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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.
211

Vergleich primärer Peritonealmakrophagen und Mikrogliazellen von jungen und alten Mäusen bezüglich ihrer Bakterienphagozytose und Freisetzung inflammatorischer Mediatoren in vitro / Comparison of primary peritoneal macrophages and microglial cells from young and aged mice regarding their phagocytosis of bacteria and release of inflammatory mediators in vitro

Kaufmann, Annika 23 November 2016 (has links)
No description available.
212

Epigenetic Alterations of Toll-Like Receptors by TET2 in Spontaneous Preterm Labor

Chumble, Anuja 01 January 2014 (has links)
Increasing evidence implicates the presence of bacteria in intrauterine tissues as an important risk factor for spontaneous preterm labor. Epigenetic alterations of innate immunity genes may increase the mother’s sensitivity to subclinical levels of bacteria. This study examined the presence of TET2, TLR-2, and TLR-9 in intrauterine tissue, and evaluated whether epigenetic alterations of these genes, as well as IL-8, changed their expression in human decidual tissue and a macrophage cell culture. Immunohistochemicalstaining was used to detect the presence of these proteins in intrauterine tissue. Gene expression changes were evaluated in stimulated monocytes and macrophages. Fluorescence immunohistochemistry was used to track translocation of TET2 in stimulated monocytes and macrophages. Secreted IL-8 concentration was detected with ELISA. Decidual expression of TET2, TLR-2, and TLR-9 increased in the order TNL < TL < sPTL < iPTL. This study found that TET2, TLR-2, TLR-9, and IL-8 are regulated by epigenetic mechanisms. This study was the first to report activation of TET2 involves its translocation from the cytosol to the nucleus in macrophages.
213

Papel do receptor toll-like 9 na falência de migração dos neutrófilos na sepse / The role of toll-like receptor 9 on failure of neutrophil migration during sepsis.

Trevelin, Silvia Cellone 20 December 2010 (has links)
O recrutamento de neutrófilos para o sítio da infecção é um evento crucial para o combate aos microrganismos e sobrevivência na sepse. A migração destes polimorfonucleares é dirigida através de um gradiente quimiotático por meio do reconhecimento de quimiocinas por receptores acoplados a proteína G (GPCRs), os quais são regulados por quinases específicas (GRKs). Estudos prévios demonstraram que na sepse ocorre uma falência na migração de neutrófilos para o foco infeccioso em função da dessensibilização de receptores quimiotáticos via GRKs induzida pela ativação de receptores toll-like (TLRs), TLR2 e TLR4. Apesar de a ausência de TLR9 em células dendriticas ter sido relacionada a maior sobrevivência de camundongos sépticos, o papel do TLR9 atuando diretamente em neutrófilos não foi avaliado. Objetivando preencher esta lacuna, propôs-se avaliar o papel direto de TLR9 na falência de migração de neutrófilos na sepse. Os camundongos TLR9-/- apresentaram maior sobrevivência a sepse polimicrobiana avaliada por meio do modelo de ligadura e perfuração do ceco (CLP). A deficiência de TLR9 também acarretou em aumento na migração de neutrófilos para o foco da infecção, menor seqüestro de neutrófilos no pulmão, bem como, menor número de bactérias no lavado peritoneal e sangue. A ativação de TLR9 por oligodeoxinucleotídeo contendo o dinucleotídeo CpG não metilado (ODN CpG) nos neutrófilos reduziu a quimiotaxia destes em direção a quimiocina CXCL2 e expressão do receptor quimiotático CXCR2. Além disso, neutrófilos estimulados com ODN CpG apresentaram aumento na expressão da quinase tipo 2 relacionada a receptores acoplados a proteína G (GRK2). Dessa forma, a ativação de TLR9 em neutrófilos circulantes no sangue é prejudicial na sepse por reduzir a quimiotaxia destes para o foco da infecção ao induzir a dessensibilização de CXCR2 via GRK2. / The recruitment of neutrophils to the site of infection is a crucial event for combating the microorganisms and survival on sepsis. The neutrophil migration is directed by a chemotactic gradient through the recognition of chemokines by G protein-coupled receptors (GPCRs), which are regulated by specific kinases (GRKs). Previous studies have shown a failure of neutrophil migration into infectious focus on sepsis due to chemotactic receptor desensitization via GRKs induced by activation of toll- like receptors (TLRs), TLR2 and TLR4. Despite the absence of activation of TLR9 in dendritic cells have been related to increase survival of septic mice, the role of TLR9 acting directly on neutrophils was not evaluated. We proposed to verify the direct role of TLR9 in the failure of neutrophil migration on sepsis. The TLR9 knockout mice (TLR9-/-) showed high survival to polymicrobial sepsis using cecal ligation and puncture model (CLP). TLR9-/- mice had high neutrophil migration to the focus of infection, low neutrophil sequestration in the lung, as well as, few bacteria in the peritoneal exudates and blood. The activation of TLR9 by oligodeoxinucleotide containing unmethylated dinucleotide CpG (CpG ODN) in neutrophils also reduced chemotaxis toward CXCL2 and the expression of chemokine receptor CXCR2. In addition, neutrophils stimulated with CpG ODN showed increased expression of kinase-related G protein-coupled receptor type 2 (GRK2). Thus, the activation of TLR9 in blood circulating neutrophils is harmful on sepsis by reducing their chemotaxis into the site of the infection by inducing CXCR2 desensitization via GRK2.
214

Characterization of differential Toll-like receptor function in human immune cells and association with susceptibility to recurrent HSV-1 reactivations and gastric cancer

Yang, Chin-An 02 February 2011 (has links)
Toll-like Rezeptoren (TLRs) sind essentielle angeborene Rezeptoren, die konservierte Strukturen von Krankheitserregern oder Gefahrsignale, die von beschädigten Zellen freigesetzt werden, erkennen können. Genetische Variationen in TLRs wie Einzel-Nukleotid-Polymorphismus (SNP) können die Funktion von TLRs beeinträchtigen und erste Studien zeigen, dass dies zu einer erhöhten Anfälligkeit gegenüber Virusinfektionen oder einem erhöhten Krebsrisiko führen kann. In dieser Studie haben wir einen Multicolor-Durchflußzytometrie-Test entwickelt, um die TLR-Funktionen in verschiedenen Subpopulationen unseparierter peripherer mononukleärer Blutzellen (PBMCs) simultan analysieren zu können. Wir konnten beobachten, dass das Ausmaß der TLR-Antworten zwischen den Probanden stark variierte, jedoch über einen Zeitraum von einem Monat gut reproduzierbar war. Zunächst untersuchten wir TLR Reaktionen bei Patienten mit rezidivierenden Herpes labilalis (HL). Im Vergleich zu asymptomatischen Personen war eine HL- Anamnese mit einer signifikant verminderten TLR3-IFN-Gamma-Antwort nach Stimulation mit poly(I:C) in NK Zellen assoziiert. Weitere molekulare Untersuchungen zeigten eine mögliche Beteiligung von TLR3 L412F SNP, welcher die oberflächliche TLR3 Expression und die IFN-Gamma-Antworten in NK-Zellen reduzierte. Einige Studien zeigen, dassTLR1 I602S, ein weiterer sehr verbreiteter SNP, in der Lage ist die TNF-Alpah-Antworten von Monozyten gegen den TLR2/1-Agonisten (Pam3Cys) zu verringern. In der hier vorliegenden Arbeit konnten wir zudem nachweisen, dass TLR1 I602S SNP auch die Funktion von NK-Zellen und CD8+ T-Zellen beeinträchtigt. Wir konnten keine Assoziation zwischen TLR2/1-Defizienz und reaktivierendem HL feststellen. Jedoch konnten wir an einer großen Kohorte von über 326 Patienten zeigen, dass der TLR1 SNP sowohl ein Risikofaktor für Magenkarzinomentstehung als auch für die Metastasierung ist. Zusammenfassend weisen unsere Ergebnisse darauf hin, dass genetische Polymorphismen von TLRs die Funktion von NK-Zellen beeinträchtigen und zu einer erhöhten Anfälligkeit für HSV-1 Erkrankung und Magenkarzinom führen können. / Toll-like Receptors (TLRs) are essential innate receptors which recognize conserved structures of pathogens, or danger signals released from damaged cells. Alterations of TLR responses might result in severe viral infections or a higher risk of cancer. Therefore, development of clinical assays to evaluate TLR functions could provide personalized information about susceptibility to these diseases. Since TLRs are differentially expressed on different subsets of human peripheral blood mononuclear cells (PBMCs), a multi-color flow cytometry-based assay was developed to detect TLR responses of individual cell types simultaneously. We observed that the magnitude of TLR responses largely varied between human subjects, but was highly reproducible over one month. To evaluate the potential role of differences in natural killer (NK) cell TLR response we studied the association of NK cell TLR function and TLR single nucleotide polymorphisms (SNPs) with susceptibility to recurrent herpes labialis (HL) and gastric cancer. Using our assay, impaired TLR3 response of NK cells was found in people with recurrent HL. In addition, we have identified enhanced levels of homozygous TLR3 L412F SNP in people with recurrent HL, which results in lower surface expression and reduced NK cell response to poly(I:C). TLR1 I602S, another common SNP, has been reported to decrease TNF-Alpha responses of monocytes toward TLR2/1 agonist, Pam3CSK4 (Pam3Cys), stimulation. In our study, we found that TLR1 I602S homozygosity also contributes to impaired IFN-Gamma responses of NK cells and CD8+T cells. Although we did not observe an association of TLR2/1 deficiency with recurrent HL, association of TLR1 I602S with risk for primary as well as metastatic gastric cancer was found in a cohort of 326 patients. To sum up, our results suggest that genetic polymorphisms of TLRs can impair TLR function of NK cells, which contribute to the increased susceptibility to HSV-1 diseases and gastric cancer.
215

Genetische Polymorphismen in Toll-like-Rezeptoren, rheumatoide Arthritis und Höhe von Rheumafaktor im Serum

Hamprecht, Axel 27 September 2005 (has links)
Die rheumatoide Arthritis (RA) ist die häufigste entzündliche Gelenkerkrankung der Welt. Sie verläuft meist chronisch-progressiv und kann schließlich zu Gelenkdestruktion und Invalidität führen. Trotz intensiver Forschungen bleibt die Pathogenese der RA weiterhin unklar. Neuere Untersuchungen weisen auf die wichtige Rolle des angeborenen Immunsystems hin, insbesondere der Toll-like-Rezeptoren (TLRs) TLR2 und TLR9. Genetische Polymorphismen in TLR2 und TLR9 könnten daher zur Erkrankung einer RA prädisponieren, davor schützen oder den Verlauf der RA beeinflussen. Zielsetzung dieser Arbeit war es, die Assoziation zwischen RA-Erkrankung, dem Rheumafaktor (RF)-Serostatus und der Höhe des RF im Serum und genetischen Polymorphismen im TLR2- und TLR9-Gen zu analysieren. Zur Untersuchung der TLR9-Polymorphismen T-1237C und T-1486C wurde ein real-time-PCR-basiertes Verfahren am LightCycler (LC) etabliert, das den schnellen Nachweis beider Polymorphismen in einer Reaktion mittels fluoreszenzmarkierter Hybridisierungssonden ermöglicht. Desweiteren wurde ein neues Puffersystem verwendet, das die LC-PCR unter Verwendung einer konventionellen Taq-Polymerase zu erheblich günstigeren Kosten ermöglicht. Die Genotypisierung der DNA von 118 RA-Patienten (89 weiblich, 29 männlich, Durchschnittsalter 56,2 Jahre) und einer geschlechtsgematchten Kontrollgruppe von 118 Personen (Durchschnittsalter 44,1 Jahre) zeigte, dass die TLR9-Polymorphismen T-1486C und T-1237C sowie der TLR2-Polymorphismus G2408A nicht für das Auftreten von RA prädisponieren. Träger des seltenen C-Allels sind signifikant häufiger RF-positiv (p=0,049) und ihre RF-Antikörperspiegel sind höher als bei Patienten, die das C-Allel nicht aufweisen (p=0,023). Der TLR9-Polymorphismus T-1486C könnte daher die Krankheitsausprägung beeinflussen. / Rheumatoid arthritis (RA) is the most common inflammatory joint disease worldwide. It is a chronic progressive disease which can eventually lead to joint destruction and disability. The pathogenesis of RA remains uncertain in spite of the intensive research in this field. Recent data indicate the important role of the innate immune system, especially of the toll like receptors (TLRs) TLR2 and TLR9 in the pathogenesis of RA. Genetic polymorphisms in the TLR2 and TLR9 gene could therefore predispose to RA, protect against it or influence its course. The aim of this work was to analyse the association of RA, the serostatus of rheumatoid factor (RF) and its levels with genetic polymorphisms in the TLR2 and TLR9 gene. A new real time PCR based method was developed on the LightCycler (LC) in order to analyse the TLR9 polymorphisms T-1237C and T-1486C. This method permits the fast detection of both polymorphisms in a single reaction using fluorescence labelled hybridization probes. Furthermore, a new reaction mix was developed which allows the use of a conventional Taq polymerase for the LC-PCR at much lower costs. The genotyping of 118 RA patients (89 female, 29 male; average age 56.2 years) and a control group of 118 healthy individuals (average age 44.1 years) showed that the TLR9 polymorphisms T-1237C and T-1486C and the TLR2 polymorphism G2408A do not predispose to RA disease. The TLR9 polymorphism T-1486C might influence the course of the disease as individuals with the rare C-allele are significantly more frequent RF-positive (p=0.049) and their RF-antibody levels are higher than in patients who do not bear the C-allele (p=0.023).
216

Vias de transdução de sinal do receptor tipo Toll 4 nas células pancreáticas e seus efeitos na secreção e produção de insulina / Toll-like receptor 4 signal transduction pathways in pancreatic cells and their effect on insulin secretion and production

Paladino, Fernanda Vieira 28 August 2012 (has links)
INTRODUÇÃO: O receptor tipo Toll 4 (TLR4) pertencente a uma família de receptores do sistema imune inato, reconhece o padrão molecular de lipopolissacarídeos (LPS), expressos por bactérias Gram negativas. Sua cascata de sinalização, nas células apresentadoras de antígeno, ocorre por duas vias principais: MyD88-dependente, que resulta na ativação de NF-B e na expressão de genes de resposta inflamatória e MyD88-independente, responsável pela ativação dos fatores IRF3 e IRF7, culminando na síntese de interferons e , envolvidos na resposta anti-viral e anti-bacteriana. Células não-imunes, de diversos tecidos, também expressam TLR4, incluindo células pancreáticas murinas e humanas. Devido ao seu papel nos processos inflamatórios, os TLR estão implicados em doenças crônicas como obesidade e diabetes. Estudo anterior do grupo identificou TLR4 como uma molécula que ativa sinais inflamatórios e provoca alterações na homeostase das células . Neste trabalho, investigamos qual via é ativada por LPS e quais os efeitos da expressão do TLR4 na viabilidade celular e na produção de insulina em células murinas. MÉTODOS: Células MIN6 (linhagem celular de insulinoma de camundongo) foram cultivadas em condições de hipo (2,8mM glicose), normo (5,6mM glicose) e hiperglicemia (11,2mM glicose), por 4 dias. Após esse período, foi adicionado LPS (50 ng/mL) por 48h e foram feitas análises por PCR em tempo real, Western Blot, ELISA e citometria de fluxo. RESULTADOS: Os resultados confirmam o aumento de TLR4 em células em condições de hiperglicemia e a via de sinalização ativada por LPS é a via MyD88-dependente, envolvida na produção de citocinas pró-inflamatórias. A via de indução de intérferons tipo 1 está ausente nestas células. Além disso, TLR4 ativado por LPS aumentou secreção de insulina em resposta a glicose, mas não induziu a morte celular. CONCLUSÃO: A expressão de TLR4 em células pancreáticas murinas é induzida em resposta ao aumento da glicemia, constituindo um novo elo entre a agressão à célula causada por altos níveis de glicose e a alteração da função celular induzida por LPS / INTRODUCTION: Toll-like receptor 4 (TLR4) belongs to a family of innate immunity receptors and recognizes the molecular pattern present in lipopolysaccharides (LPS), typical of Gram-negative bacteria. There are two TLR4 signaling pathways, typically in antigen-presenting cells: one is MyD88-dependent, activating NF-kB transcription factor and triggering inflammatory cytokine production and the other is MyD88-independent, leading to activation of IRF3 and IRF-7 and production of interferons e , involved in antiviral and antibacterial immune responses. Non-immune cells in several tissues also express TLR4, including human and murine pancreatic cells. Due to their role in inflammatory processes, TLRs have been implicated in chronic diseases like obesity and diabetes. Our previous study identified TLR4 as a molecule which activates inflammatory signals and induces changes in cell homeostasis. In this study, we investigated which of the TLR4 pathways is activated by LPS and the effects of glucose levels on cell viability and insulin production in a mouse insulinoma cell line. METHODS: MIN6 cells were maintained in low (2,8mM), normal (5,6mM) and high (11,2mM) glucose levels for 4 days, and then incubated with LPS (50 ng/mL) for 48 hours. Analyses were done by real-time PCR, Western Blot, ELISA and flow cytometry. RESULTS: Analysis confirmed increase in TLR4 gene expression in hyperglycemic conditions and showed that the signaling pathway activated by LPS is MyD88-dependent. The interferon induction pathway is absent in these cells. Furthermore, upon activation by LPS, TLR4 impacts on insulin secretion in response to glucose, but without triggering cell death. CONCLUSION: We conclude that TLR4 expression in mouse pancreatic cells is induced in response to increased glucose levels, constituting a new link in the chain of events leading to cell stress caused by high glucose levels with concomitant changes in cell function induced by LPS
217

A proteína de transferência de colesterol esterificado humana protege camundongos da sepse polimicrobiana e atenua a resposta inflamatória em macrófagos estimulados com lipopolissacarídeo / The human cholesteryl ester transfer protein protects mice from polymicrobial sepsis and attenuates the inflammatory response in macrophages stimulated with lipopolysaccharide

Venancio, Tatiana Martins 09 February 2015 (has links)
Sepse é a resposta inflamatória sistêmica decorrente de infecção grave, com alto índice de mortalidade, tornando-se um grave problema de saúde pública. Apesar dos inúmeros estudos realizados em busca de alternativas terapêuticas, o entendimento acerca dos mecanismos envolvidos na doença permanece restrito. A interação entre o metabolismo lipídico e a resposta inflamatória tem sido intensamente investigada. Neste estudo, avaliou-se a influência da proteína de transferência de colesterol esterificado (CETP) - glicoproteína plasmática que promove a transferência de lípides entre lipoproteínas - na resposta inflamatória. Inicialmente, foram comparados camundongos transgênicos para CETP humana (CETP) e controles irmãos não transgênicos (WT) submetidos ao modelo de sepse polimicrobiana de ligadura e perfuração do ceco (CLP), avaliando a taxa de sobrevida e o perfil inflamatório entre os grupos. Em seguida, a resposta inflamatória em macrófagos de peritônio de camundongos estimulados com LPS na ausência ou presença da CETP exógena (CETP humana recombinante) e endógena (macrófagos de animais CETP) foi analisada. Verificou-se que camundongos CETP apresentaram maior taxa de sobrevida, maior migração de linfócitos para o foco infeccioso, menores concentrações plasmáticas de IL-6 e menor expressão proteica do receptor Toll-like 4 (TLR4) e da enzima aciloxiacilo hidrolase (AOAH) no fígado, comparados aos WT. Nos macrófagos, observou-se que a presença da CETP recombinante foi capaz de se ligar ao LPS, pela análise da microscopia confocal, e, em cultura, reduziu de forma dose dependente a captação de LPS, a expressão de TLR4, a ativação do NF-kB (p65) e a secreção de IL-6 para o sobrenadante do cultivo celular. Os dados obtidos com os macrófagos de animais CETP corroboraram, em parte, os encontrados com a utilização da CETP exógena. Houve redução da captação de LPS e da ativação do NF-kB (p65), sem alteração na expressão de TLR4 e secreção de IL-6. Entretanto, apresentaram redução das concentrações de TNF-alfa celular e no sobrenadante de cultura. Dessa maneira, foi possível concluir que a CETP atua como agente modulador da resposta inflamatória induzida pela CLP e em macrófagos estimulados pelo LPS. Esses achados devem ser considerados nas doenças inflamatórias e nos futuros estudos relacionados à inibição da CETP, além de estabelecer novas perspectivas de tratamento da sepse / Sepsis is a systemic inflammatory response due to serious infection with high mortality rate, which has become a serious problem for public health. Despite numerous studies seeking for therapeutic alternatives, the understanding of the mechanisms involved in this disease remains limited. The interaction between lipid metabolism and inflammatory response has been intensively investigated. In the present study it was evaluated the influence of CETP (cholesteryl ester transfer protein) - plasma glycoprotein that promotes the transfer of lipids between lipoprotein - in the inflammatory response. Initially transgenic mice for human CETP (CETP) were compared to non transgenic control mice (WT) after polymicrobial sepsis induced by cecal ligation and puncture (CLP), to determine survival rate and the inflammatory profile between groups. Then, macrophages isolated from peritoneal cavity stimulated with LPS in the presence or absence of exogenous CETP (recombinant human CETP) and endogenous CETP (macrophages from CETP mice) were analyzed. It was found that CETP mice showed a higher survival rate, a greater lymphocyte migration to infectious focus, a lower IL-6 plasma concentration and a decrease in Toll-like receptor 4 (TLR4) and acyloxyacyl hydrolase enzyme (AOAH) protein expression in the liver in comparison to WT mice. In macrophages, recombinant CETP was able to bind to LPS, by confocal microscopy analysis and in cell culture, it was observed that in the presence of the recombinant CETP macrophages presented decreased in LPS uptake, TLR4 expression, NF-kB activation (p65) and IL-6 secretion into the cell culture medium. Furthermore, the results with macrophages from animals CETP corroborate partly with what was found in the exogenous experiments. LPS uptake and NF-kB activation (p65) were reduced, but no difference regarding the expression of TLR4, nor the IL-6 secretion to the cell culture medium. However, the CETP group also showed reduced levels of TNF-alfa both in macrophages and in the culture supernatant. Thus, we conclude that CETP acts as modulator of the inflammatory response induced by CLP and in the macrophages stimulated by LPS. In addition, new therapeutic perspectives could be established
218

Papel do receptor toll-like 9 na falência de migração dos neutrófilos na sepse / The role of toll-like receptor 9 on failure of neutrophil migration during sepsis.

Silvia Cellone Trevelin 20 December 2010 (has links)
O recrutamento de neutrófilos para o sítio da infecção é um evento crucial para o combate aos microrganismos e sobrevivência na sepse. A migração destes polimorfonucleares é dirigida através de um gradiente quimiotático por meio do reconhecimento de quimiocinas por receptores acoplados a proteína G (GPCRs), os quais são regulados por quinases específicas (GRKs). Estudos prévios demonstraram que na sepse ocorre uma falência na migração de neutrófilos para o foco infeccioso em função da dessensibilização de receptores quimiotáticos via GRKs induzida pela ativação de receptores toll-like (TLRs), TLR2 e TLR4. Apesar de a ausência de TLR9 em células dendriticas ter sido relacionada a maior sobrevivência de camundongos sépticos, o papel do TLR9 atuando diretamente em neutrófilos não foi avaliado. Objetivando preencher esta lacuna, propôs-se avaliar o papel direto de TLR9 na falência de migração de neutrófilos na sepse. Os camundongos TLR9-/- apresentaram maior sobrevivência a sepse polimicrobiana avaliada por meio do modelo de ligadura e perfuração do ceco (CLP). A deficiência de TLR9 também acarretou em aumento na migração de neutrófilos para o foco da infecção, menor seqüestro de neutrófilos no pulmão, bem como, menor número de bactérias no lavado peritoneal e sangue. A ativação de TLR9 por oligodeoxinucleotídeo contendo o dinucleotídeo CpG não metilado (ODN CpG) nos neutrófilos reduziu a quimiotaxia destes em direção a quimiocina CXCL2 e expressão do receptor quimiotático CXCR2. Além disso, neutrófilos estimulados com ODN CpG apresentaram aumento na expressão da quinase tipo 2 relacionada a receptores acoplados a proteína G (GRK2). Dessa forma, a ativação de TLR9 em neutrófilos circulantes no sangue é prejudicial na sepse por reduzir a quimiotaxia destes para o foco da infecção ao induzir a dessensibilização de CXCR2 via GRK2. / The recruitment of neutrophils to the site of infection is a crucial event for combating the microorganisms and survival on sepsis. The neutrophil migration is directed by a chemotactic gradient through the recognition of chemokines by G protein-coupled receptors (GPCRs), which are regulated by specific kinases (GRKs). Previous studies have shown a failure of neutrophil migration into infectious focus on sepsis due to chemotactic receptor desensitization via GRKs induced by activation of toll- like receptors (TLRs), TLR2 and TLR4. Despite the absence of activation of TLR9 in dendritic cells have been related to increase survival of septic mice, the role of TLR9 acting directly on neutrophils was not evaluated. We proposed to verify the direct role of TLR9 in the failure of neutrophil migration on sepsis. The TLR9 knockout mice (TLR9-/-) showed high survival to polymicrobial sepsis using cecal ligation and puncture model (CLP). TLR9-/- mice had high neutrophil migration to the focus of infection, low neutrophil sequestration in the lung, as well as, few bacteria in the peritoneal exudates and blood. The activation of TLR9 by oligodeoxinucleotide containing unmethylated dinucleotide CpG (CpG ODN) in neutrophils also reduced chemotaxis toward CXCL2 and the expression of chemokine receptor CXCR2. In addition, neutrophils stimulated with CpG ODN showed increased expression of kinase-related G protein-coupled receptor type 2 (GRK2). Thus, the activation of TLR9 in blood circulating neutrophils is harmful on sepsis by reducing their chemotaxis into the site of the infection by inducing CXCR2 desensitization via GRK2.
219

Analysis of Toll-Like Receptor 4 Signal Transduction and IRF3 Activation in the Innate Immune Response: A Dissertation

Rowe, Daniel C. 21 June 2006 (has links)
Over the last decade, the innate immune system has been the subject of extensive research. Often overlooked by the robustness and specificity of the adaptive immune system, the innate immune system is proving to be just as complex. The identification of several families of pattern recognition receptors (PRRs) has revealed an ancient yet multifaceted system of proteins that are responsible for initiating host defense. A wide array of pathogens, from virus to bacteria, is detected using this assortment of receptors. One such family, the Toll-like receptors (TLRs), has been at the forefront of this research. To date, 10 TLRs have been described in the human genome. Activation of TLRs leads to the induction of immune-related genes that ultimately control the response of the host. However, the signaling pathways emanating from activated TLRs and other PRRs are not fully understood. In particular, the pathway leading to the activation of interferon regulatory factor 3 (IRF3), a transcription factor crucial for the induction of type I interferon, remains undefined. IRF3 activation occurs as the consequence of viral infection and through the activation of TLRs 3 and 4 by dsRNA and lipopolysaccharide (LPS), respectively. The focus of this research is to describe components of the IRF3 activation pathway, partly through the analysis of TLR signal transduction. IRF3 normally resides in the cytoplasm of cells. Upon infection with certain viruses and bacteria, IRF3 is activated though phosphorylation at its C-terminus. Phosphorylated IRF3 homodimerizes and associates with co-activators CBP-p300. After translocating to the nucleus, the activate IRF3 complex induces the activation of type 1 interferon and interferon related genes. Little is known about the pathways that lead to the activation of IRF3, especially the kinases involved. In this study we report that the non-canonical IкB kinase homologues, IкB kinase epsilon (IKKε) and TANK-binding kinase-1 (TBK1), which were previously implicated in NF-кB activation, are also essential components of the IRF3 signaling pathway. In particular, mouse embryonic fibroblasts from TBK1 deficient mice fail to activate IRF3 in response to both viral infection and stimulation with LPS or poly (IC), a dsRNA analog. Thus, both IKKε and TBK1 play a critical role in innate immunity and host defense. In addition to viral infection, IRF3 activation also occurs via the activation of TLR3 and 4. TLRs signal through a subfamily of Toll-IL-1-Resistance (TIR) domain containing adapter molecules. One such adapter, MyD88, is crucial for all TLRs, with the exception of TLR3. MyD88 participates in a signal transduction pathway culminating in the activation of the transcription factor NF-кB. Studies from MyD88-deficient mice reveal that both TLR3 and 4 still are capable of activating NF-кB, although with slightly delayed kinetics. Another aspect of the MyD88-independent signal transduction pathway is the activation of IRF3. A second TIR domain containing adapter molecule called Mal/Tirap was discovered and originally thought to mediate the MyD88-independent pathway. However, Mal-deficient mice were found to be defective in both TLR2 and 4 mediated NF-кB activation. We hypothesized that other TIR domain containing adapters could mediate this MyD88-independent pathway of TLR3 and 4 leading to the activation of IRF3. Two additional TIR adapters were discovered, TRIF and TRAM. TRIF was shown to mediate TLR3 signal transduction. In this study, we report that both TRIF and TRAM mediate the activation of the MyD88-independent pathway in response to LPS/TLR4 activation. Unlike any of the other known TIR domain containing adapters, TRAM appears to be restricted to the LPS/TLR4 activation pathway while TRIF plays a role in both TLR3 and TLR4 pathways leading to IRF3 target gene expression. Our studies revealed that TRAM could be acting upstream of TRIF in the LPS/TLR4 pathway. To this end, we sought to determine the localization of TRAM within the cell. We found that TRAM localizes to the plasma membrane. TRAM localization is the result of myristoylation since mutation of the predicted myristoylation site (G2A) resulted in the re-distribution of TRAM from the membrane into the cytoplasm. Reconstitution of TRAM-deficient macrophages with TRAM G2A is unable to rescue LPS/TLR4 signal transduction. Thus, myristoylation and membrane association of TRAM are critical for LPS/TLR4 signal transduction. The data generated in this dissertation extends our understanding of the signaling pathways of the innate immune system. Indeed, the molecules and pathways described herein could prove to be beneficial targets for ameliorating symptoms of disease, both autoimmune and pathogen-associated. Finally, the research described here will spur further insight into the complex signaling pathways of a once ignored arm of the immune system.
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A proteína de transferência de colesterol esterificado humana protege camundongos da sepse polimicrobiana e atenua a resposta inflamatória em macrófagos estimulados com lipopolissacarídeo / The human cholesteryl ester transfer protein protects mice from polymicrobial sepsis and attenuates the inflammatory response in macrophages stimulated with lipopolysaccharide

Tatiana Martins Venancio 09 February 2015 (has links)
Sepse é a resposta inflamatória sistêmica decorrente de infecção grave, com alto índice de mortalidade, tornando-se um grave problema de saúde pública. Apesar dos inúmeros estudos realizados em busca de alternativas terapêuticas, o entendimento acerca dos mecanismos envolvidos na doença permanece restrito. A interação entre o metabolismo lipídico e a resposta inflamatória tem sido intensamente investigada. Neste estudo, avaliou-se a influência da proteína de transferência de colesterol esterificado (CETP) - glicoproteína plasmática que promove a transferência de lípides entre lipoproteínas - na resposta inflamatória. Inicialmente, foram comparados camundongos transgênicos para CETP humana (CETP) e controles irmãos não transgênicos (WT) submetidos ao modelo de sepse polimicrobiana de ligadura e perfuração do ceco (CLP), avaliando a taxa de sobrevida e o perfil inflamatório entre os grupos. Em seguida, a resposta inflamatória em macrófagos de peritônio de camundongos estimulados com LPS na ausência ou presença da CETP exógena (CETP humana recombinante) e endógena (macrófagos de animais CETP) foi analisada. Verificou-se que camundongos CETP apresentaram maior taxa de sobrevida, maior migração de linfócitos para o foco infeccioso, menores concentrações plasmáticas de IL-6 e menor expressão proteica do receptor Toll-like 4 (TLR4) e da enzima aciloxiacilo hidrolase (AOAH) no fígado, comparados aos WT. Nos macrófagos, observou-se que a presença da CETP recombinante foi capaz de se ligar ao LPS, pela análise da microscopia confocal, e, em cultura, reduziu de forma dose dependente a captação de LPS, a expressão de TLR4, a ativação do NF-kB (p65) e a secreção de IL-6 para o sobrenadante do cultivo celular. Os dados obtidos com os macrófagos de animais CETP corroboraram, em parte, os encontrados com a utilização da CETP exógena. Houve redução da captação de LPS e da ativação do NF-kB (p65), sem alteração na expressão de TLR4 e secreção de IL-6. Entretanto, apresentaram redução das concentrações de TNF-alfa celular e no sobrenadante de cultura. Dessa maneira, foi possível concluir que a CETP atua como agente modulador da resposta inflamatória induzida pela CLP e em macrófagos estimulados pelo LPS. Esses achados devem ser considerados nas doenças inflamatórias e nos futuros estudos relacionados à inibição da CETP, além de estabelecer novas perspectivas de tratamento da sepse / Sepsis is a systemic inflammatory response due to serious infection with high mortality rate, which has become a serious problem for public health. Despite numerous studies seeking for therapeutic alternatives, the understanding of the mechanisms involved in this disease remains limited. The interaction between lipid metabolism and inflammatory response has been intensively investigated. In the present study it was evaluated the influence of CETP (cholesteryl ester transfer protein) - plasma glycoprotein that promotes the transfer of lipids between lipoprotein - in the inflammatory response. Initially transgenic mice for human CETP (CETP) were compared to non transgenic control mice (WT) after polymicrobial sepsis induced by cecal ligation and puncture (CLP), to determine survival rate and the inflammatory profile between groups. Then, macrophages isolated from peritoneal cavity stimulated with LPS in the presence or absence of exogenous CETP (recombinant human CETP) and endogenous CETP (macrophages from CETP mice) were analyzed. It was found that CETP mice showed a higher survival rate, a greater lymphocyte migration to infectious focus, a lower IL-6 plasma concentration and a decrease in Toll-like receptor 4 (TLR4) and acyloxyacyl hydrolase enzyme (AOAH) protein expression in the liver in comparison to WT mice. In macrophages, recombinant CETP was able to bind to LPS, by confocal microscopy analysis and in cell culture, it was observed that in the presence of the recombinant CETP macrophages presented decreased in LPS uptake, TLR4 expression, NF-kB activation (p65) and IL-6 secretion into the cell culture medium. Furthermore, the results with macrophages from animals CETP corroborate partly with what was found in the exogenous experiments. LPS uptake and NF-kB activation (p65) were reduced, but no difference regarding the expression of TLR4, nor the IL-6 secretion to the cell culture medium. However, the CETP group also showed reduced levels of TNF-alfa both in macrophages and in the culture supernatant. Thus, we conclude that CETP acts as modulator of the inflammatory response induced by CLP and in the macrophages stimulated by LPS. In addition, new therapeutic perspectives could be established

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