• Refine Query
  • Source
  • Publication year
  • to
  • Language
  • 88
  • 19
  • 18
  • 15
  • 10
  • 8
  • 2
  • 2
  • 1
  • 1
  • Tagged with
  • 183
  • 183
  • 38
  • 32
  • 30
  • 25
  • 24
  • 22
  • 21
  • 20
  • 19
  • 19
  • 18
  • 18
  • 17
  • 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.
151

Les histones déacétylases de type 2 dans le contrôle de la mort cellulaire induite par la cryptogéine, un éliciteur des réactions de défense chez le tabac / Type-2 histones deacetylases and cryptogein-induced cell death in tabacco

Dutartre, Agnès 19 December 2011 (has links)
La cryptogéine, sécrétée par l’oomycète Phytophthora cryptogea, est un éliciteur protéique des réactions de défense qui active chez le tabac un ensemble d’événements de signalisation conduisant à la mise en place d’une mort cellulaire de type réponse hypersensible et d’une résistance systémique acquise. La caractérisation de la modulation de l’activité de kinases cytosoliques, dont SIPK et WIPK, par des événements de phosphorylation en réponse à la cryptogéine, traduit la place majeure que tiennent les modifications post-traductionnelles dans la cascade de signalisation induite dans les cellules de tabac en réponse à la cryptogéine. Il s’avère que la signalisation cellulaire induite par la cryptogéine, et impliquant ces protéines kinases, converge entre autre vers le noyau à travers la modulation de l’activité d’éléments nucléaires par phosphorylation. Dans ce contexte, d’importants travaux de purification/séquencage, visant à identifier les protéines nucléaires cibles de ces activités kinases, ont permis d’identifier deux isoformes redondantes d’histones désacétylases de type 2 nommés NtHD2a et NtHD2b qui sont rapidement phosphorylées en réponse à la cryptogéine dans les cellules de tabac.Ce travail de thèse s’inscrit dans l’étude du rôle de NtHD2a/b dans l’établissement du processus de mort cellulaire des cellules de tabac et de la RH in planta en réponse à la cryptogéine. Par des approches de pharmacologie ainsi que des approches de surexpression ou d’invalidation de l’expression de NtHD2a/b chez le tabac, nous avons d’une part confirmé l’implication de NtHD2a/b en tant que régulateurs négatifs de la mort cellulaire induite par la cryptogéine ou d’autres élicitines, et d’autre part mieux appréhendé les événements de la cascade de signalisation prépondérants dans l’établissement de cette mort cellulaire. Les mécanismes moléculaires sous-jacents à la mise en place de la mort cellulaire apparaissent complexes et semblent notamment impliquer la modulation de l’expression de gènes de défense, la synthèse de novo de protéines ainsi que l’activation de protéines kinases, dont notamment WIPK et SIPK.Des travaux relatifs à l’étude des événements de (dé)/acétylation dans les cellules de tabac traitées par la cryptogéine et invalidées dans l’expression de NtHD2a/b suggèrent le concours de modifications post-traductionnelles de protéines nucléaires telles que l’acétylation dans la mise en place de la mort cellulaire induite par la cryptogéine chez le tabac. / Cryptogein, which is secreted by the oomycete Phytophthora cryptogea, is a proteinaceous elicitor of plant defense reactions that activates a set of signaling events leading to the hypersensitive response and to systemic acquired resistance. Although the early cytosolic signaling events induced by cryptogein are well described, the only nuclear events characterized to date are the variations in free calcium concentrations and defense-related gene expression. The characterization of the activation of cytosolic protein kinases, including WIPK and SIPK, by phosphorylation in response to cryptogein highlights the key-role played by posttranslational modifications in cryptogein-induced signaling events in tobacco cells. In this context, purification/sequencing approaches revealed that two redundant isoforms of type-2 nuclear histone deacetylases, NtHD2a and NtHD2b, were rapidly phosphorylated in cryptogein-treated tobacco cells.This thesis work is part of a comprehensive study of the role of NtHD2a/b in the establishment of the cell death process in tobacco cells and of the hypersensitive response in planta, in response to cryptogein. By using a pharmacological approach and overexpression and RNA interference-based approaches, we confirmed the involvement of NtHD2a/b as negative regulators of elicitin-induced cell death and we achieved a better understanding of cell death signaling events. The molecular events that underly the cell death process appear particularly complex and seem to involve the modulation of defense-related gene expression, de novo protein synthesis and protein kinase activation such as WIPK and SIPK.The study of (de)/acetylation events in tobacco cells treated by cryptogein and invalidated in NtHD2a/b expression suggests a role for posttranslational modifications in cryptogein-induced cell death.
152

Papel de ciclina D1 na interação entre FGF-2, ACTH e outros peptídeos na sinalização em células adrenocorticais Y-1 / Role of cyclin D1 in the interaction between FGF-2, ACTH and other peptides in Y-1 adrenocortical cell signaling

Schwindt, Telma Tiemi 20 November 2001 (has links)
O principal controle do ciclo celular de mamíferos, que é dividido em G0/G1/S/G2/M, ocorre na transição G0→G1→S. Nesta tese mostramos que a proteína ciclina D1 desempenha um papel fundamental nos circuitos de transdução de sinais que regulam a transição G0→G1→S na linhagem Y-1 de células adrenocorticais de camundongo. Esta conclusão não é surpreendente, uma vez que, ao longo dos últimos anos, muitos laboratórios contribuíram para estabelecer a noção de que a atividade das diversas formas do complexo ciclina/CDK é essencial para a transição G0→G1→S, e também para outras etapas do ciclo celular. Em células Y-1, FGF-2 induz tardiamente (5-6h) a expressão do gene e da proteína ciclina D 1, através de um processo dependente de síntese de proteínas. Peptídeos hipofisários não identificados e vasopressina bloqueiam a indução de ciclina DI, antagonizando FGF-2. Por este mecanismo, vasopressina exerce um efeito anti-mitótico, bloqueando a transição G0→G1→S promovida por FGF-2. ACTH, que também exibe um forte efeito anti-mitótico sobre FGF-2 não afeta a indução de ciclina D1. A transfecção dupla de uma forma induzível de c-Myc (MycER) e constitutiva do cDNA de ciclina D1, em presença de ACTH mimetiza a ação mitogênica de FGF-2 em células Y-1 no estado G0. Estes resultados mostram que, em células adrenocorticais, c-Fos, c-Jun, c-Myc e ciclina D1 agem de forma independente e complementar, sendo necessários para a transição G0→G1→S do ciclo celular. / The main control of mammalian cell cycle, which is divided in G0/G1/S/G2/M, occurs in G0→G1→S transition. In this work we show that cyclin D1 protein plays a key role in signal transduction circuits underlying the G0→G1→S transition of mouse Y-1 adrenocortical cell line. This conclusion is not surprising, once in the last years, many laboratories have contributed to establish the notion that the activity of the distinct forms of cyclin/CDK complexes is essential for the G0→G1→S transition, and also for other phases transition of cell cycle. In Y-1 cells, FGF-2 causes a delayed (5-6h) induction of cyclin D1 gene and protein, through a process dependent on protein synthesis. Hypophisary peptides, not identified, as well as vasopressin, block cyclin D1 induction, antagonizing FGF-2. By this mechanism, vasopressin exert an antimitotic effect, blocking G0→G1→S transition promoted by FGF-2. ACTH, which also exhibit a strong anti-mitotic effect upon FGF-2, does not affect cyclin D1 induction. Double transfection of inducible c-Myc (MycER) and constitutive cyclin D1 cDNA, in the presence of ACTH, mimics the mitogenic action of FGF-2 in G0 Y-1 cells. Altogether, these results show that, in adrenocortical cells, c-Fos, c-Jun, c-Myc and cyclin D1 act in an independent and complementary manner, being necessary for the G0→G1→S transition of cell cycle.
153

Efeitos do α-tocoferol nas vias de sinalização associadas ao \"Burst\" oxidativo de neutrófilos humanos / Effects of α-tocopherol on signaling pathways associated with human neutrophil oxidative burst

Chan, Sandra Sueli 04 October 2000 (has links)
Neste estudo foi verificado os efeito do α-tocoferol (AT) nas vias de sinalização celular, dependentes de proteína quinase C (PKC) e de tirosinas quinases (TK), associadas ao \"burst\" oxidativo de neutrófilos humanos. Foram realizados também estudos comparativos com o inibidor da PKC, estaurosporina, com o inibidor de tirosinas quinases, genisteína e, com o análogo solúvel da vitamina E, Trolox. Foi feita a incorporação de AT in vitro às células, e então, estas foram estimuladas ou não com acetato de forbol miristato (PMA) ou com zymosan opsonizado (Zy). AT (40 µM) inibiu a produção de espécies reativas de oxigênio (ERO) pelos neutróflos estimulados com PMA ou Zy. Estaurosporina (10 nM), genisteína (100 µM) e Trolox (40 µM) também tiveram efeitos inibitórios. A atividade da PKC foi inibida pelo AT e pela estaurosporina, entretanto, a atividade da enzima não foi afetada pela genisteína e pelo Trolox. PMA e Zy promoveram um aumento da fosforilação em resíduos de tirosina de proteínas de neutrófilos. AT e estaurosporina provocaram um aumento adicional na fosforilação PMA-dependente, enquanto a genisteína causou uma diminiução e, Trolox não produziu nenhum efeito. Por outro lado, os quatro compostos foram inibitórios na fosforilação Zy-dependente. A atividade de tirosina fosfatases (PTPs) foi medida em neutrófilos estimulados e não-estimulados. PMA e Zy causaram uma diminuição na atividade de PTPs. A pré-incubação com AT e Trolox causou uma reversão destes efeitos inibitórios. O inibidor de serina/treonina fosfatases, caliculina A, também foi utilizado. Nós mostramos que este composto foi capaz de reverter os efeitos inibitórios do AT na produção de ERO e na atividade de PKC dos neutrófilos. Os resultados deste trabalho mostram que AT modulam ambas as via de sinalização, PKC e TK-dependentes, associadas com o \"burst\" oxidativo de neutrófilos humanos e, que esta modulação pode ser devido a ativação de fosfatases pelo AT. / The effects of α-tocopherol succinate (TS) on the signaling pathways, dependent of protein kinase C (PKC) and tirosine kinases (TK), associated with the oxidative burst of human neutrophils were analysed. Comparative studies with the PKC inhibitor, staurosporine, the TK inhibitor, genistein and the soluble analogous of vitamin E, Trolox were also performed. TS was incorporated into neutrophils and cells were then, stimulated or not with phorbol myristate acetate (PMA) or with opsonized zymosan (OZ). TS (40 µmol/l) inhibited the production of reactive oxygen species (ROS) by PMA or OZ-stimulated neutrophils. Staurosporine (10 nmol/l), genistein (100 µmol/l) and Trolox (40 µmol/l) were also inhibitory. PKC activity was inhibited by TS and staurosporine, however, the enzyme activity was not affected by genistein and Trolox. PMA and OZ promoted tyrosine phosphorylation in neutrophil proteins. TS and staurosporine caused a further increase of tyrosine phosphorylation of proteins in PMA-stimulated neutrophils, whereas, genistein diminished the levels of phosphorylation, and Trolox did not alter them. On the other hand, the four compounds decreased the tyrosine phosphorylated proteins in OZ-stimulated neutrophils. Protein tyrosine phosphatases (PTP) activity was measured in both resting and stimulated cells. PMA and OZ-stimulated neutrophils showed a decrease on PTP activity. Pre-incubation with TS or with Trolox caused partial recovery of the basal activity of stimulated neutrophils. The serine/threonine phosphatase inhibitor, calyculin A, was also utilized, and we showed that this compound was capable of reversing the inhibitory effects of TS on ROS production and PKC activity by neutrophils. These results show that TS modulates both PKC- and TK-dependent signaling pathways associated with the oxidative burst in human neutrophils, and this modulation could be due the activation of phosphatases by TS.
154

O papel de RhoA e Rac1 GTPases nas respostas celulares após danos no DNA induzidos por radiação ionizante gama / The role of RhoA and Rac1 GTPases in cellular responses after DNA damage induced by ionizing gamma radiation

Osaki, Juliana Harumi 18 June 2015 (has links)
O mecanismo pelo qual uma célula responde a algum dano no seu material genético é extremamente importante. Isto ocorre pela rápida ativação da maquinaria de reparo de danos no DNA, a qual é composta por uma rede intrincada de sinalização proteica, culminando no reparo do DNA; porém se o dano for irreparável ocorre ativação de mecanismos de morte celular. RhoA,e Rac1 pertencem a família das pequenas proteínas sinalizadoras Rho GTPases, as quais atuam como interruptores moleculares ciclando entre estado ativo (ligada a GTP) e inativo (ligada a GDP). Os componentes desta família estão relacionados ao controle dos mais diversos processos celulares como, por exemplo, remodelamento do citoesqueleto, migração, adesão, endocitose, progressão do ciclo celular e oncogênese. No entanto, apesar das proteínas Rho GTPases estarem envolvidas em um amplo espectro de atividades biológicas, há poucas informações sobre seu papel na manutenção da integridade genômica quando células são submetidas a algum agente genotóxico. Para investigar o envolvimento das GTPases RhoA e Rac1 nas respostas de células submetidas a radiação gama, foram gerados, a partir de células de carcinoma de cervix humano - HeLa, sublinhagens clonais mutantes de RhoA e Rac1 expressando exogenamente RhoA constitutivamente ativa (HeLa-RhoA V14), RhoA dominante negativa (HeLa-RhoA N19), Rac1 constitutivamente ativa (HeLa-Rac1 V12) e Rac1 dominante negativa (HeLa-Rac N17). Após estas linhagens celulares serem expostas a diferentes doses de radiação gama, observamos que ambas GTPases, RhoA e Rac1, são ativadas em resposta aos efeitos da radiação. Além disso, a modulação da atividade destas enzimas, através das mutações, levou a uma alteração das respostas celulares frente aos danos no DNA, como uma redução da capacidade de reparar quebras simples e duplas nas fitas do DNA. Por outro lado, a deficiência de RhoA ou Rac1 GTPase levou a uma redução da ativação de Chk1 e Chk2 ou da fosforilação da histona H2AX, respectivamente, prejudicando os mecanismos de detecção de danos no DNA e levando as células a permanecerem mais tempo nos pontos de checagem G1/S e/ou G2/M do ciclo celular. Esses fatores contribuíram de modo expressivo para a redução da proliferação e sobrevivência celular levando as células à morte. Por fim, ensaios celulares de reparo de danos de um DNA exógeno através de mecanismos de Recombinação Homóloga (HR) e Recombinação Não-Homóloga de extremidades (NHEJ), demonstraram que a inibição da atividade de RhoA reduz significativamente a eficiência de ambas vias de reparo. Desta maneira, este trabalho demonstra e reforça a existência de mais um viés de atuação das pequenas GTPases RhoA e Rac1, agora em células HeLa, nas respostas celulares aos danos induzidos por exposição a radiação gama, modulando a sobrevivência, proliferação e indiretamente modulando resposta ao reparo do DNA através da via de Recombinação Homóloga e Não-Homóloga / The mechanism by which a cell responds to DNA damage is extremely important. This occurs by a quick activation of the DNA damage repair machinery, which consists of an intricate protein signaling network culminating in DNA repair. But if the damages are irreparable occurs there is activation of cell death mechanisms. RhoA and Rac1 belong to family of small Rho GTPases, signaling proteins that act as molecular switches cycling between the active state (GTP-bound) and inactive state (GDP-bound). Members of this family are implicated in the control of diverse cellular process such as cytoskeletal remodeling, migration, adhesion, endocytosis, cell cycle progression, and oncogenesis. However, despite Rho proteins are involved in a broad spectrum of biological activities, there is just a few information about their roles in the maintenance of genomic integrity, that is, when the cells are subjected to some kinf of genotoxic agent. To investigate the involvement of the GTPases RhoA and Rac1 in cellular responses to gamma radiation, we generated from human cervix carcinoma cells - HeLa, clonal sublines of RhoA and Rac1 mutants, exogenous and stably expressing the constitutively active RhoA (HeLa-RhoA V14), the dominant negative RhoA (HeLa-RhoA N19), the constitutively active Rac1 (HeLa-Rac1 V12) and the dominant negative Rac1 (HeLa-Rac1 N17). After all these cell lines have been exposed to different doses of gamma radiation, we found that both GTPases, RhoA and Rac1, are activated in response to the radiation effects. Furthermore, the modulation of two enzymes activity, by using the mutant clones, led to a change in cellular responses to the DNA damage, as the reduction in the capacity of repairing DNA single and double strand breaksr. On the other hand, the deficiency of RhoA or Rac1 GTPase led to a reduction of Chk1 and Chk2 activation, or on the phosphorylation of histone H2AX, respectively, hindering the mechanisms of DNA damage detection and arresting cells in the G1/S and/or G2/M checkpoints of cell cycle. These factors significantly contributed to the reduction of cell proliferation and survival, leading cells to death. Finally, cellular assays of DNA damage repair of exogenous DNA by Homologous Recombination (HR) and Non-Homologous End Joining (NHEJ), demonstrated that RhoA inhibition significantly reduced the repair efficiency of both pathways. Thus, this work demonstrates and reinforces the existence of other biological functions of small GTPases RhoA and Rac1 in HeLa cells, by regulating cellular responses to DNA damage induced by exposure to gamma radiation, modulating the survival, proliferation and indirectly modulating the response to DNA damage repair pathway through the Homologous Recombination and Non-Homologous Recombination
155

A galectina-3 na fisiologia e no câncer de tiróide: identificação de SNPs no gene LGALS3 e estudo funcional de galectina-3 in vitro e in vivo / Galectin-3 in thyroid physiology and cancer: identification of SNPs in the LGALS3 gene and functional study of galectin-3 in vitro and in vivo.

Martins, Luciane 17 April 2008 (has links)
Neste estudo, investigamos o envolvimento de galectina-3 na fisiologia e no câncer de tiróide usando vários modelos biológicos e metodologias. Observamos que o gene LGALS3 apresenta um SNP no códon 98, mas não observamos correlação entre os genótipos deste SNP e fenótipo de câncer de tiróide. Na linhagem de tiróide de rato PCCl3, mostramos que a indução da expressão do oncogene RET/PTC promove o aumento da expressão de galectina-3, no entanto, a expressão de galectina-3, por si só, não confere vantagem de proliferação à célula. Por outro lado, na linhagem de carcinoma papilífero de tiróide TPC-1, a galectina-3 contribui para a sobrevivência da célula tumoral e progressão do ciclo celular, aumentando a expressão de c-Myc, diminuindo a expressão de p21 e caspase-3, e favorecendo a ativação de importantes vias envolvidas no controle do ciclo celular. Além disto, em modelos in vivo e in vitro, a galectina-3 interferiu na função e diferenciação da célula folicular tiroidiana, exercendo um papel indireto na regulação da expressão da tireoglobulina e atividade de TTF-1. / In this study, we investigate the involvement of galectin-3 in thyroid physiology and cancer using several biological models and methodologies. We observed that LGALS3 gene presents a SNP in codon 98, but no correlation between the genotype and the phenotype of benign or malignant thyroid tumor was observed. In the rat thyroid cell line PCCl3, we showed that the conditional induction of RET/PTC oncogene expression promotes the increase of galectin-3 expression, however, galectin-3 expression itself did not confer a proliferative advantage to cell. On the other hand, in papillary thyroid carcinoma cell line TPC-1 the galectin-3 contributes to tumor cell survival and cell cycle progression, increasing c-Myc expression, decreasing p21 and caspase-3 expression and cooperating to activation of important signaling pathways which are involved in the cell cycle control. In addition, in vitro and in vivo models the galectin-3 interferes in the differentiation and function of thyroid follicular cell, playing an indirect role in the regulation of thyroglobulin expression and TTF-1 activity.
156

Identification du xyloglucane comme nouvel éliciteur oligosaccharidique stimulant l’immunité de Vitis vinifera et d’Arabidopsis thaliana et caractérisation de deux récepteurs aux chito-oligosaccharides chez la vigne (VvLYK1-1 et VvLYK1-2) / Identification of the cell-wall derived xyloglucan as a new damage-associated molecular pattern (DAMP) eliciting plant immunity in Vitis vinifera and Arabidopsis thaliana and characterization of two chito-oligosaccharide pattern recognition receptors

Claverie, Justine 21 December 2018 (has links)
L’activation des réponses immunitaires des plantes repose sur la reconnaissance de motifs moléculaires associés aux pathogènes (aussi appelés PAMP) par des récepteurs de l’immunité, également nommés PRR (pattern recognition receptors). La chitine, principal composant de la paroi des champignons, est un PAMP bien caractérisé qui induit des réponses de défense aussi bien chez les mammifères que chez les plantes.La première partie de cette étude met en évidence que deux chito-oligosaccharides, la chitine et le chitosan, agissent comme des PAMP chez la vigne (Vitis vinifera) puisqu’ils induisent des évènements précoces de signalisation, l’expression de gènes de défense et une résistance contre des agents pathogènes. Ces résultats suggèrent que des systèmes de perception existent chez la vigne. Une analyse phylogénétique a permis d’identifier trois récepteurs kinases à domaine LysM (LysM-RK ou LYK) chez V. vinifera (VvLYK1-1, -2, -3) appartenant au même clade que le récepteur à la chitine chez Arabidopsis et nommé AtCERK1 (Arabidopsis thaliana Chitin Elicitor Receptor Kinase 1). Leur analyse fonctionnelle a été réalisée par complémentation du mutant d’Arabidopsis Atcerk1, affecté dans la perception de la chitine. Nos résultats montrent que VvLYK1-1 et VvLYK1-2, mais pas VvLYK1-3, complémentent fonctionnellement le mutant Atcerk1 en restaurant l’activation des MAPK (Mitogen-Activated Protein Kinases) et l’expression de gènes de défense induits par les chito-oligosaccharides. De plus, l’expression de VvLYK1-1 chez Atcerk1 restaure la résistance basale à l’agent de l’oïdium de la vigne (Erysiphe necator).La seconde partie du projet s’est focalisée sur les éliciteurs oligosaccharidiques de type « damage-associated molecular patterns (DAMP) ». Ces molécules endogènes peuvent provenir de la dégradation de la paroi lors d’une attaque et sont capables d’activer les réponses immunitaires de la plante. Les DAMP les mieux caractérisés actuellement sont les oligogalacturonates (OG), des fragments de pectine qui induisent des réponses immunitaires chez de nombreuses espèces végétales dont l’activation de MAPK, la production d’H2O2, l’expression de gènes de défense et le dépôt de callose. Nous avons montré dans cette étude que les xyloglucanes (Xh), des fragments d’hémicellulose pariétale purifiés, induisaient l’activation de MAPK et l’expression de gènes de défense chez la vigne et Arabidopsis, afin d’induire une résistance contre le champignon nécrotrophe Botrytis cinerea. Les Xh induisent également la production de resvératrol, une phytoalexine majoritaire chez la vigne, et un dépôt de callose chez Arabidopsis. Par une approche génétique, nous avons identifié certains composants de la signalisation induite par les Xh chez Arabidopsis. L’utilisation de mutants suggère que la résistance induite par les Xh contre B. cinerea est dépendante des voies de la camalexine, de l’acide salicylique, de l’acide jasmonique et de l’éthylène chez Arabidopsis. De manière globale, nos résultats mettent en lumière que les xyloglucanes peuvent être considérés comme de nouveaux éliciteurs de l’immunité chez la vigne et Arabidopsis. / Activation of the plant immune responses requires recognition of common pathogen-associated molecular pattern (PAMP) by their cognate pattern recognition receptors (PRR). Chitin, a major component of fungal cell walls, is a well-known PAMP that triggers defense responses in several mammal and plant species.In the first part of this study, we show that two chitooligosaccharides, chitin and chitosan, act as PAMPs in grapevine (Vitis vinifera) as they elicit immune signaling events, defense gene expression, and resistance against pathogens. These two PAMPs are active in grapevine suggesting that at least one perception system exists. Phylogenetic analysis clearly distinguished three V. vinifera LysM Receptor Kinases (VvLYK1-1, -2, -3) located in the same clade as the Arabidopsis Chitin Elicitor Receptor Kinase 1 (AtCERK1), which mediates chitin-induced immune responses. Their functional characterization was achieved by complementation assays in the Atcerk1 mutant, impaired in chitin perception. Our results provide evidence that VvLYK1-1 and VvLYK1-2, but not VvLYK1-3, functionally complement the loss of AtCERK1 function by restoring chitooligosaccharide-induced MAPK activation and immune gene expression. Moreover, expression of VvLYK1-1 in Atcerk1 restored penetration resistance to the non-adapted grapevine powdery mildew (Erysiphe necator).The second part of this study focused on damaged-associated molecular patterns (DAMP), endogenous molecules that can be released from the plant cell wall during an attack and activate the plant innate immunity. Until now, the best characterized DAMPs are oligogalacturonides (OG) coming from pectin fragments that induce innate immune responses in various plant species, including MAPK activation, H2O2 production, defense gene expression and callose deposition. In this study, we showed that purified xyloglucans (Xh), derived from the plant cell wall hemicellulose, elicit MAPK activation and immune gene expression in grapevine (V. vinifera) and Arabidopsis to trigger induced resistance against the necrotrophic fungus Botrytis cinerea. Xh also elicit the production of resveratrol, the main grapevine phytoalexin, and callose deposition in Arabidopsis. Using a genetic approach, we identified some signaling components of Xh-induced immunity. The use of Arabidopsis mutants suggests that Xh-induced resistance against B. cinerea is dependent on the camalexin, salicylate, jasmonate and ethylene pathways. Taken together, our data highlight that Xh can be considered as new elicitors of grapevine and Arabidopsis immunity.
157

Peptídeos RALF em tecido reprodutivo: caracterização e efeito dos AtRALF4, 25, 26 e 34 / RALF peptides in reproductive tissues: characterization and effect of AtRALFs 4, 25, 26 and 34

Bergonci, Tábata 30 August 2016 (has links)
Pequenos peptídeos são importantes sinalizadores celulares e estão envolvidos na comunicação célula-a-célula em diversos aspectos do desenvolvimento da planta. Durante a reprodução sexual, moléculas sinalizadoras atuam na interação entre o gametófito feminino e o masculino, controlando processos como germinação do grão de pólen, alongamento do tubo polínico e liberação das células espermáticas, entre outros. RALF é um peptídeo de sinalização codificado por genes de expressão ubíqua ou tecido-especifica e que regulam negativamente a expansão celular. Em arabidopsis, peptídeos AtRALFs podem ser agrupados em uma família de 39 membros e, interessantemente, os maiores níveis de expressão gênica dessa família são encontrados nos AtRALFs expressos em tecidos reprodutivos. / Small peptides are important cell signaling involved in several aspects of plant development. During sexual reproduction, signaling molecules act in the interaction between female and male gametophyte, controlling processes such as pollen grains germination, pollen tube elongation and sperm cells release. RALF is a signaling peptide ubiquitous or tissuespecific that negatively regulates cell growth. In arabidopsis, AtRALFs peptides can be grouped into a family of 39 members and, interestingly, the highest levels of gene expression of this family are found in AtRALFs expressed in reproductive tissues.
158

Déterminants structuraux et moléculaires de la sélectivité fonctionnelle du récepteur β2-adrénergique

Picard, Louis-Philippe 01 1900 (has links)
No description available.
159

Tetratricopeptide 39C (TTC39C) Is Upregulated During Skeletal Muscle Atrophy and is Necessary for Muscle Cell Differentiation

Hayes, Caleb 01 January 2018 (has links)
Ttc39c has been identified as a novel gene in skeletal muscle that is upregulated in response to neurogenic atrophy in mice. Quantitative PCR and Western blot analysis confirmed that Ttc39c is expressed in both proliferating and differentiated muscle cells. Furthermore, comparison of Ttc39c expression in undifferentiated and differentiated C2C12 cells demonstrated that Ttc39c levels peak in early differentiation, but decreases as cells become fully differentiated myotubes. The transcriptional regulation of Ttc39c was examined by cloning promoter fragments of the gene and fusing it with the SEAP reporter gene. The Ttc39c reporter gene constructs were transfected into muscle cells and confirmed to have significant transcriptional activity in cultured muscle cells and were also found to be transcriptionally repressed in response to ectopic expression of myogenic regulatory factors (MRF). Furthermore, conserved E-box elements in the proximal promoter region were identified, mutated, and analyzed for their role in the transcriptional regulation of Ttc39c expression. Mutation of the conserved E-box sequences reduced the activity of the Ttc39c reporter gene, suggesting that these elements are potentially necessary for full Ttc39c expression. To determine the sub-cellular location of Ttc39c in muscle cells, the Ttc39c cDNA was fused with the green fluorescent protein (GFP), expressed in muscle cells, and visualized by confocal microscopy revealing that Tct39c is localized to the cytoplasm of proliferating myoblasts and differentiating myotubes. Furthermore, Ttc39c appears to localize to the microtubule network and differentiating muscle cells developed elongated primary cilia in response to Ttc39c ectopic expression. Additionally, Ttc39c overexpression resulted in impaired muscle cell differentiation, attenuated Hedgehog and MAP Kinase signaling, and increased expression of IFT144, a component of the intraflagellar transport complex A involved in retrograde movement in primary cilia. Interestingly, Ttc39c knockdown also resulted in abrogated muscle cell differentiation and impaired Hedgehog and MAP Kinase signaling, but did not affect IFT144 expression levels. These results suggest that muscle cell differentiation is sensitive to aberrant Ttc39c expression, that Ttc39c is necessary for proper muscle cell differentiation, and that Ttc39c may participate in retrograde transport of the primary cilia of developing muscle cells.
160

Vliv proteinu HBx viru hepatitidy B na aktivaci MEK1/2-ERK signalizace a inhibici IFN typu I v hepatocelulární linii Huh7 / Effect of HBV protein HBx on activation of MEK1/2 signaling and inhibition of type I IFN in hepatoma cell line Huh7

Berehovska, Olena January 2019 (has links)
Hepatitis B virus (HBV) infection is one of the major causes of chronic and cancerous liver disease. Elimination of HBV from chronically infected patients by recombinant interferon α (IFNα) monotherapy shows that the mechanisms of the innate immunity play an important role in suppressing viral infection. However, the mechanisms of recognition of the HBV genome and its escape from the mechanisms of natural immunity are still little known. One of the principal factors enabling the virus to escape from cellular restriction mechanisms is the HBx viral protein. HBx is a 154 amino acid pleiotropic multifunctional protein affecting transcription, signal transduction, cell cycle, protein degradation, apoptosis, and chromosomal stability in the host cell. Previous results from our laboratory have shown that activation of the MEK1/2-ERK signaling pathway in plasmacytoid dendritic cells leads to inhibition of IFNα production. The aim of my work was to determine whether HBx activates the MEK1/2-ERK pathway and thus inhibits IFN type I production also in hepatocytes. For this purpose, I monitored HBx production in the Huh7 hepatoma cell line by transfecting the bicistronic plasmid pHBx- IRES-EGFP and Western blotting. Using the same method, I monitored activation of the MEK1/2-ERK signaling pathway by ERK...

Page generated in 0.1072 seconds