Global ETD Search

141	Mise au point d'une stratégie pharmacologique originale pour l'obtention de composés anti-cancéreux anti-migratoires / Setting up of an original pharmacological strategy to discover antimigration anticancerous compounds Hayot, Caroline 12 May 2006 (has links) La migration cellulaire est une étape clé intervenant à un stade précoce de la dissémination des cellules cancéreuses dans l’organisme, et est donc responsable de la formation des métastases qui tuent environ nonante pourcent des patients atteints de cancer. De plus, ces cellules migrantes résistent à l’apoptose grâce à l’activation constitutive de voies de signalisation anti-apoptotiques, et développent donc une résistance vis-à-vis des traitements anti-cancéreux actuels qui sont généralement pro-apoptotiques. Nous avons pris pour cible ce processus de migration cellulaire dans l’espoir d’identifier des agents anti-migratoires qui permettraient de lutter contre la formation des métastases et de restaurer chez les cellules migrantes une certaine sensibilité aux traitements pro-apoptotiques.<p>Dans la première partie de notre travail, nous avons analysé les effets anti-angiogéniques et anti-migratoires des agents anti-tubuline. Nous avons confirmé que le Taxol® présentait une action anti-angiogénique à des concentrations non-cytotoxiques. Nous avons ensuite démontré que d’autres agents anti-tubuline exerçaient la même action que le Taxol®, et que cette action leur était spécifique. Nous avons montré que certains de ces agents étaient également capables de réduire la migration de lignées cellulaires tumorales, toujours à des concentrations non-cytotoxiques, et que cette action pouvait s’exercer via une affectation du cytosquelette d’actine.<p>Dans la deuxième partie du présent travail, nous avons démontré l’importance de la mise au point d’une approche pharmacologique originale permettant l’identification de composés à action anti-migratoire puisque l’outil utilisé par le U.S. National Cancer Institute pour le criblage de nouvelles molécules anti-cancéreuses ne permet pas de discerner l’activité anti-migratoire des molécules testées.<p>Enfin dans la troisième partie de ce travail, après avoir souligné la raison du choix de l’actine comme cible pour inhiber la migration cellulaire, nous avons développé une stratégie pharmacologique in vitro originale de découverte de composés anti-actine à activité anti-migratoire. Grâce à une approche divisée en plusieurs étapes, à savoir un essai de cytotoxicité, une étude de la dynamique de la polymérisation d’actine en tubes ou sur cellules entières, et des essais de migration bidimensionnelle sur cellules individuelles ou sur population cellulaire, nous avons montré d’une part que des molécules connues pour affecter le cytosquelette actinique étaient capables d’affecter la migration cellulaire, et d’autre part que la méthodologie que nous avons développée permettait bien l’identification de composés affectant l’actine et capables de réduire la migration de cellules tumorales. En conclusion, cette stratégie in vitro pourrait être utilisée dans l’identification de nouvelles molécules à activité anti-migratoire pour lutter contre le cancer.<p> / Doctorat en sciences pharmaceutiques / info:eu-repo/semantics/nonPublished Sciences pharmaceutiques Antineoplastic agents Actin Cytoskeleton Anticancéreux Actine Cytosquelette actin cancer migration cytoskeleton
142	DISHEVELLED-ASSOCIATED ACTIVATOR OF MORPHOGENESIS 1 (DAAM1) IS REQUIRED FOR HEART MORPHOGENESIS Li, Deqiang 02 February 2010 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / Dishevelled-associated activator of morphogenesis 1 (Daam1), a member of the formin protein family, has been implicated in the non-canonical Wnt mediated Planar Cell Polarity (PCP) signaling pathway. Although the studies in Drosophila Daam1 and Xenopus Daam1 generated inconsistent conclusions regarding the function of Daam1, the biological function of mammalian Daam1 was not evaluated. In this study, we used a mouse promoter trap technology to create Daam1 deficient mice to analyze the role of Daam1 in embryonic development and organogenesis. Daam1 is highly expressed in the developing heart. The majority of Daam1 mutant mice died between embryonic day 14.5 and birth, exhibiting a variety of heart defects, which include ventricular noncompaction, ventricular septal defects, and double outlet right ventricle. About 10% mutant mice survive to adulthood, and these survivors do not show significantly compromised heart function based on echocardiographic analyses. However, all of these mutant survivors have ventricular noncompaction with a range of severities. A conditional rescue experiment using a cardiac specific Cre mouse line, Nkx2-5Cre, confirmed that the cardiac defects are the primary cause of death in Daam1 mutants. Both in vivo and ex vivo analyses revealed that Daam1 is essential for regulating non-sarcomeric filamentous actin assembly in cardiomyocytes, which likely contributes to cardiac morphogenesis and ventricular wall maturation. Biochemical studies further suggested that Daam1 is not a key signaling component in regulating the activation of small GTPases, such as RhoA, Rac1 and Cdc42. In conclusion, our studies demonstrated that Daam1 is essential for cardiac morphogenesis likely through its regulation of cytoskeletal architecture in the developing cardiomyocytes. / indefinitely Morphogenesis Heart -- Abnormalities Actin
143	Novel Coronin7 interactions with Cdc42 and N-WASP regulate actin organization and Golgi morphology 28 February 2020 (has links) Yes / The contribution of the actin cytoskeleton to the unique architecture of the Golgi complex is manifold. An important player in this process is Coronin7 (CRN7), a Golgi-resident protein that stabilizes F-actin assembly at the trans-Golgi network (TGN) thereby facilitating anterograde trafficking. Here, we establish that CRN7-mediated association of F-actin with the Golgi apparatus is distinctly modulated via the small Rho GTPase Cdc42 and N-WASP. We identify N-WASP as a novel interaction partner of CRN7 and demonstrate that CRN7 restricts spurious F-actin reorganizations by repressing N-WASP ‘hyperactivity’ upon constitutive Cdc42 activation. Loss of CRN7 leads to increased cellular F-actin content and causes a concomitant disruption of the Golgi structure. CRN7 harbours a Cdc42- and Rac-interactive binding (CRIB) motif in its tandem β-propellers and binds selectively to GDP-bound Cdc42N17 mutant. We speculate that CRN7 can act as a cofactor for active Cdc42 generation. Mutation of CRIB motif residues that abrogate Cdc42 binding to CRN7 also fail to rescue the cellular defects in fibroblasts derived from CRN7 KO mice. Cdc42N17 overexpression partially rescued the KO phenotypes whereas N-WASP overexpression failed to do so. We conclude that CRN7 spatiotemporally influences F-actin organization and Golgi integrity in a Cdc42- and N-WASP-dependent manner. / This work was supported by SFB 670 and DFG NO 113/22. K.B. was supported by a fellowship from the NRW International Graduate School “From Embryo to Old Age: the Cell Biology and Genetics of Health and Disease” (IGSDHD), Cologne. Actin cytoskeleton Golgi complex Coronin7 (CRN7) N-WASP Actin organization Golgi morphology
144	Coordination by Cdc42 of actin, contractility, and adhesion for melanoblast movement in mouse skin 28 February 2020 (has links) Yes / The individual molecular pathways downstream of Cdc42, Rac, and Rho GTPases are well documented, but we know surprisingly little about how these pathways are coordinated when cells move in a complex environment in vivo. In the developing embryo, melanoblasts originating from the neural crest must traverse the dermis to reach the epidermis of the skin and hair follicles. We previously established that Rac1 signals via Scar/WAVE and Arp2/3 to effect pseudopod extension and migration of melanoblasts in skin. Here we show that RhoA is redundant in the melanocyte lineage but that Cdc42 coordinates multiple motility systems independent of Rac1. Similar to Rac1 knockouts, Cdc42 null mice displayed a severe loss of pigmentation, and melanoblasts showed cell-cycle progression, migration, and cytokinesis defects. However, unlike Rac1 knockouts, Cdc42 null melanoblasts were elongated and displayed large, bulky pseudopods with dynamic actin bursts. Despite assuming an elongated shape usually associated with fast mesenchymal motility, Cdc42 knockout melanoblasts migrated slowly and inefficiently in the epidermis, with nearly static pseudopods. Although much of the basic actin machinery was intact, Cdc42 null cells lacked the ability to polarize their Golgi and coordinate motility systems for efficient movement. Loss of Cdc42 de-coupled three main systems: actin assembly via the formin FMNL2 and Arp2/3, active myosin-II localization, and integrin-based adhesion dynamics. / Cancer Research UK (to L.M.M. [A17196], R.H.I. [A19257], and S.W.G.T.) and NIH grants P01-GM103723 and P41-EB002025 (to K.M.H.). N.R.P. is supported by a Pancreatic Cancer Research Fund grant (to L.M.M.). Funding to Prof. Rottner by the Deutsche Forschungsgemeinschaft (grant RO2414/3-2). Rho GTPases Migration Actin cytoskeleton Cell motility Melanocyte Myosin Actin Adhesion Integrin Cdc42
145	WASP restricts active Rac to maintain cells' front-rear polarization 28 February 2020 (has links) Yes / Efficient motility requires polarized cells, with pseudopods at the front and a retracting rear. Polarization is maintained by restricting the pseudopod catalyst, active Rac, to the front. Here, we show that the actin nucleation-promoting factor Wiskott-Aldrich syndrome protein (WASP) contributes to maintenance of front-rear polarity by controlling localization and cellular levels of active Rac. Dictyostelium cells lacking WASP inappropriately activate Rac at the rear, which affects their polarity and speed. WASP’s Cdc42 and Rac interacting binding (“CRIB”) motif has been thought to be essential for its activation. However, we show that the CRIB motif’s biological role is unexpectedly complex. WASP CRIB mutants are no longer able to restrict Rac activity to the front, and cannot generate new pseudopods when SCAR/WAVE is absent. Overall levels of Rac activity also increase when WASP is unable to bind to Rac. However, WASP without a functional CRIB domain localizes normally at clathrin pits during endocytosis, and activates Arp2/3 complex. Similarly, chemical inhibition of Rac does not affect WASP localization or activation at sites of endocytosis. Thus, the interaction between small GTPases and WASP is more complex than previously thought—Rac regulates a subset of WASP functions, but WASP reciprocally restricts active Rac through its CRIB motif. / Cancer Research UK grants A15672, A24450, and multidisciplinary grant A20017. Actin polymerization Arp2/3 complex Cell polarity Uropod Small GTPases CRIB motif Actin cytoskeleton
146	Bundles of Semi-flexible Cytoskeletal Filaments Strehle, Dan 30 June 2014 (has links) (PDF) Schaut man durch ein Mikroskop auf eine biologische Zelle mit angefärbten Zytoskelett, so erblickt man lange, mehr oder minder gerade Objekte. Mit ziemlicher Sicherheit gehören diese zu einer von drei Arten von Zytoskelettfilamenten -- Aktin- oder Mikrofilamente, Intermediärfilamente und Mikrotubuli. Schon seit mehreren Jahrzehnten versucht man die mechanischen Eigenschaften lebender Zellen nicht nur zu beschreiben, sondern ihr Verhalten von zwei tieferen Ebenen ausgehend zu verstehen: Inwiefern beschreiben die Eigenschaften von Filamentnetzwerken und -gelen die Zellmechanik und, noch tiefgreifender, wie bestimmen eigentlich die einzelnen Filamente die Netzwerkmechanik. Das Verständnis der Mechanik homogener und isotroper, verhedderter als auch quervernetzter Gele ist dabei erstaunlich detailreich, ohne jedoch vollständig dem jüngeren Verständnis von Zellen als glassartige Systeme zu entsprechen. In den letzten Jahren sind daher anisotrope Strukturen mehr und mehr in den Fokus gerückt, die die Bandbreite möglichen mechanischen Verhaltens enorm bereichern. Die vorliegende Arbeit beschäftigt sich mit solch einem hochgradig anisotropen System -- nämlich Aktinbündeln -- unter drei Gesichtspunkten. Mit Hilfe von aktiven Biegedeformationen wird ein funktionales Modul, das eine differentielle Antwort auf verschiedenen Zeitskalen liefert, identifiziert. Es handelt sich um Aktinfilamente, die durch transiente Quervernetzer gebündelt werden. Während sich das System nach kurz anhaltenden Deformation völlig elastisch verhält, sorgt eine Restrukturierung der Quervernetzer während langanhaltender Deformationen für eine plastische Verformung des Bündels. In einem weiteren Aspekt widmet sich die Arbeit der frequenz- und längenabhängigen Biegesteifigkeit. Die Methode des Bündel-Wigglings, das Induzieren von \"Seilwellen\", wird dabei genutzt, um aus der Wellenform die Biegesteifigkeit zu berechnen. Bündel von Aktinbündeln zeigen dabei ein Verhalten, das vom klassischen Worm-like-chain-Modell abweicht und stattdessen durch das Worm-like-bundle-Modell beschrieben werden kann. Der letzte Aspekt dieser Arbeit untersucht den Musterbildungsprozess bei der Entstehung von Aktinbündeln. Gänzlich unerwartet entstehen quasi-isotrope Strukturen mit langreichweitiger Ordnung, wenn der Bündelungsprozess erst nach der Polymerisation von Filamenten frei von zusätzlichen mechanischen Einwirkungen einsetzt. Da dieser Zustand nicht von der klassischen Flüssigkristalltheorie vorhergesagt wird, soll eine Simulation eine Hypothese zum Entstehungsmechanismus testen. Die Annahme einer lateralen Kondensation von Filamenten zu Bündeln reicht demnach aus, um die beobachteten Strukturen zu erzeugen. Diese Arbeit leistet somit einen Beitrag zum Verständnis hochgradig anisotroper Strukturen und deren Überstrukturen, wie sie auch in lebendigen Zellen reichlich vorhanden sind. / Being the most basic unit of living organisms, the cell is a complex entity comprising thousands of different proteins. Yet only very few of which are considered to play a leading part in the cell’s mechanical integrity. The biopolymers actin, intermediate filaments and microtubules constitute the so-called cytoskeleton – a highly dynamic, constantly restructuring scaffold endowing the cell not only with integrity to sustain mechanical perturbations but also with the ability to rapidly reorganize or even drive directed motion. Actin has been regarded to be the protagonist and tremendous efforts have been made to understand passive actin networks using concepts from polymer rheology and statistical mechanics. In bottom-up approaches isotropic, homogeneous actin-gels are well-characterized with rheological methods that measure elastic and viscous properties on different time scales. Cells, however, are not exclusively isotropic networks of any of the mentioned filaments. Rather, actin alone can already be organized into heterogeneous and highly anisotropic structures like bundles. These heterogeneous structures have only come into focus recently with theoretical work addressing bundle networks. and, in the case of the worm-like bundle theory, individual bundles. This work aims at characterizing bundles and bundle-crosslinker systems mechanically in two complementary approaches – in the time as well as in the frequency domain. In addition, it illuminates a bundle formation mechanism that leads to bundle networks displaying higher ordering. Aktinbündel Zytoskelettfilamente Biegesteifigkeit Rheologie actin bundles cytoskeletal filaments bending stiffness rheology ddc:539 ddc:570 Actin-Filament Zellskelett Biegesteifigkeit Rheologie Actin-bindende Proteine Elastoplastizität Biorheologie
147	Etude biochimique comparative des "Actin Depolymerizing Factors"(ADFs) d'Arabidopsis : activité inattendue de pontage des filaments d'actine pour les ADFs appartenant à la sous-classe III / Comparative biochemical analysis of Arabidopsis Actin-Depolymerizing Factors (ADFs) : unexpected actin-crosslinking activity for subclass III ADFs Tholl, Stéphane 02 March 2012 (has links) L'organisation et la dynamique du cytosquelette d'actine sont finement régulées par une multitude de "actin-binding proteins" (ABPs). Parmi ces dernières, les ADFs (actin-depolymerizing factors) jouent un rôle majeur dans le turnover des filaments d'actine en induisant leur découpage et en facilitant leur dépolymérisation. Arabidopsis thaliana possède 11 protéines ADFs fonctionnelles qui peuvent être classées en 4 sous-classes sur la base de leur profil d'expression et liens phylogénétiques. Nous démontrons que l’ADF5 et l’ADF9 de la sous-classe III sont des ADFs atypiques puisqu’elles n’induisent pas la dépolymérisation des filaments d’actine. Au contraire, elles montrent une forte capacité à stabiliser et ponter les filaments d’actine en longs câbles in vitro ainsi que in vivo. Nous décrivons la caractérisation d’un nouveau mutant knockout d’Arabidopsis. Les données suggèrent un rôle d’ADF9 dans l’élongation cellulaire. Ainsi, l’hypocotyle est significativement plus long dans les mutants adf9 que dans les plantules sauvages, et ce phénotype est amplifié par des conditions de croissance à l’obscurité dans lesquelles le gène ADF9 est normalement préférentiellement exprimé. L’analyse des cellules épidermiques d’hypocotyle indique que ce phénotype est essentiellement dut à une augmentation de l’élongation cellulaire. De manière surprenante, les plantules mutantes adf9 présentent également des racines plus courtes que les contrôles, suggérant un lien complexe entre l’organisation du cytosquelette d’actine et l’élongation cellulaire. Finalement, la capacité réduite du cal issue des plantules adf9 à proliférer suggère également un rôle d’ADF9 dans la division cellulaire. / Actin cytoskeleton organization and dynamics are tightly regulated by many actin-binding proteins (ABPs). Among ABPs, the actin-depolymerizing factors (ADFs) play a major role in actin filament turnover by promoting actin filament severing and facilitating pointed end depolymerization. Arabidopsis thaliana has 11 functional proteins that can be classified into four subclasses according to their expression profile and phylogenetic relationships. We provide evidence that subclass III ADF5 and ADF9 are unconventional ADFs since they do not display typical actin filament depolymerizing activities. Instead, they exhibit opposite activities with a surprisingly high ability to stabilize and crosslink actin filaments into long and thick actin bundles both in vitro and in live cells. Competition experiments with ADF1 support that ADF9 antagonizes the depolymerizing activity of conventional ADFs. We report the characterization of a not yet described knockout Arabidopsis mutant. Data strongly suggests a role for ADF9 in cell elongation. Indeed, hypocotyls are significantly longer in adf9 mutant than in wild- type seedlings, and this phenotype is enhanced in dark growth conditions in which the ADF9 gene is normally preferentially expressed. The analysis of hypocotyl epidermal cells indicates that this phenotype is essentially due to an increase of cell expansion. Surprisingly, adf9 seedlings exhibit shorter roots than control plants, suggesting a complex link between actin cytoskeleton organization and cell elongation. Finally, the reduced ability of adf9- derived calli to proliferate supports a role for ADF9 in cell division as well. ADF Câbles d’actine Cytosquelette d’actine Arabidopsis PH Phosphorylation LIM Elongation cellulaire Actin bundles Actin cytoskeleton Actin-depolymerizing factors Arabidopsis Cell elongation LIM domain proteins PH Phosphorylation 571.6
148	Molecular and functional characterisation of the adherent properties of H7 flagella Wolfson, Eliza Briony Kate January 2013 (has links) Enterohaemorrhagic Escherichia coli (EHEC) have recently emerged as significant zoonotic pathogens. O157:H7 is one of the most common EHEC serotypes associated with human disease, which is transmitted faeco-orally from a bovine reservoir. EHEC O157:H7 preferentially colonises the bovine terminal rectum (BTR). Injection of virulence factors by type-III secretion is necessary for colonisation of cattle and results in re-modelling of the host cytoskeleton. Flagella machinery is evolutionarily related to the Type III secretion apparatus and O157 strains lacking H7 flagella show reduced adherence to the BTR. Vaccination with FliC, the main component of H7 flagella, has the potential to protect cattle against E. coli O157:H7 infection. The focus of this work was to investigate the molecular basis for H7 flagella binding to the BTR, in order to understand the basis for FliCH7 being an immuno-protective antigen. H7 flagella were shown to adhere across the surface and penetrate into BTR epithelial cells. Both the FliC shaft and the FliD cap components of flagella filaments showed the capacity to adhere to BTR epithelial cells. Preliminary studies indicate that the current FliCH7 vaccination of cattle results in FliD-specific antibodies where oral challenge with O157:H7 does not. FliD is more conserved than FliCH7, which contains a predicted 88aa structural insertion, but variation occurs along the full length of the FliD protein. There was no evidence for post-translational modification of FliCH7. A number of actin binding proteins were identified as potential FliC and FliD binding partners from BTR epithelial cell lysates. From this, a panel of purified galectin-4, cofilin-1 and βγ-actin was used to compare binding of flagella from different pathogens. H7 flagella bound more to cofilin-1 than βγ-actin, whereas phase-1 and phase-2 flagella from Salmonella Typhimurium bound more to βγ-actin, than to cofilin-1. Size-exclusion chromatography indicated that cofilin-1 alters H7 flagella filament polymerisation dynamics. αβ-ctin polymerisation and depolymerisation experiments indicate that H7, phase-1 and phase-2 flagella interactions with actin affect actin dynamics. 616.9
149	Mechanisms of Chlamydia manipulation of host cell biology revealed through genetic approaches Kokes, Marcela January 2015 (has links) <p>Chlamydia trachomatis is the most common sexually transmitted bacterial pathogen and is the leading cause of preventable blindness worldwide. Chlamydia is particularly intriguing from the perspective of cell biology because it is an obligate intracellular pathogen that manipulates host cellular pathways to ensure its proliferation and survival. This is achieved through a significant remodeling of the host cell’s internal architecture from within a membrane-bound vacuole, termed the inclusion. However, given a previous lack of tools to perform genetic analysis, the mechanisms by which Chlamydia induces host cellular changes remained unclear. Here I present genetic and molecular mechanisms of chlamydial manipulation of the host cytoskeleton and organelles. Using a forward genetics screen, InaC was identified as a necessary factor for the assembly of an F-actin structure surrounding the inclusion. InaC associated with the vacuolar membrane where it recruited Golgi-specific ARF-family GTPases. Actin dynamics and ARF GTPases regulate Golgi morphology and positioning within cells, and InaC acted to redistribute the Golgi to surround the Chlamydia inclusion. These findings suggest that Chlamydia places InaC at the inclusion-cytosolic interface to recruit host ARF GTPases and F-actin to form a platform for rearranging intracellular organelles around the inclusion. The inclusion is also surrounded by the intermediate filament vimentin and the chlamydial protease CPAF cleaves vimentin in vitro. CPAF-dependent remodeling of vimentin occurred selectively in late stages of the infection. In living cells, this cleavage occurred only after a loss of inclusion membrane integrity, suggesting that CPAF cleaves intermediate filaments specifically during chlamydial exit of host cells. In summary, I have implemented recent forward and reverse genetic approaches in Chlamydia to reveal how it employs effector proteins to manipulate the internal organization of cells in novel ways.</p> / Dissertation Microbiology Cellular biology Actin Chlamydia Cytoskeleton Genetics Organelle Pathogenesis
150	F-actin and integrin like proteins in Phytophthora cinnamomi Harland, Chad S. January 2007 (has links) Tip growth is the primary form of growth in hyphal organisms and some plant cells. Tip growth in hyphae is highly dependent on F-actin, which acts to regulate and support growth. One of the models suggested for tip growth, the amebae model of tip growth, suggests that F-actin may also be the primary source of protrusive force for tip growth in some conditions, and that proteins with a similar function to animal integrins would be present an involved in tip growth (Heath and Steinberg 1999). In this thesis we examine the role of F-actin in the growth of the oomycete Phytophthora cinnamomi and the effects on growth of the F-actin disrupting compound Latrunculin B. We demonstrate that F-actin plays a critical role in the tip growth of Phytophthora cinnamomi with it's disruption causing rapid cessation in directional growth, followed by significant subapical swelling. Further more we examine Phytophthora cinnamomi for the presence of an B4 integrin like protein that has been previously reported in the oomycete Achlya bisexualis (Chitcholtan & Garrill 2005) and show that the B4 integrin like protein is not present in Phytophthora cinnamomi. These experiments help further our understanding of tip growth in Phytophthora cinnamomi an economically important plant pathogen. tip growth hyphal organisms plant cells F-actin

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