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Development of a Novel Pck-1: eGFP Reporter Zebrafish Line for the Discovery and Evaluation of Potential Anti-Diabetic DrugsHui, Wing 27 November 2013 (has links)
Overexpression of Phosphoenolpyruvate carboxykinase - cytosolic (PEPCK, encoded by Pck-1 gene) has been found to be associated with the prevalence of hyperglycemia in Type 2 Diabetes Mellitus (T2DM) patients. The Pck-1 enzyme catalyzes the rate limiting step in endogenous glucose production. The aims of this study are to develop a Pck-1:eGFP reporter zebrafish and validate it as a potential tool for the screening of novel anti-diabetic compounds. 3.6 kb zebrafish Pck-1 promoter fragment was cloned and a Pck-1:eGFP expression vector was constructed. After DNA microinjection, we generated Pck-1:eGFP reporter zebrafish with strong eGFP expression in developing liver. Validation studies confirmed that Pck-1:eGFP zebrafish embryos responded to treatment of glucose, cAMP and dexamethasone, metformin and rosiglitazone similarly to that of humans. This novel Pck-1:eGFP reporter fish line can serve as a tool for the screening and development of novel anti-diabetic drugs that may have potential in the treatment of T2DM.
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Interaction of hepatic uptake transporters with antineoplastic compounds and regulation of the expression of organic cation transporter 3 in renal carcinoma cellsMarada, Venkata 15 January 2015 (has links)
No description available.
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Cumulative Distribution Networks: Inference, Estimation and Applications of Graphical Models for Cumulative Distribution FunctionsHuang, Jim C. 01 March 2010 (has links)
This thesis presents a class of graphical models for directly representing the joint cumulative distribution function (CDF) of many random variables, called cumulative distribution networks (CDNs). Unlike graphical models for probability density and mass functions, in a CDN, the marginal probabilities for any subset of variables are obtained by computing limits of functions in the model. We will show that the conditional independence properties in a CDN are distinct from the conditional independence properties of directed, undirected and factor graph models, but include the conditional independence properties of bidirected graphical models. As a result, CDNs are a parameterization for bidirected models that allows us to represent complex statistical dependence relationships between observable variables. We will provide a method for constructing a factor graph model with additional latent variables for which graph separation of variables in the corresponding CDN implies conditional independence of the separated variables in both the CDN and in the factor graph with the latent variables marginalized out. This will then allow us to construct multivariate extreme value distributions for which both a CDN and a corresponding factor graph representation exist.
In order to perform inference in such graphs, we describe the `derivative-sum-product' (DSP) message-passing algorithm where messages correspond to derivatives of the joint cumulative distribution function. We will then apply CDNs to the problem of learning to rank, or estimating parametric models for ranking, where CDNs provide a natural means with which to model multivariate probabilities over ordinal variables such as pairwise preferences. We will show that many previous probability models for rank data, such as the Bradley-Terry and Plackett-Luce models, can be viewed as particular types of CDN. Applications of CDNs will be described for the problems of ranking players in multiplayer team-based games, document retrieval and discovering regulatory sequences in computational biology using the above methods for inference and estimation of CDNs.
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Elucidating the Functions of the Sialylation Pathway in Drosophila melanogasterCarnahan, Mindy 2011 August 1900 (has links)
Sialylation is an important carbohydrate modification of glycoconjugates, which introduces sialic acids (SA). The relatively large nine-carbon, negatively charged sugars are typically located at the termini of carbohydrate chains. SA's are often required for functionally important molecular and cellular interactions including virus-host interactions, tumor progression and malignancy, immune system development and function, and nervous system development and function. However, the study of sialylation in vertebrates, including man, encounters serious obstacles associated with the complexity of vertebrates' biology and limitations of available experimental approaches. Drosophila is a useful model system with many advantages including quick generation time, a large number of progeny, simplified glycosylation and neurophysiology, and ease of genetic manipulations. The primary focus of this thesis is on the functions of Drosophila melanogaster CMP sialic acid synthetase (DmCSAS) and sialyltransferase (DSiaT) in the central nervous system (CNS).
A combination of genetic, immunostaining, and neurobiology approaches were used to characterize the functions of DmCSAS and DSiaT in Drosophila. This investigation revealed the expression of DmCSAS and suggested that it plays an important role in a specialized and developmentally regulated process in the nervous system of Drosophila. Further experiments examined sub-cellular localization of DmCSAS revealing that this protein has a complex mostly Golgi-associated distribution within the cell in vivo. I discovered a novel link between Drosophila sialylation and circadian rhythm regulation. I also characterized the electrophysiological phenotypes of DmCSAS mutants and compared them to the corresponding defects associated with DSiaT mutations. My experiments also revealed that the relationship between DmCSAS and DSiaT are more complex than originally thought; these genes may have independent functions while also participating in the same pathway. Taken together, these results elucidate the sialylation pathway in Drosophila and shed more light on the role of sialylation in the nervous system. My experiments provide a unique evolutionary perspective on the sialylation pathway in animals and suggest that the neural function of SA in Drosophila can be conserved in vertebrates, including humans.
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Contribution et régulation de PRR2, un facteur de transcription spécifique aux plantes, dans l'immunité végétale / Contribution and regulation of PRR2, a plant specific transcription factor, in plant immunityPerez, Manon 19 September 2017 (has links)
La capacité des plantes à répondre aux stress de l'environnement, qu'ils soient de nature biotique ou abiotique, tient au fait qu'elles sont capables d'intégrer les signaux perçus grâce à des mécanismes de transduction du signal rapides et efficaces. La perception, le décodage et la mise en place de réponses biologiques adaptées font appel à de nombreux acteurs moléculaires tels que le calcium (Ca2+), second messager majeur de la signalisation Eucaryote. Parmi les "senseurs de calcium", la calmoduline (CaM) est la protéine la plus connue. Il existe des protéines apparentées à la CaM, spécifiques aux plantes, les Calmodulin-like (CMLs). Les CMLs sont très peu étudiées et la caractérisation de leurs rôles ouvre de larges perspectives sur l'identification des réseaux de régulation. L'objectif de ce travail de thèse a concerné un partenaire nucléaire d'une de ces CMLs, AtCML9, le Pseudo-Response Regulator 2 (PRR2), une protéine atypique contenant un domaine de liaison à l'ADN de type GARP et de fonction inconnue. Au cours de ce travail, des analyses moléculaires et biochimiques ont permis de caractériser le rôle de PRR2 dans l'immunité végétale, et en particulier en réponse à Pseudomonas syringae. L'étude de lignées perte ou gain de fonction a permis de mettre en évidence que PRR2 agit comme un régulateur positif des défenses lors de l'infection par la bactérie pathogène hémibiotrophe Pst DC3000 à travers la modulation de l'acide salicylique, de composés de défense tels que la protéine PR1 et la camalexine. Les analyses phénotypiques réalisées en réponse à différentes souches de Pseudomonas ont permis de préciser que PRR2 contribue à la mise en place des défenses à travers la signalisation dépendante de l'acide salicylique et de l'injection des effecteurs bactériens. Dans une deuxième partie, l'interaction entre PRR2 et des facteurs de transcription spécifiques aux plantes, les TCPs (Teosinte Branched 1, Cycloidea and PCF), a été étudié. Ces analyses ont montré une spécificité d'interaction entre PRR2 et TCP19 ou TCP20. Ces interactions stabilisent et relocalisent PRR2 dans des domaines nucléaires spécifiques. Ces données suggèrent une forte régulation post-traductionnelle de la protéine PRR2 qui pourrait s'avérer nécessaire à sa fonction biologique. / Plants are able to perceive and respond to diverse biotic or abiotic environmental cues. This ability relies on efficient signalling pathways that are ultimately associated with genetic reprograming. These responses involve various actors of the signalling pathways such as calcium (Ca2+) transients which act as a second messenger in eukaryotic cells. The variations in intracellular Ca2+ concentrations are perceived by calcium sensors. The calmodulin (CaM) is an ubiquitous Ca2+ sensor well studied both in animal and plant cells. Comparatively, plants also possess CaM-related proteins called Calmodulin-like (CMLs) which are less studied and their role in plant physiology are emerging. The objective of this PhD work was to perform the functional analysis of PRR2 (Pseudo-Response Regulator 2), a plant specific transcription factor (with a GARP DNA binding domain) previously identified as an AtCML9-interacting partner. Using diverse genetic tools, we were able to study the role of PRR2 in plant immunity using the model plant Arabidopsis thaliana and a phytopathogenic bacteria, Pseudomonas syringae. Our study has shown that PRR2 acts as a positive regulator of plant defenses upon bacterial infection. We show that PRR2 could act by modulating the biosynthesis of the salicylic acid (SA), and the production of defense-associated compounds such as PR1 and camalexin. Collectively our data indicate that PRR2 acts as a positive regulator of plant defense associated with SA. In the aim to better understand how PRR2 could be involved in different physiological responses, we search for PRR2-interacting partners. We have more precisely worked on the interactions between PRR2 and the TCPs (Teosinte branched 1, Cycloidea and PCF) which are also plant specific transcriptions factors involved in different biological processes. We showed that PRR2 specifically interact with TCP19 or TCP20. As consequences, these interactions stabilize PRR2 and relocalize the complex in specific nuclear subdomains.
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Régulation transcriptionnelle du facteur de transcription spécifique des bâtonnets, Nrl / Transcriptional regulation of the rod-specific transcription factor, NrlKautzmann, Marie audrey 12 June 2012 (has links)
La leucine zipper de la rétine neurale (Nrl) joue un rôle central dans le développement et l'homéostasie des bâtonnets en activant I'expression de gènes tels que le photopigment Rhodopsine. Nrl est aussi associé à la Rétinite Pigmentaire, faisant ainsi de ce gène un modèle intéressant pour la compréhension des programmes contrôlant le développement et I'homéostasie des photorécepteurs.Ce travail de thèse vise à caractériser les mécanismes régulateurs de I'expression de Nr/ au cours du développement rétinien. L'électroporation in vivo de vecteurs rapporteurs dans des rétines de souris en développement, a révélé des séquences minimales de promoteur Nr/ nécessaires à une expression spécifique dans les photorécepteurs. Nous avons identifié RORI3 comme facteur requis pour cette expression, et montré que les facteurs OTX2, CRX et CREB s'accrochent aussi directement à des régions régulatrices particulières du promoteur. Nous avons construit un virus adéno-associé (AAV) contenant un promoteur minimal Nrl de 0.3 kb, et montré qu'il est adapté à la délivrance de gène spécifiquement dans les photorécepteurs.Nous avons montré que NRL, CRX et NR2E3, les régulateurs principaux de la Rhodopsine, ont une expression rythmique au cours de 24 h, et que l'expression cyclique de Nr/ peut être due à l'activation par RORp, un composant l'horloge circadienne. Enfin, nous avons identifié un nouveau facteur de transcription, NonO, au niveau de la région du promoteur proximal de la Rhodopsine, qui en combinaison avec NRL et CRX, active le promoteur de la Rhodopsine. L'invalidation de NonO au cours du développement rétinien a prouvé son implication pour le développement et I'homéostasie des bâtonnets. / The Neural Retina Leucine zipper transcription factor (Nrl) plays a central role in rod photoreceptor development and homeostasis, by activating the expression of rod-specific genes such as the visual photopigment, Rhodopsin. Nrlhave been also associated with Retinitis Pigmentosa, making this gene an interesting model for understanding genetic programs controlling photoreceptors development and homeostasis.This thesis work aimed at characterizing regulatory mechanisms of Nr/ expression during retinal development. Using in vivo electroporation of reporter vectors carrying distinct portions of Nrlpromoter into neonatal mouse retina, we identified minimal sequences required for expression photoreceptors-specific expression. We identified RORI3 as being required for this expression and showed that OTX2, CRX and CREB transcription factors also directly bind to the defined regulatory regions.We designed a novel adeno-associated virus (AAV) vector containing a minimal Nrl promoter fragment of 0.3 kb, and showed that it is well-suited for gene delivery specifically into photoreceptors.We also showed that NRL, CRX, and NR2E3, the main transcriptional regulators of Rhodopsin, display rhythmic expression over 24 h. and that Nrl might undergo cyclic activation by RORB which is part of the photoreceptor circadian clock. Finally, we investigated the role of a novel Rhodopsin transcriptional regulator, NonO, identified in theRhodopsin proximal promoter region. We demonstrated that NonO co-activates Rhodopsin promoter along with NRL and CRX. By knocking down this gene during retinal development we provided evidence for its role in rod development and homeostasis.
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Estudo da regulação da expressão do gene da proteína prion celular / Cellular prion protein gene expression regulationAna Lucia Beirão Cabral 26 July 2001 (has links)
A conversão da proteína prion celular normal (PrPc), cuja função ainda esta sob investigação, para a forma infecciosa (PrPsc) é a causa de algumas doenças neurodegenerativas em humanos e animais. Vários estudos têm sido realizados e mostram que PrPc pode participar de processos normais como memória, estresse oxidativo, neuritogênese e outros. Portanto, a elucidação dos processos de regulação de sua expressão é importante tanto para definir uma estratégia para controlar a infecção quanto para entender melhor a função fisiológica de PrPc. Este trabalho tem por objetivo avaliar a expressão do gene de PrPc, a partir da regulação da atividade de seu promotor frente a drogas que foram eleitas de acordo com a composição dos elementos de resposta a fatores de transcrição nele contidos. Para isto o promotor foi clonado em um vetor contendo o gene \"reporter\" de luciferase, células C6 e PC-12 foram transfectadas e clones com expressão estável de luciferase foram selecionados. Os resultados dos tratamentos dos clones celulares mostram que éster de forbol (TPA) e AMPc induzem a atividade do promotor de 1,5 a 3 vezes, ácido retinóico (RA) diminui esta atividade em cerca de 50% enquanto que NGF e Dexametasona não têm efeito. A dependência da conformação da cromatina na regulação deste gene também foi testada utilizando-se Tricostatina A (TSA), esta droga foi capaz de aumentar de 10 a 4.000 vezes a atividade do promotor, o que foi seguida tanto pela indução de expressão do RNAm quanto da proteína PrPc. Este efeito parece não ser generalizado a todos os promotores uma vez que esta droga não alterou expressão de GAPDH e de β-actina. Quando TPA e AMPc foram associados à TSA uma potencialização do efeito indutor destas drogas foi observada e a associação de RA e TSA mostrou que RA reduz a indução gerada por TSA. Estes novos dados indicam que a regulação de PrPc é extremamente dependente da conformação da cromatina. / Conversion of the cellular normal prion protein (PrPc), whose physiological function is still under investigation, to an infectious form called prion is the cause of some neurodegenerative diseases. Therefore, the elucidation of PrPc gene regulation is important both to define a strategy to control the infection and to better understand PrPc function. We cloned the rat PrPc gene promoter region into a luciferase reporter vector, transfected C6 and PC-12 cells and isolated clones with stable luciferase expression. The phorbol ester TPA and cAMP induced promoter activity by 1.5 to 3 times, retinoic acid decreased it by 50% while NGF and dexamethasone had no effect. We also tested the dependence of chromatin conformation for PrPc promoter activity using Trichostatin A (TSA), which was able to highly increase not only promoter activity but also PrPc rnRNA and protein leveIs. Moreover, the TSA effect seems to be restricted since any alteration was observed regarding GAPDH (Glyiceraldehyde 3-phosphate desydrogenase) and β-actin expression. When cAMP, TPA or retinoic acid were associated with TSA a potentiation of their primary effects was observed. These new data indicate that PrPc gene regulation is highly dependent on disruption of chromatin fiber assembly what permits assess of trascription factors.
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Regulação molecular da expressão atrial - específica do gene SMyHC3. / Molecular regulation of atrial-specific expression of the SMyHC3 gene.Allysson Coelho Sampaio 02 June 2010 (has links)
Para elucidar as vias genéticas controlando a formação das câmaras cardíacas, foi analisada a regulação do promotor atrial-específico do gene de codorna que codifica a isoforma lenta da cadeia pesada de miosina (slow myosin heavy chain 3 -SMyHC3). Em camundongos transgênicos, a expressão atrial-específica dos 840 pb do promotor SMyHC3 fundido ao gene repórter da fosfatase alcalina (HAP), SMyHC3-HAP, é controlada pelos 72 pb mais distais deste promotor. Este fragmento contém sítios putativos para ligação a receptores nucleares os quais foram denominados ECRRN (elemento complexo de resposta a receptores nucleares), definidos por modelagem molecular. Tratamento de embriões SMyHC3-HAP com ácido retinoico (AR) expande o domínio atrial de expressão do transgene, enquanto que a inibição da via de sinalização por AR reduz o domínio de expressão do transgene. Ensaios de gel shift revelam que os receptores de AR, RAR/RXR se ligam fracamente a esse promotor. Também, esses receptores não ativam o promotor SMyHC3 em experimentos de transfecção transiente, mesmo na presença de coativadores, tais como p300, CBP e GRIP1. Isso sugere a participação indireta de AR na regulação deste marcador atrial. Ensaios de transfecção celular demonstram que COUPTF2 é capaz de ativar o promotor SMyHC3 e, siRNA contra COUPTF2 inibe esta transativação. Embriões tratados com AR apresentam um aumento geral da expressão de COUPTF2, reforçando a idéia de que AR age indiretamente ativando este gene. Estudos de bioinformática revelam que o ECRRN está presente na região 3 do gene AMHC1 de galinha e alinhamentos indicam que pode se tratar de um elemento móvel que pode ter sido adquirido por um evento de exaptação. Em resumo, COUPTF2 e AR controlam a expressão do promotor SMyHC3, porém a natureza da relação entre os 2 elementos necessita ser elucidada. / To elucidate the genetic pathways controlling cardiac chamber formation, the atrial specific gene promoter SMyHC3 was analyzed. In transgenic mice, the atrial specific expression an 840 bp of the SMyHC3 promoter was linked to reporter gene human alkaline phosphatase (HAP), SMyHC3-HAP. By directed mutagenesis and deletion analysis we identified the more distal 72 bp of the promoter as responsible of the atrial expression. This fragment contains putative binding sites to nuclear receptors, the CNRRE (complex nuclear receptor response element), defined by molecular modeling. RA (retinoic acid) treatment in SMyHC3-HAP embryos expands the atrial domain. However, the RA effectors, RXR/RAR bind with low affinity to the SMyHC3 promoter. These receptors are not able to activate the promoter even in the presence of coactivators such as p300, CBP and GRIP1. These results suggest that RA acts indirectly to regulate this atrial marker. Cell transient transfection shows that COUPTF2 activate the SMyHC3 promoter, and COUPTF2 siRNA inhibits the transactivation of the SMyHC3 promoter. Treatment of embryos with RA increases the COUPTF2 expression reinforcing the idea that this receptor could be regulatedindirectly by RA. Bioinformatic studies revealed that CNRRE is present in the 3 region of the ortholog chicken AMHC1 gene. Alignments indicate that this CNRRE could have been acquired by an exaptation event. In conclusion, the SMyHC3 promoter seems to be controlled by RA and COUPTF2 governing atrial expression. However the nature of relationships between RA and COUPTF2 need to be elucidated.
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Caracterização funcional de fatores de transcrição da família MarR de Chromobacterium violaceum / Functional characterization of MarR family transcription factors in Chromobacterium violaceumMaristela Previato Mello 13 June 2018 (has links)
Os fatores de transcrição da família MarR atuam como sensores diretos de sinais intracelulares e regulam vários processos em bactérias, incluindo virulência e degradação de compostos aromáticos. Neste trabalho, identificamos de modo global os fatores de transcrição da família MarR envolvidos na virulência do patógeno oportunista de humanos Chromobacterium violaceum. Usando mutagênese por troca alélica, geramos mutantes nulos não polares para doze dos quinze reguladores da família MarR encontrados no genoma de C. violaceum. Em ensaios de virulência, quando injetados por via intraperitoneal em camundongos BALB/c, os mutantes ?CV_0210 (?ohrR), ?CV_0577 e ?CV_2726 foram menos virulentos, enquanto o mutante ?CV_1776 foi mais virulento, quando comparados à linhagem selvagem. Para os demais nove mutantes MarR não houve diferença na virulência. Para definir o regulon de alguns destes reguladores da família MarR, os perfis de expressão gênica foram determinados por ensaios de microarranjo de DNA e Northern blot para as linhagens mutantes ?CV_0210 (?ohrR), ?CV_1776, ?CV_1810 e ?CV_2726, para a linhagem selvagem superexpressando CV_2726 e para a linhagem selvagem em estresse oxidativo com hidroperóxido de cumeno (CHP). O regulon do repressor CV_1810 compreendeu dois operons divergentes, que codificam enzimas que possivelmente metabolizam compostos aromáticos, mas produtos do catabolismo destes compostos não funcionaram como ligantes capazes de antagonizar a repressão de CV_1810 no gene CV_1801. O regulon do ativador CV_2726, definido como quatorze genes comuns diferencialmente expressos em ensaios na ausência e na condição de superexpressão do gene CV_2726, revelou poucos genes (cstA) com potencial de estar envolvidos no fenótipo de menor virulência do mutante ?CV_2726. Os reguladores CV_0577 e CV_1776 foram alocados na subfamília UrtR de resposta a urato e provavelmente influenciam a virulência de C. violaceum com regulons sobrepostos. O regulon de CV_1776 abrangeu dezenas de genes, muitos deles relacionados ao catabolismo de aminoácidos, mas há poucos candidatos a fatores de 10 virulência clássicos (pecM, escU). Alguns genes do catabolismo/utilização de purinas (CV_0578 e CV_3771) foram regulados tanto por CV_1776 quanto por CV_0577 e responderam a presença de urato. O perfil transcricional da resposta adaptativa de C. violaceum a CHP, um ligante que oxida o regulador OhrR, revelou aumento na expressão de genes relacionados à detoxificação de peróxidos (enzimas antioxidantes e sistemas redutores de tiol), degradação da porção aromática do CHP (oxigenases) e proteção contra estresses secundários (reparo de DNA, choque térmico, limitação de ferro e nitrogênio). O regulon de OhrR revelou-se pequeno, incluindo dois genes com expressão aumentada, CV_0209 (ohrA) e CV_0208 (possível diguanilato ciclase), e três genes com expressão diminuída (hemolisina, quitinase e colagenase) no mutante ?ohrR. Assim, a virulência atenuada do mutante ?ohrR deve estar relacionada ao aumento da produção do segundo mensageiro cíclico di-GMP (c-diGMP) e à diminuição da expressão de enzimas degradativas extracelulares. Em conclusão, definimos a resposta transcricional à CHP, identificamos potenciais fatores de virulência, como a diguanilato ciclase, no regulon OhrR, e mostramos que C. violaceum utiliza os fatores de transcrição da família MarR CV_0577, CV_1776, CV_2726 e OhrR para modular sua virulência. / Transcription factors belonging to the MarR family act as direct intracellular sensors of signals and control many processes in bacteria, including virulence and degradation of aromatic compounds. In this work, we identify and characterize MarR family transcription factors controlling virulence in Chromobacterium violaceum, an opportunistic pathogen of humans. Using allelic exchange mutagenesis, we generate non-polar null mutants for twelve of the fifteen MarR family regulators found in the C. violaceum genome. In virulence tests, when introduced by intraperitoneal injection in BALB/c mice, the ?CV_0210 (?ohrR), ?CV_0577 and ?CV_2726 mutant strains were less virulent, while the ?CV_1776 was more virulent, when compared to the wild-type strain. The other nine MarR mutants showed no difference in virulence tests. To define the regulon of some MarR family transcription factors, the gene expression profiles were determined by DNA microarray analysis and Northern blot assays for the ?CV_0210 (?ohrR), ?CV_1776, ?CV_1810 and ?CV_2726 mutant strains, for the wild-type strain overexpressing CV_2726 and for the wild-type strain exposed to oxidative stress generated by cumene hydroperoxide (CHP). The CV_1810 is a repressor of a regulon that comprised two divergent operons encoding enzymes that possibly metabolize aromatic compounds, but catabolic products of these compounds did not function as ligands capable of antagonizing the repression of CV_1810 on the CV_1801 gene. The regulon of the activator CV_2726, defined as fourteen differentially expressed genes commonly found in assays in the absence and overexpression of the CV_2726 gene, revealed few genes (cstA) with potential to be involved in the phenotype of lower virulence of the ?CV_2726 mutant strain. Regulators CV_0577 and CV_1776 were allocated in the urate-responsive UrtR subfamily and probably afect the virulence of C. violaceum with overlapping regulons. The CV_1776 regulon contains dozens of genes, many of them related to amino acid catabolism, but there are few candidates for classical virulence factors (pecM, escU). Some genes related to catabolism/utilization of purine (CV_0578 and CV_3771) were 12 regulated by both CV_1776 and CV_0577 and responded to the presence of urate. The transcriptional profile of the adaptive response of C. violaceum to CHP, a ligand that oxidizes the OhrR regulator, revealed the upregulation of genes related to the detoxification of peroxides (antioxidant enzymes and thiol-reducing systems), degradation of the aromatic moiety of CHP (oxygenases), and protection against other secondary stresses (DNA repair, heat shock, iron limitation, and nitrogen starvation responses). The OhrR regulon was shown to be small, including two upregulated genes, CV_0209 (ohrA) and CV_0208 (putative diguanylate cyclase), and three downregulated genes (hemolysin, chitinase, and collagenase) in the ?ohrR mutant. Thus, the attenuated virulence of the ?ohrR mutant might be related to the increased production of the second messenger cyclic di-GMP (c-di-GMP) and the decreased expression of extracellular enzymes required for tissue dissemination, in this mutant strain. In conclusion, we have defined the transcriptional response to CHP, identified potential virulence factors such as diguanylate cyclase as members of the OhrR regulon, and shown that C. violaceum uses the transcription factors of the MarR family CV_0577, CV_1776, CV_2726 and OhrR to modulate its virulence.
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Expressão gênica diferencial durante a esporulação de Blastocladiella emersonii e estudo da sinalização por GMP cíclico / Differential gene expression during Blastocladiella emersonii sporulation and analysis of the cyclic GMP signaling pathwayAndré Luiz Gomes Vieira 24 April 2009 (has links)
Neste trabalho realizamos a análise das variações na expressão gênica global durante a fase de esporulação do fungo aquático Blastocladiella emersonii utilizando a tecnologia dos microarranjos de cDNA em lâminas contendo 3.773 genes distintos. Ao todo 615 genes foram classificados como induzidos enquanto 645 foram classificados como reprimidos ao longo da esporulação. As categorias funcionais mais representadas entre os genes induzidos foram: microtúbulo e citoesqueleto, transmissão de sinal, atividade de ligação ao íon Ca2+, proteólise (apenas no início da esporulação) e biogênese e organização do cromossomo (apenas no final da esporulação). Dentre os genes reprimidos, as categorias funcionais mais representadas foram: biossíntese de proteína, transporte de carboidratos e metabolismo energético. A comparação dos dados de expressão gênica da esporulação com aqueles obtidos recentemente em nosso laboratório para a germinação mostrou um grande número de genes regulados inversamente ao longo das duas fases de diferenciação do ciclo de vida de B. emersonii. Muitos genes induzidos na esporulação são reprimidos na germinação e vice versa. Analisamos também o efeito de glicose e triptofano sobre a expressão gênica durante a formação dos zoósporos, tendo em vista que tais nutrientes são capazes de inibir a esporulação de B. emersonii. Nossos resultados mostraram que na presença de glicose (1%) genes envolvidos na composição e atividade do citoesqueleto foram superexpressos, enquanto na presença do aminoácido triptofano houve um aumento na expressão de genes envolvidos no processo de enovelamento de proteínas e proteólise, e na resposta ao estresse oxidativo. Além disso, genes envolvidos no processo de esporulação propriamente dito foram reprimidos durante o tratamento com triptofano. Investigamos também a via de sinalização por GMP cíclico (cGMP), cujos níveis aumentam consideravelmente durante a esporulação de B. emersonii. Iniciamos o estudo com uma busca no banco de ESTs de B. emersonii (http://blasto.iq.usp.br) por seqüências que codificassem enzimas envolvidas na síntese e degradação de cGMP. Foram encontradas três ESTs que codificam domínios catalíticos que parecem pertencer a três diferentes guanilato ciclases e uma EST codificando uma fosfodiesterase com alta similaridade com fosfodiesterases que possuem alta afinidade por cGMP. Experimentos de microarranjos de cDNA validados por RT-PCR quantitativo em tempo real mostraram que os quatro transcritos são expressos durante esporulação, com picos de indução durante a fase tardia da esporulação, momento em que ocorre a biogênese dos zoósporos. Além disso, dados obtidos a partir de experimentos in vivo e in vitro utilizando inibidores das enzimas guanilato ciclase e óxido nítrico sintase, sugeriram a participação do íon Ca2+ e do radical livre óxido nítrico (•NO) na atividade de guanilato ciclase, em uma via do tipo Ca2+-•NO-cGMP. / In the present work, we analyzed global gene expression changes during the sporulation phase of the aquatic fungus Blastocladiella emersonii using cDNA microarray technology with chips containing 3773 distinct genes. A total of 615 genes were upregulated and 645 were down-regulated along the sporulation of the fungus. The overrepresented functional categories among the induced genes were: microtubule and cytoskeleton, signal transduction, Ca2+ binding activity, proteolysis (only at the beginning of sporulation), and chromosome biogenesis and organization (only at the end of sporulation). Among the down-regulated genes, the over-represented functional categories were: protein biosynthesis, carbohydrate transport, and energetic metabolism. Sporulation gene expression data were compared with those obtained recently in our laboratory for the germination phase, showing that a great number of genes are inversely regulated along the two differentiation stages of B. emersonii life cycle. We also analyzed the effects of glucose and tryptophan on gene expression during biogenesis of the zoospores, as such nutrients are able to inhibit B. emersonii sporulation. Our results showed that in the presence of glucose (1%) genes related to activity and composition of cytoskeleton were over-expressed, while in the presence of tryptophan genes involved in protein folding, proteolysis and oxidative stress were induced. In addition, genes involved in the sporulation process per se were downregulated by tryptophan treatment. We also investigated the cyclic GMP signaling pathway, as the levels of this cyclic nucleotide increase considerably during B. emersonii sporulation. Firstly, we searched for sequences encoding enzymes involved in cGMP synthesis and degradation using the B. emersonii EST databank (http://blasto.iq.usp.br). Three sequences were found encoding distinct guanylate cyclase catalytic domains, and one showed high similarity with phosphodiesterases that exhibit high affinity for cGMP. Microarray experiments, validated by real time quantitative RT-PCR, showed that the four transcripts are induced during sporulation, reaching maximum levels at the late stages of sporulation, when zoospore biogenesis occurs. In addition, data obtained from in vivo and in vitro experiments using inhibitors for the enzymes guanylate cyclase and nitric oxide synthase indicated the involvement of the ion Ca2+ and the free radical nitric oxide (•NO) in guanylate cyclase activity, suggesting the existence of a Ca2+-• NO-cGMP signaling pathway.
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