Microsporidian Spores and the Integrin Binding Loop of the MADAM Protein Are Important for Integrin Signaling and Attachment to Host Cells

Barrett, Cindy L

01 August 2023

Microsporidia are a distant fungal pathogen that have severe clinical consequences for the immunocompromised. Previous work identified a microsporidian pathogen protein termed Microsporidian ADAM or MADAM. This protein has close sequence homology to other ADAM proteins (A Disintegrin and Metalloproteinase) in two microsporidian species, Encephalitozoon intestinalis and E. cuniculi. ADAM proteins have a wide range of functions, including binding to integrins and host signaling. It is known that many pathogens manipulate integrins to invade host cells, and it is predicted that microsporidia are also exploiting this host target. Previous work with the MADAM protein demonstrated that this protein has a role in adherence to host cells. Separate work showed integrin inhibitors can also decrease spore adherence to cells. Experiments in this project complement previous research and further characterize the binding of microsporidia to host integrins and the intracellular consequences of that binding. This work found the integrin binding sequence of MADAM (MADAM peptide) is important for spore binding to host cells. Separate work shows that the host β1 integrin is also involved in spore adherence. Additional work demonstrated that spores and the MADAM peptide elicited an increase in host integrin signaling in Western blotting experiments. And finally, preliminary acellular interferometry experiments suggest the MADAM protein binds specifically to α5β1 and α6β4 integrins. Together, these results suggest microsporidia spores rely, in part, on host integrins to bind to host cells before infection.

microsporidia

cell attachment

integrins

β1 integrin

ADAM protein

Biology

Immunology and Infectious Disease

Medicine and Health Sciences

Microbiology

Identification de nouveaux acteurs moléculaires impliqués dans la mécanotransduction des chondrocytes / Identification of new molecular actors involved in chondrocytes mechanotransduction

Bougault, Carole

13 November 2009

Le phénotype des chondrocytes peut être modulé par des facteurs de croissance comme par des contraintes mécaniques. Nous avons caractérisé le potentiel chondrogénique de la "Bone Morphogenetic Protein" (BMP)-2 sur des chondrocytes murins primaires amplifiés en culture monocouche sur plastique. Nous avons aussi développé un nouveau modèle d’étude de la mécanotransduction par la compression dynamique de ces cellules incluses en hydrogel d’agarose. Nous avons ainsi confirmé l’implication des voies ERK1/2 et p38 dans ces mécanismes, révélé l’activation de Smad2/3 en réponse à la compression et identifié de nouveaux gènes mécano-sensibles. Par ailleurs, nous avons mis en évidence le rôle des intégrines-bêta-1 dans la rigidité du tissu cartilagineux. Nos résultats complètent la connaissance fondamentale des mécanismes de régulation du phénotype chondrocytaire, mais peuvent également contribuer à l'amélioration des techniques de reconstruction du cartilage dans le domaine de l'ingénierie tissulaire. / Chondrocytes phenotype can be modulated by growth factors as well as mechanical stress. We characterised Bone Morphogenetic Protein (BMP)-2 chondrogenic potential on mouse primary chondrocytes expanded in monolayer on culture plastic. Also, we developed a new model to investigate mechanotransduction by applying dynamic compression on these cells embedded in agarose hydrogel. Hence, we confirmed ERK1/2 and p38 pathways implication in such mechanisms, we revealed Smad2/3 activation in response to compression and we identified new mechanosensitive genes. Besides, we highlighted the role of beta-1-integrins in cartilage stiffness. Our results completed the basic knowledge of regulation mechanisms underlying chondrocytes phenotype, but could also contribute to improve techniques for cartilage reconstruction in the field of tissue engineering.

Cartilage

Chondrocytes

Différenciation

Mécanotransduction

Signalisation BMP/TGF-bêta

Intégrines

Cartilage

Chondrocytes

Differentiation

Mechanotransduction

Signaling BMP / TGF-beta

Integrins

571.6

Etude des mécanismes moléculaires régulant la voie Hippo via les intégrines ß1 / Study of the molecular mechanisms regulating the Hippo pathway via the integrins b1

Sabra, Hiba

29 June 2017

L'adhérence cellulaire à la matrice extracellulaire joue un rôle clé dans leur prolifération,leur différenciation ou l'apoptose. Par conséquent ce processus est critique pour undéveloppement normal et pour l'homéostasie tissulaire. La dérégulation de ce mécanismecontribue souvent à des situations pathologiques. Ainsi, la dérégulation de nombreux gènesimpliqués dans les adhérences cellule-cellule ou cellule-matrice extracellulaire sont liés à despathologies conduisant à un défaut de développement, la progression tumorale, oul'inflammation.Les intégrines sont des récepteurs transmembranaires hétéro dimériques jouant un rôlemajeur dans les interactions cellule-matrice extracellulaire. Ce rôle n'est pas limité à unesimple interaction mécanique puisqu'elles permettent également la transduction dessignaux de la matrice extracellulaire à la cellule afin de permettre à cette dernière des'adapter à son micro environnement. Dans le but d’étudier le rôle des intégrines à chaîneβ1 dans le développement osseux, le laboratoire a mis en place un modèle murind'inactivation conditionnelle du gène Itgb1 basée sur l'expression de la recombinase Cre austade pré-ostéoblastique. Les souris mutées présentent un défaut de développementosseux, dû à une faible prolifération des ostéoblastes.Contrairement à ce qui était généralement admis, cette faible prolifération desostéoblastes est indépendante de la voie classique mettant en jeu la voie classique des MAPkinases. En revanche, elle est contrôlée par la voie Hippo: cette signalisation a étérécemment identifiée chez la Drosophile et les Mammifères comme un mécanismeinhibiteur majeur de la prolifération cellulaire. Le cofacteur de transcription YAP, effecteurfinal de cette voie, est une navette nucléo-cytoplasmique. Son expression est amplifiée dansdivers cancers dont l'ostéosarcome où cette surexpression associée à celle de l’Itgb1 est unfacteur de mauvais pronostique.Mes travaux consistent à comprendre comment les intégrines à chaîne β1 contrôlent lavoie Hippo, et donc la prolifération. Nous avons confirmé que la délétion des intégrines β16active la phosphorylation de YAP et sa séquestration dans le cytoplasme. En utilisant destechniques de Biologie Cellulaire et de Biochimie, nous avons montré que suite à la délétionde l’Itgb1, les cellules présentent un défaut de trafic vésiculaire réduisant la translocationmembranaire de Rac1. La séquestration cytoplasmique de Rac1 diminue l’activation de soneffecteur majeur la kinase PAK responsable de la dissociation d'un complexe membranaired'inactivation composé de la protéine adaptatrice NF2, la kinase LATS et de son effecteurprincipal YAP. Les intégrines en provocant la perte de ce complexe induisent ladéphosphorylation de YAP, sa translocation nucléaire et donc stimulent la proliférationcellulaire. / Cell adhesion to the extracellular matrix plays a key role in their proliferation,differentiation or apoptosis. Therefore, this process is critical for normal development andtissue homeostasis. The deregulation of this mechanism often contributes to pathologicalsituations. Thus, the deregulation of many genes involved in cell-cell or cell-extracellularmatrix adhesions are linked to pathologies leading to developmental defects, tumorprogression, or inflammation.Integrins are heterodimeric transmembrane receptors that play a major role in cellextracellularmatrix interactions. This role is not limited to a simple mechanical interactionsince integrins also allow the transduction of the signals from the extracellular matrix to thecell in order to permit the latter to adapt to its microenvironment. In order to study the roleof β1 integrins in bone development, the laboratory has implemented a mouse model withconditional inactivation of the Itgb1 gene based on the expression of recombinase Cre at thepre-osteoblastic stage. The mutated mice show a defect in bone development due to a lowproliferation rate of osteoblasts.Contrary to what was generally accepted, this reduced proliferation is independent of theclassical pathway involving the classical pathway of MAP kinases. On the other hand, it iscontrolled by Hippo: this signaling pathway has recently been identified in Drosophila andMammals as a major inhibitory mechanism of cell proliferation. The transcription cofactorYAP, the end effector of this pathway, is a nucleo-cytoplasmic shuttle. Its expression isamplified in various cancers including osteosarcoma where this overexpression associatedwith that of Itgb1 is a factor of poor prognosis.My work involves understanding how β1 integrins control the Hippo pathway, and thusproliferation. We confirmed that deletion of β1 integrins activates the phosphorylation ofYAP and its sequestration in the cytoplasm. Using Cell Biology and Biochemistry techniques,we showed that following the deletion of Itgb1, the cells exhibit a defect in vesicular trafficthat reduces the membrane translocation of Rac1. The cytoplasmic sequestration of Rac18decreases the activation of its major effector, the PAK kinase. PAK is responsible for thedissociation of an inactivating membrane complex composed of the adaptor protein NF2,the LATS kinase, and its main effector YAP. The integrins by provoking the loss of thiscomplex induce the dephosphorylation of YAP, its nuclear translocation, and thus stimulatecell proliferation.

Intégrines beta 1

Voie Hippo

Trafic vésiculaire

Rac1

Pak

Beta 1 integrins

Hippo pathway

Vesicular traffic

Rac1

Pak

570

Peptídeo C16, derivado da laminina, regula invasão, dinâmica de formação e atividade de invadopódios em linhagens celulares de carcinoma epidermóide e fibrossarcoma. / Laminin-derived peptide C16 regulates invasion and invadopodia activity/dynamics in squamous cell carcinoma and fibrosarcoma cell lines.

Siqueira, Adriane Sousa de

02 June 2014

A laminina contém peptídeos que podem ser liberados por proteólise. Nosso laboratório estuda os efeitos de peptídeos da laminina em biologia tumoral. Neste trabalho, verificamos se C16 (cadeia g1) estimularia invasão e atividade de invadopódios em células de carcinoma epidermóide (CAL27) e fibrossarcoma (HT1080). C16 promoveu aumento na taxa de invasão e atividade de invadopódios em ambas às linhagens celulares, comparado ao peptídeo controle C16SX. Microscopia em time-lapse demonstrou que C16 induz aumento na atividade de invadopódios em função do tempo. C16 estimula fosforilação de Src e ERK 1/2, e inibição da via ERK reduz invasão e atividade de invadopódios relacionados ao peptídeo. C16 conjugado à rodamina foi encontrando decorando a membrana de células CAL27, sugerindo possível interação com receptores. Diminuição dos níveis de integrina b1 reduzem atividade de invadopódios em amostras tratadas com C16. Nossos dados sugerem que C16 regula invasão e atividade de invadopódios em células CAL27 e HT1080, provavelmente por meio de Src, ERK e integrina b1. / Laminin harbors bioactive peptides released upon tumor-induced proteolysis. Our Laboratory has been studying laminin peptides effects in tumor biology. Here we addressed whether C16 (g1 chain) would regulate invasion and invadopodia activity in cell lines from squamous cell carcinoma (CAL27) and fibrosarcoma (HT1080). C16 increased invasion rate and invadopodia activity compared to control peptide (C16SX). Through time-lapse microscopy, we observed that C16 stimulated invadopodia activity overtime. We searched for signaling pathways related to peptide effects. C16 stimulated Src and ERK 1/2 phosphorylation, and ERK signaling cascade inhibition decreased C16-induced invasion and invadopodia. Next, we addressed how C16 would interact with tumor cells. Rhodamine-conjugated C16 was found decorating CAL27 cell membrane, suggesting an interaction with receptors. Knockdown of b1 integrin reduced invadopodia activity of C16-treated cells. We propose that C16 regulates invasion and invadopodia activity of CAL27 and HT1080 cells through Src, ERK and b1 integrin.

Carcinoma epidermóide

Extracellular matrix

Fibrosarcoma

Fibrossarcoma

Integrinas

Integrins

Matriz extracelular

Neoplastic processes

Peptídeos

Peptides

Processos neoplásicos

Squamous cell carcinoma

Interação entre as vias de sinalização do IGF-I, do ER e da integrina 1 na regulação da transcrição do genes PHLDA1 e PAWR / IGF-I, estrogen receptor (ER) and 1 integrin interaction over PHLDA1 and PAWR transcriptional regulation

Casolari, Débora Arcieri

03 October 2008

A interação entre as vias de sinalização do ER, do IGF-I e da integrina 1 é essencial para a manutenção da homeostase da glândula mamária normal, e alterações nessas vias de sinalização estão associadas ao processo de tumorigênese da mama. Portanto, o objetivo deste trabalho foi investigar a influência e inter-relação entre as vias de sinalização do IGF-I, do ER e da integrina 1 na regulação da transcrição dos genes PHLDA1 e PAWR. Para isso, células MCF-7 foram tratadas, por diferentes tempos, com 10nM de 17- estradiol (E2), 12,5nM de IGF-I, 30M de LY294002 (inibidor da PI-3K), 30M de SB202190 (inibidor da p38MAPK) e 1M de ICI182780 (antagonista do ER), ou transfectadas com 40nM de siRNA para integrina 1. A expressão gênica foi avaliada por PCR em tempo real e a expressão protéica por Western Blot. A expressão do gene PHLDA1 aumentou após tratamento com E2 por 6h (p=0,05), e esse efeito foi inibido pelo tratamento com ICI (p<0,05). O tratamento com E2 por 24h inibiu a expressão do gene PAWR (p<0,05), e esse efeito foi dependente de ER, pois foi inibido pelo tratamento com ICI (p<0,05). O tratamento com IGF-I por 1,5h causou aumento na expressão do gene PHLDA1 (p<0,05); e o tratamento com IGF-I por 24h causou diminuição na expressão do gene PAWR (p<0,05). Foi observado aumento na expressão protéica de PHLDA1 após tratamento das MCF-7 com E2 ou IGF-I por 1:30h. A regulação da expressão do PAWR pelo IGF-I ocorreu através das vias da PI-3K e p38MAPK. O efeito do IGF-I sobre a expressão dos dois genes foi independente da ativação do ER, mas foi observado sinergismo entre E2 e IGFI na inibição da expressão dos transcritos do PAWR, com diminuição na expressão para nível menor do que o observado após tratamento com E2 ou IGF-I sozinhos (p<0,05). A repressão da expressão da integrina 1 resultou na diminuição dos níveis de expressão dos genes PHLDA1 e PAWR. Não foi observada interação entre o IGF-I e a integrina 1 na regulação dos genes PHLDA1 e PAWR. Portanto, o gene PHLDA1 é regulado positivamente pelo E2 e pelo IGF-I, mas não existe interação entre as vias. O gene PAWR é regulado negativamente pelo E2 e pelo IGF-I; o efeito do IGF-I é dependente da ativação da PI3-K e da p38MAPK, mas não do ER; e existe sinergismo entre E2 e IGF-I na regulação do PAWR / The interactions among ER, IGF-I and 1 integrin signaling pathways are essential for the maintenance of normal mammary gland homeostasis, and alterations in these pathways have been associated with mammary tumorigenesis. Therefore, the goal of this work was to investigate the influence and interaction among IGF-I, ER and 1 integrin signaling pathways on the regulation of PHLDA1 and PAWR transcription regulation. To accomplish that, MCF-7 cells were treated with 10nM 17-estradiol (E2), 12.5nM IGF-I, 30M LY294002 (a PI3-K inhibitor), 30M SB202190 (a p38MAPK inhibitor) and 1M ICI182,780 (ICI an ER antagonist), or transfected with 40nM siRNA aiming 1 integrin. Real time PCR and western blot were used to evaluate gene and protein expression, respectively. PHLDA1 mRNA expression increased after 6h of treatment with E2 (p=0.05), and this effect was inhibited by ICI (p<0.05). Treatment with E2 for 24h repressed PAWR gene expression (p<0.05) and this effect was dependent on ER, since treatment with ICI inhibited it (p<0.05). Treatment with IGF-I for 1.5h resulted in increased PHLDA1 gene expression (p<0,05) and also PHLDA1 protein expression; and treatment with IGF-I for 24h inhibited PAWR mRNA expression (p<0.05). IGF-I regulation of PAWR expression was dependent on PI3-K and p38MAPK activation. The regulation of both genes by IGF-I was independent of ER activation; however, IGF-I acted in synergism with E2 on PAWR expression resulting in lower PAWR expression than the observed after the treatments alone (p<0.05). Repression of 1 integrin expression resulted in downregulation of PHLDA1 and PAWR expression levels. No interaction was observed between IGF-I and 1 integrin on PHLDA1 and PAWR gene expression. In conclusion, PHLDA1 is positively regulated by E2 and IGF-I, but there is no interaction between them on PHLDA1 regulation. On the other hand, PAWR is negatively regulated by E2 and IGF-I; IGF-I effect is dependent on PI3-K and p38MAPK, but not on ER activation; E2 and IGF-I act synergistically on PAWR gene expression regulation

Apoptose

Apoptosis

Breast neoplasms

Expressão gênica

Gene expression

Integrinas

Integrins

Neoplasias de mama

Receptores estrogênicos

Receptors estrogen

Somatomedinas

Somatomedins

Immunhistochemische Vergleichsanalyse von Primärzellaggregaten und Ursprungsgeweben unterschiedlicher Dignität zur Charakterisirung der in-vitro Anpassung

String, Andreas Sebastian

19 April 2002

Immunhistochemische Vergleichsanalyse von Primärzellaggregaten und Ursprungsgeweben unterschiedlicher Dignität zur Charakterisierung der in-vitro Anpassung Zielsetzung: Dreidimensionale Zellkulturen stellen eine Weiterentwicklung der einschichtigen Zellkultur dar, die den in-vitro Bedingungen im Organismus näherkommt. Darüber hinaus ermöglichen organoide Kulturen, die neben der vorherrschenden Tumorzelle auch Bindegewebszellen und Immunzellen enthalten, eine Analyse der Interaktion dieser Zellen bei wichtigen Aspekten der Krebserkrankung wie Metastasierung, Angiogenese oder der Tumorimmunologie. Materialien und Methoden: Operationsresektate von Schilddrüsengeweben, -adenomen und -karzinomen, Ovarialkarzinomen und Sarkomen wurden in Einzelzellsuspensionen überführt. Nach Inkubation im Schüttler wurden innerhalb von 24-48 Stunden Primärzellaggregate gezüchtet, von denen Kryostatschnitte angefertigt wurden. Mit der APAAP-Methode wurden Epithelzell-, Leukozyten-, Makrophagen- und Endothelzellmarker sowie E-Cadherin, die a2-, a4-, a5- und av Integrinkette, IGF-I und EGF Rezeptoren, cerbB2 sowie Cathepsin D immunhistochemisch untersucht. Die Färbungen der Aggregate und der Herkunftsgewebe wurden statistisch mit dem Mann-Whitney Test verglichen. Ergebnisse: Primäraggregate konnten zu 90-100% aus Operationsresektaten kultiviert werden. Epithelzellen, Leukozyten, Makrophagen und Endothelzellen waren im Primäraggregaten und den Herkunftsgeweben ungefähr gleichmäßig vorhanden. Dies gilt auch für E-Cadherin, a4-Integrin, IGF-I und EGF Rezeptoren, cerbB2 und Cathepsin D. Die a2-, a5- und av Integrinkette trat nur in den Primäraggregaten von Schilddrüsengeweben und -adenomen nicht aber in deren Herkunftsgeweben auf, was auf eine de-novo Exprimierung schließen läßt. Schlußfolgerung: Mit der verwendeten Methode ist es relativ einfach möglich, organoide Primäraggregate zu züchten, die ein geeignetes Forschungsobjekt für verschiedene Aspekte der Tumorpathologie darstellen. Die gefundenen Unterschiede der Integrinexpression zeigen eine Anpassung and die in-vitro Kultivierung und sind möglicherweise eine Reaktion zur Vermeidung der matrix-abhängigen Apoptose. / Immunohistochemical Analysis of primary cell aggregates and their origin tissue of different pathology to evaluate adaptation to in-vitro environment Objective: Three-dimensional cell cultures reflect more closely the in-vitro environment then monolayer cultures. Furthermore, organoid cultures, which contain beside the dominant tumor cell also mesenchymal cells and leucocytes are used to study the interaction of these cells in several aspects of the tumor pathology, such as metastasis, angiogenesis and tumor immunology. Materials and Methods: Specimens obtained from thyroid tissue, thyroid adenomas and carcinomas, ovarian cancer and sarcomas were dissolved to single cell suspensions. After incubation under stirring, primary cell aggregates were cultured within 24-48 hours. Cryostat sections were made and stained with markers of epithelial cells, leucocytes, macrophages, endothelial cells as well as E-cadherin, a2-, a4-, a5- und av Integrin chain, IGF-I und EGF receptor, cerbB2 and Cathepsin D using the APAAP method. The immunhistochemical results of the aggregates and their origin tissue were statistically compared using the Mann-Whitney test. Results: Primary cell aggregates could be obtained from up to 90-100% of all probes. Epithelial cells, leucocytes, macrophages and endothelial cells were found equally in aggregates and their origin tissue. Also E-Cadherin, a4-Integrin, IGF-I und EGF receptors, cerbB2 und Cathepsin D were found equally. The a2-, a5- und av integrin chain was expressed in aggregates of thyroid tissue and adenomas, but not in their origin tissue suggesting a de-novo expression. Conclusion: Primary cell aggregates were easily obtained with the used method and could be used as a model in the study of tumor pathology. The different expressions of integrins show an adaptation to the in-vitro environment and could be a reaction to avoid matrix-related apoptosis.

Zellkultur

Primäraggregat

Integrine

Tumorpathologie

Cell culture

primary aggregates

integrins

tumor pathology

610 Medizin

33 Medizin

WX 6600

ddc:610

Rôle des cellules musculaires lisses vasculaires et des intégrines dans la génération de thrombine dans le compartiment sanguin et vasculaire / Role of vascular smooth muscle cells and integrins in the thrombin generation on vascular and blood compartments

Mohamadi, Amel

21 October 2016

Une des propriétés majeures de la thrombine est le caractère pléiotropique de ses effets physiologiques et pathologiques, à la fois dans le compartiment sanguin et tissulaire de la paroi. Notre hypothèse est que les changements phénotypiques des cellules musculaires lisses vasculaires (CMLVs) participent aux modifications des propriétés pro- et anticoagulantes de la paroi. Les objectifs ont été d’étudier : (i) le rôle prothrombotique des CMLVs dans l’hypertension chez le rat SHR et le syndrome métabolique (Smet) chez le rat Zucker, (ii) les mécanismes de régulation de la génération de thrombine par l’intégrine αvβ3 des CMLVs (récepteur de la pro- thrombine), et de développer des glyco-peptides fluorés pour l’imagerie permettant d’évaluer l’activité de cette intégrine dans la paroi, et (iii) d’évaluer l’effet de variants génétiques du locus 9p21 de susceptibilité aux maladies coronariennes sur le phénotype de coagulation. Résultats : Les CMLVs sont responsables du phénotype prothrombotique de la paroi artérielle associée à l’hypertension chez le rat SHR. Les acides gras libres et l’inflammation vasculaire augmentent la génération de thrombine dans les 2 compartiments ce qui se traduit par une fibrinolyse diminuée et une activité métallo-protéinase augmentée chez Le rat Zucker. L’invalidation de l’intégrine αvβ3 des CMLVs diminue la génération de thrombine dans les 2 compartiments et ralentit la survenue de thrombose carotidienne en réponse à une stimulation l’angiotensine. Le traçage de l’intégrine αvβ3 par des glyco-peptides comprenant une séquence RGD a été validé au niveau plaquettaire et des CMLVs. La souris invalidée pour le locus 9p21 exprime un phénotype pro-thrombotique qui est retrouvé chez l’homme pour certains variants (rs10120688 et rs1333040) dans ce locus. En conclusion, la CML est un support cellulaire clé de réactions procoagulants et pourrait être impliqué via les intégrines et/ou ses récepteurs pour la thrombine dans un couplage thrombine tissulaire – rigidité cellulaire dans les pathologies vasculaires / One of the major properties of thrombin is the pleiotropic character of its physiological and pathological effects, both in the blood compartment and the tissue of the arterial wall. We hypothesized that the phenotypic changes of vascular smooth muscle cells (VSMCs) are involved in modifications of pro- and anti-coagulant properties of the arterial wall. The objectives were to examine: (i) the prothrombotic role of VSMCs in hypertension of SHR rats and in the metabolic syndrome (Smet) of Zucker rats, (ii) regulatory mechanisms of thrombin generation by integrin αvβ3 of VSMCs (a pro-thrombin receptor), and to develop fluorinated glyco- peptides for imaging, to assess the activity of this integrin in the wall, and (iii) evaluate the effect of genetic variants of the 9p21 locus that give a susceptibility to coronary heart disease on the coagulation phenotype. Results: The VSMCs are responsible for the prothrombotic phenotype of the arterial wall associated with hypertension in SHR rats. Free fatty acids and vascular inflammation increase thrombin generation in the two compartments resulting in decreased fibrinolysis and an increased metallo-proteinase activity in the Zucker rats. The invalidation of integrin αvβ3 of VSMCs reduced thrombin generation in the two compartments and slowed angiotensin-induced carotid thrombosis. Tracing of the integrin αvβ3 by glyco-peptides including RGD was validated at the platelet level and VSMCs. Mice invalidated for the 9p21 locus express a prothrombotic phenotype that is found in humans for certain variants (rs10120688 and rs1333040) in this locus. In conclusion, the VSMC is a cell supported key to procoagulant reactions and may be involved via integrins and/or its receptors for thrombin in the ”tissular thrombin - cell rigidity” coupling in vascular pathologies

Génération de thrombine

Intégrines

Cellules musculaires lisses vasculaires

Hémostase

Generation of thrombin

Integrins

Vascular smooth muscle cells

Hemostasis

616.157

Importância da interação entre a integrina Mac-1 leucócitos e a glicoproteína Ib alfa das plaquetas para o recrutamento de leucócitos pelas plaquetas e para a resposta inflamatória à lesão vascular / The importance of the leukocyte integrin Mac-1 and platelet glycoprotein Ib? interaction for the leukocyte recruitment by platelets and for the inflammatory response to vascular injury

Zago, Alexandre do Canto

07 February 2007

INTRODUÇÃO: A interação entre leucócitos e plaquetas é fundamental para o início e a progressão da reestenose e da aterosclerose. Recentemente foi evidenciado em estudos in vitro que a integrina Mac-1 dos leucócitos se liga à glicoproteína Ibalfa (GP Ibalfa) das plaquetas e que esta interação possui uma função central na firme adesão e transmigração de leucócitos em locais de deposição de plaquetas. Entretanto, não há estudos in vivo que avaliam a importância da interação entre a integrina Mac-1 dos leucócitos e a GP Ibalfa das plaquetas (alfaMbeta2-GP Ibalfa) em modelo experimental de lesão vascular. MÉTODO: Um peptídeo denominado M2 ou anticorpo anti-M2 foi desenvolvido para bloquear a interação da integrina Mac-1 dos leucócitos com a GP Ibalfa das plaquetas, visando, deste modo, inibir a adesão de leucócitos na superfície do vaso coberta por plaquetas, a proliferação celular e a hiperplasia neointimal. Este peptídeo foi injetado e comparado com anticorpo-controle em camundongos C57B1/6J submetidos à lesão vascular da artéria femoral com corda-guia. Um dia (controle: n= 6; anti-M2: n= 6), 5 dias (controle: n= 9; anti-M2: n= 9) ou 28 dias (controle: n= 9; anti-M2: n= 9) após a lesão vascular, as artérias femorais foram retiradas para a realização de morfometria e imunohistoquímica. RESULTADOS: O bloqueio da interação alfaMbeta2-GP Ibalfa promoveu redução estatisticamente significativa de 75% do número de leucócitos na camada média no primeiro dia após a lesão vascular (controle: 7,9 ± 5,0% do total de células na camada média; versus anti-M2: 2,0 ± 1,6%; p=0,021), bem como determinou diminuição estatisticamente significativa de 42% em 5 dias (controle: 42,3 ± 12,9% do total de células na neoíntima; versus anti-M2: 24,6 ± 10,8%; p=0,047) e de 58% em 28 dias do acúmulo de leucócitos na neoíntima em desenvolvimento (controle: 7,9 ± 3,0% versus anti-M2: 3,3 ± 1,3%; p=0,012). A proliferação celular na camada média do vaso em 5 dias pós-lesão vascular apresentou redução estatisticamente significativa de 64% com o bloqueio da interação alfaMbeta2-GP Ibalfa (controle: 5,0 ± 2,9% do total de células na camada média; versus anti-M2: 1,8 ± 0,5%; p=0,043), assim como houve diminuição significativa de 47% da proliferação celular na camada íntima do vaso em 28 dias (controle: 3,8 ± 1,7% do total de células na camada íntima; versus anti-M2: 2,0 ± 1,2%; p=0,047). O bloqueio da interação alfaMbeta2-GP Ibalfa também determinou redução estatisticamente significativa de 56% do espessamento intimal em 28 dias (controle: 10.395 ± 3.549um2; versus anti-M2: 4.561 ± 4.915um2; p=0,012). CONCLUSÕES: O recrutamento de leucócitos após a lesão vascular é dependente da interação alfaMbeta2-GP Ibalfa e a neutralização desta interação inibe a proliferação celular e a formação neointimal. / INTRODUCTION: The interaction between leukocytes and platelets is fundamental for the beginning and the progression of restenosis and atherosclerosis. Recent in vitro studies have shown that the leukocyte integrin Mac-1 binds to the platelet glycoprotein (GP) Ibalfa, and this interaction plays a central role in the leukocyte firm adhesion and transmigration at sites of platelet deposition. However, there is no in vivo study evaluating the importance of the integrin Mac-1 and GP Ibalfa (alfaMbeta2-GP Ibalfa) interaction in experimental models of vascular injury. METHODS: A peptide termed M2 or anti-M2 antibody was developed to block the leukocyte Mac-1 and platelet GP Ibalfa interaction, aiming to inhibit the adhesion of leukocytes to the platelet-coated surface of vessels as well as the cellular proliferation and the neointimal hyperplasia. The peptide was injected and compared with a control-antibody in C57B1/6J mice subjected to wire-induced femoral artery injury. One day (control: n= 6; anti-M2: n= 6), 5 days (control: n= 9; anti-M2: n= 9) or 28 days (control: n= 9; anti-M2: n= 9) after vascular injury, the femoral arteries were harvested for morphometry and immunohistochemistry. RESULTS: The alfaMbeta2-GP Ibalfa interaction blockade promoted a statistically significant 75% reduction in leukocytes in the medial layer on the first day after vascular injury (control: 7.9 ± 5.0% out of the total cells in the medial layer versus anti-M2: 2.0 ± 1.6%; p=0.021), as well as determined a statistically significant 42% decrease 5 days later (control: 42.3 ± 12.9% out of the total cells in the neointima versus anti-M2: 24.6 ± 10.8%; p=0.047), and a 58% decrease in leukocyte accumulation in the developing neointima 28 days later (control: 7.9 ± 3.0% versus anti-M2: 3.3 ± 1.3%; p=0.012). The cellular proliferation in the vessel medial layer 5 days after vascular injury presented a statistically significant 64% reduction by the alfaMbeta2-GP Ibalfa interaction blockade (control: 5.0 ± 2.9% out of the total cells in the medial layer versus anti-M2: 1.8 ± 0.5%; p=0.043), and there was also a significant 47% decrease in the vessel intimal layer cellular proliferation 28 days later (control: 3.8 ± 1.7% out of the total cells in the intimal layer versus anti-M2: 2.0 ± 1.2%; p=0.047). Furthermore, the alfaMbeta2-GP Ibalfa interaction blockade determined a statistically significant 56% reduction in the intimal thickening 28 days after vascular injury (control: 10,395 ± 3,549um2 versus anti-M2: 4,561 ± 4,915um2; p=0.012). CONCLUSIONS: The leukocyte recruitment after vascular injury depends on the alfaMbeta2-GP Ibalfa interaction, and its neutralization inhibits cellular proliferation and neointimal formation.

Cell adhesion molecules

Coronary restenosis

Inflamação

Inflammation

Integrinas

Integrins

Leucócitos

Leukocytes

Moléculas de adesão celular

Plaquetas

Platelets

Reestenose

Etude du rôle des intégrines liant la laminine dans le développement et la tumorigenèse mammaires / Study of the role of laminin-binding integrins in mammary gland development and tumorigenesis

Cagnet, Stéphanie

26 November 2013

Le développement de traitements thérapeutiques du cancer du sein reste limité par le niveau de connaissance des mécanismes moléculaires et cellulaires impliqués lors du développement normal et tumoral de la glande mammaire. L’épithélium mammaire est entouré d’une matrice extracellulaire (MEC) organisée, la membrane basale, dont le constituant principal est la laminine. Des études ont montré que les interactions entre les cellules mammaires et la MEC, dépendantes des intégrines, jouent un rôle majeur dans le développement et la tumorigenèse mammaires. Ces études n’ont cependant pas permis de déterminer les hétérodimères d’intégrine spécifiquement impliqués. Dans ce contexte, mon projet de thèse a visé à définir le rôle joué par les intégrines liant la laminine (dimères contenant les sous-unités 3 et/ou 6) dans le développement mammaire, dans le maintien de cellules souches mammaires fonctionnelles dans la glande adulte et dans le développement tumoral. Les résultats de mon travail suggèrent que :(i) l’intégrine 31 présente une fonction unique au cours de la lactation. Les mécanismes moléculaires impliqués en aval de 31 font intervenir la voie FAK/Rac1/PAK1 menant à l’inhibition de la MLCK, nécessaire à la relaxation des cellules myoépithéliales mammaires et permettant de nouveaux cycles de contraction. (ii) les interactions régulées par les intégrines entre les cellules basales mammaires et la laminine sont essentielles pour régénérer l’épithélium mammaire. Cependant, les intégrines 3 et 6 présentent des fonctions redondantes dans les cellules souches mammaires. (iii) l’intégrine 31 joue un rôle clef dans le développement tumoral mammaire. L’intégrine 31 active des voies de signalisation intracellulaires FAK/Rac1/PAK1, MAPK et JNK qui favorisent la survie et la prolifération des cellules tumorales. Ensembles, ces données permettent une meilleure compréhension des mécanismes moléculaires impliqués dans le développement mammaire, la fonction de la glande adulte et la tumorigenèse. / The improvement of breast cancer therapy requires thorough analysis of the pathways leading to tumorigenesis and clear understanding of the molecular and cellular mechanisms involved in normal mammary gland development. Mammary epithelium is surrounded by a specifically organized extracellular matrix (ECM), basement membrane, and secreted glycoproteins, laminins, are among its major constituents. Integrin-mediated interactions between mammary epithelial cells and ECM have been shown to play an essential role in the control of mammary development and tumorigenesis. However, specific roles played by distinct integrin heterodimers are yet poorly understood. My thesis project aimed to define the functions of laminin-binding integrins, i.e., heterodimers, containing 3 or 6 subunits, in normal mammary gland development, in control of mammary stem and progenitor cell functions in adult gland, and in mammary tumorigenesis. The results of my work suggest that: (i31 integrin has a unique function in the control of the myoepithelial cell contractile activity during lactation; it contributes to the activation of the FAK/Rac1/PAK1 pathway leading to MLCK inhibition required for myoepithelial cell relaxation, thereby, permitting further contractile cycles. (ii) integrin-mediated interactions of mammary basal cells with laminins are essential for the regeneration of the mammary epithelium. However, 31 and 6-contaning integrins have redundant functions in mammary stem cells.(iii) 31 integrin plays a major role in mammary tumorigenesis, it promotes survival and proliferation of tumor cells activating intracellular signaling pathways involving FAK/Rac1/PAK1, MAPK and JNK pathways. Altogether, these data provide new insights into the molecular mechanisms of mammary development, adult gland function and tumorigenesis.

Intégrines

Cellules souches

Tumeurs mammaires

Beta-caténine

Épithélium

Contractilité

Integrins

Stem cells

Mammary tumors

Beta-catenin

Epithelium

Contractility

La migration des cellules et leur sensibilité aux propriétés physiques de la matrice extracellulaire : rôle d'ICAP-1, un régulateur des intégrines et de la contractilité / About cell migration and cellular response to the physical properties of the extracellular matrix : iCAP-1 regulates integrins and cell contractility.

Régent, Myriam

17 June 2011

Les cellules sont organisées en tissus dont les propriétés physiques comme la rigidité et l'élasticité sont variables. La matrice extracellulaire (MEC) est produite et remodelée par les cellules qui s'adaptent en retour aux conditions physico-chimiques de cet environnement extracellulaire. Cela nécessite une communication bidirectionnelle entre la cellule et la matrice. Les intégrines sont des protéines transmembranaires impliquées dans l'adhérence, liant la MEC au cytosquelette d'actine via une plateforme protéique appelée adhérence focale, lieu d'une double signalisation (inside-out et outside-in). Des variations de tension intracellulaire imposées par l'environnement modifient la distribution et la taille de ces adhérences. Leur dynamique est aussi contrôlée par certaines protéines cytoplasmiques comme la protéine ICAP-1, partenaire de l'intégrine b1. En cherchant à comprendre le lien entre la tension interne et l'activation des intégrines, j'ai montré qu'ICAP-1 contrôle l'étalement, la contractilité interne et la migration cellulaire en présence comme en absence de l'intégrine b1, révélant un rôle ICAP-1 indépendant de son interaction avec l'intégrine b1. Ce contrôle semble passer par l'interaction ICAP-1/ROCK et a révélé un contrôle de l'intégrine b3 par l'intégrine b1. / The physical properties of cell tissues are variable and cells adapt their behaviour to the physical and chemical extracellular environment such as rigidity and composition of the extracellular matrix (ECM) which is produced and remodelled by cells. This implicates a bidirectionnal signalling between cells and the ECM. Integrins are transmembrane proteins involved in cell adhesion, linking the ECM to the actin cytoskeleton through adaptor proteins forming adhesion site called focal adhesion (FA) where take place an inside-out and an outside-in signallings. Intracellular tension can be controlled by extracellular cues, modifying the size and distribution of FA. FA dynamics is also regulated by cytoplasmic proteins such as ICAP-1 that interacts with b1 integrin. Looking for a better comprehension of the link between cell tension and integrin activation, I show that ICAP-1 controls cell spreading, cell contractility and cell migration both in presence or absence of b1 integrins meaning that ICAP-1 has an action without its interaction b1 integrin. This action seems to implicate the interaction between ICAP-1 and ROCK and revealed a control of b1 integrin on b3 integrin.

Adhérence

Migration cellulaire

Intégrines

Rigidité extracellulaire

Tension intracellulaire

Matrice extracellulaire

Adherence

Cell migration

Integrins

Extracellular stiffness

Intracellular stress

Extracellular matrix