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The role of Stat3 in cell division and apoptosisANAGNOSTOPOULOU, AIKATERINI 27 April 2009 (has links)
The Signal Transducer and Activator of Transcription-3 (Stat3) is a transcription factor that is required for transformation by a number of oncogenes, while a constitutively active form of Stat3 alone is sufficient to induce neoplastic transformation. It was previously demonstrated that cell to cell adhesion causes a dramatic increase in the activity of Stat3 in both normal and tumour cells. This hinted for the first time at the possibility that the role of Stat3 may differ upon cellular confluence. To examine such a mechanism, it is important to evaluate the effect of Stat3 downregulation at different time-points relative to confluence. To examine this, two different approaches for Stat3 downregulation were used: (1) the introduction of high levels of peptidomimetics analogs, which block the Stat3-SH2 domain by using a technique of in situ electroporation. (2) Treatment with two platinum compounds that inhibit Stat3 binding to activated receptors and DNA.
The results demonstrated that Stat3 downregulation in vSrc or TAg transformed mouse fibroblast cells or in breast carcinoma lines, induced apoptosis which was more pronounced post-confluence at the time of its peak activity. In contrast, in sparsely growing normal mouse fibroblasts, Stat3 inhibition induced merely a growth retardation. However, in densely growing normal fibroblasts, Stat3 inhibition induced apoptosis. At least in part, apoptosis induced by Stat3 inhibition was mediated by p53, as shown by the resistance to cell death by Stat3 downregulation in colon carcinoma cells, HCT116, where the p53 gene is ablated. Overall, our observations point to the possibility that constitutive activation of Stat3 may lead to tumourigenesis by downregulating wt-53 in cancers that do not have p53 mutations. As a result, targeting Stat3 in cancers with wt-p53 may be a promising therapeutic approach for restoring p53 function, thereby inducing p53-mediated apoptosis.
Next, we examined the effect of constitutively activated Stat3 as an oncogene. Stat3C expression in rat F111 fibroblasts induced anchorage independence, but to a lower degree compared to other oncogenes, such as vSrc. Surprisingly Stat3C expression increased gap junction intercellular communication, despite the fact that other oncogenes such as vSrc or vRas effectively block gap junctions. / Thesis (Ph.D, Pathology & Molecular Medicine) -- Queen's University, 2009-04-26 01:09:21.654
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Participação da conexina 32 na fisiopatogênese da doença hepática gordurosa não alcoólica em camundongos / Role of connexin 32 in physiopatogenesis of nonalcoholic fatty liver disease in miceTiburcio, Taynã Cristina 04 March 2016 (has links)
A doença hepática gordurosa não alcoólica (DHGNA) abrange alterações desde esteatose até esteato-hepatite não alcoólica (EHNA), podendo evoluir para fibrose, cirrose e carcinoma hepatocelular. A DHGNA é considerada a doença hepática mais comum na atualidade e com prevalência mundial alarmante. Esta doença caracteriza-se, basicamente, pela deposição de triglicérides nos hepatócitos, podendo evoluir com inflamação e fibrose, e está intimamente associada com resistência à insulina (RI), diabetes mellitus tipo 2 e obesidade. Os hepatócitos representam as principais células hepáticas e se comunicam através de junções do tipo gap, formadas principalmente por conexina 32 (Cx32). Esta proteína apresenta importante função no controle da homeostase tecidual, regulando processos fisiológicos e tem sido associada como agente protetor na hepatocarcinogênese e outros processos patológicos, porem pouco se sabe sobre sua participação na DHGNA. Sendo assim, o objetivo deste trabalho foi avaliar a participação da Cx32 na fisiopatogênese da DHGNA, utilizando camundongos knockout para Cx32 (Cx32-KO) submetidos a uma dieta hiperlipídica deficiente em colina. Foram analisados dados biométricos, histopatológicos, função hepática, RI, citocinas inflamatórias, adipocinas, estresse oxidativo, peroxidação lipídica e a expressão de genes envolvidos na DHGNA. Os animais Cx32-KO apresentaram maior acumulo de triglicérides hepáticos em relação aos animais selvagens e, consequentemente, maior peso absoluto e relativo do fígado. Adicionalmente, apresentaram maior inflamação hepática demonstrado pela exacerbação da citocina TNF-α e supressão da IL-10, maior dano hepatocelular indicado pelo aumento das enzimas AST e ALT, aumento da peroxidação lipídica e alterações na expressão de genes chaves na fisiopatogênese da DHGNA, como SREBP1c. No entanto, não houve diferença nos marcadores histopatológicos, RI e estresse oxidativo hepático. Por fim, os animais Cx32-KO apresentaram maior produção de leptina e adiponectina no tecido adiposo. Todos esses resultados revelam que a Cx32 pode atuar como um agente protetor ao desenvolvimento da DHGNA, sugerindo seu potencial como novo alvo terapêutico / Nonalcoholic fatty liver disease (NAFLD) covers a spectrum of liver diseases ranging from steatosis to nonalcoholic steatohepatitis (NASH), liver fibrosis, cirrhosis and eventually hepatocellular carcinoma. NAFLD is currently the most common liver disease in the world with an alarming prevalence worldwide. This disease is characterized by the deposition of triglycerides in hepatocytes and can develop inflammation and fibrosis. NAFLD is closely associated with insulin resistance (IR), type 2 diabetes mellitus and obesity. The gap junctions mediate intercellular communication and are critical for maintaining integral cellular processes. In hepatocytes, the major type of liver cells, the gap junctions are formed mainly by connexin 32 (Cx32). This protein is important for the control of tissue homeostasis and for physiological processesregulation. It has been linked as a protective agent in hepatocarcinogenesis and other pathological processes. However, little is known about its role on NAFLD. Thus, the aim of this study was to evaluate the participation of Cx32 in the pathogenesis of NAFLD using WT and Cx32-knockout mice (Cx32-KO) subjected to a high-fat diet deficient in choline. NAFLD was evaluated based on a battery of clinically relevant read-outs, including histopathological examination, inflammatory citokines, liver damage markers, in-depth lipid analysis, assessment of oxidative stress, insulin and glucose tolerance and lipid-related biomarkers.The Cx32-KO animals showed higher accumulation of hepatic triglycerides, increased inflammation and lipid peroxidation and increased production of leptin and adiponectin in the adipose tissue when compared with WT. Moreover, there was no difference in histopathological markers, RI and hepatic oxidative stress. Taken together, all these results show that Cx32 is a protective agent to the development of the disease, suggesting its potential as a novel therapeutic target in NAFLD
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Participação das conexinas 43 e 32 no desenvolvimento da fibrose hepática: estudo em camundongos geneticamente modificados / Role of connexins 43 and 32 on the development of hepatic fibrosis: a study in genetically modified miceCogliati, Bruno 23 April 2010 (has links)
A fibrose hepática resulta da cronicidade da injúria celular, ocasionando acúmulo dos componentes da matriz extracelular (MEC) pela ativação, principalmente, de células estreladas e fibroblastos portais em miofibroblastos. Estas células se conectam através de junções comunicantes do tipo gap, formadas por proteínas denominadas conexinas (Cx). As junções gap são responsáveis pelo fluxo de moléculas e íons entre as células, desempenhando importante função no controle da homeostasia tecidual. Diversos tipos de conexinas foram descritas nas células hepáticas. Os hepatócitos expressam Cx32 e Cx26, enquanto as demais células não-parenquimatosas expressam Cx43. Alguns estudos analisaram a expressão das conexinas e das junções gap em processos de reparação e fibrogênese em diferentes tecidos, no entanto, poucos avaliaram seu papel na fibrogênese hepática. Sendo assim, o objetivo deste estudo foi avaliar os aspectos morfológicos, histopatológicos e moleculares da fibrose hepática, induzida por tetracloreto de carbono (CCl4), em animais deficientes para as conexinas 43 (Cx43+/-) ou 32 (Cx32-/-). Foram analisados dados biométricos, histopatológicos, ultra-estruturais, imuno-histoquímicos e bioquímicos, além da expressão gênica e protéica das conexinas. Os aspectos moleculares da fibrose hepática foram analisados pela expressão de genes relacionados com a deposição e degradação da matriz extracelular por PCR em tempo real. As análises macroscópicas e de varredura demonstraram um processo de micronodulação da superfície hepática mais acentuado nos camundongos Cx43+/- fibróticos em relação aos animais wild-type (Cx43+/+) fibróticos. Adicionalmente, estes animais apresentaram maior proporção volumétrica de colágeno no tecido hepático; redução na atividade necroinflamatória tecidual; redução nas concentrações séricas de AST e ALT; redução na proliferação celular dos hepatócitos e redução na expressão dos genes: colágeno tipo I, TGFβ-1, MMP-2, MMP-13 e TIMP-1. Por sua vez, os camundongos Cx32-/- fibróticos apresentaram aumento na deposição de colágeno no parênquima hepático; aumento na atividade necroinflamatória tecidual e aumento nos níveis séricos das enzimas hepáticas AST, ALT e fosfatase alcalina em comparação aos animais wild-type (Cx32+/+) fibróticos. Também foram observadas redução na proliferação hepatocelular e maior quantidade de corpúsculos apoptóticos no tecido hepático. Baseando-se em todos os resultados obtidos, observou-se que ambos os modelos animais apresentaram aumento da fibrose hepática, aparentemente ocasionada por diferentes modos de ação. Os animais deficientes em Cx43 apresentaram menor capacidade de degradação do colágeno, ocasionando seu acúmulo no tecido hepático. Por outro lado, os animais deficientes em Cx32 apresentaram maior deposição de colágeno em resposta à injúria hepatocelular mais acentuada, aliada ao desequilíbrio entre as taxas de proliferação celular e apoptose. Em conclusão, os resultados obtidos neste trabalho demonstraram a importante participação das conexinas no controle da fibrogênese hepática, e que podem representar potenciais alvos terapêuticos para o tratamento das doenças hepáticas crônicas em humanos e animais. / Hepatic fibrosis results from chronic cell injury, leading to accumulation of components of extracellular matrix (ECM) through activation mainly of hepatic stellate cells and portal fibroblasts into myofibroblasts. These cells communicate through intercellular gap junctions composed of proteins known as connexins (Cx). Gap junctions are responsible for the exchange of molecules and ions among cells, playing an important role in the control of tissue homeostasis. Several subtypes of connexins were described among hepatic cells. Hepatocytes express Cx32 and Cx26, while the other non-parenchymal cells express Cx43. Some studies analyzed the expression of connexins and gap junctions on processes of healing and fibrogenesis in different tissues; however, few studies evaluated its role on hepatic fibrogenesis. Thus, the objective of this study was to evaluate morphological, histopathological and molecular aspects of hepatic fibrosis induced by carbon tetrachloride (CCl4) in animals with connexin 43 (Cx43+/-) or 32 (Cx32-/-) deficiency. We analyzed biometric, histopathological, ultrastructural, immunohistochemical and biochemical data, besides gene and protein expression of connexins. Molecular aspects of hepatic fibrosis were analyzed with the expression of genes related to deposition and degradation of extracellular matrix by real time PCR. Macroscopic and Scanning Electron Microscopy analyses showed a process of micronodulation of hepatic surface more accentuated on Cx43+/- fibrotic mice when compared to fibrotic wild-type (Cx43+/+) animals. Additionally, these animals presented a higher collagen volumetric proportion on hepatic tissue; reduction of tissue necroinflammatory activity; reduction of serum AST and ALT; reduction of hepatocytes proliferation and reduction of expression type I collagen, TGFβ-1, MMP-2, MMP-13 and TIMP-1 genes. Fibrotic Cx32-/- mice presented an increase of collagen deposition in hepatic parenchyma; increase of tissue necro-inflammatory activity and increase of liver enzymes AST, ALT and alkaline phosphatase when compared to fibrotic wild-type (Cx32+/+) animals. Reduction of hepatocellular proliferation and a higher amount of apoptotic bodies on hepatic tissue were also observed. Based on the results obtained, we observed that both animal models showed an increase of hepatic fibrosis, apparently caused by different modes of action. Cx43 deficient animals showed a reduced capacity to degrade collagen, causing its accumulation in the hepatic tissue. Cx32 deficient animals showed an increased collagen deposition in response to accentuated hepatocellular injury, together to an unbalance between rates of cellular proliferation and apoptosis. In conclusion, results obtained on this study demonstrate an important role of connexins on the control of hepatic fibrogenesis, which could represent potential therapeutical targets for the treatment of chronic liver diseases in humans and animals.
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Participação das conexinas 43 e 32 no desenvolvimento da fibrose hepática: estudo em camundongos geneticamente modificados / Role of connexins 43 and 32 on the development of hepatic fibrosis: a study in genetically modified miceBruno Cogliati 23 April 2010 (has links)
A fibrose hepática resulta da cronicidade da injúria celular, ocasionando acúmulo dos componentes da matriz extracelular (MEC) pela ativação, principalmente, de células estreladas e fibroblastos portais em miofibroblastos. Estas células se conectam através de junções comunicantes do tipo gap, formadas por proteínas denominadas conexinas (Cx). As junções gap são responsáveis pelo fluxo de moléculas e íons entre as células, desempenhando importante função no controle da homeostasia tecidual. Diversos tipos de conexinas foram descritas nas células hepáticas. Os hepatócitos expressam Cx32 e Cx26, enquanto as demais células não-parenquimatosas expressam Cx43. Alguns estudos analisaram a expressão das conexinas e das junções gap em processos de reparação e fibrogênese em diferentes tecidos, no entanto, poucos avaliaram seu papel na fibrogênese hepática. Sendo assim, o objetivo deste estudo foi avaliar os aspectos morfológicos, histopatológicos e moleculares da fibrose hepática, induzida por tetracloreto de carbono (CCl4), em animais deficientes para as conexinas 43 (Cx43+/-) ou 32 (Cx32-/-). Foram analisados dados biométricos, histopatológicos, ultra-estruturais, imuno-histoquímicos e bioquímicos, além da expressão gênica e protéica das conexinas. Os aspectos moleculares da fibrose hepática foram analisados pela expressão de genes relacionados com a deposição e degradação da matriz extracelular por PCR em tempo real. As análises macroscópicas e de varredura demonstraram um processo de micronodulação da superfície hepática mais acentuado nos camundongos Cx43+/- fibróticos em relação aos animais wild-type (Cx43+/+) fibróticos. Adicionalmente, estes animais apresentaram maior proporção volumétrica de colágeno no tecido hepático; redução na atividade necroinflamatória tecidual; redução nas concentrações séricas de AST e ALT; redução na proliferação celular dos hepatócitos e redução na expressão dos genes: colágeno tipo I, TGFβ-1, MMP-2, MMP-13 e TIMP-1. Por sua vez, os camundongos Cx32-/- fibróticos apresentaram aumento na deposição de colágeno no parênquima hepático; aumento na atividade necroinflamatória tecidual e aumento nos níveis séricos das enzimas hepáticas AST, ALT e fosfatase alcalina em comparação aos animais wild-type (Cx32+/+) fibróticos. Também foram observadas redução na proliferação hepatocelular e maior quantidade de corpúsculos apoptóticos no tecido hepático. Baseando-se em todos os resultados obtidos, observou-se que ambos os modelos animais apresentaram aumento da fibrose hepática, aparentemente ocasionada por diferentes modos de ação. Os animais deficientes em Cx43 apresentaram menor capacidade de degradação do colágeno, ocasionando seu acúmulo no tecido hepático. Por outro lado, os animais deficientes em Cx32 apresentaram maior deposição de colágeno em resposta à injúria hepatocelular mais acentuada, aliada ao desequilíbrio entre as taxas de proliferação celular e apoptose. Em conclusão, os resultados obtidos neste trabalho demonstraram a importante participação das conexinas no controle da fibrogênese hepática, e que podem representar potenciais alvos terapêuticos para o tratamento das doenças hepáticas crônicas em humanos e animais. / Hepatic fibrosis results from chronic cell injury, leading to accumulation of components of extracellular matrix (ECM) through activation mainly of hepatic stellate cells and portal fibroblasts into myofibroblasts. These cells communicate through intercellular gap junctions composed of proteins known as connexins (Cx). Gap junctions are responsible for the exchange of molecules and ions among cells, playing an important role in the control of tissue homeostasis. Several subtypes of connexins were described among hepatic cells. Hepatocytes express Cx32 and Cx26, while the other non-parenchymal cells express Cx43. Some studies analyzed the expression of connexins and gap junctions on processes of healing and fibrogenesis in different tissues; however, few studies evaluated its role on hepatic fibrogenesis. Thus, the objective of this study was to evaluate morphological, histopathological and molecular aspects of hepatic fibrosis induced by carbon tetrachloride (CCl4) in animals with connexin 43 (Cx43+/-) or 32 (Cx32-/-) deficiency. We analyzed biometric, histopathological, ultrastructural, immunohistochemical and biochemical data, besides gene and protein expression of connexins. Molecular aspects of hepatic fibrosis were analyzed with the expression of genes related to deposition and degradation of extracellular matrix by real time PCR. Macroscopic and Scanning Electron Microscopy analyses showed a process of micronodulation of hepatic surface more accentuated on Cx43+/- fibrotic mice when compared to fibrotic wild-type (Cx43+/+) animals. Additionally, these animals presented a higher collagen volumetric proportion on hepatic tissue; reduction of tissue necroinflammatory activity; reduction of serum AST and ALT; reduction of hepatocytes proliferation and reduction of expression type I collagen, TGFβ-1, MMP-2, MMP-13 and TIMP-1 genes. Fibrotic Cx32-/- mice presented an increase of collagen deposition in hepatic parenchyma; increase of tissue necro-inflammatory activity and increase of liver enzymes AST, ALT and alkaline phosphatase when compared to fibrotic wild-type (Cx32+/+) animals. Reduction of hepatocellular proliferation and a higher amount of apoptotic bodies on hepatic tissue were also observed. Based on the results obtained, we observed that both animal models showed an increase of hepatic fibrosis, apparently caused by different modes of action. Cx43 deficient animals showed a reduced capacity to degrade collagen, causing its accumulation in the hepatic tissue. Cx32 deficient animals showed an increased collagen deposition in response to accentuated hepatocellular injury, together to an unbalance between rates of cellular proliferation and apoptosis. In conclusion, results obtained on this study demonstrate an important role of connexins on the control of hepatic fibrogenesis, which could represent potential therapeutical targets for the treatment of chronic liver diseases in humans and animals.
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Participação da conexina 32 na fisiopatogênese da doença hepática gordurosa não alcoólica em camundongos / Role of connexin 32 in physiopatogenesis of nonalcoholic fatty liver disease in miceTaynã Cristina Tiburcio 04 March 2016 (has links)
A doença hepática gordurosa não alcoólica (DHGNA) abrange alterações desde esteatose até esteato-hepatite não alcoólica (EHNA), podendo evoluir para fibrose, cirrose e carcinoma hepatocelular. A DHGNA é considerada a doença hepática mais comum na atualidade e com prevalência mundial alarmante. Esta doença caracteriza-se, basicamente, pela deposição de triglicérides nos hepatócitos, podendo evoluir com inflamação e fibrose, e está intimamente associada com resistência à insulina (RI), diabetes mellitus tipo 2 e obesidade. Os hepatócitos representam as principais células hepáticas e se comunicam através de junções do tipo gap, formadas principalmente por conexina 32 (Cx32). Esta proteína apresenta importante função no controle da homeostase tecidual, regulando processos fisiológicos e tem sido associada como agente protetor na hepatocarcinogênese e outros processos patológicos, porem pouco se sabe sobre sua participação na DHGNA. Sendo assim, o objetivo deste trabalho foi avaliar a participação da Cx32 na fisiopatogênese da DHGNA, utilizando camundongos knockout para Cx32 (Cx32-KO) submetidos a uma dieta hiperlipídica deficiente em colina. Foram analisados dados biométricos, histopatológicos, função hepática, RI, citocinas inflamatórias, adipocinas, estresse oxidativo, peroxidação lipídica e a expressão de genes envolvidos na DHGNA. Os animais Cx32-KO apresentaram maior acumulo de triglicérides hepáticos em relação aos animais selvagens e, consequentemente, maior peso absoluto e relativo do fígado. Adicionalmente, apresentaram maior inflamação hepática demonstrado pela exacerbação da citocina TNF-α e supressão da IL-10, maior dano hepatocelular indicado pelo aumento das enzimas AST e ALT, aumento da peroxidação lipídica e alterações na expressão de genes chaves na fisiopatogênese da DHGNA, como SREBP1c. No entanto, não houve diferença nos marcadores histopatológicos, RI e estresse oxidativo hepático. Por fim, os animais Cx32-KO apresentaram maior produção de leptina e adiponectina no tecido adiposo. Todos esses resultados revelam que a Cx32 pode atuar como um agente protetor ao desenvolvimento da DHGNA, sugerindo seu potencial como novo alvo terapêutico / Nonalcoholic fatty liver disease (NAFLD) covers a spectrum of liver diseases ranging from steatosis to nonalcoholic steatohepatitis (NASH), liver fibrosis, cirrhosis and eventually hepatocellular carcinoma. NAFLD is currently the most common liver disease in the world with an alarming prevalence worldwide. This disease is characterized by the deposition of triglycerides in hepatocytes and can develop inflammation and fibrosis. NAFLD is closely associated with insulin resistance (IR), type 2 diabetes mellitus and obesity. The gap junctions mediate intercellular communication and are critical for maintaining integral cellular processes. In hepatocytes, the major type of liver cells, the gap junctions are formed mainly by connexin 32 (Cx32). This protein is important for the control of tissue homeostasis and for physiological processesregulation. It has been linked as a protective agent in hepatocarcinogenesis and other pathological processes. However, little is known about its role on NAFLD. Thus, the aim of this study was to evaluate the participation of Cx32 in the pathogenesis of NAFLD using WT and Cx32-knockout mice (Cx32-KO) subjected to a high-fat diet deficient in choline. NAFLD was evaluated based on a battery of clinically relevant read-outs, including histopathological examination, inflammatory citokines, liver damage markers, in-depth lipid analysis, assessment of oxidative stress, insulin and glucose tolerance and lipid-related biomarkers.The Cx32-KO animals showed higher accumulation of hepatic triglycerides, increased inflammation and lipid peroxidation and increased production of leptin and adiponectin in the adipose tissue when compared with WT. Moreover, there was no difference in histopathological markers, RI and hepatic oxidative stress. Taken together, all these results show that Cx32 is a protective agent to the development of the disease, suggesting its potential as a novel therapeutic target in NAFLD
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Connexine als potenzielle Biomarker für den Progress oraler Plattenepithelkarzinome: Analyse der Expressionsmuster von Connexin 26, 43 und 45 und ihres Einflusses auf das Überleben / Connexins as potential biomarkers for the progression of oral squamous cell carcinoma: analysis of the expression pattern of connexin 26, 43 and 45 and their influence on survivalBrockmeyer, Phillipp 02 July 2014 (has links)
No description available.
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Les processus de différenciation et la résistance des kystes aux traitements de désinfection chez l'amibe libre Vermamoeba vermiformis / The processes of differentiation and resistance of cysts to disinfection treatments in the free-living amoeba Vermamoeba vermiformisFouque, Emilie 09 December 2013 (has links)
V. vermiformis est une amibe libre répandue dans l'environnement et les milieux artificiels comme les réseaux d'eau chaude sanitaire (RECS). Il est maintenant bien établi qu'elle joue un rôle de réservoir pour des bactéries pathogènes, comme L. pneumophila. Le contrôle de V. vermiformis dans les RECS représente donc un enjeu sanitaire important. Les amibes libres peuvent passer d'une forme métaboliquement active (trophozoïte) à une forme de résistance, le kyste, lorsque les conditions sont défavorables ce qui leur confère une résistance aux traitements. Malgré la haute prévalence de V. vermiformis dans les RECS, les processus de différenciation et la résistance de ses kystes aux traitements n'ont été que peu étudiés. Nous avons donc investigué les changements morphologiques et ultrastructuraux qui s'opèrent lors de l'enkystement et désenkystement de V. vermiformis. Il en ressort que l'enkystement est un phénomène rapide (9 h) qui conduit à la formation de kystes entourés d'une paroi double couche. Lors du désenkystement, les trophozoïtes n'émergent pas à travers un ostiole comme c'est le cas chez Acanthamoeba. Puis, nous avons étudié l'effet des conditions environnementales et de la concentration cellulaire sur l'enkystement. Nous avons observé que plus la concentration cellulaire est élevée plus l'enkystement est rapide, ce qui suggère l'existence de mécanismes de communication intercellulaire. Enfin, nous avons étudié la résistance des kystes aux traitements utilisés dans les RECS et aux protéases. Ces traitements étaient efficaces, in vitro, pour inactiver les kystes de V. vermiformis. Ces travaux ont permis d'apporter des connaissances de bases sur les processus de d / Vermamoeba vermiformis is a free-living amoeba (FLA) widespread in the environment and artificial environments such as hot water networks. It is now well established that it acts as a reservoir for many pathogenic bacteria, such as Legionella pneumophila. The control of V. vermiformis in artificial environments represents an important health issue. FLA can turn from a metabolic active form (trophozoite) to a resistance form, called cyst, when conditions are unfavorable. Cysts are more resistant to treatments. Despite the high prevalence of V. vermiformis in hot water networks, the processes of differentiation and the resistance of cysts to disinfection treatments have been poorly studied. Therefore we investigated morphological and ultrastructural changes occurring during encystment and excystment of V. vermiformis. It appears that encystment is a fast process (9 h) which leads to the formation of cysts surrounded by a double-layered wall. During excystment, trophozoites do not emerge through an ostiole as is the case with Acanthamoeba. Then, we studied the effect of environmental conditions and cell concentration on encystment. We observed that the higher cell concentration was, the faster the encystment was, which suggests the existence of intercellular communication. Finally, we studied the resistance of cysts to conventional disinfection treatments used in hot water networks and to innovative treatment with proteases. These treatments were effective, in vitro, to inactivate V. vermiformis cysts. This work provides new finding regarding differentiation processes and cysts resistance of V. vermiformis, a free-living amoeba poorly studied.
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Étude de l'implication de la Connexine 43 dans le processus d'invasion des glioblastomes humains / Study of Connexin 43 involvement in human glioblastoma invasion processChepied, Amandine 02 October 2015 (has links)
Depuis plusieurs décennies, la communication intercellulaire par jonctions gap (CIJG) est connue pour être impliquée dans la cancérogenèse. Cette implication semble complexe par le fait que les connexines pourraient augmenter la capacité d’invasion des cellules cancéreuses tout en diminuant leur prolifération. Ceci était particulièrement observé pour la connexine 43 (Cx43) dans le cas de cellules de gliomes. Or, les propriétés d’invasion des gliomes de haut grade, les glioblastomes multiformes (GBM), les rendent difficiles à supprimer par résection chirurgicale et favorisent leur récidive.<br/> Afin de préciser le rôle de la Cx43 dans le contrôle des capacités invasives de cellules de GBM, nous avons utilisé une lignée de cellules de glioblastome humaine U251 exprimant par shRNA des niveaux, en ARNm et protéiques, de Cx43 réduits. Ces clones shRNA des cellules U251 montrent une corrélation entre le niveau d’expression de la Cx43 et le processus d’invasion. Au cours de ce travail, nous avons montré, pour la première fois, que la Cx43 est localisée dans les structures protéolytiques permettant l’invasion, les invadopodes. Nous avons démontré aussi que, par sa localisation, la Cx43 favorise la formation des invadopodes en agissant comme une protéine d’échafaudage qui permet l’interaction de Src de la Cortactine. De plus, l’activité hémicanal de la Cx43, probablement inhibée par le Bisphénol A, possède des effets négatifs sur la cinétique de développement des invadopodes. Une étude du protéome et du sécrétome des cellules U251 et des clones shRNA a permis l’identification des protéines impliquées dans l’invasion et la formation et fonction des invadopodes.<br/> En conclusion, la Cx43 participe au processus invasif des cellules de GBM en favorisant la formation et la fonction des invadopodes. Cette nouvelle fonction de la Cx43 semble être la conséquence de ses propriétés de protéines d’échafaudage et hémicanal, et non de son rôle principalement décrit dans la CIJG. / Since several decades, the gap junction intercellular communication (GJIC) is known to be involved in carcinogenesis. This involvement seems complicated by the fact that connexins could increase cancer cells invasion ability while decreasing their proliferation. This was especially observed for connexin 43 (Cx43) in the case of glioma cells. But high-grade gliomas, glioblastoma multiform (GBM) has invasion properties that make it difficult to remove surgically and promote their recurrence.<br/> To clarify the Cx43 role in the control of GBM cells invasive capacities, we used the GBM U251 cell line expressing Cx43 levels, mRNA and protein, reduced by shRNA strategy. Through this approach, we confirmed that Cx43 expression level is associated with the invasive capacity of GBM cells. Furthermore we have shown, for the first time, that Cx43 is localized in invasive proteolytic structures, the invadopodia. We also show that, by its location, Cx43 promotes invadopodia formation by acting as a scaffolding protein that allows Src and Cortactin interaction. Moreover, Cx43 hemichannel activity, probably inhibited by Bisphenol A, has negative effects on invadopodia kinetics development. A proteome and secretome study of U251 cells and shRNA clones allowed the identification of proteins involved in invasion and invadopodia formation and function.<br/>In conclusion, Cx43 participates in the invasive process of GBM cells by promoting invadopodia formation and function. This new function of Cx43 seems to be the result of its scaffold proteins and hemichannel properties, but not its role described mainly in CIJG.
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The Effect of Viral Envelope Glycoproteins on Extracellular Vesicle Communication andFunctionTroyer, Zach Andrew January 2021 (has links)
No description available.
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Comparative analysis of RNA-associated proteins in the cellular and extracellular environments of HMLE cellsChen, Yiran 11 1900 (has links)
Thesis with manuscript / La communication intercellulaire joue un rôle important dans tous les organismes, car elle permet l'échange de molécules bioactives entre les cellules. La plupart des cellules peuvent sécréter des vésicules extracellulaires (VE) délimitées par une membrane, qui peuvent servir de médiateur pour le transfert sélectif de matériel génétique, en particulier de molécules d'ARN, vers des cellules réceptrices et modifier leur phénotype. Pour faciliter le ciblage de l'ARN vers les VE, les protéines de liaison de l'ARN (RBP) interagissent avec les ARN, formant des complexes ribonucléoprotéiques (RNP) et guidant leur localisation vers les sites de production des VE. Alors que la facilitation du transport de l'ARN par les RBP est bien étudiée dans les cellules, leur mécanisme dans les VE reste mal compris.
Pour mieux comprendre le chargement sélectif des ARN dans les VE, nous avons effectué un profilage RBP complet du sécrétome libéré par les cellules épithéliales mammaires humaines (HMLE), en comparaison avec le matériel des cellules entières. Nous avons d'abord utilisé la réticulation UV pour lier de manière covalente les RBP et leurs ARN associés, puis nous avons isolé le sécrétome par ultracentrifugation et purifié les RBP par extraction d'ARN lié à des protéines (XRNAX) et par spectrométrie de masse (MS). Grâce à une analyse comparative des RBP dans les environnements cellulaire et extracellulaire, nous avons identifié des collections de protéines associées à l'ARN qui étaient communes aux deux compartiments (n=189), ou qui présentaient une association plus spécifique avec l'ARN dans les échantillons cellulaires (n= 866) ou EV (n=502). Nous avons constaté que les RBP du compartiment extracellulaire (ExRBP) avaient des signatures fonctionnelles distinctes (par exemple, le métabolisme cellulaire, la structure et la modification des cellules, le repliement des protéines) par rapport aux facteurs enrichis en cellules (par exemple, le processus métabolique de l'ARN non codant). Notamment, des RBP EV bien connus, tels que ALIX, ANXA1, hnRNPR, hnRNPQ (SYNCRIP), YBX1, ainsi que des marqueurs EV de tétraspanine (CD9, CD81, TSG101), étaient enrichis dans l'ExRBP, ce qui indique le succès de XRNAX dans la purification des RBP EV. En comparant notre collection d'ExRBP aux signatures MS des VE plus pures dérivées des cellules HMLE, nous avons également pu délimiter les ExRBP qui
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sont susceptibles d'être enrichies en VE (PureEVRBP) par rapport à celles trouvées dans le sécrétome non VE (SecRBP). Il est frappant de constater que le PureEVRBP étaient enrichies en protéines de jonction cellulaire, tandis que le secRBP étaient enrichies en facteurs spliceosomaux, ce qui implique un chargement sélectif des RBP dans les VE ou leur sécrétion dans l'espace extracellulaire. Cette recherche fournit des informations précieuses sur la composition des RBP dans les EV, servant d'ensembles de données protéomiques clés pour élucider davantage les mécanismes modulant le recrutement sélectif des ARN dans les EV et améliorant notre connaissance des rôles des RBP dans la biologie des VE. / Intercellular communication plays an important role in all organisms, as it enables the exchange of bioactive molecules between cells. Most cells can secrete membrane-delimited extracellular vesicles (EVs), which can mediate the selective transfer of genetic material, in particular RNA molecules, to recipient cells and modify their phenotypes. To facilitate the targeting of RNA to EVs, RNA binding proteins (RBPs) are thought to interact with RNAs, forming ribonucleoprotein complexes (RNPs) and guiding their localization to sites of EV production. While the facilitation of RNA transportation by RBPs is well-studied in cells, their mechanism in EVs remain poorly understood.
To gain insights into the selective loading of RNAs into EVs, we conducted comprehensive RBP profiling on the secretome released by Human Mammary Epithelial (HMLE) cells, in comparison to whole cell material. We first employed UV cross-linking to covalently link RBPs and their associated RNAs, followed by secretome isolation through ultracentrifugation and purification of RBPs using Protein-Xlinked RNA Extraction (XRNAX) and mass spectrometry (MS). Through a comparative analysis of RBPs in cellular and extracellular environment, we identified collections of RNA-associated proteins that were common to both compartments (n=189), or which exhibited more specific RNA association in cellular (n= 866) or EV (n=502) specimens. We found that extracellular compartment RBPs (ExRBPs) had distinctive functional signatures (e.g. cellular metabolism, cell structure and modification, protein folding) compared to cellular-enriched factors (e.g. non-coding RNA metabolic process). Notably, well-known EV RBPs, such as ALIX, ANXA1, hnRNPR, hnRNPQ (SYNCRIP), YBX1, as well as tetraspanin EV markers (CD9, CD81, TSG101), were enriched in ExRBP, indicating the success of XRNAX in EV RBP purification. By comparing our ExRBP collection to the MS signatures of more pure HMLE cell derived EVs, we were also able to delineate ExRBPs that are likely to be EV-enriched enriched versus those found in the non-EV secretome. Strikingly, pure EV-RBPs were enriched for cell-junction proteins, while general secretome RBPs were enriched for spliceosomal factors, implying selective loading of RBPs into EVs or their secretion into the extracellular space. This research provides valuable insights into the composition of RBPs in EVs, serving as key proteomic datasets to further elucidate
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the mechanisms modulating the selective recruitment of RNAs into EVs and enhancing our knowledge of the roles of RBPs in EV biology.
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