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Estudo da expressão da enzima desubiquitinante USP2a e de sua interação com a proteina clatrina em celulas derivadas de carcinomas espinocelulares bucais e de prostata humanos / Expression of USP2a and study of its interaction with clathrin in human oral squamous carcinoma and prostate cancer cellsAgostini, Michelle 28 February 2007 (has links)
Orientador: Edgard Graner / Tese (doutorado) - Universidade Estadual de Campinas, Faculdade de Odontologia de Piracicaba / Made available in DSpace on 2018-08-09T14:11:16Z (GMT). No. of bitstreams: 1
Agostini_Michelle_D.pdf: 6485719 bytes, checksum: f82ba343c6049746e2b63420116af03c (MD5)
Previous issue date: 2007 / Resumo: O sistema ubiquitina-proteossomo degrada proteínas marcadas com etiquetas de Ub. A ubiquitinação é um processo reversível e moléculas de Ub podem ser desconjugadas pelas enzimas desubiquitinantes (DUBs), que evitam a degradação e aumentam a meia vida de seus substratos. A DUB USP2a foi identificada na próstata humana, é regulada por andrógenos e tem sua expressão aumentada em adenocarcinomas. USP2a protege a enzima ácido graxo sintase (FAS) da degradação, a qual é superexpressa em vários tipos de tumores, inclusive nos carcinomas espinocelulares (CECs) bucais. O objetivo deste trabalho foi estudar a expressão desta DUB e seu papel biológico em células derivadas de CECs bucais humanos. Foram detectados RNAs mensageiros para USP2a nas quatro linhagens celulares estudadas, principalmente nas linhagens SCC-4 e -15. Os níveis protéicos de USP2a foram semelhantes nas quatro linhagens, sendo ligeiramente maiores na SCC-9 e -25. Portanto, não foi encontrada uma correlação entre a quantidade de RNAs mensageiros e dos produtos protéicos de USP2a. Através de experimentos de imunofluorescência, demonstramos USP2a no citoplasma das células SCC-9, havendo uma concentração na região perinuclear em algumas células. A expressão forçada de USP2a nas células SCC- 9 não conferiu vantagem proliferativa, no entanto, a superexpressão de um duplomutante parece ter diminuído a proliferação. Ao contrário do que ocorre nas células LNCaP, a inibição da expressão de USP2a através de RNAi nas células SCC-9 causou discreta indução de apoptose. O tratamento das células SCC-9 com diferentes concentrações do fator de crescimento epidérmico (EGF) foi capaz de modular a expressão de USP2a, interferindo na quantidade de formas ubiquitinadas de FAS. Também foi investigada neste trabalho a possível interação entre USP2a e a proteína clatrina. De acordo com resultados prévios de experimentos realizados no laboratório do Dr. Massimo Loda, no Dana-Farber Cancer Institute, a cadeia pesada de clatrina é também substrato de USP2a. Clatrina é uma proteína que participa do processo de internalização e endocitose de proteínas localizadas na membrana plasmática. Demonstramos que USP2a e a cadeia pesada de clatrina estão co-localizadas no citoplasma de células AR-iPrEC e SCC-9 e que a produção de clatrina é regulada por andrógenos em células LNCaP. Houve uma maior produção de clatrina em células que superexpressam de forma estável USP2a. Um achado interessante foi que USP2a, além de presente no citoplasma, foi também encontrada na membrana plasmática de células LNCaP e o tratamento com EGF interferiu na localização sub-celular desta DUB, como ocorre com clatrina durante a endocitose. Estes resultados sugerem que USP2a participe do processo de endocitose mediada por clatrina / Abstract: The ubiquitin (Ub)-proteasome pathway controls cellular protein turnover by degrading targeted intracellular proteins tagged with poly-Ub chains. Ubiquitination is a reversible process and the deubiquitinating enzymes (DUBs) are proteases that specifically cleave off Ub from Ub-protein conjugates. They can act in a preproteasomal level removing the poly-Ub tag from specific substrates and preventing and modulating their degradation. The DUBs USP2a and USP2b were recently identified in the prostate of men and rats. USP2a is androgen-regulated, overexpressed in prostate cancer, and interacts with and stabilizes fatty acid synthase (FAS) and the protein murine double minute (Mdm2). FAS is overexpressed in several human malignancies, including oral squamous cell carcinoma, and is correlated with a poor prognosis for some tumors. Mdm2 is an Ub-protein ligase responsible for its own ubiquitination and ubiquitination of p53, that is degraded by the proteasome. When overexpressed in nontransformed cells USP2a exhibits oncogenic behavior both in vitro and in vivo and prevents apoptosis induced by chemotherapeutic agents. Considering that USP2a stabilizes FAS and Mdm2 and then protects tumoral cells from apoptosis, the purpose of the present study was to investigate the USP2a expression and its biological role in human oral squamous carcinoma cells. mRNAs for USP2a were detected in the four studied cell lines, mainly in SCC-4 and -15. The USP2a protein levels were similar in all cell lines, being slightly higher in SCC-9 and -25. By using immunofluorescence we showed that USP2a is located in the cytoplasm of SCC-9 cells and eventually concentrated around the nuclei. No significant differences were found in the proliferative rates of USP2a overexpressing SCC-9 cells, however, cells overexpressing mutant USP2a had lower proliferative potential. In contrast with LNCaP cells, USP2a silencing by siRNA slightly induced apoptosis. The treatment with different concentrations of EGF was able to modulate the USP2a expression in SCC-9 cells and change the amount of ubiquitinated forms of FAS. We also show in the present study experiments performed in the laboratory of Dr. Massimo Loda at the Dana-Farber Cancer Institute, in which the possible interaction between USP2a and clathrin was analyzed. Clathrin is involved in the internalization and endocytosis of proteins located in at the plasma membrane. Here we show that USP2a and clathrin heavy chain colocalize in the cytoplasm of AR-iPrEC and SCC-9 cells and that clathrin protein expression is regulated by androgens in LNCaP cells. We found higher amounts of clathrin in cells that stably express USP2a than in the controls. USP2a was found at the plasma membrane in LNCaP cells and after EGF stimulation a granular positivity for USP2a was observed in the cytoplasm. These results suggest that USP2a may have a role in the clathrin mediated endocytosis / Doutorado / Patologia
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Visualisation et perturbation de la dynamique spatio-temporelle de l’endocytose / Visualisation and Perturbation of the Spatio-Temporal Dynamics of EndocytosisRosendale, Morgane 18 June 2015 (has links)
L’endocytose dépendante de la clathrine (EDC) est un processus fondamental des cellules eucaryotes. Elle se caractérise par la formation d’invaginations à la membrane plasmique aboutissant à la création de petites vésicules par l’action de la dynamine. Dans le cerveau, elle est impliquée dans la dépression synaptique à long terme, un corrélat cellulaire de la mémoire. La morphologie complexe des neurones et le contrôle précis du code neuronal suggèrent qu’elle puisse être régulée spatialement et temporellement dans ces cellules. Le but de mon travail a été de développer de nouveaux outils pour visualiser et perturber l’EDC afin d’étudier ce type de régulation. Le premier de ces outils est pHuji, un senseur de pH rouge génétiquement encodable. Je l’ai utilisé avec un senseur de pH vert existant pour montrer que dans les cellules NIH- 3T3, le récepteur β2-adrénergique est internalisé dans une sous-population de vésicules contenant le récepteur à la transferrine constitutivement endocyté. Le deuxième est une nouvelle méthode d’imagerie permettant de visualiser l’activité d’endocytose de structures recouvertes de clathrine optiquement stables dans des neurones d’hippocampe. J’ai ainsi pu suivre pour la première fois la cinétique d’internalisation de récepteurs au glutamate de type AMPA dans des conditions de plasticité. Enfin, j'ai élaboré un test combinant imagerie et patch-clamp afin de développer un bloqueur peptidique spécifique de l'EDC. En utilisant des peptides dimériques, j’ai montré que la dynamine se lie à ses partenaires via des interactions multimériques. En conclusion, ce travail propose une boite à outils permettant d’élucider les mécanismes de l’EDC avec une grande résolution spatiale et temporelle. / Clathrin mediated endocytosis (CME) is a fundamental process of all eukaryotic cells. At the level of the plasma membrane, it is characterized by the formation of deep invaginations resulting in the creation of small vesicles after membrane scission by dynamin. In the central nervous system, it is involved in the expression of synaptic long term depression, a proposed cellular correlate of learning and memory. The complex morphology of neurons and the precise timing of neuronal firing suggest that endocytosis may be spatially and temporally regulated in those cells. The aim of the work presented here was to develop new tools to visualize and perturb CME in order to study such regulation. The first tool to be characterized was pHuji, a genetically encoded red pH-sensor. I used it in combination with an existing green pHsensor to demonstrate that in NIH-3T3 cells, the β2-adrenergic receptor was internalized in a subset of vesicles containing the constitutively endocytosed transferrin receptor. The second tool is a new imaging method that allowed me to monitor the endocytic activity of optically stable clathrin coated structures in hippocampal neurons. I was thus able to visualize for the first time the kinetics of internalization of AMPA-type glutamate receptors under plasticity inducing conditions. Finally, I set up an assay combining imaging and cell dialysis in order to develop a specific peptide-based inhibitor of CME. Using dimeric peptides, I found that the interplay between dynamin and its binding partners relies on multimeric interactions. Altogether, this work provides a toolbox to decipher the mechanisms of vesicle formation with high spatial and temporal resolution.
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Combining artificial Membrane Systems and Cell Biology Studies: New Insights on Membrane Coats and post-Golgi Carrier FormationStange, Christoph 13 December 2012 (has links)
In mammalian cells, homeostasis and fate during development relies on the proper transport of membrane-bound cargoes to their designated cellular locations. The hetero-tetrameric adaptor protein complexes (APs) are required for sorting and concentration of cargo at donor membranes, a crucial step during targeted transport. AP2, which functions at the plasma membrane during clathrin-mediated endocytosis, is well characterized. In contrast, AP1 a clathrin adaptor mediating the delivery of lysosomal hydrolases via mannose 6-phosphate receptors (MPRs) and AP3 an adaptor ensuring the proper targeting of lysosomal membrane protein are difficult to study by classic cell biology tools. To gain new insights on these APs, our lab has previously designed an in vitro system. Reconstituted liposomes were modified with small peptides mimicking the cytosolic domains of bona fide cargoes for AP1 and AP3 respectively and thereby enabling the selective recruitment of these APs and the identification of the interacting protein network.
In the study at hand we utilize above-described liposomes to generate supported lipid bilayers and Giant Unilamellar Vesicles (GUVs), large-scale membrane systems suited for analysis by fluorescence microscopy. By using cytosol containing fluorescently-tagged subunits, we visualized clathrin coats on artificial membranes under near physiological conditions for the first time. Moreover, we demonstrated clathrin-independent recruitment of AP3 coats on respective GUVs. Presence of active ARF1 was sufficient for the selective assembly of AP1-dependent clathrin coats and AP3 coats on GUVs. By using dye-conjugated ARF1, we show that ARF1 colocalized with AP3 coats on GUVs and that increased association of ARF1 with GUVs coincided with AP1-dependent clathrin coats.
Our previous study identified members of the septin family together with AP3 coats on liposomes. Here we show on GUVs, that active ARF1 stimulated the assembly of septin7 filaments, which may constrain the size and mobility of AP3 coats on the surface. Subsequent cell biology studies in HeLa cells linked septins to actin fibers on which they may control mobility of AP3-coated endosomes and thus their maturation. An actin nucleation complex, based on CYFIP1 was identified together with AP1 on liposomes before. Here we show on GUVs, that CYFIP1 is recruited on the surface surrounding clathrin coats. Upon supply of ATP, sustained actin polymerization generated a thick shell of actin on the GUV surface. The force generated by actin assembly lead to formation of long tubular protrusions, which projected from the GUV surface and were decorated with clathrin coats. Thereby the GUV model illustrated a possible mechanism for tubular carriers formation. The importance of CYFIP1-reliant actin polymerization for the generation of MPR-positive tubules at the trans-Golgi network (TGN) of HeLa cells was subsequently demonstrated in our lab.
The notion that tubulation of artificial membranes could be triggered by actin polymerization allowed us to perform a comparative mass spectrometry screen. By comparing the abundance of proteins on liposomes under conditions promoting or inhibiting actin polymerization, candidates possibly involved in stabilization, elongation or fission of membrane tubules could be identified.
Among the proteins enriched under conditions promoting tubulation, we identified type I phosphatidylinositol-4-phosphate 5-kinases. Their presence suggested an involvement of phosphatidylinositol 4,5-bisphosphate (PI(4,5)P2) in tubule formation. By cell biology studies in HeLa we show, that down regulation of these enzymes altered the dynamics of fluorescently-tagged MPRs, illustrating the importance of locally confined PI(4,5)P2 synthesis during formation of coated carriers at the TGN.
Bin–Amphiphysin–Rvs (BAR) domains are known to sense membrane curvature and induce membrane tubulation. Among various BAR domain proteins, Arfaptin2 was enriched under conditions allowing tubulation of liposomes. By microscopy studies on HeLa cells we show, that Arfaptin2 as well as its close paralog Arfaptin1 were present on AP1-coated MPR tubules emerging from the TGN. We further show, that tubule fission occurred at regions were Arfaptin1 is concentrated and that simultaneous down regulation of both Arfaptins lead to increased number and length of MPR tubules. Since fission of coated transport intermediates at the TGN is poorly understood, our findings contribute a valuable component towards a model describing the entire biogenesis of coated post-Golgi carriers. In conclusion, combining artificial membrane systems and cell biology studies allowed us to propose new models for formation as wall as for fission of AP1-coated transport intermediates at the TGN. Further we gained new insights on AP3 coats and the possible involvement of septin filaments in AP3-dependent endosomal maturation.
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Molecular mechanisms of the asymmetric pit-closing in clathrin-mediated endocytosis / クラスリン媒介エンドサイトーシスにおける非対称ピット閉鎖の分子機構Yu, Yiming 24 November 2023 (has links)
京都大学 / 新制・課程博士 / 博士(生命科学) / 甲第24983号 / 生博第512号 / 新制||生||68(附属図書館) / 京都大学大学院生命科学研究科統合生命科学専攻 / (主査)教授 荒木 崇, 教授 鈴木 淳, 教授 谷口 雄一 / 学位規則第4条第1項該当 / Doctor of Philosophy in Life Sciences / Kyoto University / DFAM
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Rapid endocytosis provides restricted somatic expression of a K+ channel in central neuronsCorrêa, Sonia A.L., Muller, Jurgen, Collingridge, G.L., Marrion, N.V. January 2009 (has links)
No / Trafficking motifs present in the intracellular regions of ion channels affect their subcellular location within neurons. The mechanisms that control trafficking to dendrites of central neurons have been identified, but it is not fully understood how channels are localized to the soma. We have now identified a motif within the calcium-activated potassium channel K(Ca)2.1 (SK1) that results in somatic localization. Transfection of hippocampal neurons with K(Ca)2.1 subunits causes expression of functional channels in only the soma and proximal processes. By contrast, expressed K(Ca)2.3 subunits are located throughout the processes of transfected neurons. Point mutation of K(Ca)2.1 within this novel motif to mimic a sequence present in the C-terminus of K(Ca)2.3 causes expression of K(Ca)2.1 subunits throughout the processes. We also demonstrate that blocking of clathrin-mediated endocytosis causes K(Ca)2.1 subunit expression to mimic that of the mutated subunit. The role of this novel motif is therefore not to directly target trafficking of the channel to subcellular compartments, but to regulate channel location by subjecting it to rapid clathrin-mediated endocytosis.
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Untersuchung zur Fettsäurezusammensetzung, subzellulären Verteilung und Funktion stressinduzierter Phosphoinositid-Pools in Pflanzen / Fatty acid-composition, subcellular distribution and physiological roles of stress-inducible phosphoinositide-pools in plantsKönig, Sabine 30 April 2008 (has links)
No description available.
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Interactome of TNRC6 W-motifs and their conserved Role in miRNA-mediated silencingMauri, Marta 15 December 2017 (has links)
MicroRNAs (miRNAs) sind kurze nicht-kodierende RNAs, die auf posttranskriptionaler Ebene die Genexpression hemmen. Dafür bilden miRNAs Ribonukleoprotein-Komplexe, deren Kernbestandteile aller Bilateria Argonaute (AGO) und GW182 /TNRC6 Proteine sind. GW182 / TNRC6-Proteine rekrutieren CCR4-NOT-Deadenylasen über kurze Tryptophan-reiche Motive (W-Motive), welche additiv wirken und fördern so die translationale Repression und den Abbau von Ziel-mRNAs. Um mehr über die Mechanismen der miRNA-abhängigen Genrepression zu erfahren, habe ich W-Motiv-abhängige Interaktionspartner humaner TNRC6C Proteine bestimmt. Hierzu habe ich, mithilfe von quantitativer Massenspektrometrie, das Interaktom von wildtyp TNRC6C Proteinen mit dem von TNRC6C Proteinen, deren W-Motive mutiert wurden, verglichen. Neben bekannten Interaktionspartnern, wie Untereinheiten des CCR4-NOT Komplexes, habe ich Komponenten von Clathrin-Vesikeln (CCVs), Stoffwechsel assoziierte Enzyme, mitochondriale Proteine, RNA Helikasen, Kinasen und Phosphatasen mit potentiellen Funktionen in der miRNA-assoziierten Repression identifiziert. Die im ersten Teil dieser Studie vorgestellten Ergebnisse legen nahe, dass CCVs die Speicherung oder das Recycling von TNRC6 und AGO Proteinen vermitteln können und somit das miRNA-Silencing modulieren.
Der zweite Teil dieser Studie befasst sich mit der Konservierung von miRNA vermitteltem Gen-Silencing in Cnidaria (Nematostella vectensis), welche sich vor 600 Millionen Jahren von der Ahnenreihe der Metazoa abspalteten. Hier zeige ich anhand humaner Zellen, dass Nematostella GW182, ähnlich wie in Bilateria, von AGO rekrutiert wird und nachfolgend in der Repression der mRNA fungiert, was darauf hinweist, dass dieser Mechanismus der miRNA-vermittelten Geninhibition bereits in den letzten gemeinsamen Vorfahren von Cnidaria und Bilateria aktiv war. / MicroRNAs (miRNAs) are short non-coding RNAs that act as post-transcriptional repressors of gene expression. To function miRNAs are assembled in ribonucleoprotein complexes, whose core components in bilaterian animals are Argonaute (AGO) and GW182/TNRC6 proteins. GW182/TNRC6 proteins additively recruit CCR4-NOT deadenylases via short tryptophan-containing motifs (W-motifs), thereby promoting translational repression and the decay of target mRNAs. To gain deeper insights into the mechanisms of miRNA silencing I determined the W-motif-specific interactome of human TNRC6C proteins. Using Stable Isotope Labeling by Amino acids in Cell Culture (SILAC) coupled to affinity purification and Mass Spectrometry (MS) I identified proteins enriched with wild type TNRC6C as compared to two mutants with disrupted W-motifs. Besides known functional interactors, such as subunits of the CCR4-NOT complex, I identified several components of clathrin-coated vesicles (CCVs), metabolic enzymes, mitochondrial proteins, RNA helicases, kinases, and phosphatases with potential functional roles in miRNA-mediated repression. The results presented in the first part of this thesis indicate that CCVs may mediate the storage or recycling of TNRC6 and AGO proteins, thus modulating miRNA silencing. The second part of the thesis addressed the conservation of the mechanisms of miRNA silencing via W-motifs in the cnidarian Nematostella vectensis, separated by 600 million years from other Metazoa. Using cultured human cells, I showed that similarly to bilaterians, GW182 in Nematostella is recruited to the miRNA repression complex via interaction with AGO proteins, and functions downstream to repress mRNA, indicating that this mechanism of miRNA-mediated silencing was already active in the last common ancestor of Cnidaria and Bilateria.
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Étude des mécanismes moléculaires des inhibiteurs de l'entrée du virus de l'hépatite C (HCV) Silibinine et Arbidol : microenvironnement hépatique et infection par le HCV / Molecular mechanisms of entry inhibitors of hepatitis C virus (HCV) and Silibinin Arbidol : hepatocyte microenvironment and HCV infectionBlaising, Julie Élisabeth Françoise 03 December 2013 (has links)
Le virus de l'hépatite C (HCV) infecte environ 180 millions de personnes à travers le monde. De nouveaux antiviraux ont récemment été mis sur le marché mais ils présentent des effets indésirables. La recherche de nouvelles cibles thérapeutiques reste donc d'actualité. Mes principaux travaux ont consisté à développer des approches de biochimie et d'imagerie sur cellules vivantes pour étudier les mécanismes moléculaires d'action des antiviraux silibinine (SbN) et arbidol (ARB) sur HCV. Nous avons montré que SbN et ARB inhibent des vésicules entourées de clathrine et ne sont pas délivrés aux endosomes précoces. SbN et ARB inhibent également l'infection d'autres virus entrant par endocytose clathrine-dépendante, ce qui expliquerait leur activité à large spectre. J'ai également contribué à un projet initié depuis quelques mois au sein de l'équipe. L'hypothèse était qu'un élément présent dans le microenvironnement hépatique (MEH) jouerait un rôle essentiel dans l'infection par HCV. Nous nous sommes intéressés au syndécan-1 (SDC1) car il est fortement exprimé à la surface des hépatocytes. Nos travaux montrent que la déplétion de SDC1 diminue fortement l'infection. SDC1 colocalise à la surface des hépatocytes non infectés avec CD81, un récepteur connu de HCV. Dans les jours suivant l'infection, cette colocalisation est perturbée. Ces données suggèrent que SDC1 serait un co-facteur d'entrée de HCV, agissant en combinaison avec CD81, et que l'infection réorganiserait les molécules du MEH, ce qui pourrait à long terme contribuer à la persistance de l'infection / Hepatitis C virus (HCV) is a global health concern infecting 170 million people worldwide. New antivirals recently received the approval for the treatment against HCV infection but they display many side effects. Research for new therapeutic targets therefore remains an important topic. My main work was to develop approaches in biochemistry and live cell imaging to study the molecular mechanisms of action of antivirals silibinin (SbN) and arbidol (ARB) on HCV infection. We show that SbN and ARB alter clathrin-mediated endocytosis. Viral particles are trapped in clathrin-positive structures and cannot be delivered to the early endosomal compartment, thereby preventing infection. SbN and ARB also prevent cell infection by viruses that enter through clathrin-mediated endocytosis, which could explain their broad spectrum activity. I also contribute to a project initiated for a few months in the lab. We hypothsized that a molecule present in the immediate surrouding of the hepatocyte microenvironment could play a role in HCV infection. We focused on the syndecan-1 (SDC1) because it is essentially anchored on the surface of hepatocytes. We show that SDC1 depletion leads to a drastic decrease of the viral infectivity. SDC1 colocalizes on the unfected hepatocyte surface with the already identified HCV recptor CD81. This colocalization vanished within days in infected cells. These data suggest that SDC1 could act as a cellular co-factor for HCV entry, in combination with CD81; thus infection could reorganized molecules of the hepatocyte microenvironment and contribute to HCV hepatotropism and the peristence of infection
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Galectins and glycosphingolipids in clathrin-independent endocytosis and cell migration / Galectines et glycosphingolipides dans l'endocytose indépendante de la clathrine et lamigration cellulaireLakshminarayan, Ramya 12 June 2012 (has links)
Les voies d’endocytose qui régissent l’internalisation d’éléments extracellulaires peuvent être classées selon que la protéine de manteau, la clathrine, est impliquée ou non dans le processus. Les voies indépendantes de la clathrine sont utilisées par de nombreuses toxines, des virus et des protéines endogènes. Les mécanismes permettant d’induire le recrutement des protéines cargoes et la déformation de la membrane plasmique dans le contexte de l'endocytose clathrine-indépendant restent encore mal compris. Cette étude montre que la galectine 3, une protéine humaine qui se lie aux glucides, induit la formation d’invaginations de la membrane plasmique de manière indépendante de la clathrine. Les glycosphingolipides (molécules jouant un rôle majeur dans la physiologie de la cellule) sont essentielles pour permettre à la galectine 3 d’induire ces invaginations et d’être internalisée dans la cellule. Les structures tubulaires induites par la galectine 3 présentent une morphologie étonnamment similaire à celle de compartiments intermédiaires de transport décrits dans la littérature pour l’endocytose indépendante de la clathrine. Des cargos utilisant la voie indépendante de la clathrine, tels que CD44 et les intégrines α5 et β1, sont retrouvés dans les tubules induits par la galectine 3. De plus, cette dernière est nécessaire à l’internalisation de CD44. Cela indique donc que la galectine 3 pourrait relier des protéines cargos glycosylés à des glycosphyngolipides de la membrane plasmique et ainsi induire une déformation de la membrane et leur internalisation dans les cellules. Ce mécanisme diffère de celui utilisé par la toxine pentamérique de Shiga et par la toxine cholérique, qui sont leur protéines cargos propores et interagissant directement avec le glycosphyngolipide leur servant de récepteur. Les tubules induits par la galectine 3 sont distincts de ceux induit par les autres lectines. Celles-ci présentent des spécificités différentes de liaison aux glucides, montrant ainsi la l'importance des interactions entre les lectines et les sucres dans ce processus. De plus, nous avons constaté que la galectine 3 module l’équilibre à l’état basal de l’intégrine β1 à la surface de la cellule. Cette protéine étant capitale pour les phénomènes d’adhésion et de migration cellulaires, nous avons donc exploré le rôle conjoint de la galectine 3 et des glycosphingolipides dans la migration cellulaire. La galectine 3 inhibe la migration des cellules humaines de carcinomes mammaires alors qu’elle stimule au contraire celle de cellules de tumeurs mammaires murines. Or, nous avons montré que la régulation par la galactine 3 de la migration de différentes lignées cellulaires est dépendante des glycosphingolipides. Il ressort donc de cette étude que la galectine 3 et les glycosphingolipides contribuent de manière synergique au processus d’induction de déformation de la membrane, à l’endocytose de protéines cargos et à la migration cellulaire. / Endocytic processes which govern the uptake of extracellular material into the cell can be classified based on their dependence on the coat protein, clathrin. Clathrin-independent mechanisms are used by many toxins, viruses and endogenous proteins. How cargo is recruited and membranes are bent is not well understood in these cases. Here, we discovered that galectin 3, a human carbohydrate binding protein induced the clathrin-independent formation of endocytic plasma membrane invaginations. Glycosphingolipids, which have established functions in key physiological processes, were found to be essential for the formation of galectin 3-induced invaginations and for the efficient uptake of the protein into the cell. Galectin 3-induced tubular structures were found to have a strikingly similar morphology to that of the clathrin-independent carriers described in literature. Clathrin-independent endocytic cargoes such as CD44, α5 and β1 integrin were present in galectin 3-induced tubules, and galectin activity and glycosphingolipids were required for the uptake of CD44. This indicated that galectin 3 could link glycosylated cargoes with glycosphingolipids for cargo recruitment and membrane bending. In contrast, the pentameric Shiga and cholera toxins are their own cargoes and drive membrane deformations by directly binding to their respective glycosphingolipid receptors. Galectin 3-induced tubules were distinct from those induced by lectins with different carbohydrate binding specificities, which revealed the importance of lectin-glycan interaction in this process. Further, we observed that galectin 3 modulated the steady state surface dynamics of β1 integrin, a protein which like CD44 is critical for cell adhesion and migration. Subsequently, we explored the interplay of galectins and glycosphingolipids in cell migration. Galectin 3 inhibited cell migration in human breast carcinoma cells, and stimulated migration in a mouse mammary tumor cell line. However, the regulation of migration by galectin 3 was in both cases found to be dependent on glycosphingolipids. In conclusion, galectin 3 and glycosphingolipids synergistically contribute to the clathrin-independent curvature generation process, cargo endocytosis and cell migration.
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Rôle des ARFs dans la migration et la régulation phénotypique des cellules du muscle lisse vasculaireCharles, Ricardo 12 1900 (has links)
No description available.
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