Chemokine Induction by Dengue Virus Infection: Mechanisms and the Role of Viral Proteins: a Dissertation

Medin, Carey L.

26 July 2005

The focus of this thesis is the role of dengue virus in the induction of chemokines. Dengue virus (DENV) occurs as four distinct serotypes, called DENV 1,2,3,and 4. Symptomatic DENV infection ranges from a self limited febrile illness, dengue fever (DF), to a more severe disease, dengue hemorrhagic fever/dengue shock syndrome (DHF/DSS). DHF is characterized by increased capillary permeability resulting in decreased plasma volume, which may be accompanied by hemorrhagic manifestations. Many factors including T cell cross reactivity, viral burden, antibody dependent enhancement and induction of chemokines and cytokines have been reported in DHF and may play a role in the pathogenesis of DENV infection. Cytokines have been shown to modulate endothelial cell permeability [1-3]. Recent studies have shown that DENV-infected endothelial cells secrete the chemokine, interleukin (IL)-8 in vitro [4]. In addition, the permeability of an endothelial cell monolayer was found to be increased by interleukin-8 (IL-8) in vitro[5]. This thesis examines the effects of DEN2V infection on the induction of chemokines, and specifically, which DEN2V viral protein(s) are involved in the induction of IL-8. The chemokine induction profile following DEN2V infection was initially assessed in various cell lines that may represent potential targets in vivo, including monocytes, liver cells and endothelial cells. We hypothesized that distinct profiles of chemokine secretion can be induced by DEN2V infection of various cell types in vitro. We found RANTES (Regulated upon Activation, Normal T cell Expressed and Secreted) and IL-8 were induced in two of the five cell lines. DEN2V infection of primary monocyte-derived dendritic cells induced RANTES and IL-8 along with macrophage inflammatory protein-1α (MIP-1α), MIP-1β and monocyte chemoattractant protein-1 (MCP-1) but at an earlier time post infection than in the cell lines. These results showed that DEN2V infection induces distinct chemokine profiles in many cell types. In addition, monocytic-derived DCs can secrete chemokines upon infection with DEN2V. Characterization of the signaling pathways induced by DEN2V revealed that DEN2V induction of chemokines in human embryonic kidney (HEK293A) cells is mainly through the nuclear factor kappaB (NFκB) pathway, as previously reported for endothelial cells and 293T cells [4,6]. Alternatively, the liver cell line (HepG2) activated mainly activator protein (AP)-l. In addition, DENV infection can induce the activation of the interferon-stimulated response element (ISRE) driven promoter. IL-8 has been shown to have multiple effects on the immune system ranging from recruiting cells to the site of infection to countering the antiviral effects of type I interferon (IFN) [7,8]. Previous reports have shown that viral proteins can induce chemokines such as seen with IL-8 induction with the nonstructural protein 5A (NS5A) and core proteins from hepatitis C virus [9,10]. We hypothesized that protein(s) from DENV could induce chemokine production. The expression of DENV proteins was analyzed for effects on IL-8 and RANTES production in HEK293A cells. The effects of viral replication on IL-8 and RANTES induction were also analyzed using a DENV replicon that contains genes for the capsid protein and the nonstructural proteins. Transfection of plasmids expressing NS5 or the DEN2V replicon induced the expression and secretion of IL-8 but not RANTES. We attributed the lack of RANTES induction to the inability of NS5 or the DEN2V replicon to induce transcription from the ISRE driven promoter. We also found that NS5 and the DEN2V replicon induced IL-8 mainly through the CCAAT/enhancer binding protein (c/EBP) and AP-1 pathways. The profile of transcription factor activation is different from what was seen with DENV infection of HEK293A cells and suggests that the transient expression of the NS5 protein and the replication and/or translation of the DEN2V genome use different pathways than viral infection to induce IL-8. In addition, we found that the expression of prM-E, known to produce virus-like particles, could induce IL-8 secretion and activate transcription from the IL-8 promoter. As with the expression of NS5, RANTES was not induced. Analysis of the transcription factors involved in IL-8 induction using luciferase reporter constructs indicated that expression of prM-E induced transcription of IL-8 through NFκB, AP-1 and c/EBP, similar to what was seen with DEN2V infection of HEK293A cells. These results suggest that production of virions or virus-like particles induce IL-8 but that another mechanism in the viral life cycle is responsible for the induction of RANTES expression by DEN2V infection. We were also interested in the effects of drugs that have been used previously to inhibit cytokine or chemokine production on chemokine induction during DEN2V infection. We hypothesized that pharmacological inhibitors of cytokines will inhibit secretion of chemokines in DEN2V infected cells. We found that the pharmacological inhibitors SB203580 and rolipram enhanced chemokine production in a DEN2V infected liver cell line (HepG2), whereas dexamethasone had the same effect in a kidney epithelial cell line (HEK293A). We conclude that drugs that inhibit signaling pathways involved in cytokine production in other experimental systems can have variable effects on chemokine induction in different cell types during DEN2V infection. The data generated in this thesis extend our understanding of how DEN2V manipulates the host cell during viral infection to produce chemokines and perhaps enhance viral propagation and dissemination through the induction of IL-8. In addition, this study provides insight into the variable effects pharmacological drug treatment may have on disease progression during DENV infection. These results increase our understanding of DENV pathogenesis and may be helpful in finding better strategies for treatment and prevention.

Chemokines

Dengue

Interleukin-8

RANTES

Amino Acids, Peptides, and Proteins

Biological Factors

Life Sciences

Medicine and Health Sciences

Viruses

Neuroinflammation & Insulinorésistance : contribution au développement physiopathologique de la maladie d’Alzheimer / Neuroinflammation & Insulinoresistance : involvement in pathophysiological development of Alzheimer Disease

Marciniak, Elodie

14 December 2015

La maladie d’Alzheimer (MA) est une maladie neurodégénérative caractérisée d’un point de vue anatomopathologique par une accumulation extracellulaire de peptides amyloïdes et d’une dégénérescence neurofibrillaire (DNF), résultant de l’agrégation intraneuronale de protéines Tau hyper-et-anormalement phosphorylées. D’autres déterminants sont également associés à la MA dont une neuroinflammation chronique et une insulinorésistance centrale qui contribueraient tous deux au développement des lésions ainsi qu’aux troubles synaptiques et mnésiques associés.La neuroinflammation observée dans la MA est caractérisée par une activation des cellules gliales, une infiltration lymphocytaire ainsi que par la libération de médiateurs inflammatoires solubles dont les chimiokines. Le CCL3 est une chimiokine hautement dérégulée dans le cerveau des patients de MA. Dans notre laboratoire, nous avons montré que dans un modèle de DNF, le CCL3 était le facteur pro-inflammatoire le plus affecté au niveau hippocampique laissant ouverte l’hypothèse d’un rôle dans les dysfonctions mnésiques associées à la pathologie Tau. Pour aborder cette question, nous avons précisément évalué l’impact du CCL3 sur le fonctionnement synaptique hippocampique et sur les fonctions mnésiques. Nos travaux montrent que l’application de CCL3 sur des tranches d’hippocampe entraine une diminution des activités basales ainsi que de la potentialisation à long terme (LTP) sans altérer le fonctionnement présynaptique ni la dépression synaptique à long terme (LTD). Par ailleurs, l’élévation intracérébrale de CCL3 par injections intracérébroventriculaires sub-chroniques affecte également la transmission synaptique basale et la LTP ainsi que la mémoire spatiale à court terme et la mémoire à long terme. La réversion de ces altérations par le Maraviroc permet de conclure que l’effet néfaste du CCL3 est dépendant du récepteur CCR5. Ainsi, ces travaux soulignent l’importance du CCL3 dans la physiopathologie de la MA, notamment en lien avec la DNF.L’insulinorésistance observée dans les cerveaux de patients atteints de la MA est connue pour favoriser le développement des lésions caractéristiques et est suggérée comme participant aux atteintes synaptiques et mnésiques. Cependant les causes de cette insulinorésistance centrale sont peu connues. Quelques études montrent que les oligomères d’Aβ, le diabète de type II ou même la neuroinflammation sont susceptibles de conduire à une insulinorésistance centrale. Néanmoins, à ce jour aucune relation n'a été établie avec la protéine Tau. La seconde partie de ce travail s’est attachée à étudier le rôle de la protéine Tau dans la régulation de la réponse centrale à l’insuline. Diverses expériences réalisées in vitro et in vivo montrent que la surexpression de la protéine Tau induit une augmentation de la sensibilité neuronale à l’insuline alors que la délétion de Tau aboutit à l’effet inverse. Cette régulation semble être liée à une interaction entre la protéine Tau et PTEN, une phospholipase inhibitrice de la signalisation de l’insuline. L’interaction entre Tau et PTEN réduirait l’activité de cette dernière, favorisant de ce fait l’action de l’insuline au niveau central. Par ailleurs, des données physiologiques indiquent que cette régulation de la signalisation centrale de l’insuline pourrait avoir une répercussion sur la régulation de l’homéostasie énergétique. En ce sens, la délétion de la protéine Tau induit une prise de poids, une hyperinsulinémie et une glucointolérance périphérique. Ces données proposent donc une nouvelle fonction de la protéine Tau dans la signalisation neuronale et le métabolisme. Cette perte de fonction dans la MA pourrait expliquer les mécanismes d’insulinorésistance centrale liés à la DNF.En conclusion, nos données mettent en évidence deux mécanismes liant la pathologie Tau aux atteintes mnésiques, l’un passant par la production de la chimiokine CCL3, l’autre impliquant une résistance neuronale à l’insuline. / Alzheimer’s disease (AD) is a neurodegenerative disorder characterized by extracellular amyloid deposits and intraneuronal neurofibrillary tangles, made of aggregated and abnormally hyperphosphorylated Tau proteins. Other components are also involved in AD pathophysiology, including chronic neuroinflammation and central insulinoresistance that would contribute both to the development of Alzheimer lesions as well as associated synaptic and memory impairments.Neuroinflammation observed in AD is characterized by glial cell activation, lymphocyte infiltration, and the release of soluble inflammatory mediators including chemokines. CCL3 is a highly upregulated chemokine in the brain of AD patients. In our lab, we have shown, in a mouse model of Tau pathology, that hippocampal CCL3 was largely upregulated and, thus, we made the assumptions that such increase could play a key-role in the memory dysfunctions associated with Tau pathology. To address to this question, we precisely evaluated the impact of CCL3 upon hippocampal synaptic activity and memory function. Our data show that CCL3 application on hippocampal slices induces a significant decrease of basal synaptic activity and long term potentiation (LTP) impairment without affecting presynaptic activity and long term depression (LTD). Further, intracerebral elevation of CCL3 by sub-chronical intracerebroventricular injections was also found to impact hippocampal basal synaptic activity and LTP but also short term spatial memory and long term memory. Reversion of these alterations by Maraviroc finally suggests that CCL3 deleterious effects are CCR5 dependent. Overall, these studies show the important role of CCL3 towards plasticity and memory as well as in AD physiopathology.Besides chronic inflammation, insulinoresistance observed in AD brain is suggested to favor the development of amyloid and Tau lesions but also to participate to synaptic impairments underlying memory loss. However, origins of the brain insulinoresistance described in AD are unclear. Previous studies ascribed central insulin-resistance to Aβ oligomers, type II diabetes or even neuroinflammation. So far, no relationship has been established with Tau protein. The aim of the second part of the present thesis was evaluate the potential role of Tau protein towards the regulation of central insulin sensitivity. Various experiments performed in vitro and in vivo show that Tau favors the neuronal response to insulin, whereas Tau deletion favors insulin-resistance. This regulation seems to be related to an interaction between Tau and PTEN, a phospholipase inhibiting insulin signaling, which results in a reduced PTEN activity, itself favoring insulin pathway activation. Regulation of brain insulin signaling is known to modulate energy homeostasis, food intake and weight gain. In line with the idea that Tau protein modulates insulin signaling, we found that Tau deletion induces weight gain, hyperinsulinemia and glucointolerance. Together, these data provide a new function for Tau in the control of neuronal signaling and peripheral metabolism. These data also highlight that the loss of Tau function in AD might explain at last in part the central insulinoresistance described as “type 3 diabetes”.In conclusion, our data highlight two mechanisms linking Tau pathology and memory deficits, one through the detrimental effect of the chemokine CCL3 and the other involving neuronal insulin resistance.

Maladie d'Alzheimer

Insulinorésistance

Métabolisme

Mémoire

Protéine Tau

Plasticité neuronale

Chimiokine CCL3

Neuroinflammation

Alzheimer's disease

Chemokines

Neuroinflammation

Tau protein

Secretion from the Leishmania flagellum as a potential mechanism of virulence factor delivery

Makin, Laura

January 2017

Protozoa of the Leishmania genus are transmitted between mammalian hosts by the sandfly and cause the neglected tropical disease leishmaniasis. Upon injection into the mammalian host by the sandfly promastigote-form parasites are phagocytosed by macrophages, where they differentiate into amastigotes. Although many virulence factors are known to modulate macrophage signalling pathways to favour infection, the delivery mechanisms are largely unknown. During differentiation to amastigotes the promastigote flagellum shortens dramatically and the fate of the excess flagellar membrane is unknown. Here we investigate the possibility that during Leishmania mexicana differentiation, shedding of the flagellar membrane is a source of extracellular vesicles (EVs) which provide a virulence factor delivery mechanism. The kinetics and structural mechanisms of EV release from promastigotes were investigated by live cell imaging and by measuring the concentration of shed EVs. Isolated EVs from a differentiating parasite culture or a control promastigote parasite culture were analysed by fluorescence and electron microscopy and mass spectrometry. To study the biological effects of EVs, macrophages were exposed to isolated EVs or live promastigotes and cytokine secretion was quantified by ELISA. An LPG1 null mutant was used to assess the contribution of virulence factor lipophosphoglycan (LPG) to the observed effects. Known protein virulence factors and LPG are present in L. mexicana EV fractions as well as known flagellar proteins. We show that there is a link between L. mexicana flagellar shortening and EV release, which is a recently discovered phenomenon in Chlamydomonas and mammalian cell research. We find that isolated EVs and live promastigotes induce changes in secreted cytokine levels from human and murine macrophages, including a substantial and previously unreported suppression of CXCL10, a chemokine which plays a protective role in Leishmania infection. LPG contributes to the effects observed on cytokine production, and EVs may be an important delivery mechanism for LPG.

Exploration de nouvelles approches pour les études de RCPG au niveau moléculaire : application aux récepteurs de chimiokines / Exploring new approaches for GPCR studies at the molecular level : application to chemokine receptors

Siauciunaite-Gaubard, Lina

15 May 2012

Les récepteurs de chimiokines sont des régulateurs essentiels de la migration cellulaire dans le cadre de la surveillance immunitaire, et le développement. Les récepteurs CCR5 et CXCR4 sont de plus spécifiquement impliqués dans les métastases cancéreuses et l'infection par le VIH. Nous avons développé un système permettant de sur-exprimer ces deux RCPGs. Afin de s'affranchir des problèmes de toxicité inhérents à l'expression des protéines membranaires en bactérie notre approche de production consiste à adresser les protéines vers les corps d'inclusion d'E. coli grâce à une fusion protéique N-terminale permettant de hauts niveaux d'expression. Après purification en conditions dénaturantes, les protéines sont alors repliées en présence de surfactants originaux, les amphipoles. La validation de cette nouvelle approche pour les récepteurs des chimiokines représente un des objectifs principaux de ce travail. Afin de tester la fonctionnalité des protéines repliées, une série d'outils a été développée : des versions modifiées des chimiokines ont été produites (RANTES pour CCR5 et SDF 1a pour CXCR4). La fonctionnalité des chimiokines a été évaluée au niveau moléculaire et cellulaire. L'interaction entre le récepteur replié en amphipole et son ligand a été testé par résonance de plasmons de surface (SPR). Différents types de surfaces fonctionalisées avec le récepteur de chimiokine replié en amphipole ont été explorés au cours de ce travail. A la fin de ce projet, la production des chimiokines et de leur récepteur a été mise au point. L'accès à ces outils ouvre la voie à de futures études moléculaires telles que la compréhension de la dimérisation du récepteur ou la détermination de la stoechiométrie du complexe. / Chemokine receptors are critical regulators of cell migration in the context of immune surveillance, inflammation and development. The GPCRs (G protein-coupled receptors) CCR5 and CXCR4 are specifically implicated in cancer metastasis and HIV-1 infection. An expression system to over-express these two GPCRs was developed. To overcome the toxicity problem of membrane protein expression in bacterial system, the production approach consists in targeting the proteins towards E. coli inclusion bodies thanks to a N-terminal fusion allowing a high yield expression. After purification under denaturing conditions, these GPCRs were then folded using original polymeric surfactants: the amphipols. The validation of this new approach for the chemokine receptor production is one of the goals of this work. In order to assess the functionality of the folded proteins, series of tools have been developed: engineered chemokine ligands (RANTES for CCR5 and SDF1a for CXCR4) were produced. The functionality of chemokines was evaluated at cellular and molecular levels. Interaction between the receptor folded in amphipols and its ligand was evaluated using Surface Plasmon Resonance (SPR) technique. Several types of surfaces, functionalized with the chemokine receptor/amphipol complex have been explored in this work. At the end of this project the productions of chemokines and their receptors has been set up. These established tools open the way to future studies, at the molecular level, in order to, for instance, investigate receptor dimerization and complex stoichiometry.

RCPG

Recepteurs de chimiokines

Chimiokines

Renaturation des RCPG

Amphipoles

Resonance de Plasmons de Surface

GPCR

Chemokine receptors

Chemokines

GPCR folding

Amphipols

Surface Plasmon Resonance

Ativa??o local da rota da quinurenina por moduladores inflamat?rios durante a meningite bacteriana.

Coutinho, Leonam Gomes

18 March 2008

Made available in DSpace on 2014-12-17T15:18:09Z (GMT). No. of bitstreams: 1 LeonamGC.pdf: 218692 bytes, checksum: 002840894937241c14e673ee875d7524 (MD5) Previous issue date: 2008-03-18 / Conselho Nacional de Desenvolvimento Cient?fico e Tecnol?gico / Activation of the kynurenine (KYN) pathway (KP) by modulators of immune system has been observed during several neurological diseases. Here we assessed the association of chemo-/cytokine levels with the concentration of KP metabolites in cerebrospinal fluid (CSF) and plasma samples from patients with bacterial meningitis (BM). All samples were collected from 42 patients diagnosed with acute bacterial meningitis (ABM), aseptic meningitis, tuberculous meningitis and patients without infection neurological disorders. CSF and plasma concentration of metabolites from the KP was assessed by high pressure liquid chromatography (HPLC) and cytokines and chemokines by Bio-plex 200 suspension array system. Concentrations of the KP metabolites KYN and kynurenic acid (KYNA) were significantly higher in CSF of patients with ABM compared to other groups. Tryptophan (TRP), anthranilic acid (AA), 3-hydroxykynurenine (3HK) and 3-hydroxyanthranilic acid (3HAA) did not show statistical significance, although some of them presented a good accumulation during ABM. The expression of TNF-alpha, IL-6, IL-1beta, IFN-gamma, IL-10, IL-1 receptor antagonist (IL-1Ra), MIP-1alpha, MIP-1beta, MCP-1 and G-CSF was about 100-fold higher in CSF from ABM patients than other infected groups. In all CSF and plasma samples, the concentration of IL-2, IL-12(p70), IL-4, IL-8 and GM-CSF was not significant. ABM still showed significant concentrations of IL-6, IL-10, IL-1Ra and MCP-1 in plasma samples. Based on the comparison of KP metabolites concentrations between plasma and CSF samples we conclude that the activation of the tryptophan pathway upon BM occurs within the brain. This increase in KP metabolites is most due to activation of the KP by molecules as IFN-gamma and TNF-alpha in response to infection. / A ativa??o da rota da quinurenina por moduladores do sistema imune tem sido observada durante diversas doen?as neurol?gicas. Neste trabalho foi avaliado a associa??o entre os n?veis de citocinas e quimiocinas com a concentra??o dos metab?litos da rota da quinurenina ( Kynurenine pathway KP) em amostras de l?quor e plasma de pacientes com meningite bacteriana. Todas as amostras foram coletadas de 42 pacientes hospitalizados com o diagn?stico de meningites bacteriana aguda, tubercul?sica, ass?ptica e pacientes cujo diagn?stico excluiu infec??o no sistema nervoso central. As concentra??es dos metab?litos da quinurenina foram avaliadas pela cromatografia l?quida de alta press?o enquanto os n?veis de citocinas e quimiocinas foram medidos pelo Bio-plex 200 suspension array system. Concentra??es de quinurenina e ?cido quinur?nico foram significativamente mais elevadas no l?quor de pacientes com meningite bacteriana aguda do que nos outros grupos. Ainda no l?quor, os n?veis de triptofano, ?cido antran?lico, 3-hidroxiquinurenina e ?cido 3-hidroxiantran?lico n?o mostraram signific?ncia estat?stica, embora alguns deles apresentaram um bom ac?mulo durante meningite bacteriana aguda. No l?quor dos pacientes com meningite bacteriana foram observados n?veis mais elevados de TNF-alfa, IL-6, IL-1beta, IFN-gama, IL-10, IL-1Ra, MIP-1alpha, MIP-1beta, MCP-1 e G-CSF do que os outros grupos infectados. Em todas as amostras, as concentra??es de IL-2, IL-12(p70), IL-4, IL-8 e GM-CSF n?o variaram significativamente. No grupo com meningite bacteriana aguda foram tamb?m observadas elevadas concentra??es de IL-6, IL-10, IL-1Ra e MCP-1 no plasma. Baseado na compara??o das concentra??es dos metab?litos da via quinurenina no l?quor e no plasma, conclui-se que a ativa??o desta via metab?lica durante a meningite ocorre primordialmente dentro do c?rebro. O aumento na concentra??o dos metab?litos da quinurenina durante a infec??o deve-se ativa??o da enzima idoleamina 2,3 dioxigenase por prote?nas da resposta imune hospedeira principalmente pelo IFN-gama, IL1beta e TNF-alfa.

Meningite bacteriana

Rota da quinurenina

Citocinas

Quimiocinas

Bacterial meningitis

Kynurenine pathway

Cytokines

Chemokines

Změny endokrinní funkce a zánětlivého profilu tukové tkáně a periferních monocytů u pacientů s obezitou: vliv fyzické aktivity a bariatrické chirurgie / The changes in endocrine function and inflammatory profile of adipose tissue and peripheral monocytes of patients with obesity: the influence of physical activity and bariatric surgery

Trachta, Pavel

January 2017

(EN) Research in the field of obesity, diabetes mellitus and their complications in recent years is increasingly focused on pathophysiological mechanisms of their onset and potential prevention and treatment. The aim of the present work was to evaluate the effects of two different interventions - sleeve gastrectomy and physical activity - on anthropometric, biochemical, hormonal parameters and mRNA expression of proinflammatory factors in subcutaneous adipose tissue along with mRNA expression in peripheral blood monocytes in patients who underwent sleeve gastrectomy. A total of 15 obese women with hypertension were included into the physical activity study. These patients underwent a 3-month training program, which included 30 minutes of aerobic exercise three times a week. 13 obese women were included into sleeve gastrectomy study and were followed-up for 2 years after surgery. Our results indicate that in both studies obese groups had at baseline significantly increased mRNA expression of proinflammatory cytokines, adipokines, chemokines and chemokine receptors relative to control groups. Both interventions decreased body weight and low-grade inflammation. Physical activity had no significant effect on blood pressure, lipid profile and mRNA expression of the components of the renin-...

Avaliação funcional de NF-κB em células dendríticas de pacientes com câncer de mama. / Functional evaluation of NF-­κB in dendritic cells of breast cancer patients.

Isabella Katz Migliori Leão de Moura

18 April 2016

Considerando que processos cruciais de diferenciação e maturação das células dendríticas (DCs) são regulados pelo fator de transcrição nuclear kappa B (NF-&#954;B), nos propusemos a estudar esta via em DCs derivadas de monócitos de pacientes com câncer de mama, partindo da hipótese de que alterações desta via contribuam, nesses indivíduos, para a geração de DCs com fenótipo e função alterados, levando ao escape tumoral. A análise da presença de NF-&#954;B no núcleo de monócitos, DCs imaturas (iDCs) e maduras indicou que as pacientes falham em modular tal fator de transcrição, de modo que a quantidade de NF-&#954;B no núcleo de iDCs de pacientes supera os níveis encontrados em controles, fenômeno possivelmente decorrente de alterações nas proteínas inibidoras do NF-&#954;B em pacientes. Observou-se menor frequência de células CD86+, CD83+ e HLA-DR+ (p < 0,05) ao final das culturas das pacientes, e aumento na concentração de IL-8 no sobrenadante das culturas. Coletivamente, estes dados corroboram a hipótese formulada. / Considering that crucial processes of differentiation and maturation of dendritic cells (DCs) are regulated by nuclear factor kappa B (NF-&#954;B), we proposed to study this pathway in monocyte-derived DCs from breast cancer patients, based on the hypothesis that alterations in such pathway may contribute in these individuals to the generation of DCs having phenotypic and functional changes, leading to tumor escape. The analysis of the presence of NF-&#954;B in the nucleus of monocytes, immature and mature DCs indicated that patients fail to modulate this transcription factor, so that the amount of NF-&#954;B in the nucleus of iDCs from patients exceeds levels found in controls, a phenomenon possibly due to alterations in inhibitory proteins of NF-&#954;B in patients. It was also observed diminished frequency of CD86+, CD83+ and HLA-DR+ cells (p <0.05) at the end of the patients cultures, as well as increased IL-8 concentration in the culture supernatants. Collectively, these data support the hypothesis previously formulated.

Fatores  de  transcrição

Células  dendríticas

Neoplasias  mamárias

Quimiocinas

Radioimunoensaio

Tolerância  imunológica

Breast  neoplasms

Dendritic  cells

Immunological  tolerance

Transcription  factors

Chemokines

Radioimmunoassay

Expressão de quimiocinas regulatórias das células Natural Killer e T-reguladoras em pacientes com endometriose profunda / Expression regulatory chemokines and Natural Killer T-regulatory cells in patients with severe endometriosis

Patrick Bellelis

20 March 2014

Introdução: A endometriose, condição inflamatória prevalente, associa-se a alterações da reposta imune na cavidade peritoneal e no útero. Evidências sugerem participação de mediadores inflamatórios, como as células Natural Killer e T-reguladoras na patogênese desta doença. A resposta destas células pode ser controlada pela atividade de algumas quimiocinas. O objetivo deste estudo foi avaliar a expressão gênica das quimiocinas reguladoras das células Natural Killer e T-reguladoras em endométrio tópico em lesões endometrióticas de pacientes com endometriose. Pacientes e Métodos: A expressão gênica das quimiocinas reguladoras da atividade das células Natural Killer (CXCL9, 10, 11, CXCL12, XCL1 e CX3CL1) e T reguladoras (CCL17 e CCL21) foi avaliada por meio de RTPCR no endométrio tópico e lesão endometriótica de 22 pacientes com endometriose de retossigmóide; 10 pacientes com endometriose retrocervical e no endométrio tópico de 32 mulheres sem endometriose comprovada por laparoscopia para laqueadura tubária. Resultados: Dentre as quimiocinas relacionadas às células Natural Killer, encontramos diferença estatística significativa na CX3CL1 e CXCL12, as quais foram mais expressas no foco de endometriose intestinal e retrocervical, quando comparadas ao endométrio tópico das pacientes e controles (p < 0,05). Das relacionadas às células T-reguladoras, a CCL17 foi mais expressa no endométrio tópico de pacientes com lesão em retossigmóide quando comparada aos demais grupos (p < 0,05). Conclusões: As quimiocinas CX3CL1 e CXCL12 foram mais expressas nos focos de endometriose intestinal e a CCL17 foi mais expressa no endométrio tópico de pacientes com lesão de retossigmóide. Estes resultados sugerem que as quimiocinas CX3CL1, CXCL12 e CXCL17 participam da resposta inflamatória que ocorre na endometriose pélvica / Objective: Endometriosis is a highly prevalent inflammatory condition associated with an altered immune response in the peritoneal cavity and uterus. Evidence suggests a participation of inflammatory mediators such as natural killer (NK) and T-regulatory (T-reg) cells in the pathogenesis of this disease while the response of these cells may be controlled by the activity of some chemokines. Patients and Methods: Gene expressions of the chemokines that regulate the activity of NK (CXCL9, CXCL10, CXCL11, CXCL12, XCL1 and CX3CL1) and T-reg cells (CCL17 and CCL21) were evaluated using real time polymerase chain reaction (PCR) in the eutopic and ectopic endometrium of 22 patients with bowel endometriosis, 10 patients with retrocervical endometriosis and 32 controls. Results: Of the chemokines associated with NK cells, the expression of CX3CL1 and CXCL12 was significantly greater in the foci of endometriosis (p < 0.05). Of those associated with T-reg cells, significant differences between groups were found in CCL17. In addition, CCL17 was expressed to a higher degree in the eutopic endometrium of the patients with rectosigmoid lesions when compared to the other groups (p < 0.05). Conclusions: Chemokines CX3CL1 and CXCL12 were more expressed in intestinal endometriosis and CCL17 expression was higher in eutopic endometrium of the patients with rectosigmoid lesions. These results suggest that those chemokines participate in the inflammatory response that occurs in pelvic endometriosis

Células matadores naturais

Endométrio

Endometriose

Linfócitos T reguladores

Quimiocinas

Chemokines

Endometriosis

Endometrium

Natural killers cells

T regulatory limphocytes

AvaliaÃÃo in vitro dos mecanismos imunossupressores induzid0s por leishmania amazonensis na resposta imune de indivÃduos sadios / In vitro evaluation of the mechanisms of transitory immunosuppression induced by L. amazonensis in healthy individuals low producers of IFN-gamma

Zirlane Castelo Branco CoÃlho

30 September 2004

CoordenaÃÃo de AperfeiÃoamento de Pessoal de NÃvel Superior / Estudos anteriores mostraram que indivÃduos expostos à Leishmania amazonensis apresentam resposta diferenciada em relaÃÃo à produÃÃo de IFN&#947;. Aqueles com baixa produÃÃo geram uma resposta Th2 e os que apresentam alta produÃÃo desta citocina, desde as primeiras horas de infecÃÃo, uma resposta Th1. Com o objetivo de avaliar o mecanismo de supressÃo induzido por L. amazonensis, foi determinado o perfil e a cinÃtica da expressÃo de quimiocinas e receptores de quimiocinas, como tambÃm de citocinas em culturas de cÃlulas mononucleadas do sangue perifÃrico de indivÃduos sadios, estimuladas com promastigotas vivas de L. amazonensis. A anÃlise semiquantitativa da expressÃo de RNAm das quimiocinas e seus receptores, atravÃs de RT-PCR, e a quantificaÃÃo das citocinas foi determinada por ELISA, apÃs 12 horas, 48 horas e 120 horas de infecÃÃo. Verificaram-se dois padrÃes de resposta em relaÃÃo à secreÃÃo de IFN&#947;. IndivÃduos com produÃÃo superior a 145,8 pg/mL foram classificados como alto respondedor (AR) e aqueles com produÃÃo inferior, como baixo respondedor (BR). Observou-se no grupo AR o desenvolvimento de uma resposta mista, com predomÃnio de Th1. Esta resposta està associada à expressÃo de quantidades relevantes de MIP-1&#945; (CCL3), RANTES (CCL5), MCP-1(CCL2), IP-10 (CXCL10), IL-8 (CXCL8), CCR1, CCR2 e CXCR3 em 12 e 48 horas de infecÃÃo. IL-12, IL-13 e IL-10 foram observadas em altas concentraÃÃes. Em relaÃÃo ao grupo BR, observou-se diminuiÃÃo da expressÃo de MIP-1&#945; (CCL3), RANTES (CCL5), MCP-1(CCL2), I-309 (CCL1), CCR2, CXCR3 e CCR5 durante todo o perÃodo avaliado e de IP-10 (CXCL10) nas primeiras 48h de infecÃÃo. IL-10 e IL-13 encontravam-se em elevadas concentraÃÃes desde 12h, tendo um pico de produÃÃo com 48h de infecÃÃo. Os resultados sugerem que apÃs 48 horas de exposiÃÃo à o momento em que hà diferenciaÃÃo na expressÃo das molÃculas. IL-10 e IL-13 parecem ter papel relevante na modulaÃÃo da supressÃo de INF&#947; induzida nos BR por L. amazonensis. / Previous studies have shown that individuals exposed to Leishmania amazonensis respond differentially with regard to interferon gamma (IFN)_ production. Individuals who have a low production of IFN_ develop a Th2 response, while those who produce high amounts of this cytokine during the early stages of infection show the Th1 response. In order to evaluate the mechanism of suppression induced by L. amazonensis, the profile and kinetics of chemokines and theirs receptors were determined, as also the cytokines in the cultures of peripheral blood mononuclear cells (PBMC) from healthy individuals, stimulated with live promastigotes of L. amazonensis. A semiquantitative analysis of mRNA expression for the chemokines and their receptor was performed by RT-PCR, and the cytokines were quantified by ELISA, at 12, 48 and 120 hours after infection. The two patterns of IFN_ response were studied. Individuals with a production higher than 145,8 pg/mL were classified as high responders (HR), and those with lower levels of production were considered as low responders (LR). Individuals in the HR group developed a mixed response, with a predominance of Th1, which was associated with the expression of relevant quantities of MIP-1_, RANTES, MCP-1, IP-10, IL-8, CCR1, CCR2 and CXCR3, within 12 and 48 hours after infection. IL-12, IL-13 and IL-10 were observed in significant quantities. In the LR group, the suppression of expression of MIP-1_, RANTES, MCP-1, I-309, CCR2, CXCR3 and CCR5 during the entire period of study, and that of IP-10 during the first 48 hours of infection, was observed. IL-10 and IL-13 were found in elevated concentrations from 12 hours of infection onwards, with a peak production at 48 hours. These results suggest that the pattern of response apparently is defined around 48 hours of infection. IL-10 and IL-13 appear to exercise a relevant role in the modulation of suppression of IFN_, induced in the LR group by L. amazonensis.

Leishmaniose

TolerÃncia ImunolÃgica

Quimiocina

Citocina

L. amazonensis

Immunossuppression

Cytokines

Chemokines

RT-PCR

IMUNOLOGIA

Laser de baixa potência no tratamento da artrite induzida por zymosan

Anjos, Lúcia Mara Januário dos

29 June 2018

Submitted by Geandra Rodrigues (geandrar@gmail.com) on 2018-10-10T10:45:14Z No. of bitstreams: 0 / Approved for entry into archive by Adriana Oliveira (adriana.oliveira@ufjf.edu.br) on 2018-10-16T13:33:10Z (GMT) No. of bitstreams: 0 / Made available in DSpace on 2018-10-16T13:33:10Z (GMT). No. of bitstreams: 0 Previous issue date: 2018-06-29 / A Artrite Reumatóide (AR) é uma doença inflamatória crônica, caracterizada por inflamação das articulações e associada à incapacidade motora e laboral dos pacientes. Tendo em vista que as estratégias atuais para o tratamento da AR podem apresentar sérios efeitos colaterais e nem sempre resultam em melhora clínica, a terapia com laser de baixa potência (LLLT) surgiu como alternativa para o tratamento da artrite, devido às suas propriedades anti-inflamatórias e de regeneração tecidual. Entretanto, os mecanismos anti-inflamatórios da LLLT nos tecidos biológicos ainda não são completamente conhecidos. Assim, o presente estudo teve por objetivo avaliar os mecanismos imunológicos e a participação das metaloproteinases de matriz (MMP) e seu inibidor (TIMP2), na resolução do processo inflamatório articular após o tratamento com LLLT. Para isso, um processo inflamatório foi induzido nas articulações talocrural e subtalar dos membros posteriores de camundongos C57BL/6, através da administração de zymosan na região periarticular. Os animais foram divididos em 4 grupos (n = 8): (ZY) artrite induzida por zymosan e não tratado, (ZY + 3Jcm-2) artrite induzida por zymosan + LLLT em 3Jcm-2, (ZY + 30Jcm-2) artrite induzida por zymosan + LLLT em 30Jcm-2 e (ZY + DEXA) artrite induzida por zymosan e tratado com dexametasona. As condições da LLLT foram: 830nm, 10mW e densidades energéticas de 3Jcm-2 e 30Jcm-2, no modo contínuo de emissão. A irradiação foi realizada durante 4 dias consecutivos, iniciando 5 horas após a indução da inflamação. Os animais foram eutanasiados 24h após a última aplicação da LLLT e as seguintes análises foram realizadas no tornozelo: morfológica, níveis relativos de mRNA de quimiocinas, citocinas, MMPs e TIMP2 por RT-qPCR, quantificação de citocinas por ELISA e quantificação da expressão tecidual de MMP13 e TIMP2 por imunohistoquímica. No linfonodo poplíteo foi realizada análise de citometria de fluxo para identificação e quantificação das populações de leucócitos. As análises morfológicas revelaram a presença de infiltrado celular no tecido conjuntivo adjacente à região periarticular, após a administração de zymosan. Foi observada diminuição dos níveis teciduais de citocinas após LLLT e alteração nos níveis de mRNA de citocinas e quimiocinas com importância na fisiopatologia da AR, diferentemente, dependendo da densidade de energia utilizada. O grupo ZY + 3Jcm-2 demonstrou aumento na maioria das populações de leucócitos analisadas, bem como na expressão de proteínas co-estimulatórias em macrófagos e células dendríticas do linfonodo proximal à inflamação. Adicionalmente, foi observado maior população de células Treg nos grupos LLLT, e no grupo ZY + 30Jcm-2, mais células Treg CD8+ expressando níveis elevados de CD25. Embora LLLT tenha diminuído os níveis de mRNA da maioria das MMPs analisadas e aumentado de TIMP2, foi observado aumento da expressão tecidual de MMP13 e TIMP2 na região inflamatória do grupo ZY + 3Jcm-2. Tendo em vista a totalidade dos resultados, o LLLT em ambas as densidades de energia, apresentou efeitos anti-inflamatórios positivos para o tratamento da AR, uma vez que diminuiu os níveis da maioria das citocinas, quimiocinas e MMPs nos tecidos inflamados, além de modificar o quantitativo e o fenótipo dos leucócitos linfonodais, especialmente de células Treg. / Rheumatoid Arthritis (AR) is a chronic inflammatory disease, characterized by joint inflammation and associated with motor and labor incapacity. Since treatment strategies could present a serious side effects and not always achieved clinic improvement, the Low Level Laser Therapy (LLLT) have being considered as an alternative to arthritis treatment, due to its anti-inflammatory and healing abilities. However, LLLT anti-inflammatory mechanisms in biological tissues is not completely understood. Then, this study aimed to evaluate immunological mechanisms and contribution of matrix metaloproteinases (MMPs) and its inhibitor (TIMP) on inflammation resolution process induced by LLLT. Arthritis was induced in C57BL/6 mice by zymosan injection into periarticular region. Experimental animals were divided in 4 groups (n=8): (ZY) arthritis induced by zymosan and untreated; (ZY + 3Jcm-2) arthritis induced by zymosan and treated with LLLT at 3Jcm-2; (ZY + 30Jcm-2) arthritis induced by zymosan and treated with LLLT at 30Jcm-2; (ZY + DEXA) arthritis induced by zymosan and treated with dexamethasone. LLLT parameters were: 830nm, 10mW energy densities at 3 Jcm-2 e 30 Jcm-2, in continuous wave emission mode. Irradiation sections and dexamethasone treatment were carried out 4 days consecutively, starting 5 hours after arthritis induction. Animals were euthanized 24h after the last treatment section and the following analysis were procedure at ankle: morphological, cytokine mRNA relative levels, chemokines, MMPs and TIMP2 by RT-qPCR, quantification of cytokines tissue expression by ELISA and MMP13 and TIMP2 by imunohistochemistry. In popliteal lymph node, leukocytes populations were identificated and quantificated by flow cytometry. Morphological analysis showed inflammatory infiltration at adjacent connective tissue of joints, after zymosan injection. After LLLT, it was observed cytokines tissue expression decrease and mRNA levels alteration of important cytokines and chemokines in pathophisiology of AR, depending of energy density used. The ZY + 3Jcm-2 group showed an increase leukocytes populations, as well as, higher expression of costimulatory proteins in macrophages and dendritic cells of popliteal lymph node. Additionally, it was observed higher Treg population in LLLT groups than ZY group. More, ZY + 30Jcm-2 showed higher Treg CD8+ population presenting CD25high. LLLT decreased mRNA levels of almost MMPs analyzed and increased of TIMP2, except for ZY + 3Jcm-2 group in which was observed MMP13 and TIMP2 tissue expression increase. Taken togheter, all results showed that LLLT, at both energy densities used, presente positive anti-inflammatory effects for RA treatment, since it decreases the levels of cytokines, chemokines and MMPs at inflammed tissues. LLLT could also alter number and phenotype leukocytes in lymph node, especially Treg cells.

CNPQ::CIENCIAS BIOLOGICAS::IMUNOLOGIA

LLLT

Artrite

Citocinas

Quimiocinas

Resposta imunológica

Metaloproteinase de matriz

LLLT

Arthritis

Cytokines

Chemokines

Immunological response

Matrix metalloproteinase