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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
11

Efeito antidipsogênico e antinatriorexigênico da IL-1β injetada no núcleo pré-óptico mediano e no órgão subfornical

Cerqueira, Diana Rodrigues de January 2012 (has links)
Submitted by Ana Maria Fiscina Sampaio (fiscina@bahia.fiocruz.br) on 2013-04-19T16:45:21Z No. of bitstreams: 1 Diana Rodrigues de Cerqueira. Efeito antidipsogenico...pdf: 2541414 bytes, checksum: 91bafe7330198ea8c8a87c6c5f8f8fd6 (MD5) / Made available in DSpace on 2013-04-19T16:45:21Z (GMT). No. of bitstreams: 1 Diana Rodrigues de Cerqueira. Efeito antidipsogenico...pdf: 2541414 bytes, checksum: 91bafe7330198ea8c8a87c6c5f8f8fd6 (MD5) Previous issue date: 2012 / Universidade Federal da Bahia. Fundação Oswaldo Cruz. Centro de Pesquisas Gonçalo Moniz / Interleucina-1β (IL-1β) pode modular funções homeostáticas controladas pelo sistema nervoso central, incluindo a atividade do eixo hipotálamo-hipófise-adrenal, termorregulação, pressão arterial e comportamento ingestivo. Estudos anteriores do Laboratório de Neurociências mostram que IL-1β injetada no terceiro ventrículo cerebral inibe a ingestão de água em animais submetidos a diferentes protocolos e inibe o apetite por sódio em animais depletados deste íon. O núcleo pré-óptico mediano (MnPO) e o órgão subfornical (SFO) são áreas importantes no controle da homeostasia hidrossalina. Assim, a proposta deste estudo foi investigar o efeito de microinjeções de IL-1β no MnPO ou SFO sobre a ingestão de sal em animais depletados de sódio. Ratos Wistar (250-270g) foram anestesiados com cetamina/xilazina (80/7mg/kg) para cirurgia estereotáxica de implante de cânula guia no MnPO ou SFO. Quatro dias após a cirurgia os animais foram submetidos à depleção de sódio por injeções de furosemida (20 mg/kg, s.c) e mantidos com livre acesso a água destilada e dieta hipossódica. 24 horas após os animais receberam microinjeções de IL-1β, nas doses 1,6, 0,8 e 0,4 ng/rato. A ingestão de sal foi monitorada por 120 minutos e ao final das sessões experimentais, os animais foram anestesiados, submetidos à perfusão transcardíaca com salina 0,9% seguido de formol 10% e os encéfalos removidos para processamento histológico. Apenas os dados dos animais cuja cânula estava no MnPO ou SFO foram analisados. IL-1β injetada no MnPO e no SFO inibe a o apetite por sódio, em animais depletados deste íon, sendo o MnPO mais sensível a ação da IL-1β que o SFO. A ação da IL-1β no MnPO e no SFO no apetite por sódio foi específica e não associada a uma deficiência locomotora ou mal estar generalizado que impossibilitasse o animal a buscar da solução sacarina, uma vez que tanto a locomoção quanto a ingestão de sacarina 0,1% dos animais não foi alterada pela IL- 1β. Observou-se também aumento da temperatura corporal após tratamento com IL-1β, sendo a hipertermia mais expressiva após injeção no MnPO do que no SFO. Os resultados obtidos com este trabalho indicam que o MnPO é mais sensível a ação da IL-1β que o SFO e sugerem papel modulatório da IL-1β sobre a homeostasia hidrossalinana, mais especificamente, no apetite por sódio. / Interleukin-1β (IL-1β) may acts on the central nervous system integrating and modulating homeostatic functions including the activity of the hypothalamic-pituitary-adrenal axis, control of blood pressure and body temperature and ingestive behavior. Previous data from our laboratory showed that intracerebroventricular injection of IL-1β inhibits sodium appetite. However, the action of IL-1β in specific brain areas controlling this behavior is unknown. It is well documented that MnPO and SFO is an important brain sites involved in the control of water and salt intake. Therefore, the purpose of this study was to investigate the effect of IL- 1β microinjections into MnPO or SFO on salt intake in sodium-depleted rats. Wistar male rats (240-270g) were implanted with guide cannula in the MnPO or SFO under anesthesia with ketamine/xylazine (80/7 mg/kg i.p). The animals were submitted to sodium depletion by injection of furosemide (20 mg/kg, sc) and maintained with free access to distilled water and low sodium diet. Salt intake was monitored for 120 minutes after microinjection and at the end of the experiments the animals were anesthetized, submitted to a transcardiac perfusions with saline followed by 10% formalin and have their brain removed for histological procedure. Only data from animals whose guide cannulas were in the MnPO or SFO were considered. The results show that microinjection of IL-1β into MnPO and SFO inhibits the hypertonic saline intake throughout the experimental session. The inhibitory effect of IL-1β in MnPO on salt intake was more intense than SFO. Furthermore, the inhibition of sodium appetite seems not to be due to inhibition of locomotor activity or to any change in palatability, since microinjections of IL-1β in MnPO or SFO failed to modify the intake of a 0.1% saccharin solution when the animals were submitted to a "dessert test" or to induce any significant locomotor deficit in the open-field test. It was also observed a rise in body temperature after treatment with IL-1β and this hyperthermia was more significant after injection into MnPO than SFO. The results of this study indicate that the MnPO is more sensitive to IL-1β in MnPO than SFO and suggest modulatory role of IL-1β in this site on hydrosaline homeostasis especially in sodium appetite.
12

Efeito da metformina sobre IL-8 e IL-1b em um modelo de células estromais endometriais hiperinsulinêmicas e hiperandrogênicas in vitro

Machado, Amanda de Barros January 2013 (has links)
O endométrio é a mucosa que reveste o útero. A receptividade uterina é definida como um estado em que o endométrio se encontra receptivo à implantação do blastocisto. E, a preparação do endométrio para a implantação não é somente uma questão de estimulação hormonal adequada, depende da interação entre o blastocisto e o endométrio. Esta interação envolve uma complexa sequência de eventos de sinalização e uma variedade de moléculas. As concentrações de interleucina-8 (IL-8) e interleucina-1β (IL-1β) estão correlacionadas com o processo de implantação. Em humanos, a taxa de insucesso desse processo é alta e ocasionada por diversos fatores. A síndrome dos ovários policísticos (SOP) é um distúrbio endócrino-ginecológico que afeta de 6 a 8 % das mulheres em idade reprodutiva, e se caracteriza, principalmente, por anovulação crônica e hiperandrogenismo, estando diretamente relacionada à infertilidade feminina. Apesar da incerteza sobre a causa primária da SOP, há relatos sobre a importância da hiperinsulinemia na sua promoção. O objetivo deste trabalho foi estabelecer um modelo de hiperinsulinemia e hiperandrogenismo em células estromais endometriais in vitro, simulando características de SOP; identificar o melhor gene normalizador para estudos de expressão gênica em amostras das células em cultivo; avaliar o efeito da metformina sobre a proliferação celular e expressão gênica da IL-8 e IL-1β no modelo proposto. O tecido endometrial foi obtido de pacientes submetidas a histerectomia. A cultura primária das células estromais foi padronizada e as células foram divididas em sete grupos de tratamento: estradiol (G1); estradiol e progesterona (G2); estradiol, progesterona e insulina (G3); estradiol, progesterona e diidrotestosterona (G4); estradiol, progesterona e metformina (G5); estradiol, progesterona, insulina e diidrotestosterona (G6); estradiol, progesterona, insulina, diidrotestosterona e metformina (G7). Foi realizada análise de imunocitoquímica para vimentina para confirmação do cultivo com células estromais. Para avaliar a viabilidade e proliferação celular ao longo do tempo foi utilizado o ensaio de MTT em dois tempos diferentes de cultivo. As extrações de RNA foram realizadas e o cDNA obtido das amostras foi utilizado para a amplificação do mRNA de cinco genes candidatos a normalizadores e para avaliar a expressão dos genes da IL-8 e IL-1β através de PCR em tempo real.O estabelecimento da cultura de células estromais foi confirmado através da coloração positiva para a proteína vimentina. As células mantiveram-se viáveis durante todo o período de cultivo, apresentando aumento significativo na proliferação celular no tempo 8 em relação ao tempo 4 em todos os grupos. O grupo G7 (tratado durante 48 horas com metformina) apresentou uma menor taxa de proliferação em relação aos grupos G2, G3 e G6. Para análise de expressão gênica nestas células, o gene que mostrou os melhores parâmetros de estabilidade de expressão no modelo celular proposto foi o gene HPRT1. Observamos uma maior expressão do gene da IL-8 no grupo G5 tratado durante 48 horas em relação ao mesmo grupo tratado durante o período de 24 horas. Verificou-se maior expressão do gene da IL-1β no grupo G5 quando comparado a todos os outros grupos no período de 48 horas de tratamento com metformina. Entretanto, o grupo G7, também tratado com metformina, não apresentou diferença estatística em relação ao tempo de tratamento em nenhum dos genes estudados. Esses resultados demonstram que o modelo de hiperinsulinemia e hiperandrogenismo em cultura de células estromais endometriais é viável. Neste modelo, em que foram testados cinco genes em relação à sua estabilidade de expressão, o gene HPRT1 apresentou uma boa estabilidade, ao contrário de outros genes frequentemente utilizados como genes de referência. O tratamento com metformina apresentou um efeito antiproliferativo nas células do grupo hiperinsulinêmico e hiperandrogênico. No período de 48 horas aumentou a expressão do gene da IL-1β no grupo tratado somente com o medicamento. Sugerindo uma ação inibitória da insulina sobre a expressão dos genes da IL-8 e IL-1β no grupo hiperinsulinêmico e hiperandrogênico. Mais estudos são necessários para melhor entendimento do efeito da metformina nos fatores envolvidos durante a implantação. / The endometrium is the mucosa lining the uterus. The uterine receptivity is defined as a condition in which the endometrium is receptive to implantation of the blastocyst. The preparation of the endometrium for implantation is not only a matter of proper hormonal stimulation, it depends on the interaction between the blastocyst and the endometrium. This interaction involves a complex sequence of events and a variety of signaling molecules. The concentrations of interleukin-8 (IL-8) and interleukin-1β (IL-1β) are correlated to the implantation process. In humans, the failure rate of this process is high and caused by several factors. The polycystic ovary syndrome (PCOS) is an endocrine-gynecological disorder that affects from 6 to 8 % of women of reproductive age. It is characterized mainly by chronic anovulation and hyperandrogenism and directly related to female infertility. Despite the uncertainty about the primary cause of PCOS, there are reports about the importance of hyperinsulinemia in promoting it. The aim of this study was to establish a model of hyperinsulinemia and hyperandrogenism in endometrial stromal cells in vitro, simulating features of PCOS; to identify the best housekeeping gene for gene expression studies in the cultured cells; to evaluate the effects of metformin on cell proliferation, as well as IL-8 and IL-1β gene expression in the proposed culture model. The human endometrial tissue was obtained from patients undergoing hysterectomy. The primary culture of stromal cells was standardized and divided into seven treatment groups: estradiol (G1); estradiol and progesterone (G2); estradiol, progesterone and insulin (G3); estradiol, progesterone and dihydrotestosterone (G4); estradiol, progesterone and metformin (G5); estradiol, progesterone, insulin and dihydrotestosterone (G6); estradiol, progesterone, insulin, dihydrotestosterone and metformin (G7). Immunocytochemistry analysis for vimentin were performed. Cell viability and proliferation were evaluated by MTT assay at two days in different times of cultivation. RNA extractions were performed and the cDNA obtained from primary culture was used to amplify five candidates to housekeeping genes mRNA and to evaluate IL-8 and IL1β expression by real time PCR. The stromal culture cell establishment was confirmed by positive staining for vimentin. The cells remained viable throughout the cultivation period, with significant cell proliferation increase at day 8 compared to day 4 in all groups. The G7 group (metformin treated for 48 hours) showed lower proliferation rate than G2, G3 and G6 groups. For gene expression analysis in these cells, the gene showing the best parameters of stability of expression was HPRT1. Increased gene expression of IL-8 was observed in G5 group treated for 48 hours compared to the same group during 24 hours. Similarly, the G5 group showed higher IL-1β gene expression when compared to all other groups treated with metformin for 48 hours. However, the G7 group, also metformin treated, did not show statistically significant difference in treatment time of any studied genes. These results suggest that model of hyperinsulinemia and hyperandrogenism in endometrial stromal cells is viable and provides a good cell sampling to molecular analysis under different experimental conditions. In this model, several genes were tested for expression stability. HPRT1 presented the best values, unlike others classical housekeeping genes. The metformin treatment showed an antiproliferative effect on cells in hyperinsulinemic and hyperandrogenic group and at 48 hours increased IL-1β gene expression in the treated group with the drug alone. It suggests an inhibitory action of insulin on these genes expression in the hyperinsulinemic and hyperandrogenic group. More studies are needed to better understand the effect of metformin on the factors involved during implantation.
13

Efeito da metformina sobre IL-8 e IL-1b em um modelo de células estromais endometriais hiperinsulinêmicas e hiperandrogênicas in vitro

Machado, Amanda de Barros January 2013 (has links)
O endométrio é a mucosa que reveste o útero. A receptividade uterina é definida como um estado em que o endométrio se encontra receptivo à implantação do blastocisto. E, a preparação do endométrio para a implantação não é somente uma questão de estimulação hormonal adequada, depende da interação entre o blastocisto e o endométrio. Esta interação envolve uma complexa sequência de eventos de sinalização e uma variedade de moléculas. As concentrações de interleucina-8 (IL-8) e interleucina-1β (IL-1β) estão correlacionadas com o processo de implantação. Em humanos, a taxa de insucesso desse processo é alta e ocasionada por diversos fatores. A síndrome dos ovários policísticos (SOP) é um distúrbio endócrino-ginecológico que afeta de 6 a 8 % das mulheres em idade reprodutiva, e se caracteriza, principalmente, por anovulação crônica e hiperandrogenismo, estando diretamente relacionada à infertilidade feminina. Apesar da incerteza sobre a causa primária da SOP, há relatos sobre a importância da hiperinsulinemia na sua promoção. O objetivo deste trabalho foi estabelecer um modelo de hiperinsulinemia e hiperandrogenismo em células estromais endometriais in vitro, simulando características de SOP; identificar o melhor gene normalizador para estudos de expressão gênica em amostras das células em cultivo; avaliar o efeito da metformina sobre a proliferação celular e expressão gênica da IL-8 e IL-1β no modelo proposto. O tecido endometrial foi obtido de pacientes submetidas a histerectomia. A cultura primária das células estromais foi padronizada e as células foram divididas em sete grupos de tratamento: estradiol (G1); estradiol e progesterona (G2); estradiol, progesterona e insulina (G3); estradiol, progesterona e diidrotestosterona (G4); estradiol, progesterona e metformina (G5); estradiol, progesterona, insulina e diidrotestosterona (G6); estradiol, progesterona, insulina, diidrotestosterona e metformina (G7). Foi realizada análise de imunocitoquímica para vimentina para confirmação do cultivo com células estromais. Para avaliar a viabilidade e proliferação celular ao longo do tempo foi utilizado o ensaio de MTT em dois tempos diferentes de cultivo. As extrações de RNA foram realizadas e o cDNA obtido das amostras foi utilizado para a amplificação do mRNA de cinco genes candidatos a normalizadores e para avaliar a expressão dos genes da IL-8 e IL-1β através de PCR em tempo real.O estabelecimento da cultura de células estromais foi confirmado através da coloração positiva para a proteína vimentina. As células mantiveram-se viáveis durante todo o período de cultivo, apresentando aumento significativo na proliferação celular no tempo 8 em relação ao tempo 4 em todos os grupos. O grupo G7 (tratado durante 48 horas com metformina) apresentou uma menor taxa de proliferação em relação aos grupos G2, G3 e G6. Para análise de expressão gênica nestas células, o gene que mostrou os melhores parâmetros de estabilidade de expressão no modelo celular proposto foi o gene HPRT1. Observamos uma maior expressão do gene da IL-8 no grupo G5 tratado durante 48 horas em relação ao mesmo grupo tratado durante o período de 24 horas. Verificou-se maior expressão do gene da IL-1β no grupo G5 quando comparado a todos os outros grupos no período de 48 horas de tratamento com metformina. Entretanto, o grupo G7, também tratado com metformina, não apresentou diferença estatística em relação ao tempo de tratamento em nenhum dos genes estudados. Esses resultados demonstram que o modelo de hiperinsulinemia e hiperandrogenismo em cultura de células estromais endometriais é viável. Neste modelo, em que foram testados cinco genes em relação à sua estabilidade de expressão, o gene HPRT1 apresentou uma boa estabilidade, ao contrário de outros genes frequentemente utilizados como genes de referência. O tratamento com metformina apresentou um efeito antiproliferativo nas células do grupo hiperinsulinêmico e hiperandrogênico. No período de 48 horas aumentou a expressão do gene da IL-1β no grupo tratado somente com o medicamento. Sugerindo uma ação inibitória da insulina sobre a expressão dos genes da IL-8 e IL-1β no grupo hiperinsulinêmico e hiperandrogênico. Mais estudos são necessários para melhor entendimento do efeito da metformina nos fatores envolvidos durante a implantação. / The endometrium is the mucosa lining the uterus. The uterine receptivity is defined as a condition in which the endometrium is receptive to implantation of the blastocyst. The preparation of the endometrium for implantation is not only a matter of proper hormonal stimulation, it depends on the interaction between the blastocyst and the endometrium. This interaction involves a complex sequence of events and a variety of signaling molecules. The concentrations of interleukin-8 (IL-8) and interleukin-1β (IL-1β) are correlated to the implantation process. In humans, the failure rate of this process is high and caused by several factors. The polycystic ovary syndrome (PCOS) is an endocrine-gynecological disorder that affects from 6 to 8 % of women of reproductive age. It is characterized mainly by chronic anovulation and hyperandrogenism and directly related to female infertility. Despite the uncertainty about the primary cause of PCOS, there are reports about the importance of hyperinsulinemia in promoting it. The aim of this study was to establish a model of hyperinsulinemia and hyperandrogenism in endometrial stromal cells in vitro, simulating features of PCOS; to identify the best housekeeping gene for gene expression studies in the cultured cells; to evaluate the effects of metformin on cell proliferation, as well as IL-8 and IL-1β gene expression in the proposed culture model. The human endometrial tissue was obtained from patients undergoing hysterectomy. The primary culture of stromal cells was standardized and divided into seven treatment groups: estradiol (G1); estradiol and progesterone (G2); estradiol, progesterone and insulin (G3); estradiol, progesterone and dihydrotestosterone (G4); estradiol, progesterone and metformin (G5); estradiol, progesterone, insulin and dihydrotestosterone (G6); estradiol, progesterone, insulin, dihydrotestosterone and metformin (G7). Immunocytochemistry analysis for vimentin were performed. Cell viability and proliferation were evaluated by MTT assay at two days in different times of cultivation. RNA extractions were performed and the cDNA obtained from primary culture was used to amplify five candidates to housekeeping genes mRNA and to evaluate IL-8 and IL1β expression by real time PCR. The stromal culture cell establishment was confirmed by positive staining for vimentin. The cells remained viable throughout the cultivation period, with significant cell proliferation increase at day 8 compared to day 4 in all groups. The G7 group (metformin treated for 48 hours) showed lower proliferation rate than G2, G3 and G6 groups. For gene expression analysis in these cells, the gene showing the best parameters of stability of expression was HPRT1. Increased gene expression of IL-8 was observed in G5 group treated for 48 hours compared to the same group during 24 hours. Similarly, the G5 group showed higher IL-1β gene expression when compared to all other groups treated with metformin for 48 hours. However, the G7 group, also metformin treated, did not show statistically significant difference in treatment time of any studied genes. These results suggest that model of hyperinsulinemia and hyperandrogenism in endometrial stromal cells is viable and provides a good cell sampling to molecular analysis under different experimental conditions. In this model, several genes were tested for expression stability. HPRT1 presented the best values, unlike others classical housekeeping genes. The metformin treatment showed an antiproliferative effect on cells in hyperinsulinemic and hyperandrogenic group and at 48 hours increased IL-1β gene expression in the treated group with the drug alone. It suggests an inhibitory action of insulin on these genes expression in the hyperinsulinemic and hyperandrogenic group. More studies are needed to better understand the effect of metformin on the factors involved during implantation.
14

Evaluation of a Serine Hydrolase Inhibitor JZL184 as an Immunomodulator against Avian Pathogenic Escherichia Coli O78 in Chickens

Ho, Cherry Pei-Yee 04 May 2018 (has links)
Chickens in the poultry industry are reared under intensive conditions where they are often exposed to opportunistic pathogens. Escherichia coli strain O78 is responsible for about half of the cases of avian colisepticemia. Potential therapeutic treatments have been proposed to inhibit the hydrolases that controls the endogenous levels of the endocannabinoid, 2-arachidonoylglycerol (2-AG). 2-AG is the full agonist at the CB2 receptors of the endocannabinoid system expressed among leukocytes and it plays a role in mediating the activation of phagocytic macrophages. It is speculated that elevating 2- AG levels could increase macrophage cytokines and promote the recruitment of immune cells at the infected tissues. The purpose of this study was to investigate the immunomodulating effect of the 2-AG hydrolase inhibitor, JZL184 in chickens. The treatments could potentially up-regulate the innate immune responses in chickens during an E. coli infection by conveying a message from the endocannabinoid system to the immune system.
15

IL-1β Amplification of Nitric Oxide Production and Its Inhibitory Effects on Glucose Induced Early Growth Response-1 Expression in INS-1 Cells

Young, Ada 15 August 2012 (has links) (PDF)
The pathophysiology of cytokines released by infiltrating white blood cells upon pancreatic beta cells is not fully understood. Early growth response gene-1 (Egr-1) expression is specifically and transiently up regulated in pancreatic beta cells in response to glucose. We hypothesized that interleukin-1 beta (IL-1▀) induction of nitric oxide alters glucose induced Egr-1 transcription levels. Egr-1 levels were assessed via western blot, nitric oxide was measured with a Griess Reagent kit and insulin levels via ELISA. Glucose induced both insulin and Egr-1 production in INS-1 cells. IL-1▀ dose dependently increased nitric oxide production over time and significantly attenuated glucose induced Egr-1 expression. Sodium nitroprusside dose dependently reduced glucose induced Egr-1 production. The data suggest a strong relationship between IL-1▀ induced nitric oxide production and the reduction of glucose stimulated Egr-1 production. The pathways altered by this cytokine could provide a better understanding of the pathophysiology leading to pancreatic beta cell death.
16

Η ανταγωνιστική δράση του αναπτυξιακού παράγοντα μετασχηματισμού-β1 (TGF-β1) στην επαγόμενη από ιντερλευκίνη-1β (IL-1β) παράγωγη της μεταλλοπρωτεΐνασης-1 (MMP-1) από ινοβλάστες ανθρώπου, εξαρτάται από την προέλευση των ινοβλαστών και πραγματοποιείται μέσω ενεργοποίησης της πρωτεϊνικής κίνασης Α (PKA)

Γιαννακούλη, Μαρία 01 September 2009 (has links)
Σκοπός της παρούσας διατριβής ήταν η μελέτη των σηματοδοτικών μονοπατιών που εμπλέκονται στην επαγόμενη από IL-1β παραγωγή της MMP-1, μιας από τις κυριότερες μεταλλοπρωτεϊνάσες του εξωκυτταρικού χώρου, από ινοβλάστες ανθρώπου και η διερεύνηση του μηχανισμού της κατασταλτικής επίδρασης του TGF-β1 στην επαγόμενη από IL-1β παραγωγή της μεταλλοπρωτεϊνάσης αυτής. Η μελέτη πραγματοποιήθηκε σε ινοβλάστες αρθρικού υμένα ασθενών με οστεοαρθρίτιδα ή ρευματοειδή αρθρίτιδα, ρινικού πολύποδα και πνεύμονα. Βρέθηκε ότι η επαγωγική δράση της IL-1 πραγματοποιείται μέσω του μονοπατιού της PKC, ενώ σημαντικό ρόλο φαίνεται να παίζουν η ενεργοποίηση του NF-kB, αλλά και των μεταγραφικών παραγόντων της οικογένειας AP-1, μέσω των MAP κινασών. Το μονοπάτι, επίσης των κινασών τυροσίνης φαίνεται να συμμετέχει. Τα μονοπάτια αυτά φαίνεται ότι είναι κοινά στις ινοβλάστες, ανεξάρτητα από την προέλευση. Η δράση αυτή της IL-1β βρέθηκε ότι καταστέλλεται από το μονοπάτι cAMP/PKA στις ινοβλάστες αρθρικού υμένα και ρινικού πολύποδα όχι όμως και πνεύμονα. Ο TGF-β1 βρέθηκε ότι στις ινοβλάστες αρθρικού υμένα και ρινιού πολύποδα είχε κατασταλτική επίδραση στην επαγόμενη από IL-1β παραγωγή της MMP-1 ενώ σε αυτές από πνεύμονα είχε συνεργειακή. Η κατασταλτική δράση του TGF-β1 βρέθηκε ότι πραγματοποιείται μέσω ενεργοποίησης της PKA, κατά τρόπο ανεξάρτητο της παραγωγής cAMP. / The aim of present work was the study of signal tranduction pathways, which are implicated in IL-1β-induced production of MMP-1, one from the predominant metalloproteinases of extacellular matrix, from human fibroblasts, and the investigation of mechanism of suppressive effect of TGF-β1 on IL-1β-induced production of this metalloproteinases. The study was performed in fibroblasts with osteoarthrits or rheumatoid arthritis, nasal polyps and lung. It was found that the IL-1β-induced production of MMP-1 from fibroblasts, independently of their origin, is carried out via PKC pathway, while the activation of transcription factors NF-kB and AP-1, via MAP kinases, seems to play significant role. The tyrosine kinases pathway may also contributes. The IL-1β effect is suppressed from the cAMP/PKA pathway and nasal polyps fibroblasts but not in lung fibroblasts. TGF-β1 is able to antagonize the IL-1β-induced production of MMP-1 from synovial and nasal polyps fibroblasts, while in lung fibroblasts it exhibits synergistic effect. This suppressive effect of TGF-β1 is carried out via PKA activation, independently of cAMP production.
17

Immunisation active à base de peptides, dérivés de l’IL-6 et de l’IL-1β, dans les maladies inflammatoires chroniques / Peptide-based active immunization against IL-6 and IL-1β in chronic inflammatory diseases

Desallais, Lucille 13 May 2013 (has links)
Les anticorps monoclonaux anti-cytokine ont constitué une révolution dans le traitement des maladies inflammatoires chroniques, mais leur utilisation présente des inconvénients (non réponse, résistance, effets secondaires, coûts élevés).Notre équipe développe une stratégie alternative originale, l’immunisation active à base de peptides de cytokines. Elle a pour but de faire synthétiser, par l’organisme même du patient, des anticorps neutralisant les effets pathogènes dus à l’excès de cytokines.Durant ma thèse, j’ai montré que l’immunisation active contre un peptide dérivé de l’IL-6 murine est protectrice dans un modèle murin de sclérodermie systémique. L’immunisation de singes avec l’équivalent humain entraîne une réduction significative des réactions inflammatoires locales suite à l’induction d’une réaction d’HSR. De plus, l’immunisation active contre deux peptides dérivés de l’IL-1β et de l’IL-23 conduit à la réduction de la sévérité de l’EAE.Ces résultats confortent l’intérêt de cibler les cytokines par l’approche d’immunisation active à base de peptides, qui pourra permettre de diversifier l’offre thérapeutique actuellement disponible. / Monoclonal antibodies have been a revolution for the treatment of chronic inflammatory diseases, but their use shows major drawbacks (non-response, resistance, side effects and prohibitive costs).Our team develops an original alternative strategy: anti-cytokine peptide-based active immunization.The aim of the approach is to make the patient’s own organism produce antibodies capable of neutralizing the pathogenic effects of cytokine overproduction.During my PhD, I have demonstrated that active immunization against an IL-6 murine peptide confers clinical protection in a murine model of systemic sclerosis. Monkeys immunized against the human peptide also showed a significant decrease of local inflammatory reactions following a delayed-type hypersensitivity reaction. Moreover, active immunization against an IL-1β and an IL-23 murinepeptide led to a reduction of the severity of the EAE in mice.These results comfort the interest of anti-cytokine peptide-based active immunization, which should eventually widen the choice of therapeutics available for the patients.
18

Regulation of sinoatrial node and pacemaking mechanisms in health and disease

El Khoury, Nabil 12 1900 (has links)
Le noeud sinusal (NS) est le centre de l‟automatisme cardiaque. Grâce à son activité électrique spontanée, il dicte la fréquence cardiaque (FC) en réponse aux demandes physiologiques. A ce jour, le NS demeure un sujet de recherche important puisque les mécanismes moléculaires responsables de sa régulation sont encore méconnus. Par exemple, les processus menant à la bradycardie sinusale et à la maladie du sinus (MS) chez les personnes âgées sont mécompris et présentement l‟implantation d‟un stimulateur cardiaque demeure le seul traitement disponible. Ainsi, l‟objectif de cette thèse était de déterminer les changements moléculaires et cellulaires se produisant au niveau du NS en réponse à divers stimuli physiologiques et pathologiques afin d'établir leurs rôles potentiels dans la régulation de la FC et le développement de la MS. Dans les deux premiers chapitres, la grossesse est présentée comme modèle physiologique. En effet, la réponse adaptative aux demandes croissantes de la mère et du foetus engendre des changements physiologiques considérables au niveau du myocarde, dont une augmentation de la FC essentielle pour la perfusion adéquate des organes. Toutefois, cette augmentation peut aussi favoriser le développement d‟arythmies. Dans le troisième chapitre, l‟inflammation, un facteur présent lors du vieillissement et dans plusieurs pathologies où la MS se manifeste, a fait l‟objet d‟une étude dans le but de déterminer son rôle dans le développement de la MS. Les résultats obtenus dans cette thèse démontrent que la grossesse induit une hausse de la FC chez la souris gestante similaire à celle retrouvée chez la femme enceinte. Cette accélération était due à un remodelage électrique du NS. Plus spécifiquement, la fréquence des potentiels d‟action ainsi que la densité et l‟expression des courants pacemaker (If) et calcique de type L (ICaL) étaient augmentées. De plus, une accélération des transitoires calciques spontanés et de la vitesse de relâche calcique du réticulum sarcoplasmique a été observée. La régulation de l‟automaticité par un stimulus pathologique, l‟interleukine-1β, est abordée par la suite. L‟interleukine-1β, une cytokine ayant un rôle majeur comme médiateur inflammatoire, se retrouve en concentrations élevées dans plusieurs maladies associées avec la ii MS. Nos résultats démontrent que l‟interleukine-1β engendre une diminution de l‟automaticité associée à une réduction de If et ICaL dans les cardiomyocytes humains de type nodal dérivés de cellules souches induites pluripotentes (hiPSC-CM). En parallèle, le phénotype électrophysiologique et moléculaire des hiPSC-CM a été caractérisé démontrant leur homologie avec les cellules du NS humain adulte, les validant comme modèle in vitro de cellules nodales humaines. En conclusion, les études présentées dans cette thèse démontrent que le NS est plus qu‟un simple tissu régulé par l‟innervation autonome. En effet, son automaticité est dynamique et peut être influencée par des facteurs physiologiques ou pathologiques. Nos résultats contribuent ainsi à une meilleure compréhension des mécanismes sous-jacents à l‟automaticité. Ces avancées sont importantes non seulement pour la santé des femmes, mais aussi pour les individus souffrant de la MS. À terme, nous espérons que ces résultats contribueront au développement de stratégies thérapeutiques pour traiter des complications liées aux troubles d‟automaticité cardiaque. / The sinoatrial node (SAN) is the dominant cardiac pacemaker. With its spontaneous automaticity, it dictates rhythm and controls heart rate in response to varying physiological demands. Despite its modest size, the SAN is a very heterogeneous and complex structure that remains the topic of research efforts due, in part, to uncertainties in the mechanisms that regulate pacemaking in various conditions. For instance, the processes that lead to severe sinus bradycardia and SAN dysfunction (SND) in the elderly are unknown and to date, the implantation of electronic pacemaker remains the only SND treatment. Accordingly, the overall objective of this thesis was to explore and highlight the molecular and cellular changes that occur within the SAN in both physiological and pathological states, while determining how they contribute to regulation of heart rate and potentially SND. In the first two chapters, we present pregnancy as a physiological model considering it is a period during which substantial adaptive changes to the myocardium and increases in heart rate occur. Paradoxically, the rapid rate, which is essential for adequate organ perfusion of both mother and foetus, may also increase vulnerability to certain arrhythmias. In the third chapter, inflammation, a central process in pathology and common factor to several diseases and even ageing, was evaluated as potential underlying circumstance contributing to the development of sinus bradycardia and SND. Combinations of in vivo, ex vivo, biochemical, molecular and cellular approaches were used in order to generate an integrated understanding of the models we examined. Our data shows that in pregnant mice, an increase in heart rate similar to that of pregnant women occurs and was due to an electrical remodelling of the SAN. Specifically, an increase in action potential frequency of isolated individual SAN cells was observed. This was attributed to increased expression and density of pacemaker (If) and L-type Ca2+ currents (ICaL) along with a rapid spontaneous Ca2+ transient rate and faster intracellular sarcoplasmic reticulum Ca2+ release. We then demonstrate that the pro-inflammatory cytokine interleukin-1β which is a major inflammatory mediator that is upregulated in several diseases associated with SND, iv dramatically slows automaticity by reducing If and ICaL density in nodal-like cardiomyocytes derived from human-induced pluripotent stem cells (hiPSC-CM). Importantly, in that study, hiPSC-CMs were also physiologically and molecularly characterized revealing their high resemblance to adult human SAN and a potential use as a novel in vitro model to study pacemaking in humans. In conclusion, the results of this thesis demonstrate that the SAN is not a simple, neurally controlled tissue, but a rather dynamic pacemaker that undergoes extensive intrinsic remodelling during states of health and disease. The results contribute to understanding physiological mechanisms of pacemaking and how they are altered by disease and may be relevant for both women‟s health and the individuals affected by SND. Ultimately, we hope these findings will be helpful in the development of therapeutic strategies to treat pacemaking-related complications.
19

La Rapamycine inhibe l’expression de l’ARNm de l’ADAMTS-4 induit par les cytokines dans les chondrocytes articulaires

Khalifé, Sarah 02 1900 (has links)
Introduction: Durant la pathogenèse d’ostéoarthrose (OA), les cytokines pro-inflammatoires IL-1β (Interleukin-1 beta) et TNF-α (Tumor necrosis factor alpha) stimulent la dégradation des agrécanes par l’aggrécanase-1 ou ADAMTS-4 (a disintegrin and metalloproteinase with thrombospondin motif). Ces cytokines peuvent stimuler plusieurs voies de signalisation conduisant ainsi à l’augmentation de l’expression des ADAMTS dans les chondrocytes humains. Les TIMPs (tissue inhibitor of metalloproteinases) présentent des inhibiteurs endogènes de l’ADAMTS. Nous avons démontré que la Rapamycine (un immunosuppresseur et un inhibiteur du mamalian target of Rapamycin (mTOR)) peut avoir des effets bénéfiques dans cette pathologie. Notre étude examine l’effet de la Rapamycine sur l’expression de l’ADAMTS-4 induit par les cytokines, son implication dans certaines voies de signalisation, et son effet sur l’expression du TIMP-3. Méthodes: Des chondrocytes normaux sont traités avec la Rapamycine seule ou stimulés aussi avec l’IL-1β et le TNF-α. Les effets de la Rapamycine sur l’expression de l’ADAMTS-4 et du TIMP-3 ont été étudiés par l’analyse RT-PCR et l’activité enzymatique a été étudiée par la technique d’ELISA. Les effets de la Rapamycine sur certaines voies de signalisation ont été étudiés par le Western blot. Résultats: Nous avons trouvé que la Rapamycine inhibe l’expression de l’ARNm de l’ADAMTS-4 induit par les cytokines pro-inflammatoires dans les chondrocytes humains. L’activité enzymatique de l’ADAMTS-4 induit par l’IL-1β a été légèrement diminuée par la Rapamycine. En plus, cette dernière a montré de différents effets sur plusieurs voies de signalisation stimulées par l’IL-1β et le TNF-α telles que les voies des MAPKs (Mitogen activated protein kinase), de l’AKT, et de la p70 S6 kinase. La Rapamycine a inhibé partiellement l’activation de la phosphorylation de l’ERK1/2 MAPK (extracellular signal-regulated protein kinase MAPK) en présence du TNF-α seulement. En outre, la Rapamycine a inhibé la phosphorylation des protéines p38 MAPK, JNK (c-Jun N-terminal kinase), et AKT activée par l’IL-1β seulement. En plus, la phosphorylation de la protéine p70 S6K stimulée par l’IL-1β et le TNF-α a été inhibée par la Rapamycine. D’autre part, nous avons démontré que le niveau du TIMP-3 a été augmenté en présence de la Rapamycine. Conclusion: Ces résultats suggèrent que la Rapamycine peut bloquer l’action de l’ADAMTS-4 via l’inhibition de l’activation des MAPKs, de l’AKT, et de la p70 S6K. La Rapamycine pourrait ainsi être considérée pour la prévention de la perte du cartilage chez les patients ostéoarthritiques. / Introduction: During the pathogenesis of osteoarthritis, the pro-inflammatory cytokines IL-1β (Interleukin-1 beta) and TNF-α (Tumor necrosis factor alpha) stimulate the degradation of aggrecans by aggrecanase-1 or ADAMTS-4 (A disintegrin and metalloproteinase with thrombospondin motif). These cytokines may stimulate several signaling pathways leading to an increased expression of ADAMTS-4 in human chondrocytes. The TIMPs (tissue inhibitor of metalloproteinases) are endogens inhibitors of ADAMTS-4. It has been shown that Rapamycin (an immunosuppressor and an inhibitor of the mammalian target of rapamycin or mTOR) may have beneficial effects in this pathology. Our study investigates the impact of Rapamycin on cytokine-induced expression of ADAMTS-4, his implication in certain signaling pathways, and his effects on the expression of TIMP-3. Methods: Human chondrocytes were pretreated with different doses of Rapamycin either alone or stimulated with IL-β and TNF-α. The effect on ADAMTS-4 expression was examined by RT-PCR analysis and enzyme activity by ELISA. Impact of Rapamycin on the activation of different signaling pathways was measured by Western blot analysis. Results: We have shown that Rapamycin down-regulated pro-inflammatory cytokines-induced ADAMTS-4 mRNA expression in human chondrocytes. The IL-1β-induced-enzymatic activity of ADAMTS-4 was slightly inhibited by Rapamycin. Furthermore, Rapamycin present different effects on pro-inflammatory cytokines-stimulated activation of certain signaling pathways such as MAPKs (Mitogen activated protein kinases), AKT, and P70 S6 kinase. Moreover, Rapamycin partially inhibits TNF-α-induced activation of phosphorylation of ERK1/2 MAPK (extracellular signal-regulated protein kinase MAPK). Thus, Rapamycin inhibit IL-1β-induced activation of phosphorylation of the proteins p38 MAPK, JNK (c-Jun N-terminal kinase), and AKT. Also, Rapamycin inhibit IL-1β and TNF-α-activation of phosphorylation of the protein p70 S6 kinase. In other way, we have shown that the level of TIMP-3 has been increased in the presence of Rapamycin. Conclusion: These results suggest that Rapamycin down-regulates the expression of ADAMTS-4 by inhibiting the cytokine activation of MAPKs, AKT, and p70 S6 kinase. Thus Rapamycin could be considered as potential therapeutic agent for prevention of cartilage loss in patient with osteoarthritis.
20

La Rapamycine inhibe l’expression de l’ARNm de l’ADAMTS-4 induit par les cytokines dans les chondrocytes articulaires

Khalifé, Sarah 02 1900 (has links)
Introduction: Durant la pathogenèse d’ostéoarthrose (OA), les cytokines pro-inflammatoires IL-1β (Interleukin-1 beta) et TNF-α (Tumor necrosis factor alpha) stimulent la dégradation des agrécanes par l’aggrécanase-1 ou ADAMTS-4 (a disintegrin and metalloproteinase with thrombospondin motif). Ces cytokines peuvent stimuler plusieurs voies de signalisation conduisant ainsi à l’augmentation de l’expression des ADAMTS dans les chondrocytes humains. Les TIMPs (tissue inhibitor of metalloproteinases) présentent des inhibiteurs endogènes de l’ADAMTS. Nous avons démontré que la Rapamycine (un immunosuppresseur et un inhibiteur du mamalian target of Rapamycin (mTOR)) peut avoir des effets bénéfiques dans cette pathologie. Notre étude examine l’effet de la Rapamycine sur l’expression de l’ADAMTS-4 induit par les cytokines, son implication dans certaines voies de signalisation, et son effet sur l’expression du TIMP-3. Méthodes: Des chondrocytes normaux sont traités avec la Rapamycine seule ou stimulés aussi avec l’IL-1β et le TNF-α. Les effets de la Rapamycine sur l’expression de l’ADAMTS-4 et du TIMP-3 ont été étudiés par l’analyse RT-PCR et l’activité enzymatique a été étudiée par la technique d’ELISA. Les effets de la Rapamycine sur certaines voies de signalisation ont été étudiés par le Western blot. Résultats: Nous avons trouvé que la Rapamycine inhibe l’expression de l’ARNm de l’ADAMTS-4 induit par les cytokines pro-inflammatoires dans les chondrocytes humains. L’activité enzymatique de l’ADAMTS-4 induit par l’IL-1β a été légèrement diminuée par la Rapamycine. En plus, cette dernière a montré de différents effets sur plusieurs voies de signalisation stimulées par l’IL-1β et le TNF-α telles que les voies des MAPKs (Mitogen activated protein kinase), de l’AKT, et de la p70 S6 kinase. La Rapamycine a inhibé partiellement l’activation de la phosphorylation de l’ERK1/2 MAPK (extracellular signal-regulated protein kinase MAPK) en présence du TNF-α seulement. En outre, la Rapamycine a inhibé la phosphorylation des protéines p38 MAPK, JNK (c-Jun N-terminal kinase), et AKT activée par l’IL-1β seulement. En plus, la phosphorylation de la protéine p70 S6K stimulée par l’IL-1β et le TNF-α a été inhibée par la Rapamycine. D’autre part, nous avons démontré que le niveau du TIMP-3 a été augmenté en présence de la Rapamycine. Conclusion: Ces résultats suggèrent que la Rapamycine peut bloquer l’action de l’ADAMTS-4 via l’inhibition de l’activation des MAPKs, de l’AKT, et de la p70 S6K. La Rapamycine pourrait ainsi être considérée pour la prévention de la perte du cartilage chez les patients ostéoarthritiques. / Introduction: During the pathogenesis of osteoarthritis, the pro-inflammatory cytokines IL-1β (Interleukin-1 beta) and TNF-α (Tumor necrosis factor alpha) stimulate the degradation of aggrecans by aggrecanase-1 or ADAMTS-4 (A disintegrin and metalloproteinase with thrombospondin motif). These cytokines may stimulate several signaling pathways leading to an increased expression of ADAMTS-4 in human chondrocytes. The TIMPs (tissue inhibitor of metalloproteinases) are endogens inhibitors of ADAMTS-4. It has been shown that Rapamycin (an immunosuppressor and an inhibitor of the mammalian target of rapamycin or mTOR) may have beneficial effects in this pathology. Our study investigates the impact of Rapamycin on cytokine-induced expression of ADAMTS-4, his implication in certain signaling pathways, and his effects on the expression of TIMP-3. Methods: Human chondrocytes were pretreated with different doses of Rapamycin either alone or stimulated with IL-β and TNF-α. The effect on ADAMTS-4 expression was examined by RT-PCR analysis and enzyme activity by ELISA. Impact of Rapamycin on the activation of different signaling pathways was measured by Western blot analysis. Results: We have shown that Rapamycin down-regulated pro-inflammatory cytokines-induced ADAMTS-4 mRNA expression in human chondrocytes. The IL-1β-induced-enzymatic activity of ADAMTS-4 was slightly inhibited by Rapamycin. Furthermore, Rapamycin present different effects on pro-inflammatory cytokines-stimulated activation of certain signaling pathways such as MAPKs (Mitogen activated protein kinases), AKT, and P70 S6 kinase. Moreover, Rapamycin partially inhibits TNF-α-induced activation of phosphorylation of ERK1/2 MAPK (extracellular signal-regulated protein kinase MAPK). Thus, Rapamycin inhibit IL-1β-induced activation of phosphorylation of the proteins p38 MAPK, JNK (c-Jun N-terminal kinase), and AKT. Also, Rapamycin inhibit IL-1β and TNF-α-activation of phosphorylation of the protein p70 S6 kinase. In other way, we have shown that the level of TIMP-3 has been increased in the presence of Rapamycin. Conclusion: These results suggest that Rapamycin down-regulates the expression of ADAMTS-4 by inhibiting the cytokine activation of MAPKs, AKT, and p70 S6 kinase. Thus Rapamycin could be considered as potential therapeutic agent for prevention of cartilage loss in patient with osteoarthritis.

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