Global ETD Search

461	Prevalência de teste tuberculínico positivo prévio ao uso de imunobiológicos em pacientes reumatológicos Garziera, Giovana January 2017 (has links) Base teórica: A introdução de agentes biológicos, especialmente os bloqueadores do fator de necrose tumoral (anti-TNF), para o tratamento de doenças reumáticas aumentou o risco de desenvolver tuberculose (TB). O rastreio para infecção tuberculosa latente (ILTB) é fortemente recomendado antes de iniciar a terapia com agentes anti-TNF. Os objetivos deste estudo foram identificar a prevalência de ILTB e TB entre pacientes com doenças reumáticas em uso dos medicamentos anti-TNF. Métodos: Estudo transversal. Foram revisados os registros médicos eletrónicos de todos os doentes adultos (≥ 18 anos) em uso da terapia anti-TNF. Todos os pacientes foram submetidos ao teste tuberculínico (TT) antes de iniciar o tratamento com os medicamentos anti-TNF. Resultados: No total, 176 pacientes foram incluídos no estudo. A idade média de todos os pacientes foi de 51,9 ± 12,4 anos, 34,7% eram do sexo masculino e 90,9% eram brancos. As doenças subjacentes mais comuns foram: Artite Reumatóide (AR) em 89 pacientes (50,6%), Espondilite Anquilosante (EA) em 49 (27,8%) e Artrite Psoriática (AP) em 31 (17,6%). A prevalência de TT positivo foi de 29,5%. O contato domiciliar com TB foi significativamente associado com TT positivo (p = 0,020). Os pacientes com AR apresentaram reações TT menores do que os pacientes com EA (p = 0,022). Houve seis casos de TB (3,4%) diagnosticados durante a terapia anti-TNF. Conclusões: Demonstrou-se alta prevalência de TT positivo (29,5%) em pacientes com doenças reumáticas em uma região com alta prevalência de TB. Nossos dados corroboram a recomendação do Colégio Americano de Reumatologia (ACR) de que os pacientes que vivem em configurações de alta incidência de TB devem ser testados anualmente para ILTB. / Background: The introduction of biological agents, especially the blockers of tumor necrosis factor (anti-TNF), for the treatment of rheumatic diseases increased the risk of developing tuberculosis (TB). Screening for latent TB infection (LTBI\|) is strongly recommended before starting therapy with anti-TNF agents. The objectives of this study were to identify the prevalence of LTBI and TB among patients with rheumatic diseases on anti-TNF drugs. Methods: Cross-sectional study. The electronic medical records of all adult patients (≥ 18 years old) undergoing anti-TNF treatment were reviewed. Every patient underwent TST test before starting anti-TNF treatment. Results: In total, 176 patients were included in the study. The mean age of all patients was 51.9 ± 12.4 years, 34.7% were males, and 90.9% were white. The most common underlying diseases were: RA in 89 patients (50.6%), AS in 49 (27.8%), and PA in 31 (17.6%). The prevalence of positive TST was 29.5%. Household contact with TB was significantly associated with a positive TST (p=0.020). RA patients had lower TST reactions than AS patients (p=0.022). There were six cases of TB (3.4%) diagnosed during anti-TNF therapy. Conclusions: We demonstrated a high prevalence of positive TST (29.5%) among patients with rheumatic diseases in a region with high TB prevalence. Our data corroborates the ACR’s recommendation that patients who live in high TB incidence settings should be tested annually for LTBI. Tuberculose latente Teste tuberculínico Mycobacterium tuberculosis Fator de necrose tumoral alfa Artrite reumatóide Latent tuberculosis Tuberculin skin test Mantoux Anti-TNF therapy Mycobacterium tuberculosis Tumor necrosis factor-alpha Rheumatoid arthritis
462	Avaliação da excreção genital do HIV-1 em mulheres menopausadas e em idade fértil: prevalência e fatores associados / HIV cervicovaginal shedding among postmenopausal and fertile-aged women: prevalence and associated factors Melo, Keli Cardoso de 14 December 2009 (has links) INTRODUÇÃO: Poucos estudos têm focado as modificações fisiológicas que ocorrem no trato genital de mulheres menopausadas infectadas pelo HIV e sua associação com a excreção genital do vírus. Nesse estudo de corte transversal, comparou-se a excreção genital do HIV em mulheres menopausadas e em idade fértil em acompanhamento em um centro especializado em São Paulo, Brasil. Investigou-se também a associação entre a excreção genital de RNA de HIV e a viremia em ambos os grupos. Fatores associados com a intensidade da excreção genital de HIV também foram pesquisados, incluindo achados ginecológicos e marcadores de progressão da infecção por HIV. MÉTODOS: 146 mulheres infectadas pelo HIV [73 menopausadas (M)/73 em idade fértil (F)] foram selecionadas em Serviço de Extensão ao Atendimento de Pacientes com HIV/Aids Casa da Aids do Hospital das Clínicas da FMUSP, São Paulo, Brasil. As mulheres menopausadas referiram tempo médio de 8,17 anos (DP=6 anos) de menopausa. A contagem de linfócitos T CD4+ foi obtida por citometria de fluxo e a quantificação do RNA do HIV no plasma e no lavado cervicovaginal (LCV) foi realizada por RT-PCR quantitativo, utilizando-se o kit Cobas Amplicor HIV-1 Monitor Test®, no método ultrasensível. Cloreto de lítio foi introduzido no tampão para obtenção do LCV e quantificado antes e depois da coleta do lavado, a fim de determinar o fator de diluição de cada amostra. A deteção do gene SRY por PCR também foi realizada a fim de eliminar amostras com eventual contaminação espermática. A prevalência de excreção genital foi estimada para ambos os grupos e os fatores associados à intensidade da excreção viral foram investigados, utilizando-se modelo de regressão linear múltipla. As variáveis com p<0,2 na análise bivariada foram incluídas na análise multivariada, assim como o grupo em estudo (M ou F). O modelo final incluiu fatores que se mostraram independentemente associados com a intensidade da excreção genital de HIV. RESULTADOS: A prevalência de excreção genital de HIV-RNA foi similar em ambos os grupos (M: 17,8%, IC 95% 9,8 28,5; F: 22%, IC 95% 13,1 33,1, p=0,678). Similarmente, a intensidade de excreção genital do HIV também não se mostrou diferente entre os grupos (mediana - M: 1,4log/mL; F: 1,4log/mL, p=0,587). A carga viral plasmática foi detectável em 34,2% das pacientes menopausadas (IC 95% 23,5 46,3) e em 42,5% entre as pacientes em idade fértil (IC 95% 31 54,6, p=0,395). Três pacientes (2 M/1 F) exibiram excreção genital de HIV-RNA na ausência de viremia detectável. Existe evidência de correlação entre a carga viral plasmática e a genital em ambos os grupos (rM: 0,658; rF: 0,684, p<0,01). Adicionalmente, o número de células CD4+ periféricas mostrou-se negativamente correlacionada à excreção genital do HIV em ambos os grupos (rM: -0,250; rF: -0,248, p<0,05). À análise multivariada, a carga viral plasmática mostrou-se independentemente associada à ocorrência de excreção genital do HIV em ambos os grupos (OR 4,03, IC 95% 2,52 6,45, p<0,001). Já a intensidade de excreção genital mostrou-se independentemente associada ao pH vaginal (p<0,001), concentração de TNF- no LCV (p=0,01), e à carga viral plasmática (p=0,001), todos com correlação positiva. CONCLUSÕES: Apesar das modificações significativas que ocorrem na mucosa vaginal da mulher menopausada, a excreção cervicovaginal do HIV parece não ser significativamente influenciada por esse estado. A carga viral plasmática e o número de células CD4+ periféricas estão correlacionadas com a excreção genital do vírus. A frequência de excreção genital mostrouse independentemente associada à intensidade de viremia. Além disso, o aumento do pH vaginal e evidência de inflamação genital, associada à concentração de TNF- no LCV, independentemente aumentam a intensidade de excreção genital nas mulheres estudadas. / BACKGROUND: Few studies have focused on physiological modifications that occur in the genital tract of HIV-infected postmenopausal women and their association with HIV cervicovaginal shedding. In this cross-sectional study we evaluated and compared HIV genital shedding among postmenopausal and fertile-aged women under care at a specialized center in Sao Paulo, Brazil, investigating the association between HIV-RNA shedding and HIV plasma viral loads in both groups. Factors associated with higher HIV shedding were also investigated, including gynaecological features and HIV disease progression markers. METHODS: 146 women living with HIV [73 postmenopausal (PM)/73 in fertile-aged (F)] were enrolled at the HIV Clinic, University of São Paulo Medical School, Brazil. Postmenopausal women referred a mean duration of 8.17y (SD=6y) since menopause. CD4+ cell counts were obtained by flow cytometry and HIV-RNA was quantified in plasma and in cervicovaginal lavages (CVL) by RT-PCR, using Cobas Amplicor HIV-1 Monitor Ultrasensitive Test. Lithium chloride was introduced into the CVL buffer and measured before and after CVL collection in order to determine the dilution factor for each specimen. SRY gene detection by PCR was also performed in all samples in order to rule out sperm contamination. Prevalence of HIV genital shedding was estimated for both groups and factors associated with the intensity of viral shedding were investigated, using a multiple linear regression model. Variables with p<0.2 in bivariate analysis were included in multivariate analysis, as well as the study group (PM and F). The final model included factors shown to be independently associated with intensity of HIV genital shedding. RESULTS: The prevalence of HIV-RNA genital shedding was similar in both groups. (PM: 17.8%, 95%CI 9.8 28.5; F: 22%, 95%CI 13.1 33.1, p=0.678). Likewise, the intensity of HIV shedding was shown not to differ between PM and F women (means - PM: 1.4log/mL; F: 1.4log/mL, p=0.587). Plasma viral loads were detectable in 34.2% of PM patients (95%CI 23.5 46.3), as compared to 42.5% among F women (95%CI 31 54.6) (p=0.395). Three patients (2 PM/1 F) exhibited HIV-RNA genital shedding in the absence of detectable viremia. We found evidence of correlation between HIV plasma viral load and HIV cervicovaginal shedding in both groups (rPM: 0.658; rF: 0.684, p<0.01). In addition, CD4+ cell counts were shown negatively correlated to HIV shedding in both groups (rPM: -0.250; rF: -0.248, p<0.05). In multivariate analysis, HIV plasma viral load was shown independently associated with occurrence of HIV genital shedding in both groups (OR 4.03, 95%CI 2.52 6.45, p<0.001). In addition, the intensity of HIV shedding was shown independently associated with vaginal pH (p<0.001), TNF- concentrations in CVL (p=0.01), and with HIV plasma viral loads (p=0.001), all of them with positive correlation. CONCLUSION: Despite the significant changes that occur in the vaginal mucosa of postmenopausal women, HIV cervicovaginal shedding does not seem to be significantly influenced by this state. Plasma viral loads and CD4+ cell counts are correlated to HIV genital shedding. The frequency of HIV genital shedding was shown independently associated with viremia intensity. Moreover, increased vaginal pH and evidence of genital inflammation associated with TNF- concentration independently enhanced the intensity of HIV shedding in postmenopausal and fertile-aged women. Bacterial vaginosis Carga viral Elderly people Excreção cervicovaginal Fator de necrose tumoral alfa Genital shedding HIV HIV HIV viral load Idoso Menopausa Menopause RT-PCR TNF-alpha Vaginose bacteriana
463	O uso de medicações anti-TNF não influencia o eixo IL-23/IL-17 em pacientes com espondilite anquilosante / IL-23/IL-17 axis is not influenced by TNF-blocking agents in ankylosing spondylitis patients Fernanda Manente Milanez 02 June 2017 (has links) Introdução: Apesar dos recentes avanços no entendimento da fisiopatologia e no tratamento da espondilite anquilosante (EA), pouco se sabe acerca da influência das medicações anti-fator de necrose tumoral (anti-TNF) sobre as novas vias inflamatórias descritas na patogênese das espondiloartrites. Objetivo: Dessa forma, o objetivo desse estudo é investigar e descrever a influência a longo prazo das medicações anti-TNF sobre o eixo da IL-23/IL-17 em pacientes com EA e sua possível correlação com o tratamento, parâmetros clínicos, laboratoriais e radiológicos. Métodos: Oitenta e seis pacientes com EA sem exposição prévia a medicações anti-TNF foram recrutados. Desses, 47 possuíam Bath Ankylosing Spondylitis Disease Activity Index (BASDAI) >= 4 (grupo EA-ativo) e haviam sido encaminhados para iniciar tratamento anti-TNF e 39 possuíam BASDAI < 4 (grupo EA-controle) em uso de anti-inflamatório não hormonal (AINH) e/ou drogas antirreumáticas modificadoras do curso de doença tradicionais. O grupo EA-ativo foi avaliado clinicamente e laboratorialmente no tempo basal e após 12 e 24 meses de uso das medicações anti-TNF e foi comparado com o grupo EA-controle e com 47 controles saudáveis (CS) pareados por idade e sexo. O escore de uso de AINH foi calculado no tempo basal, 12 meses e 24 meses. Os níveis plasmáticos das interleucinas (IL) IL-17A, IL-22, IL-23 e PGE2 e a dosagem sérica da velocidade de hemossedimentação (VHS) e proteína C-reativa (PCR) foram realizados no grupo EA-ativo no tempo basal, 12 meses e 24 meses e somente no tempo basal nos grupos EA-controle e CS. No grupo EA-ativo, a progressão radiológica foi medida pelo modified Stoke Ankylosing Spondylitis Spine Score (mSASSS) no tempo basal e após 24 meses de tratamento. Resultados: No tempo basal, o grupo EA-ativo apresentou maiores níveis plasmáticos de IL-23 e PGE2 quando comparado ao grupo EA-controle (p < 0,001 e p=0,008) e ao grupo controle saudável (p < 0,001 e p=0,02). Após 24 meses de uso de anti-TNF, os níveis plasmáticos de IL-23 e PGE2 ainda se mantiveram elevados quando comparado ao grupo CS (p < 0,001 e p=0.03) apesar da melhora de todos os parâmetros clínicos e laboratoriais (VHS/PCR) (p < 0,001). A subanálise de 27 pacientes do grupo EA-ativo que obtiveram boa resposta ao uso de anti-TNF (atingiram ASDAS-PCR< 2,1 em 24 meses, com queda >= 1,1 em relação ao ASDAS-PCR basal) revelou que, ainda assim, os níveis plasmáticos de IL-23 eram superiores aos encontrados nos CS (p < 0,001) e superiores ao grupo EA-controle com atividade de doença similar (ASDAS-PCR < 2,1; p=0,01). No grupo EA-ativo foi encontrada uma correlação positiva entre os níveis plasmáticos de IL-23 e IL-17A no tempo basal, 12 meses e 24 meses do estudo (p <= 0,001). Conclusão: Os dados apresentados sugerem que o eixo da IL-23/IL-17 não é influenciado pelas medicações anti-TNF apesar da melhora dos parâmetros clínicos e marcadores de atividade inflamatória estudados / Background: Advances in pathophysiology and treatment of ankylosing spondylitis (AS) was recently demonstrated. However, the effect of anti-tumor necrosis fator (TNF) in the newly described inflammatory pathways involved in this disease remains to be determined. Objective: The aim of our study was, therefore, investigate long-term influence of anti-TNF drugs in IL-23/IL-17 axis of AS patients and their possible correlation with treatment, clinical, laboratory and radiographic parameters. Methods: Eighty six AS anti-TNF naïve patients, 47 referred for anti-TNF therapy (active-AS group; Bath Ankylosing Spondylitis Activity Index (BASDAI) >= 4) and 39 with BASDAI < 4 (control-AS group) were included. The active group was evaluated clinically and laboratorially at baseline, 12-months and 24-months after TNF blockade and compared at baseline to control-AS group and to 47 healthy age- and gender-matched controls. Plasma levels of interleukin (IL)17A, IL-22, IL-23 and PGE2 and serum levels of erythrocyte sedimentation rate (ESR) and c-reactive protein (CRP) were measured at three study times in active-AS and at baseline in control-AS and healthy-controls. Non-steroidal anti-inflammatory drugs (NSAIDs) intake were recorded at baseline, 12 months and 24 months. Radiographic severity and progression was assessed by modified Stoke Ankylosing Spondylitis Spine Score (mSASSS) at baseline and 24 months after therapy in active-AS patients. Results: At baseline, active-AS group presented higher IL-23 and PGE2 levels compared to control-AS group (p < 0.001 and p=0.008) and to healthy controls (p < 0.001 and p=0.02). After 24-months of TNF blockade, IL-23 and PGE2 remained elevated with higher levels compared with the healthy-control group (p < 0.001 and p=0.03) in spite of significant improvements in all clinical/inflammatory parameters (p < 0.001). Further analysis of 27 anti-TNF-treated patients who achieved a good response (ASDAS-CRP < 2.1, with a drop >= 1.1) at 24-months revealed that IL-23 plasma levels remained higher than healthy controls (p < 0.001) and higher than control-AS group with similar disease activity (ASDAS-CRP < 2.1, p=0.01). In active-AS group (n=47), there was a correlation between IL-23 and IL-17A at baseline, 12-months and 24-months after anti-TNF therapy (p <= 0.001). Conclusion: This study provides novel data demonstrating that the IL-23/IL-17 axis is not influenced by TNF blockade drugs in AS patients despite clinical and inflammation improvements and NSAID intake Dinoprostona Espondilite anquilosante Fator de necrose tumoral alfa Inflamação Interleucina-17 Interleucina-23 Medicações anti-TNF Anti-TNFdrugs Dinoprostone Inflammation Interleukin-23 Interlukin-17 Spondylitis ankylosing Tumor necrosis factor-alpha
464	Inflammatory Reactions in Peritonitis and Malignant Obstructive Jaundice : Clinical and Experimental Studies with Special Emphasis on the Cellular Immune Response Österberg, Johanna January 2005 (has links) <p>Patients with peritonitis or malignant obstructive jaundice (HPB<sup>+</sup>) have an increased morbidity and mortality due to sepsis. An altered cell-mediated immunity in the intestinal mucosa might promote gut barrier failure, increased endotoxin and cytokine release and bacterial translocation (BT) in these conditions. A clinically relevant rat model of polymicrobial peritonitis induced sepsis by cecal ligation and puncture (CLP) was used. Septic animals demonstrated a superficial injury in the small intestinal mucosa, and a significant reduction in T lymphocytes in the villi, as well as increased number of macrophages in the villi and in the MLNs as compared to sham. CLP caused increased concentration of TNF-α and IL-6 in ascitic fluid. CLP + the immunomodulator Linomide decreased the TNF-α level, reduced mucosal damage and attenuated the changes in T lymphocytes and macrophages observed following CLP. CLP + selective cyclooxygenase (COX)-2 inhibitor (SC-236) or nonselective COX inhibitor (indometacin) decreased the amount of macrophages in the mucosa and the MLNs compared to untreated CLP. CLP + indometacin decreased T lymphocytes in the villi and MLNs. SC-236 + CLP reduced mucosal injury and cytokine release as compared to indometacin. An increased rate of apoptosis in both the mucosa and MLNs was seen following CLP; COX inhibitors enhanced this phenomenon in the MLNs.</p><p>BT occurred infrequently in patients with acute peritonitis and in HPB<sup>+</sup> there was no evidence of BT. Peritonitis and HPB<sup>+ </sup>causes significant inflammatory cellular reactions as increased endotoxin and cytokine plasma levels and an altered immune cell distribution in MLNs, in HPB<sup>+ </sup>a high rate of apoptosis in MLNs was observed. </p><p>An altered pattern of immunocompetent cells within the mucosa and in MLNs was found in experimental and clinical peritonitis as in HPB<sup>+</sup>.<sup> </sup>Lymphocyte depletion may be a result of increased apoptosis, which could reduce the ability of septic or jaundice patients to eradicate infection.</p> Surgery CLP sepsis peritonitis bacterial translocation malignant obstructive jaundice Linomide COX inhibitor SC-236 indometacin T lymphocyte macrophage mucosa MLN gut immune cell distribution mucosal injury cytokines TNF-α IL-6 IL-10 endotoxin caspase-3 apoptosis Kirurgi Surgery Kirurgi
465	Inflammatory Reactions in Peritonitis and Malignant Obstructive Jaundice : Clinical and Experimental Studies with Special Emphasis on the Cellular Immune Response Österberg, Johanna January 2005 (has links) Patients with peritonitis or malignant obstructive jaundice (HPB+) have an increased morbidity and mortality due to sepsis. An altered cell-mediated immunity in the intestinal mucosa might promote gut barrier failure, increased endotoxin and cytokine release and bacterial translocation (BT) in these conditions. A clinically relevant rat model of polymicrobial peritonitis induced sepsis by cecal ligation and puncture (CLP) was used. Septic animals demonstrated a superficial injury in the small intestinal mucosa, and a significant reduction in T lymphocytes in the villi, as well as increased number of macrophages in the villi and in the MLNs as compared to sham. CLP caused increased concentration of TNF-α and IL-6 in ascitic fluid. CLP + the immunomodulator Linomide decreased the TNF-α level, reduced mucosal damage and attenuated the changes in T lymphocytes and macrophages observed following CLP. CLP + selective cyclooxygenase (COX)-2 inhibitor (SC-236) or nonselective COX inhibitor (indometacin) decreased the amount of macrophages in the mucosa and the MLNs compared to untreated CLP. CLP + indometacin decreased T lymphocytes in the villi and MLNs. SC-236 + CLP reduced mucosal injury and cytokine release as compared to indometacin. An increased rate of apoptosis in both the mucosa and MLNs was seen following CLP; COX inhibitors enhanced this phenomenon in the MLNs. BT occurred infrequently in patients with acute peritonitis and in HPB+ there was no evidence of BT. Peritonitis and HPB+ causes significant inflammatory cellular reactions as increased endotoxin and cytokine plasma levels and an altered immune cell distribution in MLNs, in HPB+ a high rate of apoptosis in MLNs was observed. An altered pattern of immunocompetent cells within the mucosa and in MLNs was found in experimental and clinical peritonitis as in HPB+. Lymphocyte depletion may be a result of increased apoptosis, which could reduce the ability of septic or jaundice patients to eradicate infection. Surgery CLP sepsis peritonitis bacterial translocation malignant obstructive jaundice Linomide COX inhibitor SC-236 indometacin T lymphocyte macrophage mucosa MLN gut immune cell distribution mucosal injury cytokines TNF-α IL-6 IL-10 endotoxin caspase-3 apoptosis Kirurgi Surgery Kirurgi
466	A Systems Biology Approach to Develop Models of Signal Transduction Pathways Huang, Zuyi 2010 August 1900 (has links) Mathematical models of signal transduction pathways are characterized by a large number of proteins and uncertain parameters, yet only a limited amount of quantitative data is available. The dissertation addresses this problem using two different approaches: the first approach deals with a model simplification procedure for signaling pathways that reduces the model size but retains the physical interpretation of the remaining states, while the second approach deals with creating rich data sets by computing transcription factor profiles from fluorescent images of green-fluorescent-protein (GFP) reporter cells. For the first approach a model simplification procedure for signaling pathway models is presented. The technique makes use of sensitivity and observability analysis to select the retained proteins for the simplified model. The presented technique is applied to an IL-6 signaling pathway model. It is found that the model size can be significantly reduced and the simplified model is able to adequately predict the dynamics of key proteins of the signaling pathway. An approach for quantitatively determining transcription factor profiles from GFP reporter data is developed as the second major contribution of this work. The procedure analyzes fluorescent images to determine fluorescence intensity profiles using principal component analysis and K-means clustering, and then computes the transcription factor concentration from the fluorescence intensity profiles by solving an inverse problem involving a model describing transcription, translation, and activation of green fluorescent proteins. Activation profiles of the transcription factors NF-κB, nuclear STAT3, and C/EBPβ are obtained using the presented approach. The data for NF-κB is used to develop a model for TNF-α signal transduction while the data for nuclear STAT3 and C/EBPβ is used to verify the simplified IL-6 model. Finally, an approach is developed to compute the distribution of transcription factor profiles among a population of cells. This approach consists of an algorithm for identifying individual fluorescent cells from fluorescent images, and an algorithm to compute the distribution of transcription factor profiles from the fluorescence intensity distribution by solving an inverse problem. The technique is applied to experimental data to derive the distribution of NF-κB concentrations from fluorescent images of a NF-κB GFP reporter system. Fluorescent microscopy image analysis IL-6 signaling pathway Inverse problem K-means clustering Model simplification Mathematical modeling Observability analysis Principal component analysis Sensitivity analysis TNF-α signal transduction Transcription factor profiles
467	Immunreaktionen im zentralen Nervensystem bei Stimulation mit Bestandteilen von Borrelia burgdorferi / Immunoreactions in the central nervous system by stimulation with proteins from Borrelia burgdorferi Heinz, Torsten Joseph 08 January 2014 (has links) No description available. 610 CNS Stimulation; OspC; VlsE GOK-MEDIZIN
468	Régulations épigénétiques et rôles de la protéine Btk dans l'expression du TNF-α par la voie des TLRs Frenzel, Laurent 02 September 2013 (has links) (PDF) La Bruton tyrosine kinase ou Btk est une protéine dont le rôle dans la maturation des lymphocytes B est connu depuis plusieurs années. Par contre, son rôle dans le contrôle de l'immunité innée est moins établi. Nous avons montré que, en réponse à la voie des Toll like Receptors ou TLRs, Btk régule la stabilité de l'ARN messager du TNF-α par l'intermédiairede la protéine TTP ou Tristétraproline. Par ailleurs, nous avons montré que l'expression d'un microARN, le miR-346, régulait négativement la protéine Btk et donc la synthèse de TNF-α. L'amplification de l'expression de ce miR-346 par transfection permet d'avoir un effet anti-TNF-α et anti-Btk interessant notamment dans le modèle cellulaire de la polyarthrite rhumatoïde. Enfin, nous avons montré que, en réponse au TLRs, la modulation de l'expression du TNF-α en fonction de l'état de méthylation de l'ADN et d'acétylation des histones dépendait directement de l'expression du couple miR-346 et Btk. Btk est donc une protéine charnière dans le contrôle de l'inflammation par les mécanismes épigénétiques que sont les miARNs, la méthylation de l'ADN et l'acétylation des histones. Sur le plan thérapeutique, l'inhibition de cette protéine par ces différents mécanismes de régulation semble donc être très interessante, à la fois dans les maladies inflammatoires et néoplasiques. [SDV:IMM] Life Sciences/Immunology [SDV:IMM] Sciences du Vivant/Immunologie Btk TNF-α MicroARN MiR-346 TTP Acétylation des histones Méthylation de l'ADN Polyarthrite rhumatoïde
469	Continuous Endothelial Cell Activation Increases Angiogenesis: Evidence for the Direct Role of Endothelium Linking Angiogenesis and Inflammation Rajashekhar, Gangaraju, Willuweit, Antje, Patterson, Carolyn E., Sun, Peichuan, Hilbig, Andreas, Breier, Georg, Helisch, Armin, Clauss, Matthias 27 February 2014 (has links) (PDF) There is increasing evidence that chronic inflammation is tightly linked to diseases associated with endothelial dysfunction, including the induction of aberrant angiogenesis. While leukocytes have been described as mediators of inflammation-associated angiogenesis, the effects of direct chronic endothelial activation have not been addressed in this context. Using an uncleavable mutant of the transmembrane form of tumor necrosis factor-α (TNF-α), we have established models of stable TNF-α expression in endothelial cells in vitro and in transgenic mice in vivo. In the in vitro model, continuous endothelial activation leads to increased leukocyte cellular adhesion molecule expression and intracellular reactive oxygen species, hallmarks of a proinflammatory and dysfunctional endothelium. In addition, stable expression of TNF-α in endothelial cells increased angiogenic sprout formation in the presence but also in the absence of angiogenic growth factors. The partial neutralization of this effect by TNF-α antibodies and the inability of conditioned media from stable TNF-α-expressing endothelial cells to induce angiogenic activities in control endothelial cells suggest that this effect does not require expression of additional autocrine factors, but is an autonomous effect of the transmembrane TNF on the endothelial cells. Furthermore, using the Matrigel plug assay in vivo, increased angiogenesis was observed in endothelial TNF-α-expressing transgenic versus control mice. In conclusion, chronic inflammatory changes mediated by TNF-α can induce angiogenesis in vitro and in vivo, suggesting endothelial cell activation as a direct link between inflammation and angiogenesis. / Dieser Beitrag ist mit Zustimmung des Rechteinhabers aufgrund einer (DFG-geförderten) Allianz- bzw. Nationallizenz frei zugänglich. Angiogenese Entzündung endotheliale Dysfunktion ICAM-1 reaktive Sauerstoffspezies Tumornekrosefaktor TNF Angiogenesis Inflammation Endothelial dysfunction Intracellular adhesion molecule 1 Matrigel plug assay Reactive oxygen species Tumor necrosis factor-a ddc:610 rvk:XA 10000
470	p63 and epithelial homeostasis studies of p63 under normal, hyper-proliferative and malignant conditions / Gu, Xiaolian, January 2010 (has links) Diss. (sammanfattning) Umeå : Umeå universitet, 2010.

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