. 15 January 2008 (has links) The tobacco-specific nitrosamine 4-(methylnitrosamino)-1-(3-pyridyl)-1-butanone (NNK) is believed to play a role in human lung cancer induced by tobacco smoking. NNK biotransformation may involve the enzymes prostaglandin H synthase (PHS)-1, PHS-2 and cytochrome 450 (CYP) 2F. PHS activity is thought to be important in extrahepatic tissues, where CYP activity is low. The CYP2F subfamily contains a single functional enzyme in humans (CYP2F1) and goats (CYP2F3); these enzymes are preferentially expressed in the lung, with little or no expression in other organs. The role of these enzymes in the pulmonary biotransformation of NNK was investigated. 4.2 µM [5-3H]NNK was incubated with human lung microsomes under NADPH-dependent and arachidonic acid-dependent conditions. Metabolites reflective of NNK α-carbon hydroxylation, N-oxidation and carbonyl reduction were detected in the presence of NADPH, and metabolite levels for all three biotransformation pathways were lower in the presence of arachidonic acid compared with NADPH (p<0.05, N=4). Incubation of microsomes with the PHS-1 selective inhibitor SC-560 and the PHS-2 selective inhibitor NS-398 did not change NNK biotransformation either in the presence of NADPH or in the presence of arachidonic acid (p>0.05, N=4). Incubation of [5-3H]NNK with ovine PHS-1 or PHS-2 did not result in formation of α-carbon hydroxylation or N-oxidation metabolites; 4-(methylnitrosamino)-1-(3-pyridyl)-1-butanol (NNAL) was measurable only in the presence of PHS-2. Incubation of goat recombinant CYP2F3 with [5-3H]NNK resulted in formation of keto acid, keto alcohol and NNK-N-oxide (65.0%, 17.5% and 30.0% (µmol enzyme)-1 minute-1, respectively). Metabolite formation was inhibited by 3-methylindole (3-MI), a mechanism-based inactivator of CYP2F3. Based on an N value of 3, incubation of human lung microsomes with 3-MI inhibited N-oxidation (p<0.05) but did not alter NNK bioactivation or carbonyl reduction (p>0.05). However, when metabolite formation was examined in lung microsomes from different individuals, decreases in NNK biotransformation (ranging from 19.6 to 68.5%) were observed and were more pronounced in some patients than others, suggesting inter-individual variability in CYP2F1 activity. These studies demonstrate the ability of CYP2F to biotransform NNK and suggest inter-individual variability in the importance of CYP2F1 for this activity in human lung. They also strongly argue against the involvement of PHS enzymes. / Thesis (Master, Pharmacology & Toxicology) -- Queen's University, 2007-12-30 16:12:58.228 biotransformation pulmonary carcinogenesis prostaglandin H synthases cytochrome P450 human lung
190	Regulation of permeability of human brain microvessel endothelial cells by polyunsaturated fatty acids Dalvi, Siddhartha 04 July 2013 (has links) The blood-brain barrier, formed by brain microvessel endothelial cells, is the restrictive barrier between the brain parenchyma and the circulating blood. It was previously demonstrated in our laboratory that knock down of fatty acid transport proteins FATP-1 and CD36 attenuated apical to basolateral monounsaturated fatty acid transport across human brain microvessel endothelial cells (HBMEC). Arachidonic acid (AA; 5,8,11,14 - cis-eicosatetraenoic acid) is a conditionally essential, polyunsaturated fatty acid [20:4(n-6)] and a major constituent of brain lipids. We examined transport of AA across confluent monolayers of HBMEC. Control cells or HBMEC with knock down of FATP-1 or CD36 were cultured on Transwell® plates and incubated apically with [3H]AA and incorporation of [3H]AA into the basolateral medium was determined temporally. [3H]AA was rapidly incorporated into the basolateral medium with time in control cells. Surprisingly, knock down of FATP-1 or CD36 did not alter [3H]AA movement into the basolateral medium. The increased permeability mediated by AA was likely caused by a metabolite of AA produced de novo and was confirmed by an increased movement of fluorescent dextran from apical to basolateral medium. HBMECs expressed PGE2 synthase, cyclooxygenase-1 and -2, PGE2 receptors, tight junction proteins and prostaglandin transporters. The AA-mediated increase in membrane permeability was not attenuated by cyclooxygenase inhibitor drugs (NSAIDs). Incubation of the HBMEC monolayers with exogenous PGE2 resulted in attenuation of the AA-mediated permeability increases. The results indicate that AA increases the permeability of the HBMEC monolayer likely via increased production of metabolites or by-products of the lipoxygenase or epoxygenase pathways. These observations may explain the rapid influx of AA into the brain previously observed upon plasma infusion with AA. Blood brain barrier Arachidonic acid Polyunsaturated fatty acids Prostaglandin E2 Gene expression analysis

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