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Exploration de la diversité de Carnobacterium maltaromaticum en vue d'identifier des souches protectrices anti-Listeria monocytogenes à robustesse élevée / Exploration of the diversity of Carnobactrium maltaromaticum in order to identify highly robust anti-Listeria monocytogenes strainsEl Kheir, Sara 12 December 2016 (has links)
L'industrie alimentaire cherche constamment à améliorer les processus de conservation des aliments. La biopréservation s’impose comme une alternative à l’utilisation de conservateurs dits «chimiques» et fait appel à des micro-organismes sélectionnés en tant que cultures protectrices pour leurs propriétés antimicrobiennes naturels. L'objectif de cette étude était de tirer profit de la diversité de Carnobacterium maltaromaticum afin d’identifier des souches capables d'inhiber la croissance du pathogène alimentaire Listeria monocytogenes. Pour cela, une méthode de typage moléculaire permettant la reconnaissance fine de souches a été établie, puis une méthode de criblage d’activités antibactériennes à robustesse élevée a été mise au point. La méthode de typage moléculaire est une méthode MLVA (Multiple-locus variable-number tandem repeat (VNTR) analysis) avec 3 loci de VNTR (VNTR-A, VNTR-B, VNTR-C) permet de discriminer 15 génotypes différents au sein d’une collection de 24 souches. Cela confirme la grande diversité génotypique et phénotypique présente au sein de la population de C. maltaromaticum et la performance de la méthode. La méthode de criblage est basée sur la réalisation d’essais de compétition à haut débit où chaque membre d’une collection de C. maltaromaticum a été co-cultivé avec une souche bioluminescente de L. monocytogenes. Il a été montré que la production de luminescence est le reflet de la croissance de L. monocytogenes en micro-culture et qu’il est ainsi possible de tester la stabilité du pouvoir antagoniste de chaque membre de la collection dans de multiples conditions de cultures différentes. Cette méthode a ainsi permis d’identifier des souches de C. maltaromaticum dont la propriété anti-L. monocytogenes est peu influencée par les conditions de cultures. Outre l’intérêt fondamental que présente cette méthode pour l’étude des interactions compétitives dans l’aliment, elle a permis d’identifier des souches présentant un fort potentiel de valorisation dans le domaine de la biopréservation alimentaire / The food industry is constantly seeking to improve food preservation processes. Biopreservation imposes itself as an alternative to the use of chemical preservatives and involves micro-organisms selected as protective cultures for their natural antimicrobial properties. The aim of this study was to benefit from the diversity of Carnobacterium maltaromaticum in order to identify strains capable of inhibiting the growth of Listeria monocytogenes, a food-borne pathogen. For this purpose, a molecular typing method that enables fine strain identification has been established, then a method of screening of antibacterial activities with high robustness has been developed. The molecular typing method is a MLVA (Multiple-locus variable-number tandem repeat (VNTR) analysis) with 3 VNTR loci (VNTR-A, VNTR-B, VNTR-C). It allowed to discriminate 15 different genotypes among a collection of 24 C. maltaromaticum strains. These results confirmed the high strain diversity within this species and showed the high performance of this method. The screening method is based on high throughput competition assays where each member of a collection of C. maltaromaticum strains was co-cultivated with a bioluminescent strain of L. monocytogenes. It was established that the bioluminescence of this strains is highly correlated to bacterial growth in micro-cultures, indicating that it is possible to investigate the stability of antagonistic properties of each collection member under multiple different culture conditions. The use of this method allowed to identify C. maltaromaticum strains with bioprotection properties that are poorly influenced by culture conditions. Besides the fundamental interest of this method for investigations of competitive interactions in food, it allowed to identify strains with high potential for bioprotection applications
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Etude de la régulation du système de sécrétion de type 3 et du système de sécrétion de type 6 chez Pseudomonas aeruginosa : Approches de chémogénomique, mutagénèse aléatoire et étude d'isolat clinique / Study of the regulation of the Type III and Type VI Secretion Systems in Pseudomonas aeruginosa : Chemogenomic approaches, random mutagenesis and study of clinical isolate.Sall, Khady 28 November 2013 (has links)
Pseudomonas aeruginosa est un bacille gram négatif, ubiquiste de l'environnement. Ce pathogène opportuniste humain provoque sous sa forme planctonique des infections aiguës dont le facteur de virulence clé est le SST3. P. aeruginosa peut aussi se développer sous forme de biofilm où elle exprime entre autre le SST6-1 et induire des infections chroniques. L'expression ciblée des différents facteurs de virulence est liée à l'intégration de nombreux stimuli environnementaux transduits au moyen de systèmes à deux composants ou encore de messagers secondaires, comme le di-GMPc et l'AMPc, et conduisant à une régulation très fine, conférant une grande capacité d'adaptation à la bactérie. La nature, de même que les mécanismes impliqués dans la transduction du signal, n'ont pas encore été tous identifiés à ce jour. Le but de cette thèse était de décrypter ces mécanismes moléculaires de détection et de transduction du signal gouvernant la réponse adaptative de ce pathogène à son environnement au moyen de différentes approches : chémogénomique, mutagénèse aléatoire et d'étude d'isolat clinique. Lors de cette thèse, nous avons criblé deux chimiothèques commerciales à la recherche de molécules activatrices du SST3 et du SST6-1 et nous avons pu établir un test de criblage à haut débit robuste pour les criblages de plus larges banques de composés. En utilisant une souche avec deux rapporteurs, nous avons réalisé une banque de mutants par transposons et nous avons trouvé des mutants affectés dans leur expression du SST3, candidats intéressants pour identifier de nouveaux régulateurs du système. Enfin, grâce à l'analyse de l'isolat clinique CHA (issu d'un patient atteint de mucoviscidose), nous avons découvert qu'une délétion dans le gène codant pour le régulateur majeur GacS définissait le phénotype agressif de cette souche. / Pseudomonas aeruginosa is a gram negative bacillum present in several places. This opportunistic pathogen has the capacity to infect a wide range of hosts: plants, animals, humans. This bacterium, that shows an impressive adaptability relying on a multifactorial virulence, possesses two lifestyles. These lifestyles are associated with specific virulence patterns of expression. Under its planktonic form, P. aeruginosa can provoke acute infections thanks to the activation of T2 and T3SS or induces chronic infections in cystic fibrosis patients' lungs where it establishes a biofilm (communautary life). The expression of virulence factors is linked to the integration of several environmental cues that are transduced through two-component systems and secondary messengers like c-di-GMP and that lead to a fine tuned regulation. The nature and the mechanisms involved in this signal transduction remain largely unknown. The goal of this thesis was to decipher molecular mechanisms of signal detection and transduction that govern the adaptive pathogen response to host environment using the combination of a chemogenomics, random mutagenesis and study of clinical isolate. During this work, we screened two commercial libraries and set up a robust high throughput screening test to analyse huge molecules libraries. By setting up a double reporter-gene strain, we realized a transposon mutagenesis bank and identified interesting candidates with a down-regulated T3SS. Finally, the study of the particular clinical isolate CHA (from a cystic fibrosis patient), leads to the discovery that a deletion in the gene encoding for the important regulator GacS shapes the aggressive phenotype of this strain.
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Desenho de uma enzima ácido graxo descarboxilase para a produção enzimática de alcenos / Design of a fatty acid decarboxylase for the enzymatic production of alkenesPrause, André Richard, 1984- 10 October 2013 (has links)
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Previous issue date: 2013 / Resumo: Com o aumento da busca por novas fontes renováveis para a substituição do petróleo fóssil como substrato de derivados petroquímicos, as indústrias de plásticos, atualmente um dos ramos mais dependentes da acessibilidade do petróleo, já alcançaram um nível alto de sustentabilidade em linhas de polímeros verdes. Porém, rotas verdes para a obtenção do produto final ainda não foram implantadas industrialmente, sendo que somente precursores dos monômeros desejados são produzidos. A partir desses precursores, o processo é continuado convencionalmente através de operações químicas até a obtenção do monômero. O desenvolvimento de uma rota enzimática para esses monômeros pode ser uma alternativa para os processos praticados na indústria. Enzimas são amplamente utilizadas para a bio-conversão industrial de compostos químicos e a busca por enzimas capazes de catalisar novas reações tem se intensificado, criando uma demanda maior por processos automatizados com aplicação de protocolos de rastreamento de alto desempenho. Para a realização da produção enzimática de alcenos de cadeia curta, uma enzima nativa, apresentando um mecanismo catalítico similar à reação desejada, foi modificada pela aplicação do conceito de "desenho de proteínas", que reúne técnicas de diversificação, recombinação, clonagem, expressão heteróloga e rastreamento, utilizando a "enzima molde" como ponto de partida. A enzima P450BS?, selecionada por apresentar os melhores pré-requisitos para modificações estruturais, foi submetida ao "desenho de proteínas", gerando 5.271 versões mutantes. O rastreamento de alto desempenho automatizado dessas proteínas alteradas, utilizando uma plataforma robótica, possibilitou a obtenção de uma enzima que apresenta a nova ação catalítica da conversão de 100 ?M de ácido octanóico para 2,6 ?M de 1-hepteno. Essa nova enzima abre o caminho para a produção industrial de "bio-alcenos" em micro-organismos, criando um sistema de fermentação que poderia sustentar uma rota verde para os monômeros necessários para a produção de plásticos. / Abstract: With the increased search for renewable resources for substituting fossil petroleum as the raw material for petrochemical products, the plastics industry, currently being one of the branches with the highest dependency on petroleum availability, already reached a high level of sustainability in their green polymer lines. Still, green routes producing the final product have not been implemented industrially and only precursors of the desired are being produced. Using these precursors, the process is continued conventionally, using chemical operations for the production of the monomers. The development of an enzymatic route toward these monomers could be an alternative for current industrial processes. Enzymes are widely used in industrial bioconversion of chemicals and the search for enzymes with the potential of catalyzing new reactions has intensified, creating a higher demand for automatized processes for the application of high-throughput screening protocols. In order to realize the enzymatic production of short-chained alkenes, a native enzyme, presenting a catalytic mechanism similar to the target reaction, was modified, applying the concept of "protein design", which unites diversification, recombination, cloning, heterologous expression and screening techniques, utilizing the "template enzyme" as a starting point. The enzyme P450BS?, selected for possessing the best prerequisites for structural modifications, was submitted to "protein design", creating 5,271 mutant versions. Automatized high-throughput screening of these altered proteins, utilizing a liquid handling platform, enabled the discovery of an enzyme, which presents a new catalytic action: the conversion of 100 ?M butyric acid to 2.6 ?M 1-heptene. This new enzyme opens the way for the industrial production of "bio-alkenes" in microorganisms, creating a fermentation system, which would be able to sustain a green route toward the necessary monomers for the production of plastics. / Doutorado / Bioquimica / Doutor em Biologia Funcional e Molecular
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Vývoj chemických regulátorů drah mikroRNA a RNAi / Vývoj chemických regulátorů drah mikroRNA a RNAiBruštíková, Kateřina January 2015 (has links)
MicroRNAs are noncoding RNAs inducing sequence-specific posttranscriptional inhibition of gene expression and represent the major class of small endogenous RNAs in mammalian cells. Over 2,500 of human microRNAs potentially regulating more than 60% of human protein-coding genes have been identified. MicroRNAs participate in the majority of cellular processes, and their expression changes in various diseases, including cancer. Currently, there is no efficient small chemical compound available for the modulation of microRNA pathway activity. At the same time, small chemical compounds represent excellent tools for research of processes involving RNA silencing pathways, for biotechnological applications, and would have a considerable therapeutic potential. The presented work represents a part of a broader project, whose ultimate goal is: (i) to find a set of small molecules allowing for stimulation or inhibition of RNA silencing and (ii) to identify crosstalks between RNA silencing and other cellular pathways. This thesis summarizes results from the first two phases of the project, the development of high-throughput screening assays and the high- throughput screening (HTS) of available libraries of small compounds. To monitor the microRNA pathway activity, we developed and optimized one biochemical...
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Développement de biosenseurs fluorescents et d’inhibiteurs pour suivre et cibler CDK4/cycline D dans le mélanome / Development of fluorescent biosensors and inhibitors to probe and target CDK4/cyclin D in melanomaPrevel, Camille 11 December 2015 (has links)
Les CDK/cyclines jouent un rôle majeur dans la progression du cycle cellulaire et dans le maintien de la prolifération des cellules cancéreuses, constituant ainsi des biomarqueurs clés et des cibles pharmacologiques attractives. Plus particulièrement, l’activité de CDK4/cycline D, kinase responsable de la progression de la phase G1 et de la transition G1/S, est dérégulée dans de nombreux cancers dont le mélanome. Cette hyperactivation est associée à des mutations, à l’amplification ou à la surexpression de CDK4, cycline D, p16INK4a ou encore pRb.Comme aucune approche sensible et directe n’existe pour évaluer l’activité de CDK4/cycline D dans des conditions physiologiques et pathologiques, le premier objectif de ma thèse a consisté à développer un biosenseur fluorescent permettant d’étudier cette kinase in vitro et in cellulo. Une fois caractérisé et validé in vitro, le biosenseur a été appliqué à la détection d’altérations de CDK4/cycline D dans des biopsies de peau humaine et de xénogreffes de mélanome dans des essais fluorescents d’activité kinase, ainsi que dans des cellules cancéreuses vivantes par microscopie de fluorescence et vidéo microscopie.Par ailleurs, peu d’inhibiteurs sont actuellement disponibles pour inhiber CDK4/cycline D et la plupart d’entre eux ciblent la poche de fixation de l’ATP. C’est pourquoi le second objectif de ma thèse a consisté à identifier des inhibiteurs non compétitifs de l’ATP, soit par élaboration rationnelle de peptides, soit par criblage de petites molécules. A cette fin, deux biosenseurs fluorescents ont été développés qui permettent d’identifier respectivement des composés ciblant l’interface entre CDK4 et cycline D ou des inhibiteurs allostériques capables de perturber la dynamique conformationnelle de CDK4. Des essais de criblage par fluorescence réalisés avec ces biosenseurs ont conduit à l’identification de touches qui ont été validées et caractérisées in vitro et dans des essais de prolifération cellulaire, et qui constituent des candidats prometteurs pour une chimiothérapie sélective du mélanome. / CDK/cyclins play a central role in coordinating cell cycle progression, and in sustaining proliferation of cancer cells, thereby constituting established cancer biomarkers and attractive pharmacological targets. In particular, CDK4/cyclin D, which is responsible for coordinating cell cycle progression through G1 into S phase, is a relevant target in several cancers including melanoma, associated with mutation of CDK4, cyclin D, p16INK4a and pRb.As there are no sensitive and direct approaches to probe CDK4/cyclin D activity in physiological and pathological conditions, the first goal of my thesis has consisted in engineering a fluorescent biosensor to probe this kinase in vitro and in cellulo. Once characterized and validated in vitro, the biosensor was applied to detect CDK4/cyclin D alterations in biopsies from human skin and melanoma xenografts in fluorescence-based activity assays, and in living cancer cells by fluorescence microscopy and timelapse imaging.Moreover, only few inhibitors are currently available to target CDK4/cyclin D and most of them bind the ATP pocket. As such, the second major goal of my thesis project has consisted in identifying non-ATP competitive inhibitors, either through rational design of peptides or by screening small molecule libraries. To this aim, two fluorescent biosensors were engineered which discriminate compounds that target the interface between CDK4 and cyclin D, or that perturb the conformational dynamics of CDK4, respectively, from ATP-pocket binding compounds. Fluorescence-based screening assays performed with these biosensors lead to identification of hits, which were validated and characterized in vitro and in cell proliferation assays, and which constitute promising candidates for selective chemotherapy in melanoma.
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Identification des régulateurs de l’expression transcriptionnelle de TSPAN8 impliqués dans l’invasion précoce du mélanome cutané / Identification of the transcriptional expression regulators of TSPAN8 implicated in the early invasion of cutaneous melanomaAgaësse, Gweltaz 15 December 2016 (has links)
Le mélanome cutané est l’affection de la peau la plus meurtrière. Afin de pouvoir être traité efficacement, ce cancer nécessite un diagnostic et une exérèse chirurgicale précoce des lésions primitives non-invasives. En effet, les patients atteints de métastases ont peu de chance de survivre car les lésions de mélanome développent rapidement des résistances aux thérapies et possèdent une forte propension à disséminer des métastases dans de nombreux organes. Le franchissement de la lame basale de la peau appelée jonction dermo épidermique est la première étape cruciale dans l’invasion précoce du mélanome cutané. Notre équipe étudie cette étape depuis plusieurs années et a démontré que l’expression de la tétraspanine 8 (TSPAN8) apparait lors de la progression de ce cancer et permet l’acquisition d’un phénotype invasif par les cellules tumorales. Plusieurs membres de la famille des protéines tétraspanines sont connus pour leurs implications dans divers cancers, mais notre connaissance de leurs régulations transcriptionnelles est encore assez réduite. Les travaux présentés dans cette thèse ont permis d’identifier les premiers régulateurs transcriptionnels connus de TSPAN8, et également de commencer l’étude fonctionnelle de ces régulations sur l’invasion dépendante de TSPAN8 par le mélanome cutané. En particulier, nous montrons que l’invasion dépendante de TSPAN8 est entre autres régulée par le membre du complexe Mediator LCMR1/MED19 et par le suppresseur de tumeur p53. Ainsi, ces travaux apportent une meilleure compréhension de l’invasion précoce du mélanome cutané, ce qui devrait permettre une meilleure prise en charge des patients à l’avenir / Cutaneous melanoma is the deadliest skin condition. Curing this cancer requires an early diagnosis and surgical excision of the non-invasive primary lesions. Indeed, patients with metastasis have few chances to survive this cancer since the melanoma lesions rapidly develop treatment resistances, and can disseminate metastasis in numerous organs. Crossing the skin basal membrane called the dermal epidermal junction is the first crucial step of early melanoma invasion. Our team has studied the early invasion of melanoma for many years, and demonstrated for the first time the implication of Tetraspanin (TSPAN8) in melanoma early invasion. Indeed, the expression of this gene and the protein that it codes appears with the progression of melanoma and confers the tumor cells an invasive phenotype. Several members of the tetraspanin protein family are known for their implication in various cancers, yet their transcriptional regulation remains poorly understood. In the case of TSPAN8, nothing was known regarding its transcriptional regulation in melanoma. The experiments presented in this thesis allowed us to identify the first known regulators of TSPAN8 transcriptional expression, and also to begin the functional study of the regulators impact on TSPAN8 dependent invasion of human cutaneous melanoma. Amongst these regulators are the member of the Mediator Complex MED19/LCMR1 and the tumor suppressor p53. The results presented in the present manuscript allow a better understanding of cutaneous melanoma early invasion and should help improving the treatments against this cancer in the future
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Réduction catalytique sélective des NOx par les hydrocarbures : approches Haut-Débit et microcinétique expérimentale / Selective catalytic reduction of NOx by hydrocarbons : high throughput screening and experimental microkinetic approachesGravejat, Paul 25 June 2009 (has links)
Le but de cette étude est de trouver un matériau catalytique pour la réduction catalytique sélective des NOx par les hydrocarbures (HC-SCR) dans l’échappement Diesel par une approche haut débit (HTE : high throughput experiments). Ce matériau doit être actif à basse température et stable hydrothermiquement à hautes températures. Une bibliothèque de 150 catalyseurs a été synthétisée. Les catalyseurs sont constituées d’Ag, Au, Cu supportés sur Al2O3, TiO2, ZrO2, CeO2 qui peuvent être dopés (Ga, Mo…). Ceux-ci sont testés en parallèle dans un dispositif constitué de 16 réacteurs (SWITCH-16) au cours réaction à température programmée (TPR) avec un flux modèle (100ppm NO / 350ppm C3H6 / 15% O2 /11% H2O). Le meilleur catalyseur 5%Ag/1%P/Al2O3, testé plus avant, montre une température de light-off de 50°C en dessous de celle d’un catalyseur commercial de référence et celui-ci est stable après un vieillissement de 16h à 750°C en présence d’eau. Ce catalyseur est ensuite enduit par voie sol-gel sur un monolithe (1*2 pouces et 300 cpsi) et testé sur un mini-pilote. Les tendances obtenues en réacteur à lit fixe montés en parallèle sont confirmées sur mini-pilote. En parallèle une approche microcinétique expérimentale des étapes élémentaires de surface impliquées dans la HC-SCR du NO sur un catalyseur Ag/Al2O3 a été utilisée pour déterminer les étapes élémentaires contrôlant la conversion du NO en prenant en compte l’adsorption compétitive entre NO et CO présent dans le gaz d’échappement Diesel. Nous avons identifié l’élimination des espèces Oads adsorbées sur des sites Ag° comme étape limitante pour la production de N2 et suggéré une nouvelle orientation possible pour l’étude HTE. / The aim of this study was to discover a catalytic material for NOx reduction by HC-SCR in Diesel exhaust which is active at the lowest temperatures and hydro thermally stable at high temperatures by using High Throughtput experiments (HTE). A library of 150 catalysts was synthesized. Catalysts are supported Ag, Au, Cu on Al2O3, TiO2, ZrO2, CeO2 and further doped with different dopants (Ga, Mo, …). They were tested in a 16-parallel reactor (SWITCH-16) using a Temperature Program Reaction (TPR) protocol with a model feed (100ppm NO / 350ppm C3H6 / 15% O2 /11% H2O). The best catalyst formulation 5%Ag/1%P/Al2O3, which was further improved, exhibits a light off temperature of 50°C lower than a reference commercial catalyst and is stable after ageing at 750°C in presence of water for 16 hrs. For pilot testing, the best catalyst was deposited by sol-gel method on a 1x2 inch monolith (300 cpsi). We showed the consistency of catalytic results obtained in the parallel fixed beds match with monolith bench testing. In parallel a experimental microkinetic approach of surface elementary steps involved in the HC-SCR of NO on Ag/Al2O3 catalyst has been performed to reveal the elementary steps controlling the conversion of the NO reactant taking into account the competitive chemisorption between NO and CO that is present in an exhaust gas. We identified the elimination of Oads species adsorbed on Ag° sites as the limiting step for the N2 production and suggested a new orientation of a HTE study.
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Rift Valley fever : consequences of virus-host interactionsBaudin, Maria January 2016 (has links)
Rift Valley fever virus (RVFV) is a mosquito-borne virus which has the ability to infect a large variety of animals including humans in Africa and Arabian Peninsula. The abortion rate among these animals are close to 100%, and young animals develop severe disease which often are lethal. In humans, Rift Valley fever (RVF) presents in most cases as a mild illness with influenza-like symptoms. However, in about 8% of the cases it progresses into a more severe disease with a high case fatality rate. Since there is such a high abortion rate among infected animals, a link between human miscarriage and RVFV has been suggested, but never proven. We could in paper I for the first time show an association between acute RVFV infection and miscarriage in humans. We observed an increase in pregnant women arriving at the Port Sudan Hospital with fever of unknown origin, and several of the patients experienced miscarriage. When we analysed their blood samples for several viral diseases we found that many had an acute RVFV infection and of these, 54% experienced a miscarriage. The odds of having a miscarriage was 7 times higher for RVFV patients compared to the RVFV negative women of which only 12% miscarried. These results indicated that RVFV infection could be a contributing factor to miscarriage. RVFV is an enveloped virus containing the viral glycoproteins n and c (Gn and Gc respectively), where Gn most likely is responsible for the initial cellular contact. The protein DC-SIGN on dendritic cells and the glycosaminoglycan heparan sulfate has been suggested as cellular receptors for RVFV, however other mechanisms are probably also involved in binding and entry. Charge is a driving force for molecular interaction and has been shown to be important for cellular attachment of several viruses, and in paper II we could show that when the charge around the cells was altered, the infection was affected. We also showed that Gn most likely has a positive charge at a physiological pH. When we added negatively charged molecules to the viral particles before infection, we observed a decreased infection efficiency, which we also observed after removal of carbohydrate structures from the cell surface. Our results suggested that the cellular interaction partner for initial attachment is a negatively charged carbohydrate. Further investigations into the mechanisms of RVFV cellular interactions has to be undertaken in order to understand, and ultimately prevent, infection and disease. There is currently no vaccine approved for human use and no specific treatments for RVF, so there is a great need for developing safe effective drugs targeting this virus. We designed a whole-cell based high-throughput screen (HTS) assay which we used to screen libraries of small molecular compounds for anti-RVFV properties. After dose-response and toxicity analysis of the initial hits, we identified six safe and effective inhibitors of RVFV infection that with further testing could become drug candidates for treatment of RVF. This study demonstrated the application of HTS using a whole-cell virus replication reporter gene assay as an effective method to identify novel compounds with potential antiviral activity against RVFV.
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Triagem de enzimas associadas à biotransformação de hidrocarbonetos a partir de metagenoma de sedimentos contaminados com petroléo e metais pesados / Screening of Enzymes Related to Biotransformation of Hydrocarbons from Metagenome of Contaminated Sediments with Oil and Heavy MetalsTiago Henrique Nogueira Simões 08 July 2009 (has links)
A metagenômica trouxe novas perspectivas ao estudo de comunidades microbianas no ambiente, permitindo explorar tanto a diversidade taxonômica de microrganismos ainda não-cultivados, como o acesso direto a genes e vias metabólicas. Neste trabalho, foram construídas bibliotecas metagenômicas a partir de amostras de sedimentos de mangue da Baía de Guanabara (RJ), impactadas com hidrocarbonetos de petróleo e metais pesados. Proteobacteria (33,3%), bactérias afiliadas a redutoras-de-sulfato (29,7%) e Firmicutes (20%) representaram os grupos principais nas amostras ambientais, baseado em análises filogenéticas de rDNA 16S, ao passo que isolamentos seletivos utilizando diesel e naftaleno permitiram a recuperação preferencial de delta-Proteobacteria e actinomicetos. Bibliotecas metagenômicas dos sedimentos enriquecidos com óleo diesel, com insertos entre 25 e 35 Kb clonados em fosmídeos, foram triadas para detecção de genes catabólicos de monoxigenases (alkB1) e expressão de epóxido-hidrolases, esterases, lipases e monoxigenases em ensaios de alto desempenho (HTS, high throughput screening). Clones reativos a alkB1 foram detectados, porém não foram funcionais nas condições de HTS testadas. Nas bibliotecas de fosmídeos triadas, vários clones apresentaram atividade enzimática, sendo que dois apresentaram atividade de lipase-esterase com alta seletividade, elevada taxa de conversão de substratos e excesso enantiomérico (ee >99%). Os resultados de HTS comprovaram a eficiência do uso da clonagem direta de DNA ambiental na expressão de vias metabólicas de interesse com potencial de aplicação biotecnológica. / Metagenomics brought a new perspective to the study of microbial communities in the environment, enabling access to the taxonomic diversity of uncultured microorganisms, as well as direct access to genes and metabolic pathways. In the current study, metagenomic libraries were constructed from mangrove sediment samples of the Guanabara Bay (RJ, Brazil), impacted with oil hydrocarbons and heavy metals. Proteobacteria (33.3%), sulfate-reducing affiliated bacteria (29.7%) and Firmicutes (20%) represented the main groups in the environmental samples based upon 16S rDNA phylogenetic analysis, whereas selective isolation using diesel and naphtalene yielded delta-Proteobacteria and actinomycetes. Metagenomic libraries of diesel-enriched sediment samples, with 25 to 35 Kb fosmid inserts, were screened for detecting monooxigenase genes (alkB1) and expression of epoxide hydrolases, esterases, lipases and monooxigenases in high throughput screening (HTS) assays. Clones reactive to the alkB1 probe were detected, but were not functional under the HTS conditions used. Several functional clones were detected in the clone library, and two showed lipase-esterase activity with high rates of substrate conversion and enantiomeric ratio (ee >99%). The results obtained on HTS showed the efficiency of the direct cloning of environmental DNA for the expression of metabolic pathways with potential biotechnological application.
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Vývoj instrumentace a metod s vysokou propustností pro hledání a validaci peptidových ligandů / Development of instrumentation and high-throughput screening methods for peptide ligand discovery and validationKryštůfek, Robin January 2021 (has links)
Peptides are used as synthetically available and easily derivatizable scaffold upon which it is possible to develop ligands targeting broad spectrum of biological targets. A time-tested approach to peptide binder identification is the preparation and screening of combinatorial libraries. Bypassing of this complicated procedure is possible by using biological systems for presentation, identification and selection of peptides based on the principle of in vitro evolution - i.e. display techniques. There are two complementary automated solutions for peptide binder identification described in this work. First is the SPENSER parallel peptide synthesizer, developed as a part of this diploma project, which can be used for peptide ligand discovery and optimization as well as validation of ligands identified using display techniques. Several libraries consisting of a total of 1 052 peptides have been prepared and then used to describe its potential applications. A sample of 154 preparations, representing 14.6 % analytical coverage of the prepared libraries, showed an average purity of 67 ± 19 % according to LC-MS. The libraries presented illustrate that SPENSER is a suitable tool for the parallel synthesis of linear and disulfide-cyclized peptides with limited variability, or libraries consisting of short...
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