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Novel methods for improving rapid paper-based protein assays with gold nanoparticle detectionLama, Lara January 2017 (has links)
This thesis describes methods for improving sensitivity in rapid singleplex and multiplex microarray assays. The assays utilize the optical characteristics of colloidal gold nanoparticles for the colorimetric detection of proteins. Multiplexed detection in sandwich immunoassays is limited by cross-reactivity between different detection antibodies. The cross-reactivity between antibodies can contribute to increased background noise - decreasing the Limit-of-Detection of the assay - or generate false positive signals. Paper I shows improved assay sensitivity in a multiplexed vertical flow assay by the application of ultrasonic energy to the gold nanoparticles functionalized with detection antibodies. The ultrasonication of the antibody conjugated gold nanoparticles resulted in a 10 000 fold increase in sensitivity in a 3-plex assay. COMSOL Multiphysics was used to simulate the acoustical energy of the probe used in Paper I for obtaining an indication of the size and direction of the forces acting upon the functionalized gold nanoparticles. In Paper II, it was studied if different gold nanoparticle conjugation methods and colorimetric signal enhancement of the gold nanoparticle conjugates could influence the sensitivity of a paper-based lateral flow microarray assay, targeting cardiac troponin T for the rapid diagnostics of acute myocardial infarction. Ultrasonication and signal enhancement of the detection gold nanoparticles has the potential of improving the sensitivity of paper based assays and expanding their potential future applications. / <p>QC 20170911</p>
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Study of substrate modulation and bioreceptor anchoring for the development of high performance microarraysJiménez Meneses, Pilar 28 February 2020 (has links)
Tesis por compendio / [EN] The present PhD thesis is focused on the study of new approaches able to improve the performance of microarrays. Aspects such as the nature of the surfaces and the probes, functionalization of the substrates, probe printing, immobilization and target detection were considered in the fabrication process. Within all these features, modulation of the surface behavior and probe anchoring were the most challenging aspects, as the interface is key for the immobilization of the receptors and the later detection, which will determine the performance of the final device.
In this work, two microarray types have been developed, one for oligonucleotides and another one for antibodies. Then, a characterization of the reached achievements is done. All the routes have in common the use of light to catalyze the attachment of bioreceptors on the surface substrates, employing click-chemistry reactions.
In the first chapter, the state of the art of microarray technology is overviewed, with special focus in the main aspects of microarray design.
In the second chapter, the goals for this PhD thesis are settled. These general objectives are addressed in the following experimental chapters.
In the third chapter, the effect of hydrophobicity and probe multi-point attachment on the microarray performance are studied. Thus, modulation of glass slide surfaces with alkenyl and alkynyl motifs for the anchoring of mono and multithiolated oligonucleotide probes by thiol-ene and thiol-yne photocoupling reactions, respectively, was accomplished. Surfaces modified with the most hydrophobic silane (alkynyl), or anchoring polythiolated probes, revealed better performances. These microarray systems were applied to the discrimination of SNPs and to detect bacterial genome PCR products.
In the fourth chapter, a rational design for the preparation of microarrays of antibodies, is done. The immobilization approach displays the oriented anchoring of thiol-bearing antibody fragments to alkenylated glass slides by thiol-ene photocoupling reaction. Multiplexed detection of cardiac biomarkers is demonstrated. The designed microarray shows higher recognition capacity in comparison to whole antibody microarrays.
In the fifth chapter, improvement of a novel methodology for the anchoring of thiolated oligonucleotides has been developed. Due to the interest on modifying highly hydrophobic surfaces, a new photoinduced reaction is set up. Thanks to the features of the named "fluor-thiol photocoupling reaction", immobilization of thiolated probes to surfaces containing C-F bonds in a fast, easy and biocompatible with aqueous media way, was achieved. Hydrophobicity of the surfaces was controlled to get successful hybridizations. Because of the high hydrophobicity of the surfaces, a huge confinement of the probes is accomplished, which allows the approximation of the analytes only where the probe is linked, keeping a high repulsion in the remaining surface. The perfluorinated glass slides improved the immobilization densities and detection capacity, regarding to the alkenylated and alkynylated surfaces, and allowed the discrimination of SNPs and detection of bacterial PCR products, as well.
In the sixth chapter, other surfaces different than glass are explored. Thus, polyvinylidene fluoride membranes were employed as substrates for the development of oligonucleotide microarrays. Therefore, a fast, easy and mild functionalization process by UV irradiation and organosilane chemistry, was developed. Then, alkenyl functionalized and non-functionalized membranes were applied to microarray technology by covalent anchoring through thiol-ene and fluor-thiol photocoupling reactions, respectively. Promising results were obtained with both surfaces. / [ES] La presente tesis tesis doctoral se centra en el estudio de nuevas aproximaciones capaces de mejorar el rendimiento de los microarrays. Aspectos como la naturaleza de las superficies y las sondas, la funcionalización de los sustratos, la impresión, la inmovilización y la detección de las sondas se consideraron en el proceso de fabricación. Dentro de todas estas características, la modulación de la superficie y el anclaje de la sonda fueron los aspectos más desafiantes, ya que la interfaz es clave para la inmovilización de los receptores y la posterior detección, lo que determinará el rendimiento del dispositivo final.
En este trabajo, se han desarrollado dos tipos de microarrays, uno para oligonucleótidos y otro para anticuerpos. Luego, se ha realizado una caracterización de los logros alcanzados. Todas las rutas tienen en común el uso de la luz para catalizar la unión de los biorreceptores en los sustratos de la superficie, empleando reacciones de la química clic.
En el primer capítulo, se facilita una visión general del estado del arte de la tecnología de microarrays con un enfoque especial en los aspectos principales del diseño de microarrays.
En el segundo capítulo, se establecen los objetivos de esta tesis doctoral. Estos objetivos generales se abordan en los siguientes capítulos experimentales.
En el tercer capítulo, se estudia el efecto de la hidrofobia y el uso de sondas con múltiples puntos de unión, en el rendimiento del microarray. De este modo, se llevó a cabo la modulación de superficies vidrio con grupos alquenilo y alquinilo para el anclaje de sondas de oligonucleótidos mono y multitioladas mediante las reacciones de foto anclaje del tiol-eno y tiol-ino, respectivamente. Las superficies modificadas con el silano más hidrofóbico (alquinilo) y las sondas politioladas ancladas, revelaron mejores rendimientos. Estos sistemas de microarrays se aplicaron a la discriminación de SNPs y a la detección de productos de PCR de bacterias.
En el cuarto capítulo, se realiza un diseño racional para la preparación de microarrays de anticuerpos. El enfoque de inmovilización muestra el anclaje orientado de los fragmentos de anticuerpos que contienen tiol sobre superficies de vidrio alqueniladas mediante reacción de foto anclaje del tiol-eno. De esta forma, se demuestra la detección multiplexada de biomarcadores cardíacos. El microarray diseñado muestra una mayor capacidad de reconocimiento en comparación con los microarrays de anticuerpos completos.
En el quinto capítulo, se ha desarrollado una nueva metodología para mejorar el anclaje de oligonucleótidos tiolados. Dado el interés en modificar superficies altamente hidrófobas, se establece una nueva reacción fotoinducida. Gracias a las características de la llamada "reacción de fotoacoplamiento de fluor-tiol", se logró la inmovilización de sondas tioladas a superficies que contienen enlaces C-F de una manera rápida, fácil y biocompatible con medios acuosos. La hidrofobicidad de las superficies se controló para obtener hibridaciones exitosas. Debido a la alta hidrofobicidad de las superficies, se logra un gran confinamiento de las sondas, lo que permite la aproximación de los analitos solo donde está unida la sonda, manteniendo una alta repulsión en la superficie restante. Las superficies de vidrio perfluoradas mejoraron las densidades de inmovilización y la capacidad de detección, con respecto a las superficies alqueniladas y alquiniladas, y también, permitieron la discriminación de SNPs y la detección de productos de PCR bacterianos.
En el sexto capítulo, se exploran otras superficies diferentes al vidrio. Por lo tanto, membranas de fluoruro de polivinilideno se emplearon como sustratos para el desarrollo de microarrays de oligonucleótidos. Para ello, se desarrolló un proceso de funcionalización rápido, fácil y suave, mediante el empleo de irradiación UV y la química de los organosilanos. / [CA] La present tesi doctoral es centra en l'estudi de noves aproximacions capaces de millorar el rendiment dels microarrays. Aspectes com ara la naturalesa de les superfícies i les sondes, la funcionalització dels substrats, la impressió, la immobilització i la detecció de les sondes es van considerar en el procés de fabricació. Dins de totes aquestes característiques, la modulació de la superfície i l'ancoratge de la sonda van ser els aspectes més desafiadors, ja que la interfície és clau per a la immobilització dels receptors i la posterior detecció, la qual cosa determinarà el rendiment del dispositiu final.
En aquest treball, s'han desenvolupat dos tipus de microarrays, un per a oligonucleòtids i un altre per a anticossos. Després, s'ha realitzat una caracterització dels resultats aconseguits. Totes les rutes tenen en comú l'ús de la llum per a catalitzar la unió dels biorreceptores en els substrats de la superfície, emprant reaccions de la química clic.
En el primer capítol, es facilita una visió general de l'estat de l'art de la tecnologia de microarrays amb un enfocament especial en els aspectes principals del disseny de microarrays.
En el segon capítol, s'estableixen els objectius d'aquesta tesi doctoral. Aquests objectius generals s'aborden en els següents capítols experimentals.
En el tercer capítol, s'estudia l'efecte de la hidrofòbia i l'ús de sondes amb múltiples punts d'unió, en el rendiment del microarray. D'aquesta manera, es va dur a terme la modulació de superfícies de vidre amb grups alquenil i alquinil per a l'ancoratge de sondes de oligonucleòtids mono i multitiolades mitjançant les reaccions de foto ancoratge del tiol-doble enllaç i tiol-triple enllaç, respectivament. Les superfícies modificades amb el silà més hidrofòbic (alquinil) i les sondes politiolades ancorades, van revelar els millors rendiments. Aquests sistemes de microarrays es van aplicar a la discriminació de SNPs i a la detecció de productes de PCR de bacteris.
En el quart capítol, es realitza un disseny racional per a la preparació de microarrays d'anticossos. L'enfocament d'immobilització mostra l'ancoratge orientat dels fragments d'anticossos que contenen el grup tiol sobre superfícies de vidre alquenilades mitjançant reacció de foto ancoratge del tiol-doble enllaç. D'aquesta forma, es demostra la detecció multiplexada de biomarcadors cardíacs. El microarray dissenyat mostra una major capacitat de reconeixement en comparació amb els microarrays d'anticossos complets.
En el cinqué capítol, s'ha desenvolupat una nova metodologia per a millorar l'ancoratge de oligonucleòtids tiolats. Donat l'interés de modificar superfícies altament hidròfobes, s'estableix una nova reacció fotoinduïda. Gràcies a les característiques de l'anomenada "reacció de fotoacoplament de fluor-tiol", es va aconseguir la immobilització de sondes tioladas a superfícies que contenen enllaços C-F d'una manera ràpida, fàcil i biocompatible amb medis aquosos. La hidrofobicitat de les superfícies es va controlar per a obtindre bones hibridacions reeixides. A causa de l'alta hidrofobicidad de les superfícies, s'aconsegueix un gran confinament de les sondes, la qual cosa permet l'aproximació dels anàlits únicament on està unida la sonda i manté una alta repulsió en la superfície restant. Les superfícies de vidre perfluorades van millorar les densitats d'immobilització i la capacitat de detecció, respecte a les superfícies alquenilades i alquinilades, i també van permetre la discriminació de SNPs i la detecció de productes de PCR bacterians.
En el sisé capítol, s'exploren altres superfícies diferents al vidre. Per tant, membranes de fluorur de polivinilidé es van emprar com a substrats per al desenvolupament de microarrays d'oligonucleòtids. Per a això, es va desenvolupar un procés de funcionalització ràpid, fàcil i suau, mitjançant l'ús d'irradiació UV i la química dels organosilan / Agradecer al Ministerio de Economía y Competitividad de España, por su programa de
becas doctorales FPI / Jiménez Meneses, P. (2020). Study of substrate modulation and bioreceptor anchoring for the development of high performance microarrays [Tesis doctoral]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/137993 / Compendio
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Process Fingerprinting of Microneedle Manufacturing Using Conventional and Ultrasonic Micro-injection MouldingGulcur, Mert January 2019 (has links)
This research work investigates the development and application of process
fingerprinting for conventional micro-injection moulding and ultrasonic micro injection moulding manufacturing of microneedle arrays for drug delivery.
The process fingerprinting method covers in-depth analysis, interrogation
and selection of certain process data features and correlation of these
features with product fingerprints which are defined by the geometrical
outcomes of the microneedle arrays in micro scale. The method was
developed using the data collected using extensive sensor technologies
attached to the conventional and ultrasonic micromoulding machines.
Moreover, a machine vision based microneedle product evaluation apparatus
is presented. Micromachining capabilities of different processes is also
assessed and presented where state-of-the-art laser machining was used for
microneedle tool manufacturing in the work.
By using process fingerprinting procedures, conventional and ultrasonic
micromoulding processes has been characterised thoroughly and aspects of
the process that is affecting the part quality was also addressed for
microneedle manufacturing. It was found that polymer structure is of
paramount importance in obtaining sufficient microneedle replication. An
amorphous polymer have been found to be more suitable for conventional
moulding whereas semi-crystalline materials performed better in ultrasonic
micromoulding. In-line captured micromoulding process data for conventional and ultrasonic moulding provided detailed insight of machine dynamics and
understanding. Linear correlations between process fingerprints and micro replication efficiency of the microneedles have been presented for both micromoulding technologies. The in-line process monitoring and product quality evaluation procedures presented in this work for micro-injection
moulding techniques will pave ways for zero-defect micromanufacturing of
miniature products towards Industry 4.0.
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META-ANALYSIS OF GENE EXPRESSION STUDIESSiangphoe, Umaporn 01 January 2015 (has links)
Combining effect sizes from individual studies using random-effects models are commonly applied in high-dimensional gene expression data. However, unknown study heterogeneity can arise from inconsistency of sample qualities and experimental conditions. High heterogeneity of effect sizes can reduce statistical power of the models. We proposed two new methods for random effects estimation and measurements for model variation and strength of the study heterogeneity. We then developed a statistical technique to test for significance of random effects and identify heterogeneous genes. We also proposed another meta-analytic approach that incorporates informative weights in the random effects meta-analysis models. We compared the proposed methods with the standard and existing meta-analytic techniques in the classical and Bayesian frameworks. We demonstrate our results through a series of simulations and application in gene expression neurodegenerative diseases.
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Identification de transcrits modulés par ETV6 : un gène candidat suppresseur de tumeurBoily, Gino January 2005 (has links)
Thèse numérisée par la Direction des bibliothèques de l'Université de Montréal.
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Technologische Bewertung von Peptid-Mikroarrays als Methode der serologischen DiagnostikLück, Juliane 27 March 2012 (has links)
Die humorale Immunantwort eines Organismus auf ein Pathogen äußert sich in einer Veränderung des Antikörperrepertoires. Eine quantitative Untersuchung dieses Prozesses erfordert aufgrund der enormen Komplexität des Immunsystems, die Verwendung von Hochdurchsatztechniken, wie Peptid-Mikroarrays. Bisher gibt es nur wenige Studien, die die Verlässlichkeit von Mikroarray-Bindungsmessungen untersuchen. In dieser Arbeit werden Bewertungskriterien für die Qualität von Antikörper-Peptid-Bindungsstudien unter Verwendung der Peptid-Mikroarraytechnologie herausgearbeitet, mit dem Ziel, diese Hochdurchsatzmethode für qualitative und quantitative Antikörper-Peptid-Bindungsmessungen zu optimieren. Anhand eines Modellsystems, das aus dem monoklonalen anti-p24 (HIV-1) Antikörper CB4-1 und 26 verschiedenen Peptiden, die mit unterschiedlicher Affinität an CB4-1 binden, besteht, werden systematisch die Bindungsdissoziationskonstanten der jeweiligen Antikörper-Peptid-Komplexe mit den durch Peptid-Mikroarray-Bindungsmessungen erhaltenen Signalintensitäten verglichen. Darüber hinaus wird in dieser Arbeit die Messung von Serumantikörperbindungsprofilen gegenüber Zufallspeptidbibliotheken als Methode der serologischen Diagnostik verwendet. Anhand dreier Beispieldatensätze wird die serologische Diagnose von Infektionskrankheiten, Autoimmunkrankheiten und von Krebs mittels Zufallspeptid-Mikroarrays demonstriert. Mithilfe von Merkmalsselektion werden Peptide selektiert, die besonders geeignet sind, um zwischen gesunden und kranken Individuen zu unterscheiden. Besondere Bedeutung wird der Untersuchung der Robustheit der Methode gegenüber schwankenden experimentellen Bedingungen beigemessen. Die vorliegende Arbeit gibt Aufschluss über vorhandene Probleme der Mikroarray-Technologie, stellt Lösungsansätze vor und arbeitet bedeutende Weiterentwicklungen auf dem Weg hin zu einer minimal-invasiven serologischen Diagnostik heraus, die kein a priori Wissen über Antigene voraussetzt. / The humoral immune response to a pathogen is associated with specific changes in the antibody repertoire. Because of the enormous complexity of the immune system, a quantitative determination of this process requires high-throughput measuring tools, such as the peptide microarray technology. There are only few reports that determine the technological reliability of peptide microarray studies. By using a model system, composed of the anti-p24 (HIV-1) monoclonal antibody CB4-1 and an array of 26 different peptides for which the CB4-1 binding affinity has independently been measured, the dissociation constants of antibody-peptide complexes are systematically compared with obtained signal intensities. The assignment of serum-antibody binding profiles using random peptide microarrays for the purpose of serological diagnostics constitutes a major part of this work. By means of three sample data sets, the ability of random peptide microarrays to serve as method of serological diagnosing infectious diseases, autoimmune diseases and cancer is demonstrated. By means of feature selection, the peptides that are exceptionally appropriate to discriminate between the investigated groups are identified. This study attaches special importance to the reliability and robustness of extracted microarray data. This thesis indicates present problems of the peptide microarray technology and presents further developments on the way to minimal-invasive serological diagnostics that do not require any a priori knowledge about antigens, and thus about the investigated diseases.
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Planejamento, gerenciamento e análise de dados de microarranjos de DNA para identificação de biomarcadores de diagnóstico e prognóstico de cânceres humanos / Planning, management and analysis of DNA microarray data aiming at discovery of biomarkers for diagnosis and prognosis of human cancers.Simões, Ana Carolina Quirino 12 May 2009 (has links)
Nesta tese, apresentamos nossas estratégias para desenvolver um ambiente matemático e computacional para análises em larga-escala de dados de expressão gênica obtidos pela tecnologia de microarranjos de DNA. As análises realizadas visaram principalmente à identificação de marcadores moleculares de diagnóstico e prognóstico de cânceres humanos. Apresentamos o resultado de diversas análises implementadas através do ambiente desenvolvido, as quais conduziram a implementação de uma ferramenta computacional para a anotação automática de plataformas de microarranjos de DNA e de outra ferramenta destinada ao rastreamento da análise de dados realizada em ambiente R. Programação eXtrema (eXtreme Programming, XP) foi utilizada como técnica de planejamento e gerenciamento dos projetos de análise dados de expressão gênica. Todos os conjuntos de dados foram obtidos por nossos colaboradores, utilizando-se duas diferentes plataformas de microarranjos de DNA: a primeira enriquecida em regiões não-codificantes do genoma humano, em particular regiões intrônicas, e a segunda representando regiões exônicas de genes humanos. A primeira plataforma foi utilizada para avaliação do perfil de expressão gênica em tumores de próstata e rim humanos, sendo que análises utilizando SAM (Significance Analysis of Microarrays) permitiram a proposição de um conjunto de 49 sequências como potenciais biomarcadores de prognóstico de tumores de próstata. A segunda plataforma foi utilizada para avaliação do perfil de transcritos expressos em sarcomas, carcinomas epidermóide e carcinomas epidermóides de cabeça e pescoço. As análises com sarcomas permitiram a identificação de um conjunto de 12 genes relacionados à agressividade local e metástase. As análises com carcinomas epidermóides de cabeça e pescoço permitiram a identificação de 7 genes relacionados à metástase linfonodal. / In this PhD Thesis, we present our strategies to the development of a mathematical and computational environment aiming the analysis of large-scale microarray datasets. The analyses focused mainly on the identification of molecular markers for diagnosis and prognosis of human cancers. Here we show the results of several analyses implemented using this environment, which led to the development of a computational tool for automatic annotation of DNA microarray platforms and a tool for tracking the analysis within R environment. We also applied eXtreme Programming (XP) as a tool for planning and management of gene expression analyses projects. All data sets were obtained by our collaborators using two different microarray platforms. The first is enriched in non-coding human sequences, particularly intronic sequences. The second one represents exonic regions of human genes. Using the first platform, we evaluated gene expression profiles of prostate and kidney human tumors. Applying SAM to prostate tumor data revealed 49 potential molecular markers for prognosis of this disease. Gene expression in samples of sarcomas, epidermoid carcinomas and head and neck epidermoid carcinomas was investigated using the second platform. A set of 12 genes were identified as potential biomarkers for local aggressiveness and metastasis in sarcoma. In addition, the analyses of data obtained from head and neck epidermoid carcinomas allowed the identification of 7 potential biomarkers for lymph-nodal metastases.
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Análise da expressão de RNAs intrônicos não-codificadores em carcinomas de célula renal / Expression analysis of intronic noncoding RNAs in renal cell carcinomasBrito, Glauber da Costa de 26 November 2007 (has links)
O carcinoma de célula renal (CCR) subtipo célula clara é o câncer mais letal e prevalente do sistema urinário. A transformação maligna no CCR está possivelmente associada à mudanças no perfil de expressão de oncogenes e genes supressores de tumor, e acredita-se que estas alterações sejam críticas para o desenvolvimento do fenótipo maligno. Para identificar novos genes e vias moleculares associadas à transformação maligna no CCR célula clara, foram analisados perfis de expressão gênica de amostras pareadas de tumor e tecido não tumoral adjacente de 6 pacientes. Foi utilizada uma plataforma de microarrays de cDNA contendo 2.292 sondas mapeando éxons de genes codificadores e 822 sondas de RNAs não-codificadores mapeando em regiões intrônicas. A transcrição intrônica foi detectada em todos os tecidos normais e neoplásicos. Utilizando uma combinação de dois testes estatísticos e uma validação por leave-one-out, foi selecionado um subconjunto de 64 transcritos com expressão significativamente alterada em CCR célula clara em relação ao tecido não tumoral adjacente, estando a maior parte (86%) com expressão diminuída em CCR. Entre os transcritos com expressão diminuída, 49 mapearam em regiões não-traduzidas ou éxons de genes codificadores e 6 mapearam em regiões intrônicas de genes codificadores conhecidos. Os níveis de expressão diminuída de SIN3B, TRIP3, SYNJ2BP e NDE1 (p < 0,02), e de transcritos intrônicos derivados dos loci de SND1 e ACTN4 (p < 0,05), foram confirmados em CCR célula clara por Real-time RT-PCR. Um subconjunto de 25 transcritos se mostrou alterado em 6 amostras adicionais de CCR não célula clara, indicando alterações transcricionais comuns em CCR independentemente do subtipo histológico ou do estado de diferenciação do tumor. Além disso, foi analisado o perfil de metilação dos genes com expressão diminuída em tumor SIN3B, TRIP3, SYNJ2BP e GPX3. Nossos resultados indicam um novo conjunto de candidatos a gene supressor de tumor, que 8 podem desempenhar um papel importante na transformação maligna de células renais normais. / The clear cell subtype of renal cell carcinoma (RCC) is the most lethal and prevalent cancer of the urinary system. The carcinogenesis in RCC is thought to be associated with changes in the expression of several genes, and this alteration in gene expression is believed to be critical to the development of the malignant phenotype. To investigate new genes and molecular pathways associated with malignant transformation in clear cell RCC, gene expression profiles of matched samples of tumor and adjacent non-neoplastic tissue obtained from 6 patients were analysed. A custom-built cDNA microarray platform was used, comprising 2,292 probes that map to exons of genes and 822 probes for noncoding RNAs mapping to intronic regions. Intronic transcription was detected in all normal and neoplastic renal tissues. A subset of 64 transcripts with levels significantly deregulated in clear cell RCC relative to the matched non-tumor tissue, mostly (86%) downregulated in CCR, was
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Regulação da expressão gênica pela toxina da aranha Phoneutria nigriventer no corpo cavernoso in vivo / In vivo regulation of gene expression in the corpus cavernosum by the Phoneutria nigriventer toxinVillanova, Fabiola Elizabeth 04 September 2009 (has links)
INTRODUÇÃO: O aracnídeo Phoneutria nigriventer, também conhecido por aranha-armadeira, possui um veneno complexo, contendo vários peptídeos que ativam canais iônicos nas células. Dentre estes, só dois neuropeptídeos, Tx2-5 e Tx2-6, destacam-se por relaxar o músculo liso trabecular do corpo cavernoso, induzindo ereção peniana em camundongos e ratos. Este efeito tem sido associado à produção de oxido nítrico pela ativação de óxido nítrico sintases. No entanto, faltam estudos mais amplos para determinar o papel de Tx2-6 na indução da ereção. OBJETIVOS: Identificar os genes diferencialmente expressos no tecido erétil de camundongos após indução da ereção pela Tx2-6 utilizando microarranjos de oligonucleotídeos. Validação dos resultados obtidos nos microarranjos por PCR quantitativa e imuno-histoquímica. MATERIAIS E MÉTODOS: Camundongos machos e adultos da linhagem Swiss foram divididos em dois grupos: controle (n=10), inoculados pela via intracavernosa com 20 l de solução salina; e tratado (n=10), os quais receberam 0,006gg/animal do peptídeo Tx2-6 diluído em 20 l de salina pela via intracavernosa. Uma hora após o início da ereção no grupo tratado todos os animais foram sacrificados e retirou-se o pênis. Este último foi dividido em dois fragmentos, uma parte do material foi congelada em nitrogênio líquido e mantida a 80°C até a extração do RNA para os experimentos de microarranjos e PCR quantitativa; outra parte foi utilizada para avaliação imuno-histoquímica. RESULTADOS: No grupo tratado a ereção foi observada 30-45 minutos após aplicação de Tx2-6 e mantida durante 120 minutos. Os camundongos de grupo controle não apresentaram nenhum indício de ereção. Nos experimentos de microarranjos, onde foram analisados 34.000 genes representando o genoma total do camundongo, identificou-se 3.803 (12,3%) genes com expressão diferencial de pelo menos ±1,5 vez entre os grupos (1.823 genes superexpressos e 1.980 genes subexpressos no grupo tratado comparado ao controle). Os genes ednrb, sparc, fn1, sstr2, pdgfr foram selecionados para validação dos microarranjos por PCR quantitativa e confirmaram a superexpressão em relação aos controles. As proteínas Fn1, Sstr2 e Pdgfr resultaram aumentadas no grupo tratado após avaliação imuno-histoquímica. CONCLUSÕES: A inoculação de Tx2-6 pela via intracavernosa alterou o perfil de expressão gênica no tecido erétil de camundongos. O número de genes superexpressos foi similar ao de genes subexpressos. Serão necessários outros estudos para entender melhor as vias moleculares que Tx2-6 afeta na indução da ereção peniana. / INTRODUCTION: The Phoneutria nigriventer arachnid, also known as armed-spider, has a complex venom, composed by several peptides that affect cellular ionic channels. Among these, only two neuropeptides, Tx2-5 and Tx2-6 induce penile erection in mice and rats and this effect has been associated with the production of nitric oxide by the activation of nitric oxide synthases. Moreover, there is a scarcity of studies focusing on the role of Tx2-6 in the induction of erection. OBJECTIVES: To identify the differently expressed genes in the erectile tissue of mice after erection induction by Tx2-6 using oligonucleotide microarrays. To validate microarray results by quantitative PCR and immunohistochemistry. MATERIALS AND METHODS: Swiss adult male mice were divided in two groups: control (n=10) were injected intracavernously with 20 gl of saline solution; and treated (n=10) were injected intracavernously with 0.006gg/mouse of the Tx2-6 peptide diluted in 20 gl of saline solution. After checking the penile erection in the treated group, all mice were sacrificed one hour after the beginning of erection for the removal of the penis. Penile organ was divided into two fragments, one piece was immediately frozen in liquid-nitrogen and stored at -80°C until RNA extraction to make the microarray and quantitative PCR experiments; the other was reserved for immunohistochemistry analysis. RESULTS: In the treated group, erection was noticed 30-45 minutes after Tx2-6 inoculation and lasted for 120 minutes. Control mice did not present any sign of erection. Considering as differentially expressed genes with a ±1.5 fold expression difference, of the 34,000 genes on the microarray we identified 3,803 (12.3%) genes differentially expressed between the groups (1,823 genes up-regulated and 1,980 genes down-regulated in the treated group compared to controls). The ednrb, sparc, fn1, sstr2, pdgfr genes were selected for validation of microarray results by using quantitative PCR and confirmed the up-regulation when compared to controls. After immunohistochemistry analysis the Fn1, Sstr2 and Pdgfr proteins were found increased in the treated group. CONCLUSIONS: The intracavernous inoculation of Tx2-6 modified the gene expression profile of erectile tissue of mice. The number of upregulated and down-regulated genes was similar. Further studies are needed to understand the molecular pathways that Tx2-6 affect to induce penile erection.
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Microarray-Based Comparative Genomic Hybridization in Neurofibromatoses and DiGeorge SyndromeMantripragada, Kiran K. January 2005 (has links)
<p>Microarray-based comparative genomic hybridization (array-CGH) has emerged as a versatile platform with a wide range of applications in molecular genetics. This thesis focuses on the development of array-CGH with a specific aim to approach disease-related questions through improved strategies in array construction and enhanced resolution of analysis. In <b>paper I</b>, we applied an array covering 11 Mb of 22q, encompassing the <i>NF2</i> locus, for deletion detection in sporadic schwannoma. Hemizygous deletions and tumor heterogeneity were identified. Array-CGH was established as a reliable platform for detection of DNA dosage alterations. <b>Paper II</b> described the construction of the<i> NF2</i> gene-specific microarray for high-resolution scanning of deletions in the <i>NF2</i> locus. We report a novel PCR-based non-redundant strategy for microarray fabrication, which considerably improved the sensitivity and reliability of deletion detection. <b>Paper III</b> reported the first tiling-path array comprehensively covering a human chromosome. The usefulness of the 22q-array was demonstrated by applying it to detect DNA dosage-alterations in 22q-associated disorders. In <b>paper IV</b>, we optimized array-CGH protocols for deletion detection in 22q11 deletion-syndrome. We showed that genomic and cDNA clones are not optimal for analysis of 22q11 locus and that PCR-based non-redundant strategy is reliable for deletion detection in such regions. In <b>paper V</b>, we utilized the 22q-array for understanding the genetic basis of schwannomatosis. Two commonly deleted regions were identified within the <i>IGL</i> and the <i>GSTT1/CABIN1</i> loci. Further investigations using high-resolution arrays, bioinformatic analysis and mutational screening were performed. Missense mutations, specific to the schwannomatosis- and NF2 samples, were identified in the <i>CABIN1 </i>gene. <b>Paper VI</b> described the first array-CGH study for comprehensive and high-resolution profiling of deletions spanning the 17q11 locus. Both typical and atypical deletions were identified in NF1 samples. Bioinformatic analysis revealed novel segmental duplications, which can potentially mediate 17q11 deletions.</p>
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