Global ETD Search

111	DIFFERENTIAL GENE EXPRESSION DURING ISCHEMIA AND REPERFUSION IN AN EXTRACORPOREAL SMALL BOWEL PERFUSION MODEL IN SWINE / Differentielle Genexpression während Ischämie und Reperfusion im Modell der extrakorporalen Dünndarmperfusion am Schwein Hosseini, Seyed Mehdi 30 October 2002 (has links) No description available. 570 Biowissenschaften, Biologie Mathematics and Computer Science Ischämie-Reperfusion Differential Display IL-6 IL-2 HSP70 IFN-Gamma E-Selektin ischemia-reperfusion differential display IL-6 IL-2 HSP70 IFN-gamma E-selectin W
112	Étude de nouveaux complexes impliquant l'IL-6 et CLCF1 Chehboun, Salma 11 1900 (has links) Plusieurs recherches s’adressent à étudier les nouvelles interactions qui peuvent avoir lieu entre les différentes sous-unités des cytokines ainsi que les récepteurs associés. L’objectif général de la thèse est d’étudier la formation de nouveaux complexes impliquant le récepteur soluble EBI3 et la cytokine CLCF1, déterminer leurs voies de signalisation et examiner l’impact de ces interactions sur l’induction de nouvelles fonctions biologiques. EBI3 est un récepteur soluble qui participe à la formation de trois cytokines composites: IL-27 (EBI3/p28), IL-35 (EBI3/p35) et IL-39 (EBI3/p19). Celles-ci appartiennent à la famille IL-12 des cytokines. L’IL-27 est une cytokine pléiotropique qui exerce à la fois des fonctions pro-inflammatoires qui se caractérisent principalement par la différenciation des cellules Th1 et des fonctions anti-inflammatoires associées à l’inhibition de la différenciation des cellules Th17 et à la production du GM-CSF. L’IL-35 est une cytokine connue pour induire des effets immunosuppresseurs tandis que l’IL-39 a été récemment identifiée pour induire l’inflammation chez les souris atteintes du lupus. Étant donné que l’EBI3 ne forme pas des complexes covalents avec les sous-unités p28, p35 et p19, nous avons voulu savoir si les effets d’EBI3 pourraient passer par la formation d’un composé différent des cytokines IL-27, IL-35 et IL-39. Nous avons démontré que l’EBI3 induit une trans-signalisation en formant un complexe alternatif avec l’IL-6. Des effets similaires de type pro-inflammatoire ont été observés avec les complexes IL-6/sIL-6Rα et EBI3/IL-6. En effet, les deux cytokines activent la chaîne gp130, induisent la phosphorylation de STAT3 et augmentent l’expression des chemiokines par les cellules endothéliales humaines. CLCF1 appartient à la famille IL-6 des cytokines monomériques. L’efficacité de la sécrétion du CLCF1 augmente en présence du CLF, un récepteur soluble aux cytokines. Des mutations dans les gènes codant pour CLCF1 ou CLF induisent le syndrome de la transpiration induite par le froid appelé "Crisponi" ou "CISS". La liaison entre le CNTF, une cytokine qui peut avoir des effets protecteurs semblables au CLCF1 au niveau du système nerveux central, et l’apolipoprotéine E a été observée in vitro (1). Nous avons émis l’hypothèse que CLCF1 pourrait également former un complexe avec l’apoE. Nous avons démontré que CLCF1 se lie avec les différentes isoformes d’apoE, à savoir, apoE2, apoE3 et apoE4. L’apoE est une protéine impliquée dans le transport des lipides et qui se trouve principalement à la surface des chylomicrons, VLDL et une fraction des HDL. Nous avons observé que CLCF1 interagit avec les lipoprotéines en présence et absence d’apoE. L’impact de la liaison du CLCF1 avec l’apoE ou avec les lipoprotéines a été examiné sur les cellules qui expriment la chaîne CNTFRα. / Several researches aimed to study new interactions that take place between the different subunits of cytokines and related receptors. The general goal of this thesis is to study the formation of new complexes involving the soluble receptor EBI3 and the cytokine CLCF1, determine their signaling pathways, and examine the impact of these interactions on the induction of new biological functions. EBI3 is a soluble receptor participating in the formation of three composite cytokines: IL-27 (EBI3/p28), IL-35 (EBI3/p35), and IL-39 (EBI3/p19). These cytokines belong to the IL-12 family. IL-27 is a pleiotropic cytokine that exerts both pro-inflammatory functions characterized by the differentiation of Th1 cells, and anti-inflammatory functions associated with the inhibition of Th17 cells differentiation and the production of GM-CSF. IL-35 is known to induce an immunosuppressive effects while IL-39 has recently been identified to induce inflammation in mice with lupus. Since EBI3 doesn’t form a covalent complexes with p28, p35 and p19 subunits, we wanted to know if the effects of EBI3 could go through the formation of a different compound than that of IL-27, IL-35 and IL-39. We have shown that EBI3 induces a trans-signaling pathway by forming a complex with IL-6. Both IL-6/sIL-6Rα and EBI3/IL-6 complexes share similar pro-inflammatory effects. Indeed, both cytokines activate gp130 chain, induce phosphorylation of STAT3, and increase the expression of chemiokines by human endothelial cells. CLCF1 belongs to the IL-6 family of monomeric cytokines. CLCF1 is efficiently secreted in the presence of CLF, a soluble cytokine receptor. Mutations in the genes coding for CLCF1 or CLF cause the cold-induced sweating syndrome also called "Crisponi" or "CISS". The interaction between CNTF, a cytokine which may have similar protective effects as CLCF1 at the central nervous system, and apolipoprotein E was observed in vitro (1). We hypothesized that CLCF1 could also form a complex with apoE. We demonstrated that CLCF1 binds with different apoE isoforms, namely, apoE2, apoE3, and apoE4. ApoE is a protein involved in lipid transport and is located primarily on the surface of chylomicrons, VLDL, and a fraction of HDL. We observed that CLCF1 interacts with lipoproteins in the presence and absence of apoE. The impact of CLCF1 interaction with apoE or lipoproteins was examined on cells expressing the chain CNTFRα. EBI3 IL-6 IL-6Rα soluble Trans-signalisation Inflammation Cellules endothéliales ApoE CLCF1 Lipoprotéines EBI3 IL-6 soluble IL-6Rα Trans-signaling Inflammation Endothelial cells ApoE CLCF1 Lipoproteins
113	La voie ERK1/2 : point d’intégration et de convergence des connexions entre voies de signalisation dans les cellules épithéliales de prostate normale / ERK1/2 pathway : an integrating node of converging signaling pathways in normal prostate epithelial cells. Poncet, Nadège 14 December 2010 (has links) Le développement et l’homéostasie cellulaire de la prostate impliquent le contrôle strict des voies de signalisation induites par les androgènes et les facteurs de croissance. Ces diverses voies sont profondément altérées dans le cancer de la prostate, notamment lors des stades les plus avancés. Dans ce travail, une lignée immortalisée à partir de l’épithélium de prostate humaine, la lignée RWPE-1, a été utilisée pour étudier certains signaux régulant la prolifération cellulaire, ainsi que les connexions entre les voies de signalisation correspondantes. La prolifération des cellules RWPE-1 est sous la dépendance de l’EGF (Epidermal Growth Factor) qui intervient physiologiquement dans le développement épithélial. Les récepteurs apparentés à l’EGF-R sont également impliqués dans la prolifération au cours de la progression tumorale. La prolifération des cellules RWPE-1 en réponse à l’EGF est strictement dépendante de la voie ERK1/2, qui est donc considérée comme un point d’intégration des signaux. L’utilisation d’inhibiteurs du récepteur aux androgènes a permis de montrer le rôle essentiel qu’il joue dans l’activation d’ERK1/2 en réponse à l’EGF. Le récepteur aux androgènes s’associe avec plusieurs molécules de signalisation dans les cellules RWPE-1. Je démontre ici pour la première fois une association entre le récepteur aux androgènes et la kinase Raf-1, activatrice de la voie ERK1/2. Ainsi, le récepteur aux androgènes contrôlerait directement un processus essentiel à la prolifération épithéliale selon un mode d’action non-génomique. Par ailleurs, j’ai montré que la réponse proliférative des cellules RWPE-1 à l’IL-6 requiert l’activation de la voie ERK1/2, et l’activité kinase de l’EGF-R, suggérant la transactivation de ce récepteur par l’IL-6. L’utilisation de divers inhibiteurs chimiques a permis de démontrer que les métalloprotéases de la famille ADAM (a disintegrin and metalloprotease), notamment ADAM17, sont impliquées dans ce processus. Ainsi, l’activation de protéines ADAM par l’IL-6 conduirait au clivage d’un ligand membranaire de l’EGF-R, aboutissant à l’activation de la voie ERK1/2. Ce nouveau mécanisme pourrait être impliqué dans les situations inflammatoires conduisant à une prolifération excessive de l’épithélium prostatique, prélude à la transformation tumorale. En conclusion, les voies de signalisation étudiées sont fortement connectées dans les cellules épithéliales normales. Les deux nouveaux mécanismes décrits ici aboutissent à l’activation des kinases ERK1/2, point d’intégration et de convergence des voies de signalisation dans les cellules épithéliales de prostate normale. / Prostate development and cell homeostasis involve strict control of androgen and growth factors induced signaling pathways. These signaling pathways are deeply altered in prostate cancer, especially during late stages. In this work, the RWPE-1 immortalized cell line derived from human prostate epithelium has been used to study the signaling pathways regulating cell proliferation and their crosstalk. Optimal RWPE-1 proliferation is dependent on EGF (Epidermal Growth Factor), that also controls normal epithelial development. EGF-R family is also involved in cancer cell proliferation. EGF-dependent RWPE- 1 cell proliferation relies strictly on the ERK1/2 pathway which is then seen as a signal integrating node. Specific inhibitors showed essential role of androgen receptor in EGF mediated ERK1/2 activation. Androgen receptor is associated with several signaling molecules in RWPE-1 cells. I show here for the first time the physical interaction between the androgen receptor and the ERK1/2 activating kinase Raf1. Then, the androgen receptor could directly regulate an essential pathway for epithelial cells proliferation through a non-genomic mechanism. In addition, I showed that IL-6 dependent RWPE-1 cells proliferation requires both ERK1/2 and EGF-R kinase activities, suggesting an IL-6 mediated transactivation of EGF-R. By using several inhibitors, I showed that ADAM (a disintegrin and metalloprotease) family metaloproteases, especialy ADAM17, are involved in this process. IL-6-mediated ADAM proteins activation could lead to the cleavage of a membrane bound EGF-R ligand, leading to ERK1/2 pathway activation. This new mechanism could be involved in the inflammatory situations inducing hyperproliferation of the prostate epithelium, the first step of the transformation process. To conclude, the signaling pathways I studied are strongly connected in normal epithelial cells. The two new mechanisms described in this study lead to ERK1/2 kinases activation, an integrating node of signaling pathways in normal prostate epithelial cells. Prostate Cellules épithéliales normales Prolifération Voie ERK1/2 Récepteur aux androgènes Signalisation non-génomique IL-6 Récepteur à l’EGF Transactivation Prostate Normal epithelial cells Proliferation ERK1/2 pathway Androgen receptor Non-genomic signaling IL-6 EGF receptor Transactivation 572.8
114	Análise da biomodulação da inflamação após lesão criogênica no sistema nervoso central em ratos submetidos à fototerapia com laser em baixa intensidade / Analysis of biomodulation of inflammation after cryogenic injury in the central nervous system in rats subjected to phototherapy with low-intensity laser Moreira, Maria Stella Nunes Araujo 24 March 2010 (has links) Este estudo teve por finalidade estudar os efeitos da fototerapia com laser em baixa intensidade (Low Level Laser Therapy LLLT) sobre a inflamação e reparação após lesão criogênica realizada no sitema nervoso central (SNC) de ratos. Foram realizados 3 experimentos. Em todos os experimentos foi utilizado um modelo de deformação cortical direta induzida por lesão criogênica. A LLLT foi realizada com laser de diodo em baixa intensidade emitindo no vermelho visível (InGaAlP, 660 nm) ou no infravermelho (AlGaAr, 780 nm). Os parâmetros de irradiação foram: potência de 40 mW, área do feixe de 0,04 cm2, densidades de energia de 3 J/cm2 (3 s) ou 5 J/cm2 (5 s) determinando energias por ponto de 0,12 J e 0,20 J, respectivamente. Foram realizadas 2 irradiações com intervalo de 3 h, no modo contato e em 2 pontos por lesão. No experimento 1, 50 ratos da linhagem Wistar foram utilizados para determinar os parâmetros de LLLT capazes de influenciar na dinâmica da produção de citocinas proinflamatórias (TNF-a, IL-1b, IL-6) e antiinflamatória (IL-10). As citocinas foram mensuradas pelo teste ELISA no cérebro e no sangue dos animais, 6 e 24h após a lesão. Os grupos experimentais foram: controle (não irradiado) e 4 grupos irradiados com 3 J/cm2 ou 5 J/cm2 para cada comprimento de onda (n=10 por grupo). Para os experimentos 2 e 3 foram utilizados 40 ratos (20 não irradiados controles e 20 irradiados). A LLLT foi realizada somente com o parâmetro de irradiação do laser no infravermelho e a densidade de energia de 3 J/cm2. Nestes experimentos o processo de reparação das lesões criogênicas no SNC foi acompanhado em 6 h, 1, 7 e 14 dias após a última irradiação (n=5 por grupo por tempo experimental). No experimento 2 foi realizada a análise morfométrica da região lesionada do SNC. No experimento 3 foi analisada a distribuição das células inflamatórias (linfócitos T, leucócitos e macrófagos). Os dados de cada experimento foram comparados estatísticamente por análise de variância (ANOVA) ou Kruskal-Wallis seguido dos testes de Tukey ou de Dunn, respectivamente (F=5%). O trauma criogênico foi capaz de criar lesões focais no córtex representadas por necrose, edema, hemorragia e infiltrado inflamatório. Os achados mais marcantes foram: no experimento 1 com a irradiação do laser no infravermelho e 3 J/ cm2, o TNF- a e a IL-6 se mantiveram nos mesmos níveis em 6 e 24 h, enquanto no controle houve aumento significativo. Experimento 2: as lesões não tratadas apresentaram maior perda tecidual em 6 h que as irradiadas. Experimento 3: as lesões irradiadas apresentaram menor quantidade de leucócitos e linfócitos T nas primeiras 24 h do que nas lesões controle. A quantidade de macrófagos foi similar nos dois grupos. Conclusões: Levando em consideração as condições experimentais deste estudo concluiu-se que LLLT exerce efeitos nos processos de inflamação e reparação diminuindo a concentração de citocinas próinflamatórias (TNF-F e IL-6) no sangue e mantendo a de IL-1I no cérebro. Adicionalmente, diminui a perda tecidual inicial pós- lesão criogênica e a infiltração inicial de leucócitos e linfócitos T. / This study aimed to study the effects of phototherapy with low-intensity laser (Low Level Laser Therapy - LLLT) on inflammation and repair after cryogenic injury held in central nervous system (CNS) of rats. There were 3 experiments. In all experiments a model of deformation induced by direct cortical cryogenic injury was used. The LLLT was carried out with a low intensity diode laser emitting in the visible red (InGaAlP, 660 nm) or infrared (AlGaAs, 780 nm). The irradiation parameters were: power of 40 mW, beam area of 0.04 cm2, energy densities of 3 J/cm2 (3 s) or 5 J/cm2 (5 s) providing energy per point of 0.12 J and 0.20 J, respectively. Two irradiations were performed at 3 h-intervals, in contact mode and in 2 points for lesion. In experiment 1, 50 Wistar rats were used to determine the parameters of LLLT able to influence the dynamics of production proinflammatory cytokines (TNF-, IL-1 and IL-6) and antiinflammatory cytokine (IL- 10). Cytokines were measured by ELISA in the brain and blood of animals, 6 and 24 hours after injury. The experimental groups were: control (non-irradiated) and 4 irradiated groups [3 J/cm2 and 5 J/cm2 for each wavelength (n = 10 per group)]. For experiments 2 and 3 40 rats (20 non-irradiated - controls and 20 irradiated).were used. The LLLT was performed only with the parameter of laser irradiation on the infrared and the energy density of 3 J/cm2. In these experiments, the process of repair of cryogenic injury in the CNS was followed in 6 h, 1, 7 and 14 days after the last irradiation (n = 5 per group and time trial). In experiment 2 a morphometric analysis of the injured area of the CNS was done. In experiment 3 the distribution of inflammatory cells (lymphocytes, leukocytes and macrophages) was analyzed. Data from each experiment were compared statistically by analysis of variance (ANOVA) or Kruskal-Wallis followed by tests of Tukey or Dunn, respectively ( = 5%). Cryogenic trauma was able to create focal lesions in the cortex represented by necrosis, edema, hemorrhage and inflammatory infiltrate. The most striking findings were: in experiment 1 with the laser irradiation in the infrared and 3 J/cm 2, TNF- and IL-6 remained at the same levels at 6 and 24 h, while in the control there was a significant increase. Experiment 2: untreated lesions showed greater tissue loss than irradiated lesions in 6 h. Experiment 3: lesions irradiated had fewer leukocytes and lymphocytes in the first 24 h than control lesions. The amount of macrophages was similar in both groups. Conclusions: Considering the experimental conditions of this study it was concluded that LLLT has effects in the processes of inflammation and repair by decreasing the concentration of proinflammatory cytokines (TNF- and IL-6) in blood and holding the IL-1 in the brain. Additionally, decreases the initial tissue loss after cryogenic injury and the initial infiltration of leukocytes and lymphocytes T. Cryogenic brain injury IL-1 beta IL-10 IL-10 IL-1I IL-6 IL-6 Interleucinas Interleukins Laser de baixa potência Lesão encefálica criogênica Low power laser TNF-alfa TNF-F
115	Estudo sobre as respostas inflamatórias em modelo experimental de artrite séptica induzida por Staphylococcus aureus e suas vesículas / Study of inflammatory responses in experimental staphylococcal septic arthritis model induced by Staphylococcus aureus and extracellular vesicles Farah Fatima 06 March 2018 (has links) A artrite séptica (AS), também chamada de artrite infecciosa, é uma doença inflamatória das articulações iniciada por um agente infeccioso. O agente causal mais comum da SA é Staphylococcus aureus (S. aureus). A patogênese da SA inclui uma resposta inflamatória complexa envolvendo sistema imune inato e adaptativo. As citocinas liberadas a partir de macrófagos, tais como TNF-?, IL-1? e IL-6, foram classicamente apontadas como os principais mediadores da inflamação grave que precede a destruição da cartilagem e osso e a disfunção articular permanente mediante a AS. A evidência radiológica está frequentemente presente, mas não diferencia o afrouxamento mecânico do septo das articulações. Portanto, se houver algum indício de suspeita de infecção, deve ser aspirado para avaliação microbiológica. Recentemente, as tecnologias de imagem como a micro tomografia computadorizada (?CT) foram amplamente utilizadas para modelos pré-clínicos de distúrbios articulares auto-imunes. No entanto, as características radiológicas da AS em camundongos ainda são amplamente desconhecidas. No estudo atual, os camundongos NMRI foram inoculados intravenosamente ou intra-articularmente com a cepas de S. aureus Newman ou LS-1. Os sinais radiológicos e clínicos da artrite séptica foram acompanhados durante 10 dias usando ?CT. Avaliamos as correlações entre alterações radiológicas conjuntas e sinais clínicos, alterações histológicas e níveis séricos de citocinas. Nos dias 5-7 após a infecção intravenosa, a destruição óssea verificada por ?CT tornou-se evidente na maioria das articulações infectadas. Os sinais radiológicos de destruição óssea eram dependentes da dose bacteriana. O local mais comumente afetado pela artrite séptica foi o fêmur distal nos joelhos. A destruição óssea detectada pelo ?CT foi correlacionada positivamente com alterações histológicas na artrite séptica local e hematogênica. Os níveis séricos de IL-6 foram significativamente correlacionados com a gravidade da destruição das articulações. Coletivamente, nossos dados mostram que o ?CT é um método sensível para monitorar a progressão da doença e determinar a gravidade da destruição óssea em um modelo de artrite séptica do mouse; enquanto que a IL-6 é um potencial biomarcador de destruição óssea na artrite séptica. / Extracellular vesicles (EVs) are heterogeneous population of nano- and micro-sized vesicles secreted from almost every cell type. The process of EV secretion seems to be evolutionary conserved across the species kingdoms, ranging from simple prokaryotes to higher eukaryotes including bacteria, viruses, and parasitic protozoa such as leishmania and malarial parasites, fungi, plants and animals. Recent data suggests that Staphylococcus aureus (S. aureus) bacteria secretes EVs that could mediate host-pathogen interactions. EVs have been investigated in various bacterial species which modulate the secretion of immunoregulatory molecules such as cytokines and may have key role in infection. However, their role in S. aureus septic arthritis has not been explored yet. In current study, we postulate novel perspectives for the implementation of S. aureus-derived EVs in vitro as well as in vivo model of septic arthritis. EVs derived from S. aureus were applied to stimulate mice splenocytes in vitro as well as intra-articularly and the cytokine levels were measured. Our results showed that S. aureus derived EVs potentially provoke the production of proinflammatory cytokines. TNF-?, and IL-6 were significantly elevated in splenocytes in vitro after EV-based stimulation. Moreover, NMRI mice were injected with variable doses of EVs intraarticularly and mice were observed for 10 days to examine inflammation and development of septic arthritis. Bone and cartilage destruction was assessed by histochemistry analysis to score the joint erosion. Altogether, our results demonstrate the putative role of S. aureus-derived EVs in provoking inflammation and immunological responses suggesting that these vesicles could induce and disseminate systemic immune response during the development of septic arthritis. Artrite séptica Citocinas ELISA Histoquímica IL-6 Micro tomografia computadorizada Modelo animais Staphylococcus aureus TNF-alpha Exosomes Extracellular vesicles IL-6 Inflammation Microvesicles Septic arthritis Staphylococcus aureus TNF-alpha
116	Análise da biomodulação da inflamação após lesão criogênica no sistema nervoso central em ratos submetidos à fototerapia com laser em baixa intensidade / Analysis of biomodulation of inflammation after cryogenic injury in the central nervous system in rats subjected to phototherapy with low-intensity laser Maria Stella Nunes Araujo Moreira 24 March 2010 (has links) Este estudo teve por finalidade estudar os efeitos da fototerapia com laser em baixa intensidade (Low Level Laser Therapy LLLT) sobre a inflamação e reparação após lesão criogênica realizada no sitema nervoso central (SNC) de ratos. Foram realizados 3 experimentos. Em todos os experimentos foi utilizado um modelo de deformação cortical direta induzida por lesão criogênica. A LLLT foi realizada com laser de diodo em baixa intensidade emitindo no vermelho visível (InGaAlP, 660 nm) ou no infravermelho (AlGaAr, 780 nm). Os parâmetros de irradiação foram: potência de 40 mW, área do feixe de 0,04 cm2, densidades de energia de 3 J/cm2 (3 s) ou 5 J/cm2 (5 s) determinando energias por ponto de 0,12 J e 0,20 J, respectivamente. Foram realizadas 2 irradiações com intervalo de 3 h, no modo contato e em 2 pontos por lesão. No experimento 1, 50 ratos da linhagem Wistar foram utilizados para determinar os parâmetros de LLLT capazes de influenciar na dinâmica da produção de citocinas proinflamatórias (TNF-a, IL-1b, IL-6) e antiinflamatória (IL-10). As citocinas foram mensuradas pelo teste ELISA no cérebro e no sangue dos animais, 6 e 24h após a lesão. Os grupos experimentais foram: controle (não irradiado) e 4 grupos irradiados com 3 J/cm2 ou 5 J/cm2 para cada comprimento de onda (n=10 por grupo). Para os experimentos 2 e 3 foram utilizados 40 ratos (20 não irradiados controles e 20 irradiados). A LLLT foi realizada somente com o parâmetro de irradiação do laser no infravermelho e a densidade de energia de 3 J/cm2. Nestes experimentos o processo de reparação das lesões criogênicas no SNC foi acompanhado em 6 h, 1, 7 e 14 dias após a última irradiação (n=5 por grupo por tempo experimental). No experimento 2 foi realizada a análise morfométrica da região lesionada do SNC. No experimento 3 foi analisada a distribuição das células inflamatórias (linfócitos T, leucócitos e macrófagos). Os dados de cada experimento foram comparados estatísticamente por análise de variância (ANOVA) ou Kruskal-Wallis seguido dos testes de Tukey ou de Dunn, respectivamente (F=5%). O trauma criogênico foi capaz de criar lesões focais no córtex representadas por necrose, edema, hemorragia e infiltrado inflamatório. Os achados mais marcantes foram: no experimento 1 com a irradiação do laser no infravermelho e 3 J/ cm2, o TNF- a e a IL-6 se mantiveram nos mesmos níveis em 6 e 24 h, enquanto no controle houve aumento significativo. Experimento 2: as lesões não tratadas apresentaram maior perda tecidual em 6 h que as irradiadas. Experimento 3: as lesões irradiadas apresentaram menor quantidade de leucócitos e linfócitos T nas primeiras 24 h do que nas lesões controle. A quantidade de macrófagos foi similar nos dois grupos. Conclusões: Levando em consideração as condições experimentais deste estudo concluiu-se que LLLT exerce efeitos nos processos de inflamação e reparação diminuindo a concentração de citocinas próinflamatórias (TNF-F e IL-6) no sangue e mantendo a de IL-1I no cérebro. Adicionalmente, diminui a perda tecidual inicial pós- lesão criogênica e a infiltração inicial de leucócitos e linfócitos T. / This study aimed to study the effects of phototherapy with low-intensity laser (Low Level Laser Therapy - LLLT) on inflammation and repair after cryogenic injury held in central nervous system (CNS) of rats. There were 3 experiments. In all experiments a model of deformation induced by direct cortical cryogenic injury was used. The LLLT was carried out with a low intensity diode laser emitting in the visible red (InGaAlP, 660 nm) or infrared (AlGaAs, 780 nm). The irradiation parameters were: power of 40 mW, beam area of 0.04 cm2, energy densities of 3 J/cm2 (3 s) or 5 J/cm2 (5 s) providing energy per point of 0.12 J and 0.20 J, respectively. Two irradiations were performed at 3 h-intervals, in contact mode and in 2 points for lesion. In experiment 1, 50 Wistar rats were used to determine the parameters of LLLT able to influence the dynamics of production proinflammatory cytokines (TNF-, IL-1 and IL-6) and antiinflammatory cytokine (IL- 10). Cytokines were measured by ELISA in the brain and blood of animals, 6 and 24 hours after injury. The experimental groups were: control (non-irradiated) and 4 irradiated groups [3 J/cm2 and 5 J/cm2 for each wavelength (n = 10 per group)]. For experiments 2 and 3 40 rats (20 non-irradiated - controls and 20 irradiated).were used. The LLLT was performed only with the parameter of laser irradiation on the infrared and the energy density of 3 J/cm2. In these experiments, the process of repair of cryogenic injury in the CNS was followed in 6 h, 1, 7 and 14 days after the last irradiation (n = 5 per group and time trial). In experiment 2 a morphometric analysis of the injured area of the CNS was done. In experiment 3 the distribution of inflammatory cells (lymphocytes, leukocytes and macrophages) was analyzed. Data from each experiment were compared statistically by analysis of variance (ANOVA) or Kruskal-Wallis followed by tests of Tukey or Dunn, respectively ( = 5%). Cryogenic trauma was able to create focal lesions in the cortex represented by necrosis, edema, hemorrhage and inflammatory infiltrate. The most striking findings were: in experiment 1 with the laser irradiation in the infrared and 3 J/cm 2, TNF- and IL-6 remained at the same levels at 6 and 24 h, while in the control there was a significant increase. Experiment 2: untreated lesions showed greater tissue loss than irradiated lesions in 6 h. Experiment 3: lesions irradiated had fewer leukocytes and lymphocytes in the first 24 h than control lesions. The amount of macrophages was similar in both groups. Conclusions: Considering the experimental conditions of this study it was concluded that LLLT has effects in the processes of inflammation and repair by decreasing the concentration of proinflammatory cytokines (TNF- and IL-6) in blood and holding the IL-1 in the brain. Additionally, decreases the initial tissue loss after cryogenic injury and the initial infiltration of leukocytes and lymphocytes T. IL-10 IL-1I IL-6 Interleucinas Laser de baixa potência Lesão encefálica criogênica TNF-F Cryogenic brain injury IL-1 beta IL-10 IL-6 Interleukins Low power laser TNF-alfa
117	Estudo sobre as respostas inflamatórias em modelo experimental de artrite séptica induzida por Staphylococcus aureus e suas vesículas / Study of inflammatory responses in experimental staphylococcal septic arthritis model induced by Staphylococcus aureus and extracellular vesicles Fatima, Farah 06 March 2018 (has links) A artrite séptica (AS), também chamada de artrite infecciosa, é uma doença inflamatória das articulações iniciada por um agente infeccioso. O agente causal mais comum da SA é Staphylococcus aureus (S. aureus). A patogênese da SA inclui uma resposta inflamatória complexa envolvendo sistema imune inato e adaptativo. As citocinas liberadas a partir de macrófagos, tais como TNF-?, IL-1? e IL-6, foram classicamente apontadas como os principais mediadores da inflamação grave que precede a destruição da cartilagem e osso e a disfunção articular permanente mediante a AS. A evidência radiológica está frequentemente presente, mas não diferencia o afrouxamento mecânico do septo das articulações. Portanto, se houver algum indício de suspeita de infecção, deve ser aspirado para avaliação microbiológica. Recentemente, as tecnologias de imagem como a micro tomografia computadorizada (?CT) foram amplamente utilizadas para modelos pré-clínicos de distúrbios articulares auto-imunes. No entanto, as características radiológicas da AS em camundongos ainda são amplamente desconhecidas. No estudo atual, os camundongos NMRI foram inoculados intravenosamente ou intra-articularmente com a cepas de S. aureus Newman ou LS-1. Os sinais radiológicos e clínicos da artrite séptica foram acompanhados durante 10 dias usando ?CT. Avaliamos as correlações entre alterações radiológicas conjuntas e sinais clínicos, alterações histológicas e níveis séricos de citocinas. Nos dias 5-7 após a infecção intravenosa, a destruição óssea verificada por ?CT tornou-se evidente na maioria das articulações infectadas. Os sinais radiológicos de destruição óssea eram dependentes da dose bacteriana. O local mais comumente afetado pela artrite séptica foi o fêmur distal nos joelhos. A destruição óssea detectada pelo ?CT foi correlacionada positivamente com alterações histológicas na artrite séptica local e hematogênica. Os níveis séricos de IL-6 foram significativamente correlacionados com a gravidade da destruição das articulações. Coletivamente, nossos dados mostram que o ?CT é um método sensível para monitorar a progressão da doença e determinar a gravidade da destruição óssea em um modelo de artrite séptica do mouse; enquanto que a IL-6 é um potencial biomarcador de destruição óssea na artrite séptica. / Extracellular vesicles (EVs) are heterogeneous population of nano- and micro-sized vesicles secreted from almost every cell type. The process of EV secretion seems to be evolutionary conserved across the species kingdoms, ranging from simple prokaryotes to higher eukaryotes including bacteria, viruses, and parasitic protozoa such as leishmania and malarial parasites, fungi, plants and animals. Recent data suggests that Staphylococcus aureus (S. aureus) bacteria secretes EVs that could mediate host-pathogen interactions. EVs have been investigated in various bacterial species which modulate the secretion of immunoregulatory molecules such as cytokines and may have key role in infection. However, their role in S. aureus septic arthritis has not been explored yet. In current study, we postulate novel perspectives for the implementation of S. aureus-derived EVs in vitro as well as in vivo model of septic arthritis. EVs derived from S. aureus were applied to stimulate mice splenocytes in vitro as well as intra-articularly and the cytokine levels were measured. Our results showed that S. aureus derived EVs potentially provoke the production of proinflammatory cytokines. TNF-?, and IL-6 were significantly elevated in splenocytes in vitro after EV-based stimulation. Moreover, NMRI mice were injected with variable doses of EVs intraarticularly and mice were observed for 10 days to examine inflammation and development of septic arthritis. Bone and cartilage destruction was assessed by histochemistry analysis to score the joint erosion. Altogether, our results demonstrate the putative role of S. aureus-derived EVs in provoking inflammation and immunological responses suggesting that these vesicles could induce and disseminate systemic immune response during the development of septic arthritis. Artrite séptica Citocinas ELISA Exosomes Extracellular vesicles Histoquímica IL-6 IL-6 Inflammation Micro tomografia computadorizada Microvesicles Modelo animais Septic arthritis Staphylococcus aureus Staphylococcus aureus TNF-alpha TNF-alpha
118	Biomarcadores de sepsis en sangre de cordón para el diagnóstico de sepsis neonatal precoz Sancho Rodríguez, Natalia 23 July 2012 (has links) La sepsis neonatal precoz actualmente es una importante causa de morbilidad y mortalidad en el período neonatal, y su rápido diagnóstico puede ayudar a instaurar un tratamiento antibiótico eficaz. El objetivo de este trabajo es estudiar la relación de diferentes marcadores de sepsis, tanto bioquímicos como hematológicos, en muestras de sangre de cordón procedentes de neonatos; que previamente fueron clasificados en grupos de estudio en función de la presencia o ausencia de factores de riesgo (infeccioso, prematuridad, otras causas, o sepsis neonatal precoz confirmada). Los marcadores bioquímicos de sepsis (PCR, PCT e IL-6) y hematológicos en sangre de cordón no han resultado de utilidad en el diagnóstico de sepsis neonatal precoz, y los datos clínicos continúan siendo los más determinantes. Las nuevas técnicas de biología molecular en sangre de cordón fueron indicativas de la presencia de sospecha de infección en aquellos neonatos con uno o varios factores de riesgo infeccioso. / Early-onset neonatal sepsis is currently a major cause of morbidity and mortality in the neonatal period, and its rapid diagnosis can help to establish an effective antibiotic treatment. The objective of this work is to study the relationship of different markers of sepsis, both biochemical and haematological, in cord blood samples taken from infants; that were previously classified in groups according to the presence or absence of risk factors (infectious, prematurity, other causes, or confirmed early neonatal sepsis). Biochemical markers sepsis (CRP, PCT and IL-6) and haematological in cord blood have not proved useful in the diagnosis of early neonatal sepsis, and clinical data continue to be the most decisive. New techniques of molecular biology in cord blood were indicative of the presence of suspected infection in those neonates with one or several factors of risk of infection. Sepsis neonatal precoz sangre de cordón Proteína C Reactiva (PCR) Procalcitonina (PCT) Interleuquina-6 (IL-6) Septifast Early-onset neonatal sepsis cord blood C Protein Reactive (CRP) Procalcitonine (PCT) Interleukin-6 (IL-6) Septifast Ciencias de la salud 577 579 616.9
119	Molecular mechanisms of the cytokine-dependent induction of the heme oxygenase-1 gene: in vivo and in vitro studies / Molekulare Mechanismen der Zytokin-abhängigen Induktion des Hämoxygenase-1 Gens: in vivo und in vitro Studien Tron, Kyrylo 30 June 2004 (has links) No description available. 570 Biowissenschaften, Biologie Mathematics and Computer Science Akute-Phase Reaktion Hepatozyten HO-1 IL-6 Leber Muskel STAT Terpentinöl Acute phase response hepatocytes HO-1 IL-6 liver muscle STAT turpentine oil 42.13 WF 200: Molekularbiologie
120	De novo Induktion von Anaphylatoxin C5a-Rezeptoren in Hepatocyten der Ratte durch den Entzündungsauslöser Lipopolysaccharid in vivo / Vermittlung durch die Entzündungsmediatoren Interleukin-6 und -1ß / De novo induction of anaphylatoxin C5aR in rat hepatocytes by bacterial lipopolysaccharide in vivo / Mediation by the proinflammatory cytokines interleukine-6 and -1ß Koleva, Milena 03 May 2001 (has links) No description available. 000 Allgemeines, Wissenschaft Mathematics and Computer Science C5aR C5a Leber Hepatocyten LPS IL-6 Entzündungen Abwehrreaktionen der Leber C5aR C5a liver hepatocytes LPS IL-6 Inflammation Liver defence reactions 42.15 Zellbiologie WF

Search results