Cell Surface GRP78 and α2-Macroglobulin in Kidney Disease / THE PROFIBROTIC ROLE OF CSGRP78/ ACTIVATED α2M SIGNALING IN THE PATHOGENESIS OF DIABETIC AND CHRONIC KIDNEY DISEASE

Trink, Jacqueline

January 2023

Diabetic kidney disease (DKD) is the leading cause of end stage renal disease worldwide and occurs in up to 40% of patients with diabetes. The standard of care for DKD treatment has not kept up with the current health epidemic, which has led to a heavy economic toll and substantial health burden. Targeting either cell surface (cs)GRP78, activated α2-macroglobulin (α2M*) or preventing their interaction may provide a novel anti-fibrotic therapeutic target for the treatment of DKD and potentially non-diabetic chronic kidney disease (CKD) as well. Previously our lab has shown that HG-induced csGRP78 is a mediator of PI3k/Akt signaling and downstream extracellular matrix (ECM) protein production in glomerular mesangial cells (MC). However, the ligand responsible for activating high glucose (HG)-induced csGRP78 had not yet been determined. We have shown thus far that α2M is endogenously produced, secreted, and activated (denoted α2M*) in HG by MC, which leads to its binding to and activation thereof csGRP78. Further, α2M knockdown or α2M* neutralization attenuated Akt activation, the production of the profibrotic cytokine connective growth tissue factor (CTGF) and ECM proteins fibronectin and collagen IV. We have also shown that integrin β1 (Intβ1), a transmembrane receptor, associated with csGRP78 under HG conditions and likely acts as a tether to present csGRP78 completely extracellularly on MC. Interestingly, Intβ1 activation, even in the absence of HG, was sufficient to induce csGRP78 translocation. Further, inhibition of either csGRP78 or Intβ1 prevented synthesis, secretion and signaling of TGFβ1. This data implicates a role for Intβ1 as a required signaling partner for csGRP78-mediated profibrotic signaling. To further our understanding of csGRP78/ α2M*’s role in DKD, we investigated their ability to mediate TGFβ1 signaling through its non-proteolytic activator thrombospondin-1 (TSP1). Here, HG-induced TSP1 expression, ECM deposition, and activation of TGFβ1 was regulated by the PI3k/Akt pathway via csGRP78/α2M* in MC. Furthermore, we assessed whether this csGRP78/ α2M* axis is relevant to promoting profibrotic signaling in other renal cell types, including proximal tubule epithelial cells (PTEC) and renal fibroblasts (RF), that contribute to the pathogenesis of both later stage DKD and non-diabetic CKD. We show evidence here that HG and direct treatment with TGFβ1, a key pathologic regulator of kidney fibrosis, induce GRP78 surface translocation as well as the endogenous production and activation of α2M in both PTEC and RF. Inhibition of either csGRP78 or α2M* prevented TGFβ1 signaling measured as Smad3 activation as well as downstream ECM production. Interestingly, inhibition of this pathway under direct TGFβ1 treatment did not prevent Smad3 activation, implicating a role for Smad-independent TGFβ1 signaling through this axis. We identified the known noncanonical TGFβ1 signaling partners, yes associated protein (YAP) and transcriptional co-activator with PDZ binding motif (TAZ), are mediated by csGRP78 and α2M*. Lastly, we evaluated the potential therapeutic benefit of inhibiting csGRP78/α2M* interaction in the kidney fibrosis model, unilateral ureteral obstruction (UUO). Here, we show evidence that inhibition of this signaling axis using an inhibitory peptide can prevent renal fibrosis. Whether this peptide also prevents fibrosis in DKD is currently being assessed. Together, these studies strongly implicate targeting csGRP78/α2M* interaction as a novel anti-fibrotic therapeutic intervention for early and late stage DKD, as well as a potential role in non-diabetic CKD. / Thesis / Doctor of Philosophy (Medical Science) / Diabetic kidney disease is the leading cause of kidney failure in developed nations. This progressive disease leads to the loss of kidney function due to an accumulation of scar proteins in the kidney over time. High glucose is a major factor that causes this to occur. Our lab studies specific kidney cells called mesangial cells, proximal tubule epithelial cells, and fibroblasts that produce scar proteins in the presence of high glucose. We have shown that when these cells are treated with high glucose, this causes the movement of a protein called GRP78 that normally resides inside the cell to move to the cell’s surface where it can interact with other proteins. My research has established that the proteins alpha 2-macroglobulin (ɑ2M), integrin β1 (Intβ1), and thrombospondin-1 (TSP1) can bind to GRP78 on the cell surface and cause cells to make scar proteins. Preventing ɑ2M or Intβ1 from binding to GRP78 or preventing TSP1 production prevents mesangial cells from making scar proteins when exposed to high glucose. In a mouse model that overproduces these scar proteins, we showed that preventing cell surface GRP78 and α2M interaction prevents scar protein production and is thus a novel potential treatment option for kidney disease.

cell surface GRP78

alpha 2-macroglobulin

fibrosis

diabetic kidney disease

chronic kidney disease

TGFβ1

Integrin β1

Thrombospondin-1

The effects of TGF-β on the behaviour of a keratinocyte cell line: implications in wound repair

Berends, Rebecca F.

January 2011

TGF-β isoforms are important signalling molecules in wound repair in the skin. Transforming growth factor β3 (TGF-β3) has been implicated in scarless healing. In both animal and human models the application of exogenous TGF-β3 causes a reduction in the inflammatory response and improves the architecture of the neodermis. Research into the influence of TGF-β on scarring has tended to focus on fibroblasts. However, keratinocytes play a major role in scarring both indirectly, as a result of their influence over the behaviour of fibroblasts and also by directly influencing wound contraction. Thus, experiments were carried out to investigate the influence of TGF-β3 on the behaviours of a keratinocyte cell line (HaCaT). Incubation with TGF-β3 increased cell spreading and appeared to reduce cell-surface contacts indicated by both SPR imaging and a detachment assay. TGF-β3 also caused a decreased cell alignment response to microcontact printed protein patterns, in part due to the deposition of laminin which is associated with the TGF-β induced cell migration. There is evidence that TGF-β isoforms differentially influence the outcome of wound healing. Similar to the results produce following addition of exogenous TGF-β3, the neutralisation of TGF-β1 and 2 has been shown to reduce scar formation in the adult wounds. During reepithelialisation keratinocytes experience a dynamic environment. Both extracellular matrix proteins and growth factors influence the progression of wound repair which includes both cell migration and proliferation. Few studies have examined collective cell behaviour in response to TGF-β isoforms and ECM coated substrates. Thus both wound closure and cell proliferation assays were conducted for different ECM proteins fibronectin, laminin and collagen type I and for TGF-β1, 2 and 3. Rates of wound closure were significantly reduced on laminin coated substrates while cell proliferation rates were increased. TGF-β2 and 3 induced significant increases in wound closure rates. This appeared to correspond with an increase in the number of cells independently migrating out from the wound margins. Only TGF-β3 caused a significant decrease in cell proliferation over a 4 day period. Laminin332 deposition is central to the reepithelialisation process and is known to be induced in response to TGF-β. Thus experiments were carried out to investigate HaCaT cell laminin332 deposition in response to TGF-β1, 2 and 3. Both an immunofluorescence staining technique and an ELISA based semi-quantification method was used. Following 4 day incubation all TGF-β isoforms significantly increased laminin332 deposition; however TGF-β2 and 3 caused the most significant increases. Integrin receptors enable cell-matrix interactions during wound repair. TGF-β is known to influence the expression of integrin subunits. Thus, experiments were carried out to compare the influence of each TGF-β isoform on the expression of subunits α3, α2, α5, β1 and β4. All TGF-β isoforms significantly increased all subunit expression. TGF-β3 caused the most significant increase in β4 and both TGF-β2 and 3 caused the most significant increase in α2. While there were differences in cell responses to each isoforms, TGF-β3 did not stand out from the other two isoforms. Interestingly, TGF-β2 shared more similarities with TGF-β3 than it did with TGF-β1, in its role in enhancing wound closure and LN332 deposition. These comparative studies have shown that differences exist in the way TGF-β isoforms influence HaCaT cell behaviour, namely migration, laminin deposition and integrin expression. / EPSRC and DTA grant

HaCaT

; Keratinocyte

; Transforming growth factor β

; ECM

; Wound repair

; Laminin and integrins

; Signalling molecules

; Human skin

; Scarring

; Integrin

; Laminin

Regulation of tumor growth by synthetic disintegrins or depletion of PIN1

Schneider, Ryan Anthony

17 December 2010

No description available.

Molecular Biology

Oncology

Pharmaceuticals

Pharmacology

Pharmacy Sciences

Cancer

integrin

disintegrin

PIN1

proline-isomerase

VEGF

HIF-1alpha

caspase-3

Biophysical characteristics of cells cultured on cholesteryl ester liquid crystals

Soon, Chin Fhong, Omar, W.I.W., Berends, Rebecca F., Nayan, N., Basri, H., Tee, K.S., Youseffi, Mansour, Blagden, Nicholas, Denyer, Morgan C.T.

2013 October 1914

No / This study aimed at examining the biophysical characteristics of human derived keratinocytes (HaCaT) cultured on cholesteryl ester liquid crystals (CELC). CELC was previously shown to improve sensitivity in sensing cell contractions. Characteristics of the cell integrin expressions and presence of extracellular matrix (ECM) proteins on the liquid crystals were interrogated using various immunocytochemical techniques. The investigation was followed by characterization of the chemical properties of the liquid crystals (LC) after immersion in cell culture media using Fourier transform infrared spectroscopy (FTIR). The surface morphology of cells adhered to the LC was studied using atomic force microscopy (AFM). Consistent with the expressions of the integrins α2, α3 and β1, extracellular matrix proteins (laminin, collagen type IV and fibronectin) were found secreted by the HaCaT onto CELC and these proteins were also secreted by cells cultured on the glass substrates. FTIR analysis of the LC revealed the existence of spectrum assigned to cholesterol and ester moieties that are essential compounds for the metabolizing activities of keratinocytes. The immunostainings indicated that cell adhesion on the LC is mediated by self-secreted ECM proteins. As revealed by the AFM imaging, the constraint in cell membrane spread on the LC leads to the increase in cell surface roughness and thickness of cell membrane. The biophysical expressions of cells on biocompatible CELC suggested that CELC could be a new class of biological relevant material.

Keratinocyte

Liquid crystals

Cell adhesion

Cell surface morphology

AFM

FTIR

Integrin

Cell surface roughness

Cholesteryl ester

Extracellular matrix proteins

ROLE OF OXIDATIVE STRESS AND T CELL HOMING IN THE DEVELOPMENT OF MURINE SYNGENEIC GRAFT-VERSUS-HOST DISEASE

Perez-Rodriguez, Jacqueline

01 January 2009

Syngeneic graft-versus-host disease (SGVHD) is induced by reconstituting lethally irradiated mice with syngeneic BM cells followed by a 21 day treatment with the immunosuppressive agent cyclosporine A (CsA). Clinical symptoms of the disease appear 2-3 weeks following cessation of CsA therapy and disease-associated inflammation occurs primarily in the colon and liver. The development of SGVHD is a complex process resulting from the cooperative interaction of multiple effector cell populations including NK cells, T cells and macrophages. TH1 cytokines (IL-12, TNF-α, IFN- γ), produced by these effector cells, serve as inflammatory mediators contributing to the pathogenesis of SGVHD. The SGVHD conditioning agents, irradiation and CsA, are both required for the development of disease and contribute to the production of oxidative stress. Time course studies revealed increased reactive oxygen and nitrogen species (ROS/RNS), as well as, increased colon mRNA levels for TNF-α and iNOS in CsA-treated versus control BMT animals. Since ROS/RNS are known to mediate CsA toxicity, studies were undertaken to determine the effect of oxidative stress on the induction of SGVHD. In vivo treatment with the antioxidant MnTBAP caused a reduction in colon mRNA levels for iNOS and TNF-α, as well as delayed disease development, suggesting a role for oxidative stress in the development of SGVHD. In addition, CD4+ T cells have been shown to play an important role in the inflammatory response observed in the gut of SGVHD mice. Time course studies revealed significant increases in the migration of CD4+ T cells as early as day 14 post- BMT into the colon of CsA mice as well as significant elevated mRNA levels of cell adhesion molecules. Homing studies revealed that a labeled CD4+ T cell line, generated from SGVHD mice, migrated in larger numbers into the gut of CsA-treated mice compared to control animals. This study demonstrated that CD4+ T cells responsible for the pathogenesis observed in murine SGVHD are present early after BMT in colons of CsA-treated mice, suggesting that during the 21 days of immunosuppression therapy functional mechanisms are in place that result in increased homing of effector cells to colons of CsA-treated mice.

Medical Toxicology

Le réseau d'interactions de l'endostatine, une matricryptine du collagène XVIII / The interaction network of endostatin, a matricryptin of collagen XVIII

Faye, Clément

23 October 2009

L’endostatine est le fragment C-terminal du collagène XVIII libéré dans la matrice extracellulaire par clivage enzymatique. C'est un inhibiteur endogène de l’angiogenèse et de la croissance tumorale. L'endostatine inhibe la prolifération et la migration des cellules endothéliales induite par le Fibroblast Growth Factor-2 ou le Vascular Endothelial Growth Factor et elle inhibe la croissance de 65 types de cellules tumorales. L’endostatine fait actuellement l’objet d’essais cliniques pour le traitement de différents cancers son mécanisme d’action est encore mal connu. Nous avons caractérisé par résonance plasmonique de surface (SPR) les interactions établies par l'endostatine avec les intégrines αvβ3 et α5β1 qui sont surexprimées à la surface des cellules endothéliales activée. Nous avons identifié le site de fixation l'endostatine sur les intégrines, proposé un modèle de structure du complexe formé par l'endostatine et l'intégrine αvβ3 et montré que l'endostatine ne peut pas se lier simultanément aux intégrines et aux chaînes d'héparane sulfate présentes à la surface cellulaire. Pour identifier des partenaires supplémentaires de l'endostatine, nous avons développé des puces à protéines et à glycosaminoglycanes basées sur la SPR et capables de suivre jusqu'à 400 interactions simultanément. Nous avons identifié neuf partenaires de l'endostatine (le dermatane sulfate, la transglutaminase-2, les collagènes I, IV et VI, le peptide amyloïde β1-42, et des protéines matricellulaires dont SPARC et thrombospondine-1). Nous avons montré que l’endostatine se fixe avec une forte affinité (KD ~ 6 nM) sur la transglutaminase-2 et que cette interaction nécessite la présence de calcium mais que l'endostatine n'est pas un substrat donneur d'acyle de l'enzyme. Nous avons montré que le réseau d'interactions de l'endostatine est enrichi en protéines contenant des modules EGF (Epidermal Growth Factor). Cela offre de nouvelles perspectives pour l'identification d'autres partenaires et donc de nouvelles fonctions de l'endostatine. Des protéines contenant des modules EGF comme la fibrilline-1, composant des fibres élastiques, et des protéines de l'immunité innée par exemple sont des partenaires potentiels de l'endostatine / Endostatin is the carboxyl-terminal fragment of collagen XVIII released in the extracellular matrix by proteolytic cleavage. It inhibits angiogenesis and tumor growth. Endostatin inhibits the proliferation and migration of endothelial cells induced by Fibroblast Growth Factor-2 and Vascular Endothelial Growth Factor and it inhibits 65 different tumor types. Endostatin is currently under clinical trials for several tumors. We have used surface plasmon resonance (SPR) binding assays to characterize interactions between endostatin and α5β1 or αvβ3 integrins which are over-expressed at cell surface of actived endothelial cell. We have identified the binding site of endostatin on those integrins, and we have built a molecular modeling of the endostatin/integrin αvβ3 complex. We have shown that endostatin can not bind simultaneously to integrins and to heparan sulfate. In order to identify new partners of endostatin we have developed glycosaminoglycan and protein arrays based on SPR detection. We have found nine new partners of endostatin include glycosaminoglycans (chondroitin and dermatan sulfate), matricellular proteins (thrombospondin-1 and SPARC), collagens (I, IV and VI), the amyloid peptide Aβ(1-42), and transglutaminase-2 (TG-2). We have shown that endostatin binds to transglutaminase-2 with an high affinity (KD ~ 6 nM) in a calcium-dependent manner. Enzymatic assays indicated that, in contrast to other extracellular matrix proteins, endostatin is not a glutaminyl substrate of TG-2, but would rather be an acyl acceptor. The endostatin network comprises a number of extracellular proteins containing EGF domains (Epidermal Growth Factor), and able to bind calcium. Depending on the trigger event, and on the availability of its members in a given tissue at a given time, the endostatin network might be involved either in the control of angiogenesis, and tumor growth, or in neurogenesis and neurodegenerative diseases

Angiogenèse

Endostatine

Glycosaminoglycane

Intégrines

Interactome

Matrice extracellulaire

SPR array

Transglutaminase-2

Angiogenesis

Endostatin

Glycosaminoglycan

Integrin

Interactome

Extracellular matrix

SPR array

Tranglutaminase-2

572

Construction et analyse de réseaux d’interactions extracellulaires / Construction and analysis of extracellular interactions networks

Chautard, Émilie

21 September 2010

La matrice extracellulaire est constituée d'un réseau tridimensionnel de protéines et de polysaccharides complexes, les glycosaminoglycanes. Elle apporte un support structural aux tissus et aux cellules dont elle est capable de moduler la prolifération, la migration et la différenciation. Nous avons créé une base de données d'interactions extracellulaires protéine-protéine et protéine-glycosaminoglycane, MatrixDB, qui est disponible sur le Web (http://matrixdb.ibcp.fr). Nous avons intégré des données expérimentales, des données issues de l’analyse de la littérature et des données issues de bases de données d'interactions publiquement disponibles. Nous avons respecté les standards de curation et d’échange de données du consortium IMEx dont fait partie MatrixDB. MatrixDB permet la construction et la visualisation de l'interactome extracellulaire entier et de plusieurs types de réseaux d'interactions, spécifiques d'une molécule, d'un tissu, d'une pathologie ou d'un processus biologique. Nous avons ainsi caractérisé le réseau d’interactions extracellulaire associé au vieillissement et mis en évidence le rôle important des glycosaminoglycanes et du calcium dans ce réseau. Nous avons construit le réseau d'interactions d'une matricryptine anti-angiogénique et anti-tumorale, l'endostatine, qui est issue du collagène XVIII. Les analyses structurales et fonctionnelles de ce réseau ont montré que les partenaires de l’endostatine sont majoritairement impliqués dans l’adhésion cellulaire et que les domaines EGF (Epidermal Growth Factor) sont surreprésentés. Cette propriété nous a permis d'identifier expérimentalement d'autres partenaires de l'endostatine possédant un ou plusieurs domaines EGF et de nouvelles fonctions de l’endostatine. Nous avons modélisé les complexes formés par l'endostatine avec deux de ses partenaires pour identifier les sites d'interactions. Ces prédictions, associées aux données expérimentales, ont permis de déterminer des interactions susceptibles d'être établies simultanément par l'endostatine. L'intégration de ces données et des paramètres cinétiques et d'affinité dans le réseau d'interactions de l'endostatine sera utilisée pour proposer un modèle de son mécanisme d'action qui reste mal connu / The extracellular matrix is composed of a tridimensional network of proteins and complex polysaccharides called glycosaminoglycans. It provides a structural support to tissues and modulates cell proliferation, migration and differenciation. We have created a database of protein-protein and proteinglycosaminoglycan extracellular interactions, MatrixDB (http://matrixdb.ibcp.fr). We have integrated experimental data, data issued of the literature curation and data from interaction databases publicly available. We have respected the curation and exchange standards of the IMEx consortium that includes MatrixDB. MatrixDB allows the construction and the visualization of the entire extracellular network and other types of interaction networks specific of a molecule, a tissue, a disease or a biological process. We have characterized the aging-related extracellular interaction network and underlined the important role of glycosaminoglycans and calcium in this network. We have constructed the interaction network of an antitumoral and anti-angiogenic matricryptin, endostatin, issued from collagen XVIII. Functional and structural analysis of their network showed that partners of endostatin are mostly involved in cell adhesion and that EGF domains are overrepresented. This has allowed us to to identify experimentally other partners of endostatin possessing one or more EGF domains and to propose new functions of endostatin. We have modelled complexes formed by endostatin with two of its partners to identify the binding sites.These predictions, associated with experimental data, allowed us to determine interactions able to be established simultaneously by endostatin. Integration of these data and of kinetics and affinity parameters in the interaction network of endostatin will be used to build a model of its mechanism of action that is not fully elucidated

Angiogenèse

Bases de données

Endostatine

Intégrines

Réseaux d’interactions

Interactomes

Matrice extracellulaire

Vieillissement

Angiogenesis

Database

Endostatin

Integrin

Interactions networks

Interactome

Extracellular matrix

Aging

572

Effets des contraintes mécaniques cycliques sur la génération de thrombine à la surface des cellules musculaires lisses de rat / Effects of cyclic mechanical stretch on thrombin generation at the surface of rat vascular smooth muscle cells

Mao, Xianqing

09 January 2012

Les cellules musculaires lisses (CML) vasculaires les composants cellulaires principaux de la paroi artérielle, sont exposées constamment aux contraintes mécaniques. Les contraintes mécaniques cycliques régulent de nombreuses fonctions des CML vasculaires via les intégrines. Parmi les intégrines, l'[alpha]v[gamma]3 est non seulement un mécano-transducteur mais aussi le récepteur de la prothrombine à la surface des CML. L?activation de l'intégrine [alpha]v[gamma]3 par les contraintes mécaniques pourrait favoriser l'adhésion des CML à la prothrombine et aussi accélérer la génération de thrombine à la surface des CML. Pour vérifier cette hypothèse, nous avons étudié l'effet des contraintes mécaniques sur la génération de thrombine par les CML et identifié les voies de la signalisation impliquées. Nous avons utilisé un modèle de Flexcell utilisant les CML aortiques de rat, soumises à un étirement cyclique (10%, 1Hz). L'exposition à l'étirement cyclique pendant 1h et 6h induit un phénotype de différenciation et non-apoptotique des CML et une augmentation de l'expression de l'intégrine [alpha]v[gamma]3. Il y a aussi une augmentation de la phosphorylation de Src, FAK, AKT de façon temps dépendant et une augmentation de la phosphorylation de l'ILK à 15 min et du clivage de taline de 5 à 60 min. L'étirement cyclique augmente l'adhésion des CML à la prothrombine et la génération de thrombine avec un effet maximum à 6h de 67% et 30% respectivement. Le peptide mimétique de l'intégrine [alpha]v[gamma]3 (cRGDPV) et le siARN [alpha]v bloquent tous les effets de l'étirement cyclique sur les CML. Le siARN taline inhibe l'expression de la sous-unité [alpha]v et également la phosphorylation de Src, AKT et ILK. Le siARN ILK n'a pas d'effet sur l'expression de l'[alpha]v mais inhibe la phosphorylation d'AKT et le clivage de taline à 6h de l'étirement cyclique. Ainsi, l'étirement cyclique induit une plus forte génération de thrombine par les CML vasculaires via l'activation des voies de signalisation dépendante de l'[alpha]v[gamma]3. Cette étude suggère que la génération de thrombine intravasculaire peut être régulée par des antagonistes de l'intégrine [alpha]v[gamma]3 et peut devenir une nouvelle cible thérapeutique chez les patients avec une pression pulsée élevée / Vascular smooth muscle cells (SMC), the main cellular components of the arterial wall, are constantly exposed to mechanical stretch. Cyclic mechanical stress regulates many functions of vascular SMC via integrins. Among the integrins, [alpha]v[gamma]3 is not only a mechanotransducer but also the receptor of prothrombin in the vascular SMC. Activation of integrin [alpha]v[gamma]3 by mechanical stretch may promote SMC adhesion to prothrombin and also accelerate thrombin generation on the surface of SMC. To test this hypothesis, we have studied the effect of mechanical stretch on the generation of thrombin by SMC and identified possible signaling pathway involved. We used a Flexcell model using rat aortic SMC subjected to cyclic stretch (10%, 1Hz). Exposure to cyclic stretch for 1h and 6h induced a phenotype of differentiation and non-apoptosis of SMC and an increased expression of integrin [alpha]v[gamma]3. There was also an increase in phosphorylation of Src, FAK, and AKT in a time dependent manner, increased phosphorylation of ILK at 15min and the cleavage of talin from 5 to 60min. Cyclic stretch increased the adhesion of prothrombin to the SMC, and thrombin generation with a maximum effect of 67% and 30% respectively. A peptide mimetic of integrin [alpha]v[gamma]3 (cRGDPV) and [alpha]v siRNA both blocked all the effects of cyclic stretch on SMC. A talin siRNA inhibited the expression of [alpha]v and the phosphorylation of Src, AKT and ILK. An ILK siRNA has no effect on the expression of [alpha]v but inhibited the phosphorylation of AKT and the cleavage of talin at 6h of stretch. Thus, cyclic stretch induced a higher thrombin generation by vascular SMC via activation of signaling pathways dependant on [alpha]v[gamma]3. This study suggests that intravascular thrombin generation can be regulated by antagonists of integrin [alpha]v[gamma]3 and can become a new therapeutic target for the patients with a high pulse pressure

Contraintes mécaniques cycliques

CML vasculaire

Thrombine

Intégrine [alpha]v[gamma]3

Mécanotransduction

Cyclic mechanical stretch

Vascular SMC

Thrombin

Integrin [alpha]v[gamma]3

Mechanotransduction

575.75

611.018 6

Peptídeo AG73, derivado da laminina-111, induz migração, invasão e secreção de proteases em linhagem celular derivada de carcinoma epidermóide oral através de sindecana-1 e integrina b1 / Laminin-111-derived peptide AG73 regulates migration, invasion and protease activity of cell line derived from oral squamous cell carcinoma through syndecan-1 and b1 integrin.

Siqueira, Adriane Sousa de

24 September 2009

Carcinona epidermóide é um prevalente tumor de cabeça e pescoço relacionado a altas taxas de mortalidade. Neste trabalho, verificamos se AG73 (RKRLQVQLSIRT, cadeia a1), peptídeo derivado da laminina-111, regula migração, invasão e secreção de protease em células de carcinoma epidermóide oral (OSCC). Cadeia a1 da laminina e MMP9 estão expressas neste tumor in vivo e in vitro. AG73 induziu aumento da taxa migratória de células OSCC em ensaios de ferida e migração, e também estimulou invasão em ensaio em câmaras bipartites com Matrigel. Células OSCC crescidas sobre AG73 exibiram aumento dose-dependente de MMP9, detectado por zimografia. Buscamos receptores de AG73 que regulariam atividade nesta linhagem. Células OSCC crescidas sobre AG73 exibiram colocalização de sindecana-1 e integrina b1, e silenciamento desses receptores com RNA de interferência promoveu diminuição de migração e invasão dependente de AG73 nestas células. Esses resultados sugerem que sindecana-1 e integrina b1, ativados por AG73, podem regular migração, invasão e secreção de MMPs em células OSCC. / Oral squamous cell carcinoma is a prevalent head and neck tumor, related to high mortality rates. Here we studied the role played by AG73 (RKRLQVQLSIRT, a1 chain) on migration, invasion and protease secretion of a cell line (OSCC) from human oral squamous cell carcinoma. Laminin a1 chain and MMP9 are expressed in oral squamous cell carcinoma cells in vivo and in vitro. AG73 increased migratory activity of OSCC cells, as shown by monolayer wound assays and migration assays. This peptide also stimulated cell invasion in chemotaxis chambers coated with Matrigel. OSCC cells cultured on AG73 showed a dose-dependent increase of MMP9 secretion, detected by zymography. We searched for AG73 receptors regulating activities in this cell line. OSCC cells grown on AG73 exhibited colocalization of syndecan-1 and b1 integrin, and siRNA knockdown of these receptors decreased AG73-dependent migration and invasion of OSCC cells. Our results suggest that syndecan-1 and b1 integrin signaling downstream of AG73 regulate migration, invasion and MMP secretion by OSCC cells

AG73 peptide

Carcinoma epidermóide

Integrina \'beta\'1

Laminin

Laminina

Matrix metalprotease

Metaloprotease de matriz

Peptídeo AG73

Sindecan-1

Squamous cell carcinoma

Syndecan-1

\'Beta\' 1 integrin

Adesão e atividade de protease são reguladas pelo peptídeo derivado da laminina AG73, sindecan-1 e integrina 1 em linhagem celular derivada de carcinoma adenóide cístico / Ahesion and protease activity are regulated by the laminin-derived peptide AG73, syndecan-1 and bintegrin in cell line derived from adenoid cystic carcinoma.

Oliveira, Elaine Cyreno

01 October 2009

Estudamos indução da atividade de MMP pelo peptídeo da laminina a1 AG73 em linhagem celular (CAC2) de carcinoma adenóide cístico. CAC2 cultivadas em laminina-111 com AG73 geraram espaços pseudocísticos. Inibidor de MMP diminuiu tais espaços, sugerindo ação de MMPs. CAC2 crescidas sobre AG73 mostraram aumento dose-dependente de MMP9. RNAi para MMP9 diminuiu remodelação em cultura 3D. Buscamos receptores de AG73 ligados à atividade de MMP9. CAC2 crescidas sobre AG73 exibiram colocalização de sindecan-1 e integrina b1. RNAi para sindecan-1 ou para integrina b1 geraram, isolados, redução na adesão a AG73 e nas atividades de remodelação e de protease. Duplo RNAi estudou a cooperação entre os receptores e promoveu diminuição na adesão a AG73 e na atividade de MMP. Distinção de receptores foi feita por cromatografia de afinidade e espectrometria de massa, através de colunas de afinidade com AG73 acoplado, que resultou em possíveis receptores, como integrinas b1 e aV. Sugerimos que AG73 regula adesão e secreção de MMP em células CAC2 através de sindecan-1 e integrina b1. / We studied induction of MMP activity by b1-laminin peptide AG73 in adenoid cystic carcinoma cell line (CAC2). Cells grown inside AG73-enriched laminin-111 exhibited pseudocystics spaces. MMP inhibitor decreased those spaces, suggesting MMPs action. Cells grown on AG73 showed a dose-dependent increase of MMP9 secretion. MMP9 siRNAi decreased remodeling in 3D culture. We searched for AG73 receptors regulating MMP9 activity. CAC2 grown on AG73 exhibited colocalization of syndecan-1 and b1 integrin. Syndecan-1 siRNA or siRNA b1 integrin showed reduction in adhesion to AG73 and in remodeling and protease activities. Double-knockdown explored syndecan-1 and 1 integrin cooperation and showed decrease in adhesion to AG73 and in MMP activity. Receptors characterization was made by affinity chromatography followed by mass spectrometry through AG73-affinity columns and showed putative receptors, like b1 and aV integrins. We suggest that AG73 peptide regulates adhesion and MMP secretion in CAC2 cells through syndecan-1 and b1 integrin.

AG73 peptide

Beta 1 integrin

Integrina beta 1

Laminin

Laminina

Matrix metaloprotease

Metaloprotease de matriz

Neoplasia de glândula salivar

Peptídeo AG73

Salivary gland neoplasm

Sindecan-1

Syndecan-1