Atividade antiluteolítica no microambiente uterino durante o período crítico para o estabelecimento da gestação em bovinos / Antiluteolytic activity in the uterine microenvironment during the critic period to pregnancy establishment in bovines

Vanessa Belentani Marques

14 December 2006

A inibição da secreção pulsátil de prostaglandina F2alfa (PGF2α) uterina (atividade antiluteolítica) pela ação do interferon-tau (IFN-τ) trofoblástico, mantêm a secreção de progesterona pelo corpo lúteo, fundamental ao estabelecimento da gestação nas fêmeas bovinas. Supõe-se que essa atividade antiluteolítica esteja presente no microambiente uterino bovino, portanto objetivou-se estudá-la. Dada à inexistência de ensaios que meçam especificamente a atividade antiluteolítica propôs-se elaborar um ensaio biológico para tal. Observou-se que células BEND tratadas com forbol 12,13 dibutirato (PdBu) por 6 horas em cultivo sintetizam PGF2α e tal síntese é inibida na presença de interferon-tau recombinante bovino (rbIFN-τ). Em outro estudo definiu-se que 25 ng/mL de PdBu promove estímulo consistente à síntese de PGF2α. A partir da análise de regressão do percentual de inibição à síntese de PGF2α estimulada por PdBu, em função da concentração de interferon-tau recombinante (rbIFN-τ), calculou-se a concentração de rbIFN-τ que inibiu em 50% a síntese máxima de PGF2α (observada na presença apenas de PdBu). Definiu-se a atividade antiluteolítica como o recíproco da concentração proteica requerida para atingir esse percentual de inibição (50%), e que a solução com uma unidade antiluteolítica é aquela que com um micrograma exerça tal efeito. Caracterizou-se a utilização dessa isoforma como padrão do ensaio antiluteolítico e calculou-se a atividade antiluteolítica do mesmo, 9,61 x 10² UA/µg de proteína. Em estudo seguinte observou-se a modulação da síntese de PGF2α estimulada por PdBu, em função da concentração proteica de um pool de lavados uterinos ou meios condicionados por conceptos obtidos no décimo sétimo dia de gestação. Notou-se que para cada fluido testado há um intervalo de concentrações onde observa-se aumento linear na atividade antiluteolítica em função do acréscimo proteico. A partir da análise por regressão linear desse evento calculou-se a atividade antiluteolítica de cada amostra. Para o pool de lavados uterinos calculou-se 1,63 x 10-¹ UA/ µg de proteína, e para o pool de meios condicionados por conceptos 1,66 x 10² UA/µg de proteína. Estes estudos permitiram desenvolver uma metodologia para observar a atividade antiluteolítica em humores biológicos. Aplicando o ensaio antiluteolítico estudou-se a atividade antiluteolítica presente em lavados uterinos obtidos durante o período crítico de fêmeas bovinas prenhes ou cíclicas ( respectivamente, 56,2 e 33,9 UA/µg de proteina), notou-se que a atividade antiluteolítica foi maior no microambiente uterino de fêmeas gestantes. Tal resultado associado à potente atividade antiluteolítica observada para os meios condicionados por conceptos indicam a participação do IFN-τ secretado pelo concepto na modulação da síntese de PGF2α. Entretanto, observou-se atividade antiluteolítica nos lavados uterinos obtidos de fêmeas cíclicas, o que indica que a síntese de PGF2α estimulada por PdBu pode ser modulada por outras proteínas, além do IFN-τ. Sugere-se que a atividade antiluteolítica, observada através do ensaio biológico proposto, é resultante da atuação de fatores estimulatórios e inibitórios presentes nos humores biológicos. Conclui-se que a atividade antiluteolítica pode ser mensurada pelo ensaio biológico proposto, no entanto outros estudos devem ser conduzidos para correlacionar essa atividade com a atuação do IFN-τ. / The inhibition of pulsatile secretion of PGF2α mediated by interferon-tau (IFN) is fundamental on the maternal recognition of pregnancy, maintaining the progesterone secretion by corpus luteum. Therefore the measurement of interferon activity in the uterine microenvironment was studied. Due to a lack of assays those measure specific antiluteolytic capacities we suggest develop a biological assay for it. In this research we observed that BEND cells treated with PdBu synthesize PGF2α, wich is inhibited by the presence of recombinant bovine interferon-tau (rbIFN-τ). Following we defined 25ng/mL as PdBu (phorbol 12,13 dibutirate) stimulus at the PGF2α synthesis to be applied in this biological assay. Studies about the modulation of PdBu-stimulated PGF2α synthesis by the rbIFN-τ validate the use of this isoform as a reference, defining a standard-curve and allowing estimating the antiluteolytic activity of 9.61 x 10² antiluteolytic units per microgram (UA/µg) of protein. Further, we observed the modulation of PdBu-stimulated PGF2α synthesis exerted by a pool of uterine flushings or conceptus conditioned medium, and for each tested fluid, there is a range of concentrations where is observed an increasing rate on the inhibition of PGF2α synthesis. A restrict analysis on this concentrations range shows a linear behavior and allow calculate the antiluteolytic activity of each sample1.63 x 10-¹ UA/ µg of protein from a pool of uterine flushings, and 1.66 x 10² UA/µg from conceptus conditioned medium. These studies validated a method to observe the antiluteolytic activity from biological fluids. Using the antiluteolytic assay, we studied the antiluteolytic activity present in uterine flushings obtained during the critic period by pregnant or cyclic bovine females cíclicas (respectively 56,2 e 33,9 UA/µg of protein). We observed higher antiluteolytic activity from pregnant uterine microenvironment than in cyclic uterine microenvironment. This result linked with the high antiluteolytic activity observed to conceptus conditioned medium, suggest the participation of IFN-τ secreted by the conceptus in the PGF2α synthesis modulation. However, we observed the antiluteolytic activity in uterine flushing obtained by cyclic cows, suggesting that the PGF2α synthesis could be modulated by another proteins. We believe that the antiluteolytic activity, observed by the antiluteolytic assay, ensue the action of inhibitors or stimulators factors in the biological fluids. We conclude that the antiluteolytic assay could be measured by the proposed biological assay, nevertheless another studies must be done in order to correlate this activity with the interferon action.

bovinos

ensaio biológico

interferons

prostaglandina F2&alpha

reconhecimento da gestação

biological assay

bovines

interferons

pregnancy recognition

prostaglandin F2&alpha

Expressão ex vivo de fatores antivirais em mães infectadas por HIV-1 e recém-natos. / Ex vivo expression of antiviral factors in mothers infected by HIV-1 and newborns.

Natalli Zanete Pereira

16 April 2013

A transmissão vertical mãe-recém-nato é a principal fonte de infecção pediátrica. O tratamento antirretroviral vem reduzindo a transmissão vertical, mas também tem elevado o número de infantes expostos não infectados, os quais vêm mostrando maior risco de morbidade e mortalidade. Este dado salienta a importância de avaliar as características imunológicas, relacionadas à resposta inata no binômio mãe e recém-nato. A proposta do trabalho foi avaliar a expressão de fatores antivirais em células mononucleares (CMN), tecido placentário e no colostro de mães infectadas por HIV e cordão umbilical (RN), comparadas com mães-RN controle não infectadas. Os dados mostram que há uma ativa expressão dos fatores antivirais, sejam constitutivos ou induzíveis por IFN, nas mães infectadas por HIV e nos RN expostos. No sítio de interface materno-fetal, decídua e face fetal da placenta, foi detectado um perfil alterado de expressão dos fatores antivirais, especialmente da proteína APOBEC3G. Apesar da relativa imaturidade imunológica dos RNs, a infecção materna por HIV gerou um perfil semelhante de expressão dos fatores antivirais nos RN, por uma complexa interação de fatores relacionados a gestação e a infecção. / Vertical transmission mother-newborn is the main source of pediatric infection. The antiretroviral therapy has reduced vertical transmission, but also has increased the number of exposed uninfected infants, which have shown increased risk of morbidity and mortality. This finding emphasizes the importance of evaluating the immunological characteristics, related to innate response in both the mother and newborn. The purpose of this study was to evaluate the expression of antiviral factors in mononuclear cells (MNC), placental tissue and colostrum of HIV-infected mothers and umbilical cord (RN), compared with control mothers-uninfected infants. The data show that the active expression of antiviral factors, are constitutive or inducible by IFN in HIV-infected mothers and newborns exposed. At the site of maternal-fetal interface, decidua and placental villi, a profile was detected altered expression of antiviral factors, especially the APOBEC3G protein. Despite the relative immunological immaturity of the newborn, maternal HIV infection generated a similar profile of expression of antiviral factors in RN, by a complex interaction of factors related to pregnancy and infection.

Fatores imunológicos

Gravidez

Imunidade natural

Infecções por HIV

Interferons

Recém-nascido

HIV infections

Immune factors

Interferons

Natural immunity

Newborn

Pregnancy

Efeito do interferon-gamma sobre defeitos de \"splicing\" que levam à doença granulomatosa crônica ligada ao cromossomo X. / Interferon-gamma effect on splicing defects that cause chronic granulomatous disease linked to X chromosome.

Frazão, Josias Brito

06 April 2009

Os fagócitos contêm uma nicotinamida adenina dinucleotídeo fosfato (NADPH) oxidase associada à membrana, que gera superóxido e outros reativos intermediários do oxigênio. Defeitos nesta oxidase em seres humanos resultam na doença granulomatosa crônica (DGC). Mutações próximas aos sítios de splicing que interferem com o processamento do RNA mensageiro, acarretando deleção de um ou mais exons, são cada vez mais freqüentes na literatura científica, nesses casos, os mecanismos moleculares que levam a DGC nem sempre são totalmente esclarecidos, assim como o efeito do IFN-g, seja sobre o processamento da mensagem ou estabilidade dos transcritos. Com base nessas informações o objetivo geral deste trabalho é investigar o efeito do IFN-g sobre a regulação do sistema NADPH oxidase fagocítico humano. Através dos resultados obtidos, não se pode constatar melhora na produção de ânions superóxido após o tratamento com IFN-g em pacientes com defeito de splicing, no entanto detectou-se aumento da expressão do gene CYBB através de PCR convencional e através de real-time PCR além de um aumento na marcação de proteínas do spliceossoma através do FAN. / Phagocytes have a nicotinamide adenine dinucleotide phosphate-oxidase (NADPH) associated to plasmatic membrane that generates superoxide and other oxygen reactive intermediates. Defects on this oxidase in humans result in a disorder called Chronic Granulomatous Disease (CGD). Mutations next to splicing sites that interfere with the mRNA processing leading to deletion of one or more exons, are even more frequent on scientific literature, in these cases, the molecular mechanisms causing CGD are not always completetly clear, as well as the effect of IFN-g on the mRNA processing or on the stability of transcripts. Based on this information our aim is to investigate the effect of IFN-g on the regulation of the human NADPH oxidase phagocyte system.. With the obtained results it wasnt possible to see an increase in anion superoxide production after the IFN-g treatment in patients with splicing defects, however it was detected an increase on the expression of CYBB gene by conventional and real-time PCR besides an increase in the marking of spliceossomal proteins by FAN.

Chronic granulomatous disease

Doença granulomatosa crônica

Doenças imunológicas

IFN-gama

IFN-gama

Immunologic diseases

Immunology

Imunologia

Interferons

Interferons

Ligado ao X

Splicing

X linked

\"Splicing\"

Resposta celular Th1 /Th2 na doen?a periodontal experimental, em ratos: um estudo imuno-histoqu?mico

Lemos, Jana?na Cavalcante

28 February 2009

Made available in DSpace on 2014-12-17T15:32:28Z (GMT). No. of bitstreams: 1 JanainaCL.pdf: 1946389 bytes, checksum: 9edf9a3e8f8e033293bf82a3b2344d4d (MD5) Previous issue date: 2009-02-28 / Host response plays a major role in the pathogenesis of periodontal disease. Mediators such as inflammatory cytokines which are secreted during the immune response to bacterial challenges have ambiguous functions that may or may not lead to protection of the attacked tissue. In this context, experimental evidence suggests that T-helper 1 (Th-1) and T-helper 2 (Th-2) mediated responses are potentially important during the disease process. The aims of this study therefore were to further clarify the role played by Th2 cells during different time points of the active phase of periodontal disease, as well as, to investigate whether there was any evidence of a Th1 response in the periodontal disease microenvironment. Experimental periodontitis was induced in 30 Wistar male rats by placing cotton ligatures around the mandibular first molars. The rats were then randomly divided into two groups. Group1 (G1=15) and Group 2 (G2=15). In G1 the ligatures were maintained for 2 days, whereas in G2 the ligatures were left for 15 days, a time point that corresponds to the advanced stage of periodontal disease The contra-lateral teeth served as controls (no ligatures). Immunohistochemical investigation for the presence in gingival tissue of Th2 specific transcription factor (GATA3) and the subunit of the IFN-γ receptor was carried out after the disease induction period. Light microscopy analysis revealed a decrease in the expression of GATA-3 as bone loss progressed. On the other hand, although IFN-γ R1 was detected at an early stage of the active phase of disease its expression remained unaltered during the remaining period of the study. These results indicate that the Th2 response have a protective role during the pathogenesis of periodontal disease and that the progression of the periodontal disease is related with the unbalance of the responses Th1/Th2 / A resposta do hospedeiro tem um importante papel na patog?nese da doen?a periodontal. Mediadores como as citocinas liberadas por c?lulas inflamat?rias durante a resposta imune, frente a um ataque bacteriano, desempenham pap?is antag?nicos que podem culminar com a prote??o ou n?o do tecido agredido, o que fundamenta o paradigma da resposta Th1/Th2 na doen?a periodontal. Na tentativa de esclarecer a participa??o das c?lulas Th2, em diferentes tempos, na fase ativa da doen?a periodontal, bem como observar se o microambiente encontrava-se preparado para uma resposta Th1, induziu-se doen?a periodontal experimental em 30 ratos Wistar machos, atrav?s da coloca??o de ligaduras de algod?o ao redor dos primeiros molares mandibulares. Os animais foram divididos, aleatoriamente, em dois grupos: Grupo 1 (G1 = 15) e Grupo 2 (G2 = 15). Em G1 as ligaduras foram mantidas por 2 dias, que configurou o est?gio inicial da doen?a periodontal e no G2, as ligaduras foram mantidas por 15 dias, que foi considerado o est?gio avan?ado da doen?a periodontal. Os dentes contralaterais serviram de controle (sem ligaduras). Avalia??o imuno-histoqu?mica para o fator de transcri??o espec?fico para c?lula Th2 (GATA-3) e da subunidade IFN- γ R1 do receptor para IFN-γ (principal citocina da resposta Th1) foram avaliados nos tecidos gengivais dos ratos ap?s o per?odo de indu??o da doen?a. Ap?s an?lise microsc?pica observamos que o fator de transcri??o GATA-3 teve sua express?o diminu?da com o avan?o da perda ?ssea induzida e a subunidade IFN-γ R1 passou a se expressar na fase ativa da doen?a experimental, contudo n?o se alterou com a progress?o da destrui??o tecidual. Estes resultados indicam que a resposta Th2 pode estar associada a uma resposta protetora na patog?nese da doen?a periodontal e que a progress?o da doen?a periodontal est? relacionada com o desequil?brio das respostas Th1/Th2

Doen?as periodontais

Linf?citos T

Citocinas

Imunologia

Imuno-histoqu?mica

Interferons

Periodontal disease

Limphocytes

Cytokines

Immunology

Immunohistochemistry

Interferons

CNPQ::CIENCIAS DA SAUDE::ODONTOLOGIA

Efeito do interferon-gamma sobre defeitos de \"splicing\" que levam à doença granulomatosa crônica ligada ao cromossomo X. / Interferon-gamma effect on splicing defects that cause chronic granulomatous disease linked to X chromosome.

Josias Brito Frazão

06 April 2009

Os fagócitos contêm uma nicotinamida adenina dinucleotídeo fosfato (NADPH) oxidase associada à membrana, que gera superóxido e outros reativos intermediários do oxigênio. Defeitos nesta oxidase em seres humanos resultam na doença granulomatosa crônica (DGC). Mutações próximas aos sítios de splicing que interferem com o processamento do RNA mensageiro, acarretando deleção de um ou mais exons, são cada vez mais freqüentes na literatura científica, nesses casos, os mecanismos moleculares que levam a DGC nem sempre são totalmente esclarecidos, assim como o efeito do IFN-g, seja sobre o processamento da mensagem ou estabilidade dos transcritos. Com base nessas informações o objetivo geral deste trabalho é investigar o efeito do IFN-g sobre a regulação do sistema NADPH oxidase fagocítico humano. Através dos resultados obtidos, não se pode constatar melhora na produção de ânions superóxido após o tratamento com IFN-g em pacientes com defeito de splicing, no entanto detectou-se aumento da expressão do gene CYBB através de PCR convencional e através de real-time PCR além de um aumento na marcação de proteínas do spliceossoma através do FAN. / Phagocytes have a nicotinamide adenine dinucleotide phosphate-oxidase (NADPH) associated to plasmatic membrane that generates superoxide and other oxygen reactive intermediates. Defects on this oxidase in humans result in a disorder called Chronic Granulomatous Disease (CGD). Mutations next to splicing sites that interfere with the mRNA processing leading to deletion of one or more exons, are even more frequent on scientific literature, in these cases, the molecular mechanisms causing CGD are not always completetly clear, as well as the effect of IFN-g on the mRNA processing or on the stability of transcripts. Based on this information our aim is to investigate the effect of IFN-g on the regulation of the human NADPH oxidase phagocyte system.. With the obtained results it wasnt possible to see an increase in anion superoxide production after the IFN-g treatment in patients with splicing defects, however it was detected an increase on the expression of CYBB gene by conventional and real-time PCR besides an increase in the marking of spliceossomal proteins by FAN.

Doença granulomatosa crônica

Doenças imunológicas

IFN-gama

Imunologia

Interferons

Ligado ao X

\"Splicing\"

Chronic granulomatous disease

IFN-gama

Immunologic diseases

Immunology

Interferons

Splicing

X linked

The role of type I interferons in regulating intestinal inflammation

Kole, Abhisake

January 2013

Intestinal homeostasis is a delicate balance between suppression of immune responses against innocuous antigens and stimulation of immune responses against pathogens. Type I interferon (IFN-1) cytokines have both immunostimulatory and immunomodulatory effects. Colon mononuclear phagocytes (MP) constitutively produced IFN-1 in a TRIFdependent manner. We explored the function of endogenous IFN-1 in the colon using the T cell adoptive transfer model of colitis. Transfer of CD4⁺CD45RB^hi naïve T cells from wild type (WT) or IFNAR subunit 1 knockout (IFNAR1^-/-) mice into RAG^-/- hosts resulted in similar onset and severity of colitis. In contrast, RAG^-/- x IFNAR1^-/- double knockout (DKO) mice developed accelerated severe colitis compared to RAG^-/- hosts when transferred WT CD4⁺CD45RB^hi T cells. Although WT or IFNAR1^-/- regulatory T (Treg) cells equally prevented disease caused by CD45RB^hi naïve T cells, WT Treg cells co-transferred with naïve CD4⁺ T cells into DKO recipients failed to expand or maintain Foxp3 expression and gained effector functions in the colon. IFNAR signaling on host hematopoietic cells inhibited T cell-mediated colitis, but not innate colitis. MPs isolated from the colon lamina propria (cLP) required IFNAR signaling for the production of the anti-inflammatory cytokines, IL-10, IL-27, and IL-1RA, but not for the production of classic pro-inflammatory cytokines. IFN-1-dependent secretion of IL-1RA was particularly important in inhibiting the migration of inflammatory DCs with potent T cell proliferative capacity from the cLP to the mesenteric lymph nodes. Finally, preliminary results suggested that IFN-1 may shape the commensal microbiota, but is not essential for controlling specific colitis-inducing bacteria.

616.07

IBDV-mediated antiviral responses by TLR3 signaling pathways

Wong, Tsz-yeung., 王子揚.

January 2009

published_or_final_version / Biological Sciences / Doctoral / Doctor of Philosophy

Cell receptors.

Interferons.

Cellular signal transduction.

Chickens - Virus diseases.

Chickens - Immunology.

Viral genetics.

Etude de la différence de susceptibilité des lentivirus de primates aux interférons de type I / Study of the different susceptibility of primate lentiviruses to type I Interferons

Cordeil, Stéphanie

11 December 2012

Les IFN-I (interférons de type I), principalement IFN et , constituent un mécanisme de défense primordial de l’hôte contre les pathogènes. Pourtant, dans le cas du VIH-1 (virus de l’immunodéficience humaine), la relation entre les IFN-I et la réplication virale apparaît plus complexe. En effet, si les IFN-I inhibent la réplication du VIH-1 ex vivo, un état d’hyperactivation permanent de la réponse IFN-I a été récemment associé à la progression vers le SIDA ainsi qu’à une forte virémie chez les patients infectés par le VIH-1. De même, la dérégulation de la réponse IFN-I est un critère déterminant dans l’issue pathogénique de certains modèles d’infection virale chez le singe. Si l’hypothèse du rôle pathogénique des IFN-I s’avère correcte, le VIH-1 pourrait avoir évolué afin de se répliquer même en présence d’une telle réponse, qui semble être au final, plus délétère pour l’hôte que pour le virus. L’objectif de ce travail a été d’évaluer la résistance du VIH-1 aux IFN. Dans ce contexte, le VIH-1 a été comparé au VIH-2 et au SIVmac (virus de l’immunodéficience simienne), virus phylogénétiquement proches mais peu ou pas pathogènes pour l’homme, lors de l’infection de plusieurs types cellulaires tels que des lymphocytes, des macrophages et des cellules dendritiques. En accord avec l’hypothèse initiale de travail, les expériences réalisées ont montré que le VIH-1 est capable de se répliquer dans les cellules primaires prétraitées avec des doses d’IFN comparables à celles mesurées in vivo, alors que la réplication des virus VIH-2/SIVmac est complètement bloquée, même à des concentrations très faibles d’IFN. Ce travail a permis de démontrer que le blocage induit par l’IFN s’exerce au niveau des phases précoces de l’infection et plus précisément à l’étape de la transcription inverse. En effet, les données obtenues suggèrent que l’IFN induit l’expression d’un effecteur cellulaire qui affecte différentiellement la stabilité des complexes viraux, ce qui se traduit par un défaut d’accumulation de l’ADN viral plus important pour le VIH-2 et le SIVmac, que pour le VIH-1. La différence de susceptibilité des lentivirus de primates aux IFN-I pourrait ainsi expliquer en partie, les différents niveaux de réplication de ces virus, associés à leurs degrés de pathogénicité in vivo. / Type I Interferons (IFN-α/β, herein IFNs) provide an important mechanism of defense against pathogens and regulate in a paracrine and autocrine manner both intrinsic and adaptive immune responses. In the case of HIV-1 however, the relationship between IFNs and viral replication appears more complex. Indeed, if IFNs have been described to interfere with HIV-1 at basically all phases of its life cycle ex vivo, an IFN-induced state is linked to AIDS progression and to high viral loads in HIV-1 infected individuals. Similarly, a deregulated and prolonged IFN production/state seems one of the main distinguishing features between pathogenic and non-pathogenic SIV infection in primate animal models, suggesting that a deregulated IFN-state may be more detrimental to the host than to the virus itself in vivo.If this hypothesis is correct and if HIV-1 plays an active role in the perpetration of this antiviral state, it is possible that HIV-1 may have overall evolved to cope with this environment, remaining able to replicate despite it.To determine whether HIV-1 was better armed to replicate in the presence of an IFN-state environment than other primate lentiviruses, we compared HIV-1 to SIVmac and more importantly to HIV-2 that albeit capable of inducing AIDS in humans does so in a much less aggressive manner. In agreement with the initial hypothesis, our results indicate that HIV-1 is better fit to replicate in primary cells in the presence of amounts of IFN comparable to the ones measured in vivo, while the replication of HIV-2/SIVmac viruses is completely blocked even in the presence of low levels of IFN. By decorticating the effects of IFNs on the early and late phases of the viral life cycle in primary macrophages, we show here that the main target of the differential action of IFNs are the early phases of infection. More specifically, with time kinetics that we determine herein, IFNs induce cellular factor/s that differentially affect the stability of pre-reverse transcription complexes of HIV-2, but not of HIV-1. Our results could underlie a different evolutionary adaptation of primate lentiviruses to interferons that might be responsible for their different pathogenicity in vivo.

Lentivirus de primate

Interférons

Pathogenèse lentivirale

Macrophages

Primate lentiviruses

Interferons

Lentiviral pathogenesis

Macrophages

Effects of the strictly enteric helminth, Heligmosomoides polygyrus, on respiratory syncytial virus (RSV) infection

McFarlane, Amanda Jayne

January 2014

RSV is the most common cause of infant bronchiolitis, leading to morbidity and mortality in both infants and the elderly. The relationship between RSV and asthma development further highlights the need to fully understand the immune responses involved in order to develop effective vaccines and therapeutics to aid prevention and treatment of RSV infection respectively. Helminths have long been studied both as a major pathogen of humans, infecting approximately 3 billion people worldwide, and also their ability to modulate the host immune response to allow survival and chronic infection to ensue. Specifically, helminth infections are thought to modulate the host immune response through regulatory mechanisms which are not fully understood. This not only confers protection and survival of the parasites themselves, but also modulates the immune response to unrelated antigens and pathogens. In this thesis, the potential role of a strictly enteric helminth infection, with Heligmosomoides polygyrus, in the modulation of respiratory syncytial virus (RSV) infection was investigated and the associated immune mechanisms were investigated. Firstly, the effects of prior H. polygyrus infection on RSV infection and immune responses in the lung were analysed. H. polygyrus significantly reduced the number of natural killer cells, CD8+ T cells, B cells and conventional dendritic cells in the lung following RSV infection. Co-infection also reduced the production of pro-inflammatory cytokines IL-6 and TNF-α in the lungs. All of these reductions were associated with significantly lower viral titres on day 4 of RSV infection. Interestingly, this attenuation of immune responses and viral titres, correlated with reduced severity of clinical disease, as assessed by weight loss and lung function. H. polygyrus excretory secretory product (HES) was not found to be the immune-modulatory factor in this system, as HES failed to suppress viral titres and reduce immune cell responses to RSV infection. However, irradiated larvae with stunted maturation to adult worms, revealed that larval stages were sufficient to suppress viral titres. Next, the role of type 2 signalling for H. polygyrus effects on RSV infection were examined, using IL-4Rα-/- mice. H. polygyrus infection maintained the ability to attenuate RSV infection and subsequent immune responses in IL-4Rα-/- mice. Furthermore, the presence of the adaptive immune response was not required for H. polygyrus-induced attenuation of RSV infection, as demonstrated in recombinase-activating gene (RAG-/-) deficient mice. H. polygyrus induces innate type 2 immune responses indicating the release of the innate alarmin, IL-33, in the lung and consequently an accumulation of group 2 innate lymphoid cells (ILC2). Their contribution to H. polygyrus effects remain to be fully elucidated. Finally, the role of antiviral responses was explored in H. polygyrus and RSV co-infection. H. polygyrus infection alone induced expression of antiviral genes, IFN-β, OAS1A, Viperin and the antimicrobial peptide CRAMP, in both the duodenum and the lung. Expression of these genes was still higher in the lung 1 hour after RSV in H. polygyrus co-infected mice compared to controls without co-infection. The importance of type I IFN signalling pathway was demonstrated using mice deficient in the type I IFN receptor in H. polygyrus co-infection, which failed to suppress RSV titres and subsequent lung immune cell infiltration. These data highlight the ability of the strictly enteric helminth H. polygyrus to attenuate RSV infection and subsequent immune responses in the lung through the potentiation of type I IFN signalling and consequent upregulation of antiviral immune responses in the lung.

616.2

Analyse de la contribution des inflammasomes et de l’interleukine-1β dans un modèle murin d’inflammation microcristalline / Analysis of the contribution of inflammasomes and interleukin-1β in a murine model of microcrystalline inflammation

Mariotte, Alexandre

26 March 2019

La goutte est une maladie inflammatoire particulièrement prévalente causée par la formation de dépôts articulaires et péri-articulaires de cristaux d’urate monosodique (UMS ou MSU) et dépendante de la cytokine interleukine-1β (IL-1β). En 2006, l’inflammasome NLRP3 a été montré comme nécessaire pour la maturation de l’IL-1β, in vitro, en réponse aux cristaux de MSU. Néanmoins, sa nécessité in vivo est un sujet de controverse. Mon travail de thèse a porté sur la caractérisation d’un modèle murin d’inflammation aiguë uratique et l’analyse de la contribution des inflammasomes dans cette pathologie. J’ai d’abord montré que notre modèle par injection sous-cutanée de cristaux de MSU donne lieu une forte inflammation des tissus mous comme cela est souvent observé lors des crises de goutte chez l’Homme. L’emploi de souris invalidées génétiquement et d’inhibitions pharmacologiques m’a permis de décrire son indépendance vis-à-vis de plusieurs composants des inflammasomes et confirme le rôle majeur de l’IL-1β. De manière intéressante, j’ai ensuite montré qu’il est possible de réduire fortement l’inflammation dans ce modèle par un traitement topique à base d’imiquimod (crème ALDARA®), un ligand synthétique de TLR7. Des expériences réalisées in vivo et in vitro m’ont permis de relier l’effet de l’imiquimod à une baisse importante de l’Il1b au niveau transcriptionel, via une signalisation faisant probablement intervenir les interférons de type I et possiblement le facteur RUNX3. Mes données montrent donc que la production d’IL-1β, dans ce modèle, est visiblement indépendante de NLRP3 mais peut être fortement abaissée par l’application topique d’imiquimod. L’imiquimod pourrait ainsi représenter une piste thérapeutique attractive. / Gout is a prevalent inflammatory disease caused by the deposition of monosodium urate crystals (MSU) in articular/periarticular areas, which strongly depends on interleukine-1β (IL-1β). In 2006, the NLRP3 inflammasome has been shown to perform IL-1β maturation in vitro after MSU crystal exposure. However, its in vivo dependence is still matter of controversy. In my thesis project, I focused on the characterization of a murine acute uratic inflammation and analysed the contribution of inflammasome components. I first showed that the subcutaneous injection of MSU crystals in mice generate a strong soft tissue inflammation as observed in human gouty crises. Then, by using genetically-modified mouse lines and pharmacological inhibitions, I demonstrated that this model is inflammasome-independent, while still requiring IL-1β secretion. Interestingly, I observed that the topical application of imiquimod (ALDARA® cream), which is a synthetic TLR7 ligand, strongly dampens inflammation. In vivo and in vitro experiments further demonstrated that this effect is linked to reduced Il1b gene expression, which linkely involves type I interferon signaling and eventually the transcription factor RUNX3. Altogether, my results show that IL-1β production is NLRP3-independent in this mouse model but can be strongly decreased by topical application of imiquimod. Therefore, imiquimod might be an attractive therapeutic option for gouty patients.

Goutte

Inflammasomes

Interleukine-1β

Interférons

Imiquimod

Gout

Inflammasomes

Interleukin-1β

Interferons

Imiquimod

572.8

615.7

616.7