995 resultados para DNA - Modelos


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Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)

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Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

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Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)

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La computación molecular es una disciplina que se ocupa del diseño e implementación de dispositivos para el procesamiento de información sobre un sustrato biológico, como el ácido desoxirribonucleico (ADN), el ácido ribonucleico (ARN) o las proteínas. Desde que Watson y Crick descubrieron en los años cincuenta la estructura molecular del ADN en forma de doble hélice, se desencadenaron otros descubrimientos, como las enzimas de restricción o la reacción en cadena de la polimerasa (PCR), contribuyendo de manera determinante a la irrupción de la tecnología del ADN recombinante. Gracias a esta tecnología y al descenso vertiginoso de los precios de secuenciación y síntesis del ADN, la computación biomolecular pudo abandonar su concepción puramente teórica. El trabajo presentado por Adleman (1994) logró resolver un problema de computación NP-completo (El Problema del Camino de Hamilton dirigido) utilizando únicamente moléculas de ADN. La gran capacidad de procesamiento en paralelo ofrecida por las técnicas del ADN recombinante permitió a Adleman ser capaz de resolver dicho problema en tiempo polinómico, aunque a costa de un consumo exponencial de moléculas de ADN. Utilizando algoritmos de fuerza bruta similares al utilizado por Adleman se logró resolver otros problemas NP-completos, como por ejemplo el de Satisfacibilidad de Fórmulas Lógicas / SAT (Lipton, 1995). Pronto se comprendió que la computación biomolecular no podía competir en velocidad ni precisión con los ordenadores de silicio, por lo que su enfoque y objetivos se centraron en la resolución de problemas con aplicación biomédica (Simmel, 2007), dejando de lado la resolución de problemas clásicos de computación. Desde entonces se han propuesto diversos modelos de dispositivos biomoleculares que, de forma autónoma (sin necesidad de un bio-ingeniero realizando operaciones de laboratorio), son capaces de procesar como entrada un sustrato biológico y proporcionar una salida también en formato biológico: procesadores que aprovechan la extensión de la polimerasa (Hagiya et al., 1997), autómatas que funcionan con enzimas de restricción (Benenson et al., 2001) o con deoxiribozimas (Stojanovic et al., 2002), o circuitos de hibridación competitiva (Yurke et al., 2000). Esta tesis presenta un conjunto de modelos de dispositivos de ácidos nucleicos capaces de implementar diversas operaciones de computación lógica aprovechando técnicas de computación biomolecular (hibridación competitiva del ADN y reacciones enzimáticas) con aplicaciones en diagnóstico genético. El primer conjunto de modelos, presentados en el Capítulo 5 y publicados en Sainz de Murieta and Rodríguez-Patón (2012b), Rodríguez-Patón et al. (2010a) y Sainz de Murieta and Rodríguez-Patón (2010), define un tipo de biosensor que usa hebras simples de ADN para codificar reglas sencillas, como por ejemplo "SI hebra-ADN-1 Y hebra-ADN-2 presentes, ENTONCES enfermedad-B". Estas reglas interactúan con señales de entrada (ADN o ARN de cualquier tipo) para producir una señal de salida (también en forma de ácido nucleico). Dicha señal de salida representa un diagnóstico, que puede medirse mediante partículas fluorescentes técnicas FRET) o incluso ser un tratamiento administrado en respuesta a un conjunto de síntomas. El modelo presentado en el Capítulo 5, publicado en Rodríguez-Patón et al. (2011), es capaz de ejecutar cadenas de resolución sobre fórmulas lógicas en forma normal conjuntiva. Cada cláusula de una fórmula se codifica en una molécula de ADN. Cada proposición p se codifica asignándole una hebra simple de ADN, y la correspondiente hebra complementaria a la proposición ¬p. Las cláusulas se codifican incluyendo distintas proposiciones en la misma hebra de ADN. El modelo permite ejecutar programas lógicos de cláusulas Horn aplicando múltiples iteraciones de resolución en cascada, con el fin de implementar la función de un nanodispositivo autónomo programable. Esta técnica también puede emplearse para resolver SAP sin ayuda externa. El modelo presentado en el Capítulo 6 se ha publicado en publicado en Sainz de Murieta and Rodríguez-Patón (2012c), y el modelo presentado en el Capítulo 7 se ha publicado en (Sainz de Murieta and Rodríguez-Patón, 2013c). Aunque explotan métodos de computación biomolecular diferentes (hibridación competitiva de ADN en el Capítulo 6 frente a reacciones enzimáticas en el 7), ambos modelos son capaces de realizar inferencia Bayesiana. Funcionan tomando hebras simples de ADN como entrada, representando la presencia o la ausencia de un indicador molecular concreto (una evidencia). La probabilidad a priori de una enfermedad, así como la probabilidad condicionada de una señal (o síntoma) dada la enfermedad representan la base de conocimiento, y se codifican combinando distintas moléculas de ADN y sus concentraciones relativas. Cuando las moléculas de entrada interaccionan con las de la base de conocimiento, se liberan dos clases de hebras de ADN, cuya proporción relativa representa la aplicación del teorema de Bayes: la probabilidad condicionada de la enfermedad dada la señal (o síntoma). Todos estos dispositivos pueden verse como elementos básicos que, combinados modularmente, permiten la implementación de sistemas in vitro a partir de sensores de ADN, capaces de percibir y procesar señales biológicas. Este tipo de autómatas tienen en la actualidad una gran potencial, además de una gran repercusión científica. Un perfecto ejemplo fue la publicación de (Xie et al., 2011) en Science, presentando un autómata biomolecular de diagnóstico capaz de activar selectivamente el proceso de apoptosis en células cancerígenas sin afectar a células sanas.

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In vitro and in animal models, APE1, OGG1, and PARP-1 have been proposed as being involved with inflammatory response. In this work, we have investigated if the SNPs APE1 Asn148Glu, OGG1 Ser326Cys, and PARP-1 Val762Ala are associated to meningitis and also developed a system to enable the functional analysis of polymorphic proteins. Patients with bacterial meningitis (BM), aseptic meningitis (AM) and controls (non-infected) genotypes were investigated by PIRA-PCR or PCR-RFLP. DNA damages were detected in genomic DNA by Fpg treatment. IgG and IgA were measured from plasma and the cytokines and chemokines were measured from cerebrospinal fluid samples using Bio-Plex assays. The levels of NF-κB and c-Jun were measured in CSF by dot blot assays. A significant (P<0.05) increase in the frequency of APE1 148Glu allele in BM and AM patients was observed. A significant increase in the genotypes Asn/Asn in control group and Asn/Glu in BM group was also found. For the SNP OGG1 Ser326Cys, the genotype Cys/Cys was more frequent (P<0.05) in BM group. The frequency of PARP-1 Val/Val genotype was higher in control group (P<0.05). The occurrence of combined SNPs increased significantly in BM patients, indicating that these SNPs may be associated to the disease. Increasing in sensitive sites to Fpg was observed in carriers of APE1 148Glu allele or OGG1 326Cys allele, suggesting that SNPs affect DNA repair activity. Alterations in IgG production were observed in the presence of SNPs APE1Asn148Glu, OGG1Ser326Cys or PARP-1Val762Ala. Reductions in the levels ofIL-6, IL-1Ra, MCP-1/CCL2and IL-8/CXCL8 were observed in the presence of APE1148Glu allele in BM patients, however no differences were observed in the levels of NF-κB and c-Jun considering genotypes and analyzed groups. Using APE1 as model, a system to enable the analysis of cellular effects and functional characterization of polymorphic proteins was developed using strategies of cloning APE1 cDNA in pIRES2-EGFP vector, cellular transfection of the construction obtained, siRNA for endogenous APE1 and cellular cultures genotyping. In conclusion, we obtained evidences of an effect of SNPs in DNA repair genes on the regulation of immune response. This is a pioneering work in the field that shows association of BER variant enzymes with an infectious disease in human patients, suggesting that the SNPs analyzed may affect immune response and damage by oxidative stress level during brain infection. Considering these data, new approaches of functional characterization must be developed to better analysis and interactions of polymorphic proteins in response to this context

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Ceramic membranes were fabricated by in situ synthesis of alumina nanofibres in the pores of an alumina support as a separation layer, and exhibited a high permeation selectivity for bovine serum albumin relative to bovine hemoglobin (over 60 times) and can effectively retain DNA molecules at high fluxes.

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Synchronous fluorescence spectroscopy (SFS) was applied for the investigation of interactions of the antibiotic, tetracycline (TC), with DNA in the presence of aluminium ions (Al3+). The study was facilitated by the use of the Methylene Blue (MB) dye probe, and the interpretation of the spectral data with the aid of the chemometrics method, parallel factor analysis (PARAFAC). Three-way synchronous fluorescence analysis extracted the important optimum constant wavelength differences, Δλ, and showed that for the TC–Al3+–DNA, TC–Al3+ and MB dye systems, the associated Δλ values were different (Δλ = 80, 75 and 30 nm, respectively). Subsequent PARAFAC analysis demonstrated the extraction of the equilibrium concentration profiles for the TC–Al3+, TC–Al3+–DNA and MB probe systems. This information is unobtainable by conventional means of data interpretation. The results indicated that the MB dye interacted with the TC–Al3+–DNA surface complex, presumably via a reaction intermediate, TC–Al3+–DNA–MB, leading to the displacement of the TC–Al3+ by the incoming MB dye probe.

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To further investigate the use of DNA repair-enhancing agents for skin cancer prevention, we treated Cdk4R24C/R24C/NrasQ61K mice topically with the T4 endonuclease V DNA repair enzyme (known as Dimericine) immediately prior to neonatal ultraviolet radiation (UVR) exposure, which has a powerful effect in exacerbating melanoma development in the mouse model. Dimericine has been shown to reduce the incidence of basal-cell and squamous cell carcinoma. Unexpectedly, we saw no difference in penetrance or age of onset of melanoma after neonatal UVR between Dimericine-treated and control animals, although the drug reduced DNA damage and cellular proliferation in the skin. Interestingly, epidermal melanocytes removed cyclobutane pyrimidine dimers (CPDs) more efficiently than surrounding keratinocytes. Our study indicates that neonatal UVR-initiated melanomas may be driven by mechanisms other than solely that of a large CPD load and/or their inefficient repair. This is further suggestive of different mechanisms by which UVR may enhance the transformation of keratinocytes and melanocytes.

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Cell proliferation is a critical and frequently studied feature of molecular biology in cancer research. Therefore, various assays are available using different strategies to measure cell proliferation. Metabolic assays such as AlamarBlue, WST-1, and MTT, which were originally developed to determine cell toxicity, are being used to assess cell numbers. Additionally, proliferative activity can be determined by quantification of DNA content using fluorophores, such as CyQuant and PicoGreen. Referring to data published in high ranking cancer journals, 945 publications applied these assays over the past 14 years to examine the proliferative behaviour of diverse cell types. Within this study, mainly metabolic assays were used to quantify changes in cell growth yet these assays may not accurately reflect cellular proliferation rates due to a miscorrelation of metabolic activity and cell number. Testing this hypothesis, we compared metabolic activity of different cell types, human cancer cells and primary cells, over a time period of 4 days using AlamarBlue and fluorometric assays CyQuant and PicoGreen to determine their DNA content. Our results show certain discrepancies in terms of over-estimation of cell proliferation with respect to the metabolic assay in comparison to DNA binding fluorophores.

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Recent studies have shown that human papillomavirus (HPV) DNA can be found in circulating blood, including peripheral blood mononuclear cells (PBMCs), sera, plasma, and arterial cord blood. In light of these findings, DNA extracted from PBMCs from healthy blood donors were examined in order to determine how common HPV DNA is in blood of healthy individuals. Blood samples were collected from 180 healthy male blood donors (18-76 years old) through the Australian Red Cross Blood Services. Genomic DNA was extracted and specimens were tested for HPV DNA by PCR using a broad range primer pair. Positive samples were HPV-type determined by cloning and sequencing. HPV DNA was found in 8.3% (15/180) of the blood donors. A wide variety of different HPV types were isolated from the PBMCs; belonging to the cutaneous beta and gamma papillomavirus genera and mucosal alpha papillomaviruses. High-risk HPV types that are linked to cancer development were detected in 1.7% (3/180) of the PBMCs. Blood was also collected from a healthy HPV-positive 44-year-old male on four different occasions in order to determine which blood cell fractions harbor HPV. PBMCs treated with trypsin were negative for HPV, while non-trypsinized PBMCs were HPV-positive. This suggests that the HPV in blood is attached to the outside of blood cells via a protein-containing moiety. HPV was also isolated in the B cells, dendritic cells, NK cells, and neutrophils. To conclude, HPV present in PBMCs could represent a reservoir of virus and a potential new route of transmission.