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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
11

New Approaches to Studies of Paracellular Drug Transport in Intestinal Epithelial Cell Monolayers

Tavelin, Staffan January 2003 (has links)
<p>Studies of intestinal drug permeability have traditionally been performed in the colon-derived Caco-2 cell model. However, the permeability of these cell monolayers resembles that of the colon rather than that of the small intestine, which is the major site of drug absorption following oral administration. One aim of this thesis was therefore to develop a new cell culture model that mimics the permeability of the small intestine. 2/4/A1 cells are conditionally immortalized with a temperature sensitive mutant of SV40T. These cells proliferate and form multilayers at 33°C. At cultivation temperatures of 37 – 39°C, they stop proliferating and form monolayers. 2/4/A1 cells cultivated on permeable supports expressed functional tight junctions. The barrier properties of the tight junctions such as transepithelial electrical resistance and permeability to hydrophilic markers resembled those of the human small intestine <i>in vivo</i>. These cells lacked functional expression of drug transport proteins and can therefore be used as a model to study passive drug permeability unbiased by active transport. The permeability to diverse sets of drugs in 2/4/A1 was comparable to that of the human <i>jejunum</i> for both incompletely and completely absorbed drugs, and the prediction of human intestinal permeability was better in 2/4/A1 than in Caco-2 for incompletely absorbed drugs. The small intestinal-like paracellular permeability of 2/4/A1 thus enables better predictions of drug permeability in the small intestine than does Caco-2. </p><p>The studies of the paracellular route and its importance for intestinal drug permeability was also in focus in the second part of this thesis, in which a new principle for tight junction modulation was developed, based on the primary structure of the extracellular tight junction protein occludin. Peptides corresponding to the N-terminus of the first extracellular loop increased the permeability of the tight junctions, but lacked apical effect. This problem was solved by conjugation of one peptide to a lipoamino acid, resulting in two diastereomers with different effects. The L-isomer had a sustained apical effect, while that of the D-isomer was transient. In conclusion, conjugated occludin peptides constitute a new class of tight junction modulators that can enhance the tight junction permeability.</p>
12

New Approaches to Studies of Paracellular Drug Transport in Intestinal Epithelial Cell Monolayers

Tavelin, Staffan January 2003 (has links)
Studies of intestinal drug permeability have traditionally been performed in the colon-derived Caco-2 cell model. However, the permeability of these cell monolayers resembles that of the colon rather than that of the small intestine, which is the major site of drug absorption following oral administration. One aim of this thesis was therefore to develop a new cell culture model that mimics the permeability of the small intestine. 2/4/A1 cells are conditionally immortalized with a temperature sensitive mutant of SV40T. These cells proliferate and form multilayers at 33°C. At cultivation temperatures of 37 – 39°C, they stop proliferating and form monolayers. 2/4/A1 cells cultivated on permeable supports expressed functional tight junctions. The barrier properties of the tight junctions such as transepithelial electrical resistance and permeability to hydrophilic markers resembled those of the human small intestine in vivo. These cells lacked functional expression of drug transport proteins and can therefore be used as a model to study passive drug permeability unbiased by active transport. The permeability to diverse sets of drugs in 2/4/A1 was comparable to that of the human jejunum for both incompletely and completely absorbed drugs, and the prediction of human intestinal permeability was better in 2/4/A1 than in Caco-2 for incompletely absorbed drugs. The small intestinal-like paracellular permeability of 2/4/A1 thus enables better predictions of drug permeability in the small intestine than does Caco-2. The studies of the paracellular route and its importance for intestinal drug permeability was also in focus in the second part of this thesis, in which a new principle for tight junction modulation was developed, based on the primary structure of the extracellular tight junction protein occludin. Peptides corresponding to the N-terminus of the first extracellular loop increased the permeability of the tight junctions, but lacked apical effect. This problem was solved by conjugation of one peptide to a lipoamino acid, resulting in two diastereomers with different effects. The L-isomer had a sustained apical effect, while that of the D-isomer was transient. In conclusion, conjugated occludin peptides constitute a new class of tight junction modulators that can enhance the tight junction permeability.
13

Le stress et les maladies inflammatoires cryptogénétiques de l'intestin (MICI) : rôle anti-inflammatoire de la neurostimulation vagale (NSV) / Stress and cholinetgic system in intestinal homeostasis

Pelissier-Rota, Marjolaine 17 December 2014 (has links)
Les maladies inflammatoires chroniques de l'intestin (MICI) se caractérisent par des altérations de la structure épithéliale intestinale conduisant à une augmentation de la perméabilité intestinale. Cette altération de la barrière intestinale, par l'activation du système immunitaire, amène à l'inflammation. Le stress, par la production de neuromédiateurs spécifiques (le « corticotropin-releasing factor », CRF, et ses apparentés les urocortines, Ucn1-3) et de leurs récepteurs (CRF1 et CRF2) pourrait jouer un rôle prépondérant dans l'initiation et la récidive des poussées inflammatoires. Dans une étude préliminaire, nous avons montré que l'activation du CRF2 par l'Ucn3 entraîne une augmentation de la perméabilité intestinale par l'altération des JA. Le stress entraîne également une inhibition du système parasympathique vagal. La stimulation des efférences vagales (VNS) exerce un effet anti-inflammatoire périphérique par la libération d'acétylcholine (ACh) qui, en se liant aux récepteurs nicotiniques (nAChR), inhibe la réponse immuniataire (voie cholinergique anti-inflammatoire). Les récepteurs cholinergiques (nAChR et mAChR) sont également présents au niveau de l'épithélium intestinal, nous avons précédemment observé que les nAChR aurait un effet protecteur de la perméabilité en stabilisant les JA. A l'inverse, les mAChR aurait un effet pro-inflammatoire en potentialiser les effets du stress sur la perméabilité épithéliale. / Inflammatory Bowel Disease (IBD) patients, such as Crohn's disease or ulcerative colitis suffer from chronic and relapsing intestinal inflammation that favours the development of colitis associated cancer (CAC). This inflammation is initiated by aberrant activations of the innate immune responses associated to intestinal barrier defects. The conventional medical therapies consist to decrease the inflammatory response, which also decrease the risk of colon carcinoma but lead to severe side-effects. Recently, a number of animal studies have demonstrated that innate immune responses are attenuated by stimulation of the efferent arm of vagus nerve (VN) through its neurotransmitter acetylcholine (ACh) that acts on resident macrophages α7 nicotinic receptor (α7 nAChR). ACh also acts as a signalling molecule in epithelial cells through cholinergic receptors such as nAChR or muscarinic (mAChR) receptors. In the current study, we aimed to extend these findings to CAC prevention by treating human adenocarcinoma cell lines through targeting cholinergic receptors with nicotine (which binds nAChR) and ACh (which binds both cholinergic receptors). Using HT-29 and Caco-2 cell lines, we demonstrated that ACh-induced activation of mAChR results in cell dissociation together with changes in expression and localization of intestinal tight and adherens junction proteins. ACh-induced modulation of cell adhesion proprieties correlates with the acquisition of invasive potential. By contrast, nicotine-mediated activation of nAChR maintains epithelial cell organisation. ACh-released by VN stimulation (VNS) could effectively preserve epithelium integrity thus limiting inflammatory response and tumor development. However, attention should be paid on the nature of the cholinergic receptor solicited. Indeed, regarding to the protective effects of nAChR signalling on epithelial cells, activation of mAChR would worsen the disease and led to increase inflammation. These data have important repercussions on the therapeutic potential of VNS in IBD and CAC, which may represent “the yin and yang” of the intestinal homeostasis.
14

Utilização de zinco, na forma de óxido de zinco nanoparticulado, em dietas para leitões recém-desmamados / Dietary zinc supplementation, as zinc oxide nanoparticles, in weanling pig diets

Natália Cristina Milani 18 November 2016 (has links)
O objetivo deste estudo foi avaliar os efeitos da suplementação de Zn (na forma de ZnO nanoparticulado) em dietas para leitões recém-desmamados sobre o desempenho, a ocorrência de diarreia, a digestibilidade dos nutrientes, a excreção de Zn nas fezes, os parâmetros sanguíneos, a histologia do epitélio intestinal, a morfometria de órgãos e a contagem bacteriana no conteúdo intestinal em comparação ao uso de dose farmacológica de Zn (na forma de ZnO). Foram utilizados 192 leitões desmamados aos 21 dias, em um experimento em blocos casualizados, com 6 tratamentos, 8 repetições (blocos) e 4 animais por unidade experimental (baia). Os tratamentos foram: controle negativo - dieta basal com 100 mg de Zn/kg de ração (na forma de ZnO); controle positivo - dieta basal com 2400 mg de Zn/kg de ração (na forma de ZnO), e dieta basal com 12, 24, 48 ou 96 mg de Zn/kg de ração (na forma de ZnO-N). Os leitões foram alimentados com as dietas experimentais, durante os primeiros 21 dias de experimento. Dos 22 aos 35 dias, todos os animais foram alimentados com uma única dieta, com níveis basais de Zn. A ocorrência de diarreia foi registrada diariamente. Amostras de fezes foram coletadas para determinação da digestibilidade dos nutrientes da dieta e quantificação do Zn excretado. Amostras de sangue foram coletadas no 19° dia do experimento para análise dos parâmetros sanguíneos. No 21º dia, um animal de cada baia foi abatido para a realização da morfometria dos órgãos, histologia do epitélio intestinal e contagem bacteriana. Os dados foram submetidos à análise de variância e à regressão polinomial. Contrastes ortogonais foram utilizados para comparar o tratamento controle positivo com cada um dos níveis de Zn (na forma de ZnO-N). Não foram observados efeitos dos níveis de Zn (ZnO-N) sobre o desempenho, a excreção de Zn nas fezes, o hemograma, a morfometria de órgãos, a histologia do epitélio intestinal e a contagem bacteriana no conteúdo intestinal. O aumento dos níveis de Zn (ZnO-N) aumentou linearmente a digestibilidade aparente dos nutrientes da dieta. Foi observado efeito quadrático dos níveis de Zn (ZnO-N) sobre a frequência da ocorrência de diarreia entre os dias 1 e 7 e sobre a concentração plasmática de Zn. No período de 1 a 21 dias foi observado um menor consumo diário de ração para os níveis de Zn (ZnO-N) em comparação ao controle positivo. Não foram observados diferenças entre o controle positivo e os níveis de Zn (ZnO-N) para as variáveis de desempenho e a frequência da ocorrência de diarreia durante o período de 21 a 35 dias. Foi observada uma menor excreção de Zn nas fezes, e uma menor concentração plasmática de Zn para os níveis de Zn (ZnO-N) em comparação ao controle positivo. A suplementação de Zn, na forma de ZnO-N, não foi capaz de substituir a dose farmacológica de Zn (ZnO) no controle da diarreia após o desmame. Os níveis de Zn, na forma de ZnO-N, não ocasionaram toxicidade nos animais e propiciaram uma redução na excreção de Zn nas fezes. / The purpose of this study was to evaluate the effects of dietary Zn (as ZnO nanoparticles) on performance, diarrhea occurrence, nutrient digestibility, Zn excretion in the feces, blood parameters, histology of gut epithelium, organs morphometry and intestinal bacterial count of weanling pigs compared to the use of pharmacological doses of Zn (as ZnO). One hundred and ninety-two 21d-weaned pigs (5.90±0.83 kg BW) were used in a randomized complete block design experiment with 6 treatments, 8 replications per treatment, and 4 animals per experimental unit (pen). The treatments were: negative control (NC): basal diet (based on corn, soybean meal, dried whey and dried plasma) with 100 mg Zn (as ZnO)/kg diet; positive control (PC): basal diet with 2,400 mg Zn(as conventional ZnO, 150nm)/kg diet and basal diet with 12, 24, 48 or 96 mg Zn (as ZnO-N, 70nm)/kg diet. Pigs were fed dietary treatments from 1 to 21 d feeding period followed by a common diet (same diet for all treatments) from 22 to 35 d feeding period. Diarrhea occurrence was recorded daily. Feces samples were collected to determine the digestibility of the diet and to quantify the Zn excreted. Blood samples were collected on the 19th day of the experiment for analysis of blood parameters. On the 21th day one pig per pen was slaughtered for the analyses of organs morphometry, intestinal epithelium histology and bacterial count. ANOVA and polynomial regression analysis (for levels of Zn as ZnO-N) were performed. Orthogonal contrasts were used to compare positive control with each level of Zn (as ZnO-N). No effects of Zn levels (as ZnO-N) were observed on performance, Zn excretion on feces, blood count, organs morphometry, intestinal epithelium histology and intestinal bacterial count. Increased levels of Zn (as ZnO-N) linearly increased the apparent digestibility of nutrients. It was observed a quadratic effect of Zn levels (as ZnO-N) on the frequency of diarrhea occurrence between 1 and 7 d and on the Zn plasma concentration. From 1 to 21 d of experimental period, lower daily feed intake for Zn levels (as ZnO-N) was observed compared to positive control. No differences were observed among the positive control and levels of Zn (as ZnO-N) for performance and diarrhea occurrence during the period 21 to 35 d. Lower Zn excretion in feces and lower Zn plasma concentration were observed for Zn levels (as ZnO-N) compared to the positive control. Zn supplementation, as ZnO-N, could not to replace the pharmacological dose of Zn (ZnO) to control diarrhea after weaning. The levels of Zn, as ZnO-N, did not cause toxicity of weanling pigs and reduced Zn excretion in the feces.
15

Desenvolvimento de novo método ex vivo para estudo da permeabilidade de fármacos utilizando epitélio intestinal de rã-touro (Rana catesbeiana) / Development of a new ex vivo method to study drugs permeability using intestinal epithelium of frog (Rana catesbeiana)

Talita Ferreira Monteiro 07 December 2012 (has links)
Este trabalho teve como objetivo propor novo método para estudar a permeabilidade de fármacos, utilizando epitélio intestinal de rã-touro (Rana catesbeiana) em método ex vivo, empregando células de Franz. Por utilizar epitélio intestinal, um material de descarte proveniente de um animal utilizado como alimento humano, pode ser considerado um método alternativo, pois não implica no sacrifício de animais. A quantidade de fármaco permeada foi determinada por método de eletroforese capilar com detecção ultravioleta e validado para os antivirais lamivudina, zidovudina e aciclovir, na presença de metoprolol e floridizina. O fármaco escolhido como modelo nos ensaios de permeabilidade foi a lamivudina. Para estabelecimento do protocolo experimental dos estudos de permeabilidade, foi proposta uma análise de variância three-way para verificar a influência na permeabilidade dos fármacos, das seguintes variáveis: secção intestinal, pH da solução de Ringer e temperatura. Foram determinados a quantidade total de fármaco permeado (Qt), o coeficiente de permeabilidade aparente (Papp) e a constante de absorção de primeira ordem (ka). A partir da análise do planejamento experimental, os efeitos das variáveis não foram significativos, exceto para a secção intestinal. Os resultados de coeficiente de permeabilidade aparente (Papp) obtidos foram de 0,09 x 10-4 cm/s para lamivudina e de 0,22 x 10-4 cm/s para o metoprolol. O valor de Papp obtido de para o metoprolol é próximo dos valores encontrados na literatura para outras técnicas. Para a lamivudina, entretanto, a diferença encontrada em comparação às células Caco-2 pode ser devida às diferentes técnicas empregadas. / This work aimed to propose a new method for studying drug permeability using frog intestinal epithelium (Rana catesbeiana) in ex vivo method, using Franz cells. By using intestinal epithelium, a disposal material from an animal used as human food, can be considered an alternative method, because it doesn\'t involve the sacrifice of animals. The amount of permeated drug was determined by capillary electrophoresis method with UV detection and validated for antiviral drugs lamivudine, zidovudine and acyclovir in the presence of metoprolol and floridizina. The drug chosen as a model in permeability studies was lamivudine. To establish the experimental protocol for the permeability studies, a three-way analysis of variance was proposed to check the influence of intestinal section, pH of Ringer\'s solution and the temperature on the permeability. Total amount of drug permeated (Qt), apparent permeability coefficient (Papp) and first-order constant absorption (ka) were determined. By the analysis of experimental design, the effects of the variables were not significant, except for intestinal section. The results of apparent permeability coefficient (Papp) obtained were 0.09 x 10-4 cm/s for lamivudine and 0.22 x 10-4 cm/s for metoprolol. The value of Papp obtained for metoprolol is quite close to the values found in literature for other methods. For lamivudine, however, the difference found in comparison to Caco-2 cells may be due to different techniques.
16

Rôle de la GTPase atypique RhoU dans l'homéostasie intestinale / Role of the atypical GTPase RhoU in the intestinal homeostasis

Slaymi, Chaker 04 December 2014 (has links)
L'épithélium intestinal se renouvelle tous les 4 à 6 jours chez les mammifères grâce aux cellules souches localisées au fond des cryptes. Le renouvellement dépend des signaux émis par le microenvironnement et requiert une phase de prolifération des cellules souches, de différenciation et d'apoptose/desquamation des cellules épithéliales. La signalisation Wnt, joue un rôle majeur dans l'homéostasie intestinale par l'action de deux gradients inversés le long de l'axe crypte/lumière ; la signalisation Wnt canonique, active au fond des cryptes, contrôle la prolifération alors que la signalisation non-canonique, active vers le haut des cryptes contrôle la différenciation. Il a été montré que ces deux voies contrôlent l'activité de la GTPase atypique RhoU/Wrch1. RhoU fait partie des GTPases qui s'activent spontanément, son activité est donc directement proportionnelle à son niveau d'expression dans la cellule. Enfin, cette GTPase atypique est sous exprimée dans de nombreuses tumeurs gastriques et colorectales.Compte tenu de ces données, nos objectifs étaient donc de caractériser les changements morphologiques induits par l'invalidation conditionnelle de RhoU dans l'épithélium intestinal murin et d'en déterminer les mécanismes d'action. Nos résultats montrent que la déplétion de RhoU n'est pas létale, cependant elle a induit une augmentation de 20% de la densité cellulaire et une désorganisation de la structure de l'épithélium dans le haut des cryptes du colon. Cette augmentation concerne aussi bien les lignages sécrétoires et absorptifs, cependant, l'absence de RhoU a induit une sur-représentation du lignage sécrétoire. Dans la lignée de tumeur colorectale DLD-1, nous avons montré que l'absence de RhoU mime le phénotype d'augmentation de la densité cellulaire observé chez la souris. L'invalidation de RhoU ne modifie pas la distribution des phases du cycle cellulaire ni de celle de la mitose, cependant, elle réduit le nombre des cellules en apoptose dans le colon des souris et dans les cellules DLD-1. L'invalidation de RhoU a réduit la signalisation Hippo et a altéré la contractilité cellulaire via une augmentation de la phosphorylation de la protéine MLC2. Des travaux récents ont montré que la diminution du niveau MLC2 phosphorylée est nécessaire pour l'activation des caspases par un stimulus apoptotique. Ceci suggère que cette perturbation de la contractilité peut être à l'origine de cette diminution de l'apoptose qui est la cause majeure responsable de ce phénotype. En conclusion, RhoU est un régulateur de l'homéostasie intestinale chez la souris via son rôle modérateur de la mort cellulaire. / In Mammals, the intestinal epithelium is renewed every 4-6 days through the stem cells located at the bottom of crypts. The renewal depends on signals from the micro-environment and requires a proliferation phase of stem cells, then a differentiation and apoptosis/desquamation phases of epithelial cells. Wnt signaling plays a major role in intestinal homeostasis by the action of two reversed gradients along the axis crypt/ lumen: canonical Wnt signaling, active in the bottom of crypts, control proliferation while non canonical signaling, active in the top of the crypts control cell differentiation. It was shown that these two pathways are regulator of the atypical GTPase RhoU/Wrch1. The RhoU protein activates spontaneously, its activity is directly proportional to its expression level in the cell and is expressed as in gastric and colorectal tumors. In view of these informations, our objectives were therefore to characterizethe morphological changes induced by conditional invalidation of RhoU in the intestinal epithelium of mice and to determine the mechanisms of action. Our results show that RhoU depletion is not lethal. However, it induces an increase of cell density (+20%) and a disruption of the epithelium structure in the top of the colonic crypts. This increase affects both absorptive and secretory lineages. However, the absence of RhoU induced over-representation of secretory lineage. In colorectal tumor cell line DLD-1, we have shown that the absence of RhoU mimics the phenotype of cell density increase observed in mice. RhoU invalidationdid not change the distribution of cell cycle phases and mitosis, however, it reduces the number of apoptotic cells in the colon of mice and in the DLD-1 cells. RhoU invalidation reduced Hippo signaling and altered cell contractility via the increase of the protein MLC2 phosphorylation. Recent work has shown that the reduction of MLC2-P level is necessary for the caspase protein activation by an apoptotic stimulus. Suggesting that the perturbation of contractility may be the cause of this apoptosis decrease which is the main cause responsible of this phenotype. Finally, RhoU is a regulator of the intestinal homeostasis in micevia its moderating role of cell death.
17

Study of Musashi1-Expressing cells and of Musashi1 function in mouse intestinal physiopathology / Etude des cellules exprimantes Musashi1 et de la fonction de Musashi1 dans la physiopathologie intestinale de la souris

Cambuli, Francesca Maria 20 December 2012 (has links)
L’épithélium intestinal est une monocouche de cellules qui tapisse la lumière intestinale, constitué d’un compartiment différencié, les villosités dans l’intestin grêle et les plateaux épithéliaux dans le colon, et d’un compartiment prolifératif, les cryptes de Lieberkühn. Ce tissue se renouvelle de façon rapide et continue tout au long de la vie de l’individu, grâce à la présence de cellules souches adultes dans le fond des cryptes. Ces cellules s’autorenouvellent et donnent naissance à des progéniteurs prolifératifs (capables d’engendrer les différents cytotypes épithéliaux) qui se différencient tout en migrant vers le compartiment différencié. Mon travail de these a porté sur l’étude d’une marqueur putatif de ces cellules souches épithéliales intestinales: Musashi1 (Msi1).Dans ce contexte, mon premier axe d’étude s’est focalisé sur l’isolement et la caractérisation des cellules souches épithéliales intestinales chez la souris. Pour cela, nous avons généré des souris transgéniques exprimant la protéine fluorescente GFP sous le contrôle du promoteur de Msi1. Les cellules souches intestinales de ces souris coexpriment donc Msi1 et la GFP. Ce modèle a été validé et nous à permis de isoler les cellules GFP/Msi1 positives dans l’intestin. A l'aide de différentes approches cellulaires et moléculaires, nous avons confirmé leur nature de cellules souches et nous avons apporté des nouvelles données sur la composition de la zone proliférative de l’épithélium intestinal murin.Le second axe de mes travaux de thèse a porté sur l’étude de la fonction de Msi1 dans l'homéostasie de l’épithélium intestinal chez la souris, par son sur-expression tous au long de l’épithélium. Nous avons montré que la sur-expression de cette protéine, qui est un régulateur des voies Wnt et Notch, perturbe l’architecture intestinale, a propriétés pro-prolifératives et un potentiel tumorigènique. / The intestinal epithelium is a monolayer of cells surrounding the intestinal lumen. It consists of a differentiated compartment, the villi in the small intestine and a flat surface in the colon, and a proliferative compartment, the crypts of Lieberkühn. This tissue self-renews rapidly and continuously throughout life, due to the presence of adult stem cells in the bottom of the crypts. These cells are capable of self-renewing and give rise to proliferating progenitors (capable of generating all the different epithelial cytotypes) that differentiate and migrate toward the differentiated compartment. My thesis focused on the study of the intestinal epithelial stem cells marker Musashi1 (Msi1).In this context, the first part of my thesis work focused on the isolation and characterization of the intestinal epithelial stem cells that express Msi1 in the mouse. For this, we generated transgenic mice expressing the fluorescent protein GFP under the control of the promoter of Msi1. The intestinal stem cells of these mice co-express Msi1 and GFP. This model has been validated and allowed us to isolate GFP+/Msi-expressing cells in the intestine. By using different cellular and molecular approches, we confirmed their nature of stem cells and provided new data on the composition of the proliferative zone in the murine intestinal epithelium.The second part of my thesis has focused on the study of the function of Msi1 in the intestinal epithelium homeostasis in the mouse, by its over- and ectopic expression all along the epithelium. We have shown that the over-expression of this protein, which is a regulator of the Wnt and Notch pathways, perturbs the intestinal architecture, has pro-proliferative properties and tumorigenic potential.
18

Rôle de la Protéine Cellulaire du Prion (PrPc) dans l'homéostasie de l'épithélium intestinal / Role of the cellular prion protein in the intestinal epithelium homeostasis

Besnier, Laura 31 January 2014 (has links)
La Protéine Cellulaire du Prion (PrPc), isoforme non pathogène de la Protéine Scrapie, est une protéine ubiquitaire qui a été impliquée dans de nombreux processus cellulaires tels que la prolifération, la migration, l’adhésion, la différenciation et l’apoptose, par des mécanismes qui restent en grande partie à élucider. L’épithélium intestinal est en constant renouvellement et son homéostasie repose sur une régulation fine et coordonnée de l’ensemble de ces processus. Notre équipe s’est intéressée au rôle de la PrPc dans l’épithélium intestinal et a mis en évidence son expression dans le type cellulaire majoritaire de cet épithélium, les entérocytes, et sa double localisation selon leur état de différenciation. En effet, dans les cellules différenciées, la PrPc est majoritairement présente au niveau des desmosomes, alors que dans les cellules prolifératives, elle est principalement nucléaire. Nous mettons en évidence que la PrPc desmosomale est impliquée dans le maintien et l’intégrité de l’ensemble des jonctions intercellulaires (jonctions serrées, adhérentes et desmosomes) et contribue à la fonction de barrière de l’épithélium intestinal. La PrPc nucléaire, quant à elle, interagit avec plusieurs effecteurs de la voie de signalisation Wnt : la -caténine, la -caténine et le facteur de transcription TCF7L2. Dans ce contexte, nous révélons la capacité de la PrPc nucléaire à moduler l’expression de gènes cibles de la voie Wnt canonique. L’ensemble de ces travaux permet de révéler la PrPc comme un nouvel élément clé de l’homéostasie de l’épithélium intestinal – du maintien de la fonction de barrière jusqu’à la régulation de l’expression de gènes – et de définir la PrPc comme un nouveau membre de la famille des protéines NACos. / The cellular Prion Protein (PrPc), the normal conformer of the Scrapie protein, is a ubiquitous protein, which has been involved in several cellular processes such as proliferation, migration, adhesion, differentiation and apoptosis, through mechanisms that are not fully characterized. Intestinal epithelium is renewing constantly and its homeostasis requires a fine and coordinated regulation of all these processes. Our team has focused on PrPc functions in this tissue and has demonstrated that it is expressed in enterocytes, the major cell type in the intestinal epithelium, with a dual localization depending on the differentiation state of the cells. Indeed, in differentiated cells PrPc is localized in desmosomes while being mostly in the nucleus in proliferative cells. We demonstrated the involvement of desmosomal PrPc in the maintenance and integrity of all the intercellular junctions (tight, adherens junctions and desmosomes) and its requirement for the intestinal barrier function. PrPc in the nucleus interacts with key effectors of the Wnt pathway: -catenin, -catenin and the transcription factor TCF4/TCF7L2. In this context, we revealed the ability of nuclear PrPc to modulate the expression of a subset of Wnt target genes. Altogether, this work highlights the role of PrPc as a new key element of the intestinal epithelial homeostasis – from the barrier function to gene regulation – and allows considering PrPc as a new member of the NACos family proteins (proteins associated with the Nucleus and Adhesion Complexes).
19

Étude du rôle de la Nétrine-1 dans l'ontogénèse et le maintien de l'homéostasie de l'épithélium intestinal murin / Investigating Netrin-1 functions during the ontogenesis and the homeostatic maintenance of the mouse intestinal epithelium

Vieugué, Pauline 15 December 2017 (has links)
L'épithélium intestinal adulte des mammifères est un tissu hautement organisé entièrement renouvelé tous les 5 à 7 jours, grâce à la présence de cellules souches intestinales (CSI). Localisées à la base des cryptes, les CSI sont capables de s'auto-renouveler et de générer l'ensemble des types cellulaires de ce tissu. Afin de préserver l'équilibre entre leur auto-renouvellement et leur différenciation, véritable garant de l'homéostasie de l'épithélium intestinal, les CSI résident dans un microenvironnement finement régulé, « la niche », leur procurant l'ensemble des signaux nécessaires à leurs fonctions. La Nétrine-1, molécule sécrétée et apparentée à la famille des Laminines, est exprimée dans l'environnement des cryptes intestinales, mais également au cours du développement intestinal. Initialement découverte pour son rôle dans le guidage axonal, cette protéine est à ce jour considérée comme une molécule pléïotropique impliquée dans divers processus physiologiques tels que la morphogénèse, la migration, l'adhésion cellulaire, la prolifération mais également pathologiques comme la tumorigénèse. Considérant ces observations nous nous sommes donc intéressés au rôle potentiel de la Nétrine-1 dans la régulation du compartiment souche intestinal adulte, ainsi que lors de l'ontogénèse intestinale. Dans une première partie, nous montrons qu'ex vivo la Nétrine-1 promeut la croissance des entéroïdes et régule l'expression génique de certains marqueurs spécifiques des CSI. Dans une seconde partie, nous montrons, grâce à la génération et caractérisation de nouveaux modèles murins, que la Nétrine-1 est impliquée dans le développement de l'épithélium intestinal grêle et que sa délétion conduit à un retard d'émergence des villi / The adult intestinal epithelium is a highly organized tissue, which is completely self-renewed every 5 to 7 days, due to a pool of multipotent intestinal stem cells (ISC). Located at the base of intestinal crypts, ISC have the ability to self- renew and to give rise to all epithelial intestinal cell types. To preserve the balance between their self-renewal and their differentiation, and therefore to maintain the epithelial tissue homeostasis, ISC reside in a tightly regulated microenvironment - called “niche”- that provides them all factors required for their functions. Netrin-1, a laminin-related secreted protein, is expressed in the microenvironment of the crypt, and is also expressed during intestinal development. Initially described as an axonal guidance cue, Netrin-1 is now considered as a pleiotropic molecule involved in many different processes such as morphogenesis, cell migration, cell adhesion, proliferation and also tumorigenesis. Based on these observations, we hypothesized that Netrin-1 could play a role in the maintenance of the adult intestinal stem cell compartment, and also in the intestinal ontogenesis. In a first part, we showed that Netrin-1 promotes the growth of enteroids ex vivo while regulating gene expression of specific intestinal stem cell markers. In the second part, we demonstrated, by using two novel genetically engineered mouse models, that Netrin-1 is involved in the embryonic development of the intestinal epithelium and that its deletion leads to a delay in villi emergence
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Analysis of genetic interactions and hierarchies of Wnt-signaling components in vivo

Schelp, Nadine 06 December 2012 (has links)
Der Wnt/β-catenin Signalweg reguliert zusammen mit anderen Signalkaskaden die Embryogenese sowie auch die Homöostase und die Proliferation der Stammzellen im adulten Organismus. Mutationen in Komponenten dieses Signaltransduktionsweges führen zu einer aberranten Aktivierung von β-catenin und wurden in vielen verschieden Krebsarten einschließlich Darmkrebs beobachtet. Die transkriptionelle Akivität von β-catenin wird von verschiedenen nukleären Kofaktoren beeinflusst. Hierzu zählen insbesondere die Proteine der Pygopus Familie, die in Drosophila eine essentielle Rolle im kanonischen Wnt-Signalweg spielen, in Vertebraten allerdings vielmehr Kontext abhängig agieren. Insbesondere Pygo2 ist hierbei vermutlich auch an der malignen Transformation verschiedener Zelltypen mit anschließender Ausbildung von Tumoren beteiligt. Auch wenn bereits gezeigt werden konnte, dass Pygo2 in Darmtumoren überexprimiert wird, ist bisher unbekannt, ob es tatsächlich eine Rolle bei der Entstehung von intestinalen Tumoren spielt. Anhand von genetischen Experimenten in der Maus zeigt diese Arbeit zum ersten Mal in vivo, dass Pygo2 für die normale Homöostase des Darms nicht essentiell ist, aber an der Ausbildung von Darmtumoren, welche durch eine Stabilisierung von β-catenin induziert werden, beteiligt ist. Weder im embryonalen noch im adulten Darm beeinflusste der konditionale Villin-Cre bedingte Knock-out von Pygo2 in epithelialen Zellen die normale embryonale Entwicklung oder die Homöostase im adulten Darm. Auch für die Regulation von Zielgenen des Wnt/β-catenin Signalweges unter physiologischen Bedingungen scheint Pygo2 funktionell redundant zu sein. Im Gegensatz dazu verhinderte der Verlust von Pygo2 die Entstehung von β-catenin induzierten intestinalen Tumoren und normalisierte die damit verbundene Hyperproliferation sowie die erhöhte Expression von Wnt/β-catenin Zielgenen und intestinalen Stammzellmarkern. Überraschenderweise konnte die Ausbildungen von Adenomen in ApcMin/+ Mäusen durch Deletion von Pygo2 nicht verhindert werden. Der Vergleich beider Mausmodelle ergab eine erhöhte Expression von BCL9-2 in den Adenomen der ApcMin/+ Mäuse aber nicht in den Hyperplasien, die durch aktiviertes β-catenin induziert wurden. Dies könnte darauf hinweisen, dass in Apc mutierten epithelialen Zellen BCL9-2 für die Tumorprogression verantwortlich ist. Weiterhin konnte gezeigt werden, dass sowohl der knock-down von Pygo2 als auch von BCL9-2 in human Kolonkarzinomzellen die Proliferation reduzierte. Anhand von immunohistochemischen Analysen des Phosphorylierungsstatus von ERK1/2, einem „downstream“ Effektor von K-ras, konnten außerdem pERK1/2 positive Zellen in den intestinalen Adenomen von ApcMin/+ Mäusen, nicht aber in hyperproliferierenden Zellen mit stabilisierten β-catenin nachgewiesen werden. Zusammenfassend weisen die Ergebnisse dieser Arbeit daraufhin, dass die Funktion von Pygo2 im Darm Kontext abhängig ist. Während in normalen epithelialen Zellen des Darms Pygo2 offensichtlich funktionell redundant ist, scheint es für die Ausbildung von intestinalen Tumoren, welche durch dereguliertes Wnt/β-catenin induziert werden, essentiell zu sein. Daher könnte Pygo2 ein idealer Angriffspunkt für die zielgerichtete Therapie von Darmtumoren mit β-catenin Mutation sein.

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