Identification de nouvelles cibles thérapeutiques dans le cancer de la prostate / Identification of new therapeutic targets in prostate cancer

Rakotondrahaso, Valomanda

07 October 2019

En France, le cancer de la prostate est le premier cancer par son incidence ainsi que la troisième cause de mortalité pour cette pathologie. La progression de la maladie est dépendante des androgènes. Ainsi l’un des traitements majeurs du cancer de la prostate est la déprivation androgénique : le blocage de la production ou de l’action des androgènes conduit à inhiber la croissance tumorale. La plupart des patients répondent à cette thérapie, cependant l’évolution de la pathologie vers un stade d’insensibilité à la castration est inévitable, ce qui est associé à un mauvais pronostic. Au cours de la progression du cancer de la prostate, la voie de signalisation des androgènes demeure active grâce au récepteur des androgènes. Ce récepteur est une cible idéale afin de traiter et de bloquer la progression tumorale. Une telle inhibition du récepteur des androgènes peut être faite par l’utilisation d’un anti-androgènes de seconde génération : l’Enzalutamide. Cette molécule perturbe l’interaction entre le récepteur des androgènes et son ligand, elle peut bloquer la translocation nucléaire du récepteur activé mais elle empêche aussi son interaction avec l’ADN. Bien que l’utilisation de l’Enzalutamide ait contribué à améliorer la survie des patients, son utilisation conduit à l’émergence d’une résistance à l’Enzalutamide, ce qui constitue un défi thérapeutique considérable.L’objectif principal de mes travaux de thèse est d’identifier de nouvelles protéines afin d’améliorer les effets thérapeutiques de l’Enzalutamide ou de surmonter la résistance à ce médicament. Ainsi dans notre étude, nous avons supposé que le traitement à l’Enzalutamide induit l’activation de voies de signalisation spécifiques, pouvant être impliquées soit dans le mécanisme d’action du médicament ou dans la résistance à ce dernier. Cette hypothèse nous a conduit à l’identification des protéines MAPKs p38, qui sont activées lors d’un traitement avec l’Enzalutamide. Nos résultats démontrent que la combinaison d’Enzalutamide et d’inhibiteur de la MAPK p38 a un effet antitumoral significatif aussi bien in vitro que in vivo. Le mécanisme d’action de cet effet cytotoxique et synergique reste à l’étude. Ces données permettraient d’approfondir la compréhension des mécanismes de résistance lors d’un traitement à l’Enzalutamide et contribuer à la potentialisation de l’effet thérapeutique de cet antiandrogènes. / In France, prostate cancer is the most frequently diagnosed male cancer and its progression is tightly associated with the androgen signals. One of the major treatments for prostate cancer is androgen deprivation therapy which is based on blocking the production or action of the androgens to induce a tumor growth inhibition. Most patients respond to this therapy, however they still reach a castration-resistant stage which is associated with a poor prognosis. Since the progression till this late cancer stage is still driven by the androgen signaling pathway, the second-line therapy is focused on targeting the active androgen receptor by using a second-generation anti-androgens: the Enzalutamide. This molecule disrupts the interaction between the androgen receptor and its ligand, it can block the nuclear translocation of the receptor and it also prevents the receptor interaction with DNA. Although Enzalutamide treatment has enhance the patient survival, some drug resistance still arises which is a considerable therapeutic challenge.The main objective of my thesis is to identify new proteins in order to improve the therapeutic effects of Enzalutamide or to overcome resistance to this drug. Thus, in our study, we assumed that Enzalutamide treatment induces the activation of specific signaling pathways which may be involved in the cancer cell response to the treatment. This hypothesis led us to identify the MAPKs p38 proteins, which are activated during treatment with Enzalutamide. Our results show that the combination of Enzalutamide and p38 inhibitor has a significant antitumor effect both in vitro and in vivo. The mechanism of action of this cytotoxic and synergistic effect remains under study. These data would allow a better understanding of the Enzalutamide resistance mechanisms and contribute to the enhancement of the therapeutic effect of this anti-androgen.

Cancer de la prostate

Résistance aux traitements

Nouvelles cibles

Synergie

MAPK p38

Prostate cancer

Drug resistance

New therapeutic targets

Synergy

P38 mapk

Characterization of a MAPK module involved in Arabidopsis response to wounding / Caractérisation d'un module MAPK impliqué dans la réponse à la blessure chez Arabidopsis thaliana

Sözen, Cécile

29 November 2017

Les plantes ne pouvant pas se déplacer sont continuellement soumises aux stress environnementaux. La blessure, l’un des stress les plus fréquents auxquels la plante est soumise, peut causer d’important dégâts et faciliter l’entrée de pathogène dans les tissus de la plante. Pour répondre efficacement à la blessure, la plante a développé des mécanismes lui permettant de guérir ses tissus endommagés et d’empêcher l’infection pathogène. Les stress environnementaux sont perçus grâce à la présence de récepteurs spécifiques activant des voies de signalisation qui, à terme, conduisent à la mise en place de réponses de défense. Les modules de MAPK, composés de 3 kinases (MAP3K, MAP2K et MAPK) activées en cascades, représentent d’importantes voies de signalisation impliquées en réponse à divers stress biotiques et abiotiques. Grâce aux approches de tests de phosphorylation in vitro très maîtrisées dans le groupe « Stress signaling », j’ai pu identifier un module MAPK impliquant la MAP2K MKK3 et les MAPKs du groupe C (MPK1, 2, 7 et 14) activé par la blessure. Les MAP3Ks du sous-clade III (MAP3K13 à 20) sont transcriptionnellement induites par divers stress ce qui semble être un mécanisme assez conservé. Certains membres du sous-clade III sont induits par la blessure et parmi eux la MAP3K14 semble avoir un rôle majeur en amont du module MKK3/MPK1-2-7-14. Enfin, j’ai pu montrer que l’acide jasmonique (JA), une phytohormone importante produite en réponse à la blessure, tient un rôle important en amont du module. Ce-dernier est également activé en réponse à l’insecte herbivore Spodoptera littoralis et au champignon nécrotrophe Botrytis cinerea. Dans le contexte de blessure par l’insecte herbivore, MKK3 semble réguler la production de deux phytohormones, le JA et l’Acide Salicylique (SA). / Plants are sessile organisms. They have to cope continuously with environmental stresses. Injury, one of the most frequent stress conditions that plants must face may cause harsh damages to the plant tissues and facilitate the entry of pathogens. Therefore, plants have evolved mechanisms to respond efficiently to wounding by healing damaged tissues and preventing further pathogen infection. Wounding is a complex stress which is perceived by specific receptors which activate signaling pathways leading to those responses. Mitogen-Activated Protein Kinases modules are composed of 3 kinases (MAP3K, MAP2K and MAPK) activated in cascade and represent important signaling pathways involved in response to various biotic and abiotic stresses as well as in developmental processes. During my Ph.D I identified a MAPK module activated 30 minutes after wounding and involving the MAP2K MKK3 acting upstream of C-group MAPKs MPK1-2-7-14. In the past, the laboratory has shown that this module is dependent on the transcriptional regulation of sub-clade III MAP3Ks (MAP3K13 to 20). Some were found induced by wounding and among them MAP3K14 seems to have an important role upstream MKK3/C-group MAPKs. Finally I was able to show that Jasmonic Acid (JA), a major phytohormone produced upon wounding and involved in the mediation of defense responses, was shown to have an important role upstream the MKK3/C-group MAPKs module. The module is also activated by the herbivore Spodoptera littoralis and the necrotrophic fungus Botrytis cinerea. Upon insect feeding, MKK3 negatively regulates JA and SA levels. My work helped to better understand stress signaling events occurring upon wounding.

Blessure

MAPK

Signalisation

Acide jasmonique (JA)

Acide salicylique (SA)

Wounding

MAPK

Stress signaling

Jasmonic acid (JA)

Salicylic acid (SA)

Sprouty4 regulates the balance between pluripotency and trophectoderm differentiation in mouse embryonic stem cells

Chap, Christna

22 December 2010

Unbegrentzte Selbsterneuerungkapazität und Pluripotenz sind charakteristische Merkmale von embryonalen Stammzellen (ES-Zellen). Dennoch sind die molekularen und zellulären Mechanismen, die für das Schicksal der ES-Zellen zuständig sind, noch nicht genau definiert. Um regulierende Faktoren des undifferenzierten Zustands von ES-Zellen zu identifizieren, wurden undifferenzierte ES Zellen, "Embryoid Bodies", spontan differenzierte und mit Retinsäure differenzierte ES Zellen mittels Microarray-Analysen verglichen. Neben bereits etablierten Pluripotenz-Markern, wurde Sprouty4 als eines der am stärksten degerulierten Transkripte unter diesen Bedingungen identifiziert. Sprouty4 ist als Inhibitor des ERK (Extracellular signal-regulated protein kinase)-Signalweges bekannt, aber seine Rolle in ES-Zellen wurde noch nicht definiert. Mittels Genexpression und Western BlotAnalysen konnte gezeigt werden, dass Sprouty4 in undifferenzierten ES-Zellen stark exprimiert ist und im Verlauf der Differenzierung schnell herunterreguliert wird. In vivo war Sprouty4 auf die innere Zellmasse (ICM) der Mausblastozyste beschränkt. Außerdem wurde gezeigt, dass der Sprouty4 Promotor durch direkte Bindung der PluripotenzMarkern Nanog, Klf4 und Stat3 reguliert wird. ES-Zellen, die Sprouty4 konstitutiv exprimieren, waren resistent gegen Differenzierung durch Zugabe von Retinsäure oder Bildung von Embryoid Bodies. Hingegen führte die Expression einer dominant-negativen Mutante von Sprouty4 zu einer erhörten Sensitivierung von ES-Zellen gegenüber der Differenzierung und zur Bildung extraembryonaler Gewebe begleitet von Endoreduplikation. Zusammenfassend konnten unsere Ergebnisse zeigen, dass die enge Regulation des ERK-Signalweges und warscheinlich anderer Signalwege durch Sprouty4 notwendig ist, um die Balance zwichen Pluripotenz und Differenzierung embryonaler Stammzellen zu kontrollieren. / A hallmark feature of embryonic stem (ES) cells is the ability to self-renew indefinitely while maintaining pluripotency. However, the molecular and cellular mechanisms underlying ES cell fate are poorly understood. To identify signaling pathway molecules that maintain the uncommitted state of ES cells, a microarray analysis was performed comparing undifferentiated ES cells, mature embryoid bodies, spontaneously differentiated and retinoic acid-induced differentiated ES cells. Among several well-validated pluripotency markers, Sprouty4 was identified as one of the most highly deregulated transcripts under these conditions. Sprouty4 is known as an inhibitor of the extracellular signal-regulated protein kinase (ERK/MAPK) pathway however its role in ES cells has not yet been defined. Gene expression and western-blot analyses have shown that Sprouty4 is highly expressed in ES cells and strongly downregulated upon differentiation whilst in vivo, Sprouty4 is confined to the founder population of ES cells, the inner cell mass of mouse blastocysts. Moreover, the Sprouty4 promoter was found to be regulated via the direct binding of the intrinsic pluripotency-associated factors Nanog, Klf4 and Stat3. ES cells engineered to constitutively express a wild-type version of Sprouty4 were found to be resistant to differentiation induced by retinoic acid or embryoid bodies formation. Conversely, expression of a dominant negative Sprouty4 mutant activating the ERK/MAPK pathway in a sustained manner sensitized ES cells to differentiation and triggered endoreduplication leading to the formation of extraembryonic tissue. Taken together, these results highlight the essential role of Sprouty4 in the tight regulation of the ERK/MAPK pathway- and probably others- for the balance between pluripotency and lineage commitment in mouse embryonic stem cells.

Differenzierung

Sprouty

MAPK

ES Zellen

Pluripotenz

differentiation

Sprouty

MAPK

ES cells

pluripotency

570 Biologie

32 Biologie

WE 5320

ddc:570

Couplage du récepteur à sept domaines transmembranaires GABA-B1 aux voies intracellulaires de signalisation en absence de GABA-B2

Richer, Maxime

02 1900

Le GABA est le principal neurotransmetteur inhibiteur du SNC et est impliqué dans le développement du cerveau, la plasticité synaptique et la pathogénèse de maladies telles que l’épilepsie, les troubles de l’anxiété et la douleur chronique. Le modèle actuel de fonctionnement du récepteur GABA-B implique l’hétérodimérisation GABA-B1/B2, laquelle est requise au ciblage à la surface membranaire et au couplage des effecteurs. Il y est cependant des régions du cerveau, des types cellulaires et des périodes du développement cérébral où la sous-unité GABA-B1 est exprimée en plus grande quantité que GABA-B2, ce qui suggère qu’elle puisse être fonctionnelle seule ou en association avec des partenaires inconnus, à la surface cellulaire ou sur la membrane réticulaire. Dans le cadre de cette thèse, nous montrons la capacité des récepteurs GABA-B1 endogènes à activer la voie MAPK-ERK1/2 dans la lignée dérivée de la glie DI-TNC1, qui n’exprime pas GABA-B2. Les mécanismes qui sous-tendent ce couplage demeurent mal définis mais dépendent de Gi/o et PKC. L’immunohistochimie de récepteurs endogènes montre par ailleurs que des anticorps GABA-B1 dirigés contre la partie N-terminale reconnaissent des protéines localisées au RE tandis des anticorps C-terminaux (CT) marquent une protéine intranucléaire. Ces données suggèrent que le domaine CT de GABA-B1 pourrait être relâché par protéolyse. L’intensité des fragments potentiels est affectée par le traitement agoniste tant en immunohistochimie qu’en immunobuvardage de type western. Nous avons ensuite examiné la régulation du clivage par le protéasome en traitant les cellules avec l’inhibiteur epoxomicine pendant 12 h. Cela a résulté en l’augmentation du marquage intranucléaire de GABA-B1-CT et d’un interacteur connu, le facteur de transcription pro-survie ATF-4. Dans des cellules surexprimant GABA-B1-CT, l’induction et la translocation nucléaire d’ATF-4, qui suit le traitement epoxomicine, a complètement été abolie. Cette observation est associée à une forte diminution du décompte cellulaire. Étant donné que les trois derniers résidus de GABA-B1-CT (LYK) codent un ligand pseudo-PDZ et que les protéines à domaines PDZ sont impliquées dans la régulation du ciblage nucléaire et de la stabilité de protéines, en complément de leur rôle d’échaffaud à la surface cellulaire, nous avons muté les trois derniers résidus de GABA-B1-CT en alanines. Cette mutation a complètement annulé les effets de GABA-B1-CT sur l’induction d’ATF-4 et le décompte cellulaire. Cette deuxième série d’expériences suggère l’existence possible de fragments GABA-B1 intranucléaires régulés par le traitement agoniste et le protéasome dans les cellules DI-TNC1. Cette régulation d’ATF-4 dépend des résidus LYK de GABA-B1-CT, qui modulent la stabilité de GABA-B1-CT et favorisent peut-être la formation d’un complexe multiprotéique incluant GABA-B1-CT, ATF-4, de même qu’une protéine d’échaffaudage inconnue. En somme, nous démontrons que les sous-unités GABA-B1 localisées au RE, lorsque non-hétérodimérisées avec GABA-B2, demeurent capables de moduler les voies de signalisation de la prolifération, la différentiation et de la survie cellulaire, via le couplage de protéines G et possiblement la protéolyse régulée. Les mécanismes de signalisation proposés pourraient servir de nouvelle plate-forme dans la compréhension des actions retardées résultant de l’activation des récepteurs 7-TMs. / GABA is the principal inhibitory neurotransmitter in the CNS and is implicated in brain development, synaptic plasticity and the pathogenesis of diseases such as epilepsy, anxiety disorders and chronic pain. In the current model of GABA-B function, there is a requirement for GABA-B1/B2 dimerization for targetting to the cell surface and effector coupling. However, there are certain brain regions (putamen), cell types (glial cells) and times during brain development where GABA-B1 is expressed in higher amounts than GABA-B2, suggesting that GABA-B1 might be functional alone or in association with unidentified partners, either at the cell surface or on the ER membranes. In this thesis, we first show the capacity of endogenous GABA-B1 receptors to activate the MAPK-ERK1/2 pathway in the DI-TNC1 glial-derived cell line which does not express GABA-B2. The underlying mechanisms remain incompletely defined but depend on Gi/o and PKC. Immunohistochemistry of endogenous receptors shows that GABA-B1 N-terminal antibodies recognize ER-localized proteins and that C-terminal (CT) antibody shows intranuclear distribution. This data suggests that fragments of the GABA-B1 receptor are generated by proteolysis and indeed we show that agonist treatment affects the intensity of certain C-terminal GABA-B1 fragments both in immunohistochemistry and western blots suggesting that the GABA-B1 receptor is subjected to regulated proteolysis. Since a 13-residue potential PEST sequence was localized immediately distal to the ER retention motif in the GABA-B1 CT, we examined proteasome regulation of the cleavage event. Following a 12h treatment with the proteasome inhibitor, epoxomicin, we detected increases in intranuclear staining for both GABA-B1 and a known interactor, the pro-survival transcription factor ATF-4, using confocal microscopy and by western blotting of nuclear extracts. These increases are due either to proteasome inhibition or activation of the ER stress pathway. In cells overexpressing GABA-B1-CT, ATF-4 induction and nuclear translocation, which normally follows epoxomicin treatment, was completely abolished. This observation was associated to a strong decrease in cell number. Since the last three residues of GABA-B1-CT (LYK) encode a pseudo-PDZ ligand and that PDZ domain protein regulate nuclear targeting and protein stability, in complement to their role in scaffolding at the cell surface, we mutated the last three residues of GABA-B1-CT to alanines. This mutation completely reversed the effect of GABA-B1-CT on ATF-4 induction and on cell number. This second set of data suggests the existence of agonist and proteasome-regulated intranuclear GABA-B1 fragments in DI-TNC1 cells. Further, the GABA-B1-CT pseudo-PDZ ligand appears to be critically important in regulating ATF-4 induction by modulating GABA-B1-CT stability and perhaps by favoring the formation of a multiprotein complex with ATF-4, ATF-4 interactors and an unknown scaffolding protein. Overall, we show that ER-localised GABA-B1 subunits, when not dimerized with GABA-B2, can still modulate proliferation, differentiation and survival pathways, both through G-protein coupling and regulated proteolysis. The signalling mechanisms which we propose could serve as a new platform in understanding the long term effects of 7-TM receptor activation.

RCPGs

GABA-B

Signalisation MAPK-ERK1/2

ATF-4

Protéolyse

PDZ

GPCRs

Signaling

MAPK

Proteolysis

Modélisation et analyse des dérégulations tumorales du réseau MAPK chez l'homme / Integrative modelling and analysis of MAPK network deregulations in human cancers

Grieco, Luca

03 May 2013

Le réseau des MAPK est composé de pathways de signalisation fermement entrecroisés impliqués dans le cancer. Toutefois, les mécanismes précis qui sous-tendent son influence sur l'équilibre entre la prolifération et la mort cellulaire demeurent insaisissablesDes données publiques ont été intégrés dans une carte de réactions détaillée, représentant l'influence du réseau des MAPKs sur la décision du destin cellulaire. Cette carte a ensuite été utilisée pour des analyses informatiques spécifiquesTout d'abord, les dynamiques du réseau des MAPKs dans les cancers de la vessie ont été analysés.Un modèle Booléen a été construit, représentant la réponse du réseau aux inputs d'intérêt.Les résultats de simulations systématiques ont été trouvés globalement cohérents avec des données publiques, et ont permis de déchiffrer les principaux événements qui sous-tendent les différents comportements observés dans le cancerEnsuite, la carte a été exploitée pour réanalyser des données publiques d'expression de gènes, avec l'objectif d'identifier les principaux acteurs de la transduction des signaux prolifératifs, dans des types cellulaires spécifiques.Des analyses du réseaux et des calculs statistiques ont conduit à l'identification de régions dérégulées dans le réseau des MAPKs, et à la délinéation de points d'intervention optimales dans cinq stades du cancer de la vessie et dans quatre sous-types de lymphome TL'ensemble de ces résultats a conduit à la formulation de nouvelles hypothèses concernant le fonctionnement du réseau des MAPKs dans différents états pathologiques, et à la sélection de composants cibles qui pourraient être envisagées pour le développement de nouveaux traitements / MAPK network consists of tightly interconnected signalling pathways. Although several studies established the involvement of this network in cancer deregulations, the precise mechanisms underlying its influence on the balance between cell proliferation and death remain elusive.Public data were integrated into a detailed reaction map, accounting for the influence of MAPK network on cell fate decision. This map was then used for computational analyses addressing specific cancer-related questions.First, the dynamics of MAPK network in bladder cancers were analysed. A Boolean model was built, accounting for the response of the network to selected inputs. The results of systematic simulations were found globally coherent with published data. Based on in silico experiments, the main events underlying different observed cancer cell behaviours were then deciphered.Next, the MAPK reaction map was exploited to reanalyse public high-throughput gene expression data. The goal was to identify key actors for the transduction of proliferative signals, in specific cell types. Network analyses and statistical computations led to the identification of deregulated MAPK network regions, and to the delineation of optimal intervention points aimed at blocking the proliferative signals transduced from such regions. This approach was used to study five different tumour stages and four different subtypes of T-cell lymphoma.Altogether, these results led to the formulation of novel hypotheses concerning the functioning of MAPK network in different pathological conditions, and to the selection of target components that might be considered for the development of novel treatments.

MAPK

Biologie des systèmes

Carte de réactions

Modélisation logique

Analyse de pathways

Cancer

MAPK

Systems biology

Reaction maps

Logical modelling

Pathway analysis

Cancer

572

Sensibilização central induzida pelo vírus HSV-1: uma análise de mecanismos de dor crônica em modelo experimental de neuralgia pós-herpética / Central sensibilization inducted by HSV-1 virus: an analysis of chronic pain mechanisms in experimental model of post herpetic neuralgia

Rossi, Laís Regina

11 January 2018

A dor é descrita como uma sensação sensorial e emocional desagradável de extrema importância para sobrevivência e integridade do organismo. As dores crônicas de origem neuropática são de difícil tratamento e seus mecanismos fisiopatológicos pouco conhecidos. Este estudo foi realizado após inoculação do vírus HSV-1 na pata traseira esquerda de camundongos machos da linhagem Balb/C, e teve como objetivo investigar comportamentalmente o desenvolvimento de alodínia mecânica e hipernocicepção nas fases herpética e pós herpética, caracterizar a atividade de vias intracelulares de sinalização das proteínas JNK, AKT CREB, P38, ERK, Glutamina Sintetase e Stat 3, através de western blot na coluna dorsal da medula espinal nas fases herpética e pós herpética, além de verificar a presença do vírus HSV-1 na medula espinal e gânglio dos animais por meio da reação em cadeia da polimerase em tempo real (RT-PCR). Os resultados evidenciaram alteração de sensibilidade nos animais a partir do 7º dia que permaneceu até o 28º dia após a inoculação do vírus. Houve uma mudança na expressão das proteínas MAPKs, com aumento na expressão de JNK, AKT e CREB no corno dorsal da medula no 8º e 21º dia após a inoculação do vírus HSV-1, aumento na expressão de P 38 e P ERK no 8º dia após inoculação do vírus e uma diminuição na expressão da proteína Stat 3 no 8º e 21º dia após a inoculação do vírus, sugerindo assim a participação dessas proteínas na alteração de sensibilidade tanto no período herpético quanto pós herpético. Também ocorreu um aumento na amplificação do DNA viral HSV-1 na medula espinal e gânglio espinal esquerdo no período herpético após inoculação do vírus HSV-1 / The pain is described as a sensorial and emotional unpleasant sensation of extreme importance for survival and integrity of the organism. The chronic pains that has neuropathic source are hard to treat and its physiopathologic mechanisms not well known. This study was performed after inoculation of the virus HSV-1 in the left back foot of male Balb/C mouse, and had as main objectives to behaviorally investigate the development of mechanical allodynia and hyper nociception during the herpetic and post-herpetic phase, characterize the activity of the intracellular signalization paths of the proteins JNK, AKT CRB, P38, ERK, glutamine synthetase and Sat 3 during herpetic and post-herpetic phase using Western Blot, besides checking as well for the presence of HSV-1 viral load in the spinal cord and ganglions using RT-PCR. The results evidenced alteration of sensitivity in the animals from the 7th day that remained until the 28th day after inoculation of the virus, a change in the MAPKs proteins expression, with a raise of expression of JNK, AKT e CREB in the dorsal horn of the spinal cord in the 8th and 21st day after the HSV-1 virus inoculation, thus suggesting the participation of these proteins in the alteration of sensitivity both in the herpetic and post herpetic periods. It is also possible to observe the presence of viral load in the spinal cord and left spinal ganglion in the herpetic period after HSV-1 virus inoculation

CREB

CREB

Dor neuropática

Glutamine synthetase

HSV-1 virus

MAPK

MAPK

Neuralgia pós herpética

Neuropathic pain

Post Herpetic Neuralgia

Vírus HSV-1

Papel do fator de transcrição AP-1 na hipernocicepção neuropática em camundongos / Role of the AP-1 transcription factor in neuropathic hypernociception in mice.

Poloni, Rafael

24 February 2014

A dor neuropática pode ser causada por lesões e/ou disfunções no sistema somatossensorial. Nestes tipos de dores, alterações plásticas ao longo de todo o sistema sensorial nociceptivo estão associadas à cronificação do processo doloroso. A plasticidade observada pode ser resultante da indução e/ou repressão de genes, os quais geralmente são modulados por fatores de transcrição. Um dos principais fatores de transcrição até então conhecido é a proteína ativadora-1 (AP-1), que pode ser estruturalmente formado principalmente por proteínas das famílias Jun e Fos. Entretanto, na dor neuropática, a participação e o papel do AP-1 não estão bem elucidados. Dessa forma, a hipótese deste trabalho é que a ativação do AP-1 contribua para a indução e/ou manutenção da dor neuropática, através da ativação de células gliais e de proteinocinases ativadas por mitógenos (MAPK) e por indução da produção e liberação de mediadores pró-inflamatórios, bem como de metaloproteinases da matriz extracelular (MMP) na medula espinal. Esses fatores contribuem para sensibilização central causada pela SNI, facilitando a transmissão dolorosa. Assim, a inibição do AP-1 seria uma potencial estratégia terapêutica no tratamento da dor neuropática. Foi utilizado o modelo experimental de dor neuropática de lesão limitada do nervo isquiático (SNI, Spared Nerve Injury) em camundongos, os quais receberam injeção intratecal (i.t.) do inibidor de AP-1, SR11302, ou seu veículo (DMSO, tween® 20 e salina). O tratamento com o inibidor de AP-1 reduziu a hipernocicepção mecânica causada pela SNI, e o perfil de redução sugeriu que esse fator de transcrição esteja relacionado com a manutenção da dor neuropática. No sétimo dia após a SNI, observou-se na medula espinal dos camundongos, ativação da microglia, dos astrócitos e das MAPK, além de aumento na expressão de TNF-, interleucina (IL)-6, IL-1, IL-17A, quimiocina derivada de queratinócito (KC), proteína quimiotáxica de monócitos (MCP-1), óxido nítrico (NO), NO sintase induzível e das MMP-2 e -9. Todos esses eventos estão associados à sensibilização central, portanto, contribuem para a facilitação da transmissão nociceptiva. O tratamento com o inibidor de AP-1 SR11302 impediu, pelo menos parcialmente, a ativação das células gliais e das MAPK e bloqueou o aumento na expressão de todos esses mediadores pró-inflamatórios e das MMPs na medula espinal. Assim, o fator de transcrição AP-1 e, consequentemente, suas vias a jusante (downstream) são potenciais alvos farmacológicos no tratamento da dor neuropática. / Neuropathic pain results from nerve damage or dysfunction, which is associated to the painful process of chronification. This process may include participation of the inducible genes, which may be modulated by transcription factors, including the activator protein-1 (AP-1), which can structurally be formed by proteins from Jun and Fos families. However, the participation and the role of AP-1 neuropathic pain remain unclear. Our hypothesis is that the activation of AP-1 would contribute for the induction and/or maintenance of neuropathic pain, by inducing the glial cells activation and mitogen-activated protein kinases, and by inducing the production/release of pro-inflammatory mediators and extracellular matrix metalloproteinase (MMP) in mices spinal cord. All these factors are contributing to SNI-evoked central sensitization, facilitating pain transmission. Thus, inhibition of AP-1 would be a potential drug target in the treatment of neuropathic pain. The animals received inhalatory anesthesia (2% isoflurane) and were submitted to an experimental model of neuropathic pain Spared Nerve Injury (SNI). The animals were treated intrathecally (i.t.) with AP-1 inhibitor SR11302 or vehicle (DMSO, tween®20 and saline). Treatment with AP-1 inhibitor reduced the SNI-induced mechanical hypernociception, suggesting that this transcription factor is related to the maintenance of neuropathic pain. On the seventh day after SNI, there was in the spinal cord of mice microglia, astrocytes and MAPK activation, increased of expression of TNF-, interleukin (IL)-6, IL-1, IL-17A, keratinocyte-derived chemokine (KC), monocyte chemoattractant protein-1 (MCP-1), nitric oxide (NO) and inducible NO synthase, and increased the expression of MMP-2 and -9. All of these effects are related with central sensitization, thus facilitating nociceptive transmission. However, treatment with SR11302 prevented, at least partially, activation of MAPK and glial cells, as well as prevented the increase in expression of all these pro-inflammatory mediators and MMPs in the spinal cord. Thus, inhibition of AP-1 and hence its way downstream is a potential pharmacological target in the treatment of neuropathic pain.

AP-1

AP-1

Células gliais

Glial cells

Hipernocicepção neuropática

MAPK

MAPK

Mediadores pró-inflamatórios

MMP

MMP

Neuropathic hypernociception

Pro-inflammatory mediators

Contribuição do estresse oxidativo para a ativação das vias NF-kB, FOXO e MAPK para atrofia muscular associada à insuficiência cardíaca: efeito do treinamento físico aeróbico / Contribution of oxidative stress to NF-kB, FOXO and MAPK signaling pathway activation in atrophy induced by heart failure: role of aerobic exercise training

Cunha, Telma Fátima da

20 January 2015

A musculatura esquelética tem um papel fundamental para a manutenção da homeostase do organismo. A perda de massa muscular está relacionada a prejuízos na qualidade de vida de indivíduos saudáveis, além de piorar o prognóstico de pacientes com doenças sistêmicas, como o câncer, o diabetes e a insuficiência cardíaca. Em quadros mais graves de insuficiência cardíaca, a perda excessiva de massa muscular associada a um reduzido consumo de oxigênio de pico, são considerados como preditores independentes de mortalidade. O aumento do estresse oxidativo tem sido apontado como um dos principais desencadeadores do aumento da degradação de proteínas na atrofia muscular. Na presente tese, investigamos a contribuição do estresse oxidativo para a ativação das vias de sinalização NF-kB, FOXO e MAPK na atrofia muscular desencadeada pela insuficiência cardíaca. Para compreender melhor os mecanismos envolvidos na ativação dessas vias pelo estresse oxidativo, utilizamos a linhagem de células musculares C2C12. Observamos que o tratamento com peróxido de hidrogênio (1,2mM, 12h) induziu um aumento do estresse oxidativo, o qual foi capaz de aumentar a atividade do proteassoma, desencadeando a atrofia dos miotúbulos. Verificamos também um aumento da expressão proteica de alguns componentes dessas vias de sinalização, como p-p38 e NF-kB; apontando para uma ativação diferenciada dessas vias pelo estresse oxidativo. Para verificar se essas vias de sinalização relacionadas ao estresse oxidativo estavam também relacionadas à atrofia desencadeada pela insuficiência cardíaca, avaliamos um modelo experimental de ratos com insuficiência cardíaca induzida pelo infartado do miocárdio. Observamos uma redução da área de secção transversa do músculo plantar, acompanhada de um aumento da inflamação sistêmica, de p38 e das atividades de NF-kB e do proteassoma. Como o treinamento físico aeróbico tem se apresentado como uma estratégia terapêutica não farmacológica eficaz na redução do estresse oxidativo e no restabelecimento da atividade do sistema ubiquitina proteassoma, submetemos os ratos infartados ao treinamento físico aeróbico em esteira rolante. O treinamento físico aeróbico preveniu a perda de massa muscular, reduzindo a inflamação sistêmica e as atividades de NF-kB e do proteassoma. Em conjunto, os resultados apontam para o estresse oxidativo como um fator preponderante para o aumento da degradação de proteínas relacionada à atrofia muscular, seja por indução de inflamação (TNF-α) ou por sua ação direta. Além disso, observamos que as vias de sinalização são ativadas de forma diferenciada nos dois modelos, sugerindo que a degradação de proteínas nos miotúbulos está relacionada ao controle de qualidade de proteínas e, nos ratos infartados, às alterações do metabolismo, servindo como fonte de energia. Já o treinamento físico aeróbico comprovou sua eficácia no restabelecimento da atividade do proteassoma, reduzindo a inflamação e a atividade de NF-kB, prevenindo assim, a perda de massa muscular / About 40% of human body mass consists of skeletal muscles, which are involved in all aspects of movement including breathing, eating, posture, walking and reflexes. Skeletal muscle is also important as a source of heat generation and as a regulator of intermediary metabolism. Loss of skeletal muscle mass and function (skeletal muscle atrophy) leads to several functional impairments, affecting health and quality of life. It occurs in several chronic diseases such as cancer, diabetes and heart failure. In heart failure, atrophy is considered an independent predictor of poor prognosis. Oxidative stress has a crucial role in atrophy, activating different signaling pathways capable of stimulating the ubiquitin proteasome system to degrade proteins. In this study, we investigated the oxidative stress contribution to NF-kB, FOXO and MAPK signaling pathway activation in heart failure-induced atrophy. To better understand the mechanisms involved with oxidative stress and signaling pathways activation in atrophy, we have used C2C12 skeletal muscle cells. We observed that, even in high hydrogen peroxide concentrations, oxidative stress increased proteasome activity, phosphorylated p38 and NF-kB protein expression, causing myotubes atrophy. In an experimental heart failure model of infarcted rats, we evaluated plantaris muscle and verified a reduced cross sectional area, accompanied by increased systemic inflammation, p-38 protein expression and increased both NF-kB and proteasome activities. As aerobic exercise training causes a lot of beneficial effects on skeletal muscle structure and function in chronic diseases, we submitted infarcted rats to 8 weeks of aerobic exercise training on a treadmill. Aerobic exercise training prevented atrophy by reducing inflammation and both NF-kB and proteasome activities. Collectively, our data suggest a differentiated activation by oxidative stress in muscle cells and animal models. In the first case, protein degradation was involved with protein quality control; and, in the other, oxidative stress is a second messenger, stimulating protein degradation to provide substrates to metabolism. Aerobic exercise training re-established proteasome activity by reducing inflammation and NF-kB activity, preventing muscle atrophy

Aerobic exercise training

Atrofia

Atrophy

Estresse oxidativo

FOXO and MAPK

FOXO e MAPK

Músculo esquelético

NF-kB

Oxidative stress

Signaling pathways

skeletal muscle

Treinamento físico aeróbico

Vias NF-kB

Influência do excesso de iodo na ativação do oncogene RET/PTC3 na linhagem PCCL3 de tiróide de rato. / Influence of iodine excess in RET/PTC3 oncogene activated PCCL3 thyroid cell lineage.

Fiore, Ana Paula Zen Petisco

04 August 2008

Carcinomas papilíferos (CP) estão relacionados à ativação da via de sinalização MAPK por diversos oncogenes. Estudos têm relacionado a incidência de CP com a disponibilidade de iodo, um dos mais importante reguladores da função tiroidiana. Recentemente, nosso grupo descreveu que a inibição da via de sinalização TGF<font face=\"symbol\">b pode estar vinculada ao desenvolvimento de CP. Nosso objetivo foi avaliar os efeitos do excesso de iodo na transformação de células tiroidianas. Utilizamos células PCCL3 com indução do oncogene RET/PTC3, tratadas com excesso de iodo. Observamos que o iodo reduziu a proliferação, sem alterar a morte das células e recuperou a expressão de genes específicos tiroidianos, evento geralmente vinculado à transformação maligna tiroidiana. O tratamento com excesso de iodo, ainda, reduziu a expressão de proteínas envolvidas na via MAPK e promoveu o restabelecimento da expressão da via TGF<font face=\"symbol\">b, uma importante via inibitória da proliferação de células tiroidianas. Concluímos que o excesso iodo tenha uma ação antioncogênica durante a transformação maligna tiroidiana. / Papillary Carcinomas (PC) are frequently related to MAPK signaling pathway, activation by several oncogenes. Recent studies had related PC incidence and iodine availability, one of the most important thyroid function regulators. Our group has recently showed that TGF<font face=\"symbol\">b pathway inhibition is directly related to PC development. Our aim was to evaluate iodine excess effects during thyroid cells transformation. We used the PCCL3 cells with RET/PTC3 oncogene induction, treated with iodine excess. We observed that iodine reduced the cell proliferation, not altering cell death and recovered thyroid specific genes expression, event frequently liked to thyroid cells malignant transformation. Iodine excess treatment also reduced MAPK proteins expression and reestablished TGF<font face=\"symbol\">b pathway components expression, an important inhibitory pathway of epithelial cells. We can conclude that iodine excess treatment plays an antioncogenic role during thyroid malignant transformation.

Carcinoma papilífero

Cell culture

Cultura de células

Glândula tireóide

Iodine

Iodo

MAPK pathway

Oncogenes

Oncogenes

Papillary carcinoma

Thyroid gland

Via de sinalização MAPK

Cartographie des interactions virus-hôtes pour le virus de la fièvre catarrhale ovine et mise en évidence d'une nouvelle fonction portée par la protéine NS3 / Mapping virus-host interactions for bluetongue virus and highlighting a new function carried by NS3 protein

Kundlacz, Cindy

18 December 2018

Le virus de la fièvre catarrhale ovine (Bluetongue virus, BTV) est l’agent étiologique de la maladie du même nom, une arbovirose non contagieuse transmise aux ruminants domestiques et sauvages par l’intermédiaire de morsures de moucherons hématophages du genre Culicoides. Il existe actuellement 27 sérotypes décrits de BTV à travers le monde qui se distinguent par les pathologies qu’ils induisent et leur capacité à infecter et se propager chez leur(s) hôte(s) mammifère(s). Le premier objectif de mon projet de thèse visait à identifier les interactions cellulaires spécifiques des sérotypes 8 et 27 pour identifier des facteurs de pathogénicité/virulence et/ou de franchissement de barrière d’espèces. Pour atteindre cet objectif, l’ensemble des protéines virales du BTV a été criblé par la méthode du double-hybride en levure contre deux banques d’ADN complémentaires, l’une d’origine bovine et l’autre d’origine culicoïde. A l’issue de 70 cribles, une centaine de nouvelles interactions virus-hôtes a été mise en évidence et révèle un enrichissement pour quatre processus cellulaires : l’épissage des ARNm, les ribosomes, la SUMOylation et l’apoptose. Cette étude nous a ainsi permis de réaliser le premier interactome pour le BTV qui se poursuit au travers de multiples validations biochimiques et fonctionnelles des interactions identifiées. En parallèle de ce travail de protéomique, le second objectif de mon projet de thèse a été de déterminer l’impact du BTV sur la voie MAPK/ERK, une voie cellulaire essentielle à la prolifération et différenciation cellulaire et classiquement modulée lors d’infections virales. En plus de son rôle antagoniste sur la voie des interférons de type I, nous avons démontré la capacité de la protéine NS3 de BTV à activer la voie MAPK/ERK. En effet, nous avons démontré que NS3 a la capacité d’augmenter le niveau de phosphorylation des protéines kinases ERK1/2 mais également du facteur de traduction eIF4E. Cette fonction, qui semble être spécifique au BTV par rapport aux autres orbivirus, implique l’interaction de NS3 avec la protéine cellulaire BRAF, une protéine MAP3 kinase jouant un rôle majeur dans l’activation de la voie MAPK/ERK. L’activation cette voie par NS3 pourrait être un mécanisme de détournement de la traduction cellulaire au profit de celle du virus mais aussi constituer un élément de réponse pour expliquer l’hyper-inflammation observée dans le cas d’une infection par ce virus / Bluetongue virus (BTV) is the etiological agent of the bluetongue (BT) disease, a non-contagious arbovirus that affects a wide range of wild and domestic ruminants. It is transmitted by blood-feeding midges of the genus Culicoides. There are currently 27 serotypes described of BTV in the world that are distinguished by their differences in term of pathology/virulence and their capacity to infect and disseminate in their mammalian host(s). The first objective of my thesis project was to identify specific cellular interactions of serotype 8 and 27 to reveal new factors of pathogenicity/virulence and/or cross species barrier. To reach this goal, all the proteins encoded by BTV were used as baits to screen, by a high-throughput yeast two-hybrid (Y2H) approach, two complementary DNA libraries originating from hosts naturally infected by BTV : Culicoides and cattle. Therefore, 70 screens were performed to identify a hundred of new virus-host interactions and reveal an enrichment for four cellular processes : mRNA splicing, ribosomes, SUMOylation and apoptosis. This study allowed us to build the first interactome of BTV which continues through multiple biochemical and functional validations of the identified interactions. In parallel to this proteomics work, my second objective was to determine the impact of BTV on the MAPK/ERK pathway, a cellular pathway essential for cell proliferation and differentiation usually modulated during viral infections. In addition to its antagonist role on the type I interferon pathway, we have demonstrated the ability of BTV-NS3 to activate the MAPK/ERK pathway. Indeed, we have demonstrated that NS3 has the ability to increase the level of phosphorylation of ERK1/2 protein and the eIF4E translation factor. This function, which seems to be specific to BTV compared to other orbiviruses, involves the interaction of NS3 with BRAF cellular protein, a MAP3 kinase protein that plays a major role in the regulation of the MAPK/ERK pathway. These results could provide a better understanding of the molecular basis underlying the hijacking of the translation machinery to support virus replication but also constitute a hypothesis to explain the hyperinflammation observed in the BTV infection context

Virus de la fièvre catarrhale ovine

Interactions virus-Hôtes

Protéine NS3

Voie MAPK/ERK

Bluetongue virus

Virus-Host interactions

NS3 protein

MAPK/ERK signaling pathway