Implication de la protéine Rnd3/RhoE dans la physiologie et la carcinogenèse hépatiques / Role of Rnd3/RhoE in hepatic physiology and carcinogenesis

Paysan, Lisa

15 December 2014

L'étude des mécanismes moléculaires de la carcinogenèse hépatique a montré l'implication de la RhoGTPase, Rnd3/RhoE. La protéine Rnd3 est sous-exprimée dans le carcinome hépatocellulaire et la diminution de son expression engendre, in vitro, une augmentation de l'invasion des hépatocytes tumoraux. Sur la base de ces travaux, ce projet de thèse s'est décomposé en deux axes. Le premier axe a été d'étudier le rôle de Rnd3 dans la carcinogenèse ainsi que dans la physiologie hépatique in vivo. Ce projet a débuté par la génération d'un modèle murin présentant un KO conditionnel ethépato-spécifique de Rnd3 {KORnd3). L'utilisation de plusieurs stratégies s'est révélée nécessairepour obtenir une extinction protéique de Rnd3 dans la majorité des hépatocytes chez les souris KO. Après hépatectomie des deux tiers, les premiers résultats montrent un retard de régénération hépatique chez les souris KORnd3. En ce qui concerne la carcinogenèse hépatique, nous avons mis en place un modèle de carcinogène chimique en utilisant le diéthylnitrosamine et un modèle de carcinogénèse spontanée chez les animaux KORnd3Hep. Le deuxième axe a porté sur l'étude des invadosomes, structures d'actine impliquées dans l'invasion cellulaire. Nous avons établi une signature minimum pour les invadosomes, impliquant la GTPase Cdc42 et la protéine d'échafaudage TksS. Nos résultats suggèrent également une implication de Rnd3 dans la fonction de dégradation des invadosomes. Ce travail de thèse a ainsi permis d'apporter de nouveaux outils et de nouvellespistes quant à l'implication de Rnd3 dans la physiopathologie hépatique et dans l'invasion cellulaire. / The study of the molecular mechanisms involved in hepatic carcinogenesis revealed the significant down-regulation of the RhoGTPase Rnd3/RhoE in hepatocellular carcinoma as compared to non- tumor liver. Rnd3 down-regulation provides an invasive advantage to tumor hepatocytes suggesting that RND3 might represent a metastasis suppressor gene in hepatocellular carcinoma. This PhD work was divided in two axes. We first studied the role of Rnd3 in the mouse liver using carcinogenesis and liver regeneration protocols. We thus generated conditional and liver specific Rnd3 KO mice (KORnd3Hep). The first results obtained after partial hepatectomy suggest a delay in liver regeneration for the KORnd3Hep mice. We also developed a carcinogenesis strategy in KORnd3Hep mice using diethylnitrosamine treatment. The second axis focused on invadosomes, which are actin-based structures involved in cell invasion. We have determined a minimal and universal molecular signaturefor functional invadosomes, which involves the RhoGTPase Cdc42 and the adaptor protein TksS. We also highlighted the role of Rnd3 in invadosome degradation. ln conclusion, this work provides new tools and new insights on Rnd3 function in hepatic physiopathology and cellular invasion.

RND3/RhoE GTPase

Souris

Regeneration hépatique

Invasion

Carcinoma hépatocellulaire

Invadosomes

RND3/RhoE GTPase

Mice

Liver regeneration

Invasion

Hepatocellular carcinoma

Invadosomes

Rôle de la protéine NLRP7 dans la placentation normale et tumorale : cas du choriocarcinome / Role of NLRP7 protein in normal and tumor pregnancies

Reynaud, Déborah

21 December 2018

Les môles hydatiformes complètes (MHC) sont des lésions bénignes précancéreuses du placenta qui dans 5% des cas évoluent vers un cancer très prolifératif dénommé, choriocarcinome (CC). Différents travaux ont rapporté une corrélation entre le développement des MHC récurrentes et les mutations du gène NLRP7. Ce gène code pour la protéine NLRP7 de l’inflammasome dont l’activation contribue à la production d’IL-1 et IL-18. La majorité des travaux publiés à ce jour se sont intéressés à l’étude des mutations de NLRP7. En revanche, aucune étude n’a caractérisé son rôle dans la placentation normale et tumorale. L’objectif de mon projet de thèse était de caractériser le rôle de cette protéine dans le placenta normal et tumoral. Trois approches ont été utilisées, i) Clinique, en collaboration avec le CHU de Casablanca ; le centre de référence Français des Maladies Gestationnelles Trophoblastiques (MGT) et l’Université Mc Gill pour l’accès aux tissus et sera collectés chez des patientes MHC ou CC; ii) In Vitro/Ex Vivo, pour la caractérisation du rôle du NLRP7 dans les processus clés du développement placentaire normal et tumoral dans des systèmes de cultures en 2D et 3D. Deux lignées trophoblastiques ont été utilisées, les cellules non tumorales HTR-8 Sv/Neo et la lignée JEG3 issue d’un CC humain ; iii) In Vivo, par l’injection orthotopique de cellules JEG3, invalidées ou non pour l’expression du gène NLRP7 (stratégie ShRNA), dans le placenta de souris gestantes. L’impact tumoral des JEG3 suite à leur injection dans la corne utérine et dans la veine de la queue de souris non gestantes a également été étudié.Mes travaux ont démontré que la protéine NLRP7 est abondamment exprimée dans le placenta normal au cours du premier trimestre de la grossesse, que son expression est régulée positivement par l’hypoxie, paramètre clé du développement du placenta et que cette protéine contrôle les processus clés du développement placentaire comme la prolifération et la différentiation trophoblastique. Par ailleurs, j’ai aussi démontré que NLRP7 joue un rôle compensatoire important dans la pathologie du retard de croissance intra-utérin. En relation avec le développement tumoral placentaire, mes travaux ont démontré que, i) la protéine NLRP7 est augmentée dans le placenta de patientes MHC et CC, et que les protéines de la machinerie des inflammasomes sont aussi dérégulées, ii) les cellules tumorales JEG3 surexpriment le NLRP7 comparé au HTR-8 Sv/Neo, iii) l’invalidation de NLRP7 dans les JEG3 induit une baisse de leur prolifération et augmentation de leur migration et invasion dans les systèmes de culture 2D et 3D. L’étude in vivo a démontré que l’invalidation de NLRP7 diminue le développement et la métastase du CC humain dans les trois modèles étudiés. Les analyses immunohistologiques, RNAseq et anticorps-array ont permis la caractérisation des mécanismes régulés par la protéine NLRP7 dans les JEG3. L’ensemble de mes travaux ont mis en évidence le rôle critique de la protéine NLRP7 dans le développement placentaire normal et tumoral et proposent la machinerie NLRP7 comme cible potentielle pour le traitement du CC. / Complete hydatidiform moles (CHM) are benign precancerous lesions of the placenta that evolve in 5% of cases into a highly proliferative cancer called choriocarcinoma (CC). Numerous studies have reported correlations between the development of recurrent CHM and mutations in the NLRP7 gene. NLRP7 protein belongs the NLRP7-inflammasome, whose activation contributes to the production of mature IL-1 and IL-18. Most of the work published on NLRP7 was focused on the study of NLRP7 mutations in CHM. Though, no study has characterized its role in normal and tumor placental development. The aim of my thesis project was to characterize the role of this protein in the normal and tumor placenta. Three approaches were used, i) A clinical approach, in collaboration with Casablanca University Hospital; the French reference center of Trophoblastic Gestational Disease and with McGill University. These collaborations allowed for tissue access from MHC and CC patients; ii) An in Vitro / Ex Vivo approach for the characterization of the role of NLRP7 in key processes of normal and tumor placental development using 2D and 3D culture systems. Two trophoblastic cell types were used, a non-tumor cell line, the HTR-8 Sv/Neo and the JEG3 cells, derived from human CC; iii) An In Vivo approach through orthotopic injection of JEG3 cells, invalidated or not for the expression of the NLRP7 gene (ShRNA strategy), in the placenta of gravid mice. The tumor impact of JEG3 following their injection into the uterine horn and the vein of the tail of non-pregnant mice was also examined.The first part of my work showed that NLRP7 protein is abundantly expressed in the normal placenta during the first trimester of pregnancy, that its expression is upregulated by hypoxia, a key parameter in placental development, and that this protein controls key processes of placental development such as proliferation and differentiation. Importantly, I have also demonstrated that NLRP7 plays an important compensatory role in the pathology of intrauterine growth retardation. The second part of my work concerning the role of NLRP7 protein in the placental tumor development demonstrated that i) NLRP7 protein levels are increased in the placenta of MHC and CC patients, and that components of the inflammasome machinery are also deregulated, ii) the JEG3 cells overexpress NLRP7 compared to HTR-8 Sv/Neo, iii) NLRP7 knock-down in JEG3 induced a significant decrease in their proliferation and an increase in their migration and invasion both in the 2D and 3D culture systems. The in vivo study demonstrated that the knock-down of NLRP7 decreased the development and metastasis of human CC in the three tested routes. Immunohistological, RNAseq and antibody-array analyses allowed the characterization of the pathways regulated by the NLRP7 protein in JEG3 cells.Altogether my PhD project characterized the critical role of the NLRP7 protein in normal and tumor placental development and proposes the NLRP7 machinery as a potential target for CC treatment.

Placenta

Moles hydtiformes

Choriocarcinome

Invasion tumorale

Métastases

Nlrp7

Placenta

Hydatiform moles

Choriocarcinoma

Tumor invasion

Metastasis

Nlrp7

570

Investigation of inhibitors of polysialyltransferase as novel therapeutics for neuroblastoma. Development of in vitro assays to assess the functionality and selectivity of novel small-molecule inhibitors of polysialyltransferases for use in neuroblastoma therapy

Saeed, Rida F.

January 2015

Polysialic acid is aunique carbohydrate that decorates the surface of the neural cell adhesion molecule. Polysialic acidis an onco-developmental antigen, expressed in tumours principally of neuroendocrine origin, notably neuroblastoma,strongly correlating with invasion and metastasis. Polysialylation is regulated by two polysialyltransferase enzymes, PST(ST8SiaIV)and STX(ST8SiaII),withSTX dominant in cancer. Post-development polysialic acid expression is only found at low levels in the brain, thus this could be a novel target for cancer therapy. It is hypothesized that inhibition of polysialyltransferasecould lead to control of tumour dissemination and metastasis.The aims of this thesis were to develop tools and in vitro assays to screen novel polysialyltransferaseinhibitors. A panel of tumour cell lines were characterised in terms of growth parameters (using the MTT assay) and polysialic acid expression. This includes a pair of isogenic C6 rat glioma cells (C6-STX and C6-WT) and naturally polysialic acid expressing neuroblastoma cells(SH-SY5Y). Following this, an in vitro assay was validated to screen modulation of polysialic acid expression by removing pre-existing polysialic acid expression using endoneuraminidase N and evaluated the amount of re-expression of polysialic acid using immunocytochemistry. Then, a functional assay was developed and validated for invasion, the matrigel invasion assay. Cytidine monophosphate (tool compound) significantly reduced polysialic acidsurface expression and invasion. A panel of six novel polysialyltransferase inhibitors was screened for cytotoxicity, polysialic acidsurface expression and invasion. Of the potential polysialyltransferase inhibitorsevaluated, ICT3176 and ICT3172 were identified from virtual screening of Maybridge library and were emerged as the most promising inhibitors, demonstrating significant (p<0.05)reduction in cell-surface polysialic acidre-expression and invasion in polysialic acid expressing cells.Furthermore, the specificity of compounds for polysialyltransferase (α-2,8-sialyltransferase) over othermembers of the wider sialyltransferase family (α-2,3-and α-2,6-sialyltransferases) was confirmed using differential lectin staining. These results demonstrated that small molecule inhibitors as STX is possible and provides suitable in vitrocell based assays to discovery more potent derivatives.

Ukrainakrigets rötter : En motivanalys av Rysslands invasion av Ukraina 2022 / The roots of the Ukraine war : A motive analysis of Russia's 2022 Invasion of Ukraine

Thoms Jensen, Christoph

January 2023

This study is a qualitative case study, with a theory-consuming approach and motive analytical structure that aims to examine Russia's ulterior motives, for the full-scale military invasion of Ukraine in February 2022. The analysis is based on a theoretical framework of two different international relations theories: realism and constructivism. Realism highlights security, military power and the survival of state in the international system while constructivism highlights the interactions between different constructed identities, norms and ideas within the international system. Together with the theoretical framework the analysis uses Kremlin's own statements, to see if it corresponds with the theoretical findings. The study concludes that the two theoretical perspectives complement each other in explaining Russia's ulterior motives and that Kremlin's own statements on Ukraine was able to correspond with the theoretical findings.

Russia

Ukraine

Invasion

Motive analysis

International relations

Realism

Constructivism

Ryssland

Ukraina

Invasion

Motivanalys

Internationella relationer

Realism

Konstruktivism

Political Science

Statsvetenskap

The role of the adaptor protein lamellipodin in glioblastoma cell invasion and radiosensitivity

Moritz, Stefanie

19 September 2022

Background: Highly infiltrative growth and resistance to radiation as well as chemotherapy contribute to a poor prognosis of glioblastoma. To improve the survival of patients with glioblastoma, further research to uncover the complex signaling network is essential. Due to the central role of the signaling adaptor lamellipodin in nervous system development and cell migration, a function of lamellipodin in glioblastoma is conceivable. However, the specific function of lamellipodin in the invasion and radioresistance of glioblastoma is so far entirely unknown. Therefore, the present work investigates the invasion and radioresistance of glioblastoma cells and the underlying signaling mechanism under the influence of lamellipodin. Material and Methods: Expression of lamellipodin was evaluated in human astrocytes and nine glioblastoma cell lines by Western blot analysis. Localization of lamellipodin in glioblastoma cells was analyzed by applying immunofluorescence staining. The effects of lamellipodin silencing by siRNA on the glioblastoma characteristics invasion, survival, and residual DNA double strand breaks (DSB) upon X-ray irradiation, proliferation, apoptosis, and senescence were investigated. Alterations in molecular signaling were analyzed by phosphoproteome analysis upon control and lamellipodin depletion combined with/-out X-ray irradiation in A172 cells. Colony formation assays were performed after single and double knockdown of lamellipodin and the affected proteins to connect latter findings to clonogenic survival. Direct lamellipodin binding partners were explored using mass spectrometry analysis. Validation of protein-protein interaction was determined by immunoprecipitation and proximity ligation assay. Clonogenic survival assay was performed after triple knockdown of lamellipodin, previous proteins identified by phosphoproteome, and the direct interaction partner of lamellipodin. Hierarchical analysis was performed by analyzing the expression and phosphorylation of the determined proteins by immunoblot. Results: Lamellipodin was shown to be expressed and phosphorylated in varying amounts in the glioblastoma cell culture panel, with a preferential localization in membrane protrusions and the cytoplasm. The siRNA-specific depletion of lamellipodin tremendously decreased glioblastoma invasion and proliferation while exerting no impact on apoptosis or senescence. Moreover, seven of the nine studied glioblastoma cell lines were radiosensitized by lamellipodin silencing without affecting the number of residual DNA double strand breaks, while its overexpression improved radiation survival. Mechanistically, the loss of lamellipodin impaired the phosphorylation of nine proteins (EIF2A, EGFR, FOS, MKK6, NFKBIA, PRKAA2, RSK2, SRC, and TAK1), which are mostly implicated in the EGFR-MAPK signaling. The combinational silencing of lamellipodin and the relevant proteins achieved overall radiosensitization in A172 and U343MG cells. Furthermore, mass spectrometric analysis of lamellipodin immunoprecipitates demonstrated that the lamellipodin interactome alters in response to X ray irradiation conditions. RICTOR was confirmed as a direct linker of lamellipodin to the EGFR-MAPK signaling by immunoprecipitation and proximity ligation assay. In addition, triple depletion of lamellipodin, RICTOR, and EGFR resulted in similar degrees of radiosensitization as reported for lamellipodin knockdown, highlighting their superimposable role in glioblastoma radiation response. In line, lamellipodin silencing increased EGFR expression and phosphorylation, while lamellipodin phosphorylation was decreased upon EGFR deficiency. Conclusion: The results uncover the crucial function of lamellipodin for invasion, proliferation, and radiosensitivity of glioblastoma cells. Based on molecular analyses, lamellipodin was discovered as a determinant of EGFR signaling by interacting with RICTOR. Based on these data, the complexity of the signaling networks conducting radiation survival is broadened by adding the adaptor protein lamellipodin. / Hintergrund: Ein stark infiltrierendes Wachstum und Resistenzen gegenüber Bestrahlung und Chemotherapie tragen zu einer schlechten Prognose des Glioblastoms bei. Um die Therapie des Glioblastoms zu verbessern, ist die weitere Erforschung des komplexen Signalnetzwerkes notwendig. Aufgrund der essentiellen Rolle des Signaladaptors Lamellipodin für die Entwicklung des Nervensystems und der Migration von Zellen ist eine Funktion von Lamellipodin im Glioblastom vorstellbar. Die spezifische Funktion von Lamellipodin in der Invasion und Strahlenresistenz des Glioblastoms ist allerdings bisher völlig unbekannt. Die vorliegende Arbeit untersucht daher die Invasion und Strahlenresistenz von Glioblastomzellen sowie den zugrundliegenden molekularen Mechanismus im Hinblick auf Lamellipodin. Material und Methoden: Die Expression von Lamellipodin wurde in humanen Astrozyten und neun Glioblastom-Zelllinien mittels Western Blot Analyse untersucht. Die Lokalisierung von Lamellipodin in Glioblastomzellen wurde mit Immunfluoreszenzfärbung analysiert. Die Auswirkungen eines Lamellipodin-Knockdown mittels siRNA auf die Glioblastom-Eigenschaften Invasion, Überleben und residuale DNA-Doppelstrangbrüche (DSB) bei Röntgenbestrahlung, Proliferation, Apoptose und Seneszenz wurden untersucht. Veränderungen in molekularen Signalwegen wurden durch Phosphoproteomanalyse nach Kontroll- und Lamellipodin-Knockdown in Kombination mit und ohne Röntgenbestrahlung in A172 Zellen analysiert. Koloniebildungsassays wurden nach einfachem und doppeltem Knockdown von Lamellipodin und den betroffenen Proteinen durchgeführt, um letztere Ergebnisse mit dem klonogenen Überleben in Verbindung zu bringen. Direkte Lamellipodin-Bindungspartner wurden mittels massenspektrometrischer Analyse untersucht. Die Validierung der Protein-Protein-Interaktion wurde durch Immunpräzipitation und Proximity Ligation Assay bestimmt. Ein klonogenes Überlebensassay wurde nach dreifachem Knockdown von Lamellipodin, durch das Phosphoproteom identifizierten Proteinen und dem direkten Interaktionspartner von Lamellipodin durchgeführt. Die hierarchische Analyse erfolgte durch Analyse der Expression und Phosphorylierung der ermittelten Proteine mittels Immunblot. Ergebnisse: Die Expression und Phosphorylierung von Lamellipodin war unterschiedlich in den Glioblastomzelllinien. Die siRNA-vermittelte Deletion von Lamellipodin verringerte die Invasion und Proliferation von Glioblastomzellen enorm, während die Reduktion von Lamellipodin keine Auswirkungen auf Apoptose oder Seneszenz hatte. Darüber hinaus wurden sieben der neun untersuchten Glioblastomzelllinien durch das Ausschalten von Lamellipodin radiosensibilisiert, ohne dass sich dies auf die Anzahl der residualen DNA-Doppelstrangbrüche auswirkte, während die Überexpression von Lamellipodin das Überleben nach Bestrahlung verbesserte. Mechanistisch beeinträchtigte der Verlust von Lamellipodin die Phosphorylierung von neun Proteinen (EIF2A, EGFR, FOS, MKK6, NFKBIA, PRKAA2, RSK2, SRC und TAK1), die hauptsächlich an der EGFR-MAPK-Signalübertragung beteiligt sind. Die kombinierte Ausschaltung von Lamellipodin und den relevanten Proteinen führte zu einer allgemeinen Radiosensibilisierung in den Zelllinien A172 und U343MG. Darüber hinaus zeigte die massenspektrometrische Analyse von Lamellipodin-Immunpräzipitaten, dass sich das Lamellipodin-Interaktom als Reaktion auf Röntgenbestrahlung verändert. RICTOR wurde durch Immunpräzipitation und Proximity Ligation Assay als direktes Bindeglied von Lamellipodin zum EGFR-MAPK-Signalweg identifiziert. Darüber hinaus führte die dreifache Deletion von Lamellipodin, RICTOR und EGFR zu einem ähnlichen Grad an Radiosensibilisierung wie der Knockdown von Lamellipodin, was ihre gemeinsame Rolle bei der Strahlenreaktion von Glioblastomen unterstreicht. Darüber hinaus erhöhte die Ausschaltung von Lamellipodin die EGFR-Expression und -Phosphorylierung, während die Lamellipodin-Phosphorylierung bei EGFR-Mangel verringert wurde. Schlussfolgerung: Die Ergebnisse decken die entscheidende Funktion von Lamellipodin für die Invasion, Proliferation und Radiosensitivität von Glioblastomzellen auf. Basierend auf molekularen Analysen wurde Lamellipodin als eine Determinante der EGFR-Signalübertragung durch Interaktion mit RICTOR identifiziert. Auf der Grundlage dieser Daten wird die Komplexität des Signalnetzwerks, welches das Überleben durch Strahlung reguliert, durch das Adaptorprotein Lamellipodin erweitert.

info:eu-repo/classification/ddc/610

ddc:610

Standardisering eller differentiering? : En studie om företags bibehållande av legitimitet i krigstider

Enander Sjökvist, Evelina, Olsson Islani, Nina

January 2024

Abstract   Title: Standardization or differentiation? - A study on companies' maintenance of legitimacy in times of war.   Level: Bachelor's thesis in Business Administration. Authors: Evelina Enander Sjökvist and Nina Olsson Islani. Supervisor: Asif M Huq. Date: May 2024.   Aim: "The purpose of the study is to examine the impact of war on companies' maintenance of legitimacy. How Nordic companies operating in Russia have communicated regarding this crisis to uphold their legitimacy".   Method: A qualitative research method with an abductive approach has been chosen in the form of a document study. A content analysis will be used on documents obtained from the Retriever database or companies websites.   Results and Conclusions: The results show that companies use different strategies when it comes to crisis management of the war between Russia and Ukraine. Clear standardization and differentiation exist both between companies and industries, showing their unique strengths and standards that the companies adhere to. A central conclusion that has characterized the study from the beginning is that this concerns sensitive information.   Contributions: The study has contributed to the research area of companies maintaining legitimacy in times of war and crisis management, the study focuses on companies that have acted in the war. An additional contribution is the analysis model that has been constructed.   Suggestions for future research: A suggestion for further research is to study the full consequences of the war and the sensitivity of information over time. It would be interesting to conduct a study focusing on comparing different years in the annual reports. / Sammanfattning    Titel: Standardisering eller differentiering? - En studie om företags bibehållande av legitimitet i krigstider.    Nivå: Kandidatuppsats i företagsekonomi. Författare: Evelina Enander Sjökvist och Nina Olsson Islani. Handledare: Asif M Huq. Datum: Maj 2024.    Syfte: “Studiens syfte är att studera krigets påverkan på företagens bibehållande av legitimitet. Hur nordiska företag med verksamhet i Ryssland kommunicerat angående denna kris för att upprätthålla sin legitimitet”.   Metod: En kvalitativ forskningsmetod med en abduktiv ansats har valts i form av en dokumentstudie. En innehållsanalys kommer att användas på dokument inhämtade från databasen Retriever och företags webbsidor.        Resultat och Slutsats: Resultaten visar på att företag använder sig av olika strategier när det gäller krishantering av kriget mellan Ryssland och Ukraina. Tydlig standardisering och differentiering finns både mellan företag och branscher, som visar på deras unika styrkor och standarder som företagen förhåller sig till. En central slutsats som präglat studien från början är att detta gäller känslig information.     Bidrag: Studien har bidragit till forskningsområdet kring företags bibehållande av legitimitet i krigstider samt krishantering då studien riktar sig mot företag som agerat gentemot kriget. Ett ytterligare bidrag till framtida forskning är den analysmodell som konstruerats.     Förslag till vidare forskning: Förslag till vidare forskning är att studera krigets fullständiga konsekvenser samt informationens känslighet längre fram i tiden. Det hade varit intressant att utföra en studie där jämförelse mellan olika årtal på årsredovisningarna varit i fokus.

Legitimacy

Crisis Management

Russia's invasion of Ukraine

Annual Reports.

Legitimitet

Krishantering

Rysslands invasion av Ukraina

Årsredovisning.

Business Administration

Företagsekonomi

Neutrophil antimicrobial proteins enhance Shigella flexneri adhesion and invasion

Eilers, Björn

04 November 2009

Shigella flexneri verursacht im Verlauf der Infektion eine massive Enzündungsreaktion sowie Schädigung des humanen Darmepithels. Neutrophile sind die ersten Zellen des angeborenen Immunsystems, welche den Infektionsherd infiltrieren. Diese Zellen greifen Mikroorganismen mittels Phagozytose, Neutrophiler extrazellulärer Fallen (Neutrophil Extracellular Traps, NETs) oder Degranulierung an. In dieser Arbeit haben wir untersucht, wie die Degranulierung von Neutrophilen die Virulenz von Shigellen beeinflußt und konnten zeigen, dass die Exposition von Shigellen mit Proteinen aus den Granula von Neutrophilen die Invasion in Epithelzellen stark erhöht. Während dieser Exposition binden kationische Proteine der Granula an die Oberfläche von Shigella und bewirken eine verstärkte Adhesion, welche dann schließlich zu “Hyperinvasion” führt. Dieser Effekt wird durch Änderungen der Oberflächenladung bewirkt, da eine Lipopolysaccharid (LPS) Mutante mit negativer Oberflächenladung eine zusätzliche erhöhte Hyperinvasion im Vergleich zu Wildtyp Shigellen zeigt. Zusätzlich zur Hyperinvasion bewirkt die Infektion von Epithelzellen mit Shigellen, die mit Granula Proteinen in Kontakt gekommenen sind, eine Verminderung der IL-8 Sekretion. Dieses Zytokin bewirkt eine starke Rekrutierung von Neutrophilen. Daher stellen wir die Hypothese auf, dass Shigella in der Lage ist, antimikrobielle Proteine des Wirtes zur Erhöhung seiner Virulenz durch Hyperinvasion zu verwenden sowie eine weitere Rekrutierung von Neutrophilen durch Inhibition der IL-8 Sekretion zu verhindern. Somit unterwandert Shigella das angeborenen Immunsystem und nutzt dessen Angriff zu seinem Vorteil. / Shigella flexneri is an enteric pathogen that causes massive inflammation and destruction of the human intestinal epithelium. Neutrophils are the first cells of the innate immune system recruited to the site of infection. These cells can attack microbes by phagocytosis, Neutrophil Extracellular Trap (NET) formation and degranulation. Here, we investigated how neutrophil degranulation affects virulence and show that exposure of Shigella to granular proteins enhances infection of epithelial cells. During this process, cationic granular proteins bind to the Shigella surface causing increased adhesion which ultimately leads to hyperinvasion. This effect is mediated by changes in the surface charge, since a lipopolysaccharide (LPS) mutant with a negative surface shows enhanced hyperinvasion compared to wild-type Shigella. In addition, infection with Shigella exposed to granular proteins leads to the inhibition of secretion of the neutrophil attracting cytokine IL-8. We propose that Shigella uses host defense molecules to enhance its virulence by increased infection of its host cells and reduced recruitment of neutrophils after hyperinvasion through inhibition of IL-8 secretion. With this Shigella subverts the innate immune system and uses its attack for its own benefit.

Shigella

Neutrophile

Antimikrobielle Proteine

Invasion

Shigella

Neutrophils

Antimicrobial proteins

Invasion

570 Biologie

32 Biologie

WF 7250

ddc:570

The Distribution, Dynamics & Impacts Of Invasive Lantana Camara In A Seasonal Forest Of Mudumalai, Southern India

Ramaswami, Geetha

06 1900

Species that become naturalized in a new geographical range, subsequently multiply and spread, and persist to the detriment of resident communities, are known as alien invasive species. Two aspects of species invasion – spread and ecological impact – were examined using Lantana camara L. (henceforth lantana) as the study system, specifically in the context of a seasonally dry tropical forest ecosystem of the Mudumalai Wildlife Sanctuary and National Park. Lantana is a thicket-forming woody shrub of South and central American origin, which is now widespread across the tropics. The thesis is divided broadly into two parts -the first part examines the influences of environmental factors on the distribution and spread of lantana while the second part focuses on the effects of lantana on the distribution, survival and growth of native woody species. Much of the work presented in this thesis was conducted within a 50 ha permanent plot (the Mudumalai Forest Dynamics Plot, MFDP hereon) in Mudumalai, chiefly because the history of invasion by lantana has been recorded here since 1989. The influence of changing resources on lantana invasion was explored at two scales -small spatial but fine temporal scale in the MFDP and at the level of the landscape. Available data on an 18 year chronosequence of changes in the qualitative density of lantana from the MFDP and field studies between the years 2009 and 2010 were used to determine the environmental correlates of lantana spread in time and space. It was found that biotic factors such as the presence of the shrub Helicteres isora and abiotic factors such as proximity to drainages and the combination of fire and drought promoted the intensification of lantana invasion in time while proximity to streams, higher total annual rainfall and low fire frequency contributed to lantana invasion at the landscape level. The impacts of lantana on the seedlings of native woody species were assessed in 10m x 10m plots within the MFDP. An initial enumeration of 60 such plots revealed that animaldispersed, dry forest habitat preferring species were most affected by the presence of dense lantana. A follow-up study comprising of growth and survival measurements made on 1105 seedlings over two years (2008-2010) further confirmed that dry forest preferring species were most affected by the presence of dense lantana and that this response at the community level was most likely influenced by the most abundantly sampled species in this habitat preference guild – Catunaregam spinosa. In conclusion, while the environmental correlates of lantana most likely promoted its invasion, only certain guilds of native species seemed to be negatively affected by the presence of lantana.

Alien Invasive Species

Lantana Camara

Lantana Invasion

Lantana Camara Invasion

Mudumalai Forest Dynamics Plot (MFDP)

Native Woody Species

Invasive Species

Ecology

Apport de l'approche évolutive pour l'étude de l'invasion de l'acarien rouge de la tomate, Tetranychus evansi / Contribution of an evolutionary approach to study the invasion of the red tomato spider mite, Tetranychus evansi

Boubou, Angham

22 November 2010

L'acarien rouge de la tomate Tetranychus evansi (Tetranychidae) est considéré comme une espèce invasive à fort impact économique sur les cultures de solanacées. Il a été découvert pour la première fois en 1954 au Brésil, d'où il est probablement originaire. Historiquement, T. evansi a d'abord été signalé en Afrique et plus récemment en Europe et en Asie. L'objectif de cette thèse était de reconstruire les routes de colonisation de T. evansi et de dégager le scénario évolutif décrivant le mieux l'histoire de l'invasion. Nous avons d'abord analysé des échantillons collectés dans son aire actuelle de distribution, à l'aide des séquences d'un fragment du gène codant pour la sous-unité I de la Cytochrome Oxydase (COI) de l'ADN mitochondrial et de la région ITS1-5,8S-ITS2 de l'ADN nucléaire ribosomique. Les données soutiennent l'hypothèse d'une origine sud américaine de cette espèce et ont révélé que des événements d'invasions multiples et cryptiques ont eu lieu lors de la colonisation de l'Europe. L'invasion résulte de deux lignées génétiquement divergentes et originaires de deux régions géographiques distantes au Brésil. Ces deux lignées semblent avoir des potentiels invasifs contrastés. Elles s'hybrident au laboratoire ainsi que dans la nature. Grâce à 16 locus microsatellites que nous avons développés et utilisés comme marqueurs, nous avons déterminé les zones géographiques de cette hybridation. Nous avons également pu estimer des paramètres historiques de l'invasion et confronter différents scénarios d'introduction, par la comparaison de la composition génétique des populations récemment introduites avec celles de l'aire d'origine de T evansi, et par l'utilisation de la méthode d'inférence bayésienne (Approximate Bayesian Computation, ABC). Les résultats ABC contredisent partiellement le scénario d'invasion basé uniquement sur des données historiques. Ils suggèrent que T. evansi serait d'abord arrivé en Europe dans le sud de l'Espagne (en Andalousie) bien avant les signalements historiques. Ainsi, l'Andalousie semble avoir servi de source de colonisation pour des nouvelles zones en Afrique, d'autres régions méditerranéennes et d'Asie. Les résultats de cette thèse ouvrent des perspectives d'étude visant à comprendre pourquoi certaines populations d'une espèce allochtone réussissent à s'établir et à envahir un nouvel écosystème / The red tomato spider mite Tetranychus evansi (Tetranychidae) is regarded as an invasive species having an important economic impact on solanaceous crops. It was first discovered in Brazil in 1954, where it probably originated. Based on historical records, T. evansi was first reported in Africa and more recently in Europe and Asia. This work aims at reconstructing the colonization routes of T. evansi and identifies the scenario that best describes the evolutionary history of the invasion. To do this, we first analyzed samples collected from most parts of the world where the mite is currently known to occur. We used sequence variation of a fragment of the mitochondrial Cytochrome Oxidase I (COI) sub-unit I gene and the ITS1-5.8S-ITS2 of the nuclear ribosomal DNA. Our results were consistent with the hypothesis of a South American origin of this species. They also suggested that the invasion of south Europe resulted from multiple cryptic introductions from two genetically divergent lineages originated from two distant geographical regions in Brazil. These two lineages seem to have a differential invasive potential. Despite the high genetic divergence, crosses between mites stemming from the two lineages do occur both in the laboratory and in nature. Second, we used 16 microsatellite loci that we developed for this study and in association with Approximate Bayesian Computation (ABC) methods; we reconstructed the historical events of the cryptic invasion of the pest. ABC results challenge the invasion scenario captured by historical data only. They suggest that T. evansi first arrived to Europe in Southern Spain (Andalusia) long before historic records. Thus, Andalusia seems to have served as a source for colonization of new areas in Africa and other Mediterranean regions. The results obtained in this thesis provide an interesting framework to further study and understand why some populations of an exotic species might become invasive.

Tetranychus evansi

Espèce invasive

Routes de colonisation

Microsatellites

ADN mitochondrial

Invasion cryptique

Tetranychus evansi

Invasive species

Colonization routes

Microsatellites

Mitochondrial DNA

Cryptic invasion

Implication de la protéine tyrosine phosphatase DEP-1/PTPRJ dans la promotion de l’invasion des cellules du cancer épithélial de l’ovaire

Roussy, Jacinthe

01 1900

Le cancer épithélial de l’ovaire (CÉO) est le cancer gynécologique le plus létal. Bien que certains progrès aient été accomplis, une meilleure compréhension des mécanismes moléculaires impliqués dans le développement de ce cancer est requise. Notre laboratoire a démontré que la protéine tyrosine phosphatase DEP-1 était impliquée dans l’activation de Src, la survie, la migration et l’invasion des cellules endothéliales en réponse au VEGF. Des études ont proposé que Src ait également un rôle important dans la progression tumorale du CÉO. Ainsi, nous nous intéressons au rôle de DEP-1 dans le potentiel invasif du CÉO. Nous avons observé des niveaux d’expression variables de DEP-1 dans 6 lignées cellulaires du CÉO et constaté que ceux-ci corrèlent positivement avec le potentiel invasif des cellules dans le Matrigel. Des expériences d’ARNi ont démontré que la réduction de l’expression de DEP-1 inhibe des voies de signalisation pro-invasives telles que la phosphorylation de Src et de Cortactine, ainsi que la localisation de Cortactine aux lamellipodes. Cette déplétion de DEP-1 a également eu pour effet de diminuer d’autres voies de signalisation pro-tumorales, tel que la phosphorylation de l’EGFR et de P65 (NfκB). Conséquemment, la déplétion de DEP-1 par transfection d’ARNi se traduit par une perte du potentiel invasif des cellules, et une diminution de la résistance des cellules au Carboplatin. L’analyse de l’expression de DEP-1 par immunohistochimie dans les tumeurs ovariennes révèle l’existence d’une corrélation positive entre l’expression en protéine de DEP-1 et le cancer de l’ovaire de grade élevé et la survie des patientes, qui a également été confirmé sur une puce à ARN. Nos résultats suggèrent que DEP-1 favoriserait la progression tumorale du cancer épithélial de l’ovaire. Nous avons démontré que DEP-1 est impliquée dans l’invasion in vitro, et que son expression est associée à un cancer de l’ovaire plus agressif, faisant ainsi de DEP-1 une cible thérapeutique potentiellement intéressante. / Epithelial ovarian cancer (EOC) is the most lethal gynecological cancer. Our laboratory has previously shown that the protein tyrosine phosphatase DEP-1 is involved in Src activation, survival, migration and invasion of endothelial cells in response to VEGF. Studies have shown that Src may be implicated in the progression of epithelial ovarian cancer progression. Thus, we were interested in determining if DEP-1 had a role in the promotion of the Src invasive pathway in EOC. First, we have observed a variable protein expression of DEP-1 in six EOC cell lines, and that there was a positive correlation with invasion in Matrigel. We also showed in RNAi experiments that inhibition of DEP-1expression resulted in the decreased phosphorylation of Src and Cortactin, also loss of Cortactin localisation at the cellular membrane. We also observed dysregulation of other pro-tumoral pathways like EGFR and P65 (NfκB) diminution of phosphorylation. Consequently, DEP-1 depletion resulted in loss of invasive capacities of most of the cell lines, and diminution of chemoresistance in response to Carboplatin. Analysis of DEP-1 in EOC tumors revealed the existence of a positive correlation with an aggressive form of ovarian cancer, high grade status, and poorer survival. These results suggest a positive role of DEP-1 in tumor progression of EOC. Our results show for the first time that DEP-1 is implicated in invasion in vitro, and is associated with the most aggressive form of EOC. Thus, DEP-1 is an interesting therapeutical target for EOC.

Invasion cellulaire

DEP-1

progression tumorale

immunohistochimie

Src

In vitro

In situ

Invasion

tumor progression

immunohistochemistry