931 resultados para SDS - PAGE
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Objectives: The inflammatory response to pulpal injury or infection has major clinical significance. The aim of the study is to investigate the presence and regulation of expression of neuropeptide receptors on human pulp fibroblasts and whole pulp tissue. This study will investigate the expression of Substance P (NK-1) and Neuropeptide Y (NPY-Y1) receptors on pulp fibroblasts, determine the effects of Transforming Growth Factor Beta-1 (TGF-b1) and Interleukin 1-Beta (IL-1b) on the expression of NK-1 and NPY-Y1 receptors on pulp fibroblasts and examine the levels of receptor expression in whole pulp samples. Methods: Primary pulp fibroblast cell lines were obtained from patients undergoing extractions for orthodontic reasons. The cells were grown to confluence and stimulated for 5 days with IL-1b or TGF-b1. Pulp tissue fragments were obtained from freshly extracted sound and carious teeth, snap frozen in liquid nitrogen and cracked open using a vice. The monolayer was removed with cell scrapers and pelleted. The cell membranes of the cultured cells and the whole tissue were isolated using a Mem-PER® Eukaryotic Membrane Protein Extraction Reagent Kit (Pierce, UK). The membrane proteins were separated by SDS-PAGE and Western blotting was used to detect the presence of NK-1 and NPY-Y1. Results: Initial results demonstrated the presence of NK-1 and NPY-Y1 in cultured pulp fibroblasts. Following the 5 day incubation with TGF-b1, the cells appeared not to express NK-1. IL-1b had a slight stimulatory effect on NK-1 expression. The NPY-Y1 expression was not affected by either TGF-b1 or IL-1b. In whole pulp samples, levels of NK-1 were increased in carious teeth compared to caries-free teeth. The NPY-Y1 levels were similar in carious and non-carious teeth. Conclusion: These findings give an insight into how pulp cells react to inflammatory stimuli with regards to neuropeptide receptor expression and their roles in health and disease
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A inativação fotodinâmica tem sido usada com sucesso na inativação de microorganismos. Diversos aspetos da inativação fotodinâmica foram já estudados para diferentes microrganismos, contudo, existe ainda pouca informação disponível no que diz respeito à inativação de bacteriófagos por processos fotodinâmicos. Este trabalho pretendeu elucidar e avaliar vários aspetos da fotoinativação de vírus, em particular de bacteriófagos, incluindo (i) o efeito de diversos parâmetros de luz utilizados na fotoinativação de bacteriófagos; (ii) a eficiência da inativação fotodinâmica de diferentes tipos de bacteriófagos (fagos do tipo DNA e RNA); (iii) o principal mecanismo através do qual a inativação fotodinâmica tem lugar; (iv) o efeito da fotoinativação nas proteínas do bacteriófago; e (v) o possível desenvolvimento de resistência e recuperação da viabilidade após vários tratamentos fotodinâmicos consecutivos. Para avaliar o efeito dos diferentes parâmetros de luz, suspensões fágicas com 107 UFP mL-1 foram irradiadas com diferentes fontes e doses de luz, intensidades luminosas e tempos de irradiação (30,90 e 270 min) na presença de 0,5; 1,0 e 5,0 μM dos derivados porfirínicos catiónicos Tri- Py+-Me-PF e Tetra-Py+-Me. A eficiência da fotoinativação de diferentes fagos do tipo DNA e RNA, foi avaliada através da irradiação da suspensão fágica com luz branca (40 W m-2) durante 270 min na presença de 0,5 e 5,0 μM do derivado porfirínico Tri-Py+-Me-PF, respetivamente para os fagos do tipo RNA e DNA. O mecanismo através do qual a fotoinativação de fagos de DNA (fago do tipo T4) e de RNA (fago Qb) tem lugar foi avaliado por exposição da suspensão fágica à luz branca com uma potência de 40 W m-2, na presença de fotossensibilizador (Tri-Py+-Me-PF e Tetra-Py+-Me) e inibidores, quer do oxigénio singuleto (azida de sódio e L-histidina) quer de radicais livres (Dmanitol e L-cisteína). Os danos nas proteínas do fago do tipo T4, induzidos pelas espécies reativas de oxigénio geradas por 5,0 μM Tri-Py+-Me-PF, foram avaliados pelo método convencional de SDS-PAGE e por espectroscopia de infravermelho. O possível desenvolvimento de resistência e recuperação da viabilidade após a inativação fotodinâmica dos bacteriófagos foi avaliado após dez ciclos consecutivos de tratamento fotodinâmico incompletos (120 min sob irradiação de luz branca a uma potência de 40 W m-2) na presença de 5,0 μM do derivado porfirínico Tri-Py+-Me-PF. Os resultados deste trabalho mostraram que (i) quando uma quantidade de energia (dose de luz) determinada foi aplicada numa suspensão fágica, a partir de uma mesma fonte irradiação, a fotoinactivação do fago foi tanto mais eficiente quanto mais baixa foi a potência luminosa aplicada; (ii) os bacteriófagos foram eficientemente inativados até ao limite de deteção (redução de 6-7 log); (ii) os fagos do tipo RNA foram inativados mais facilmente do que os fagos do tipo DNA (tempos de exposição mais curtos e com concentração de fotossensibilizador dez vezes menor do que a usada para inativar os fagos do tipo DNA); (iii) o mecanismo do tipo II (via produção de oxigénio singuleto) foi o principal mecanismo através do qual a fotoinativação dos bacteriófagos teve lugar; (iv) foi possível detectar danos no perfil proteico após tratamento fotodinâmico e a espectroscopia de infravermelho apresentou-se como uma metodologia promissora de screening para avaliação dos danos induzidos pela inativação fotodinâmica em proteínas; e (v) após dez ciclos consecutivos de tratamento fotodinâmico, o fago do tipo T4 não revelou nenhum tipo de resistência ao tratamento fotodinâmico nem recuperou a sua viabilidade. Como conclusão, a inativação fotodinâmica microbiana é uma tecnologia bastante eficaz para a fotoinativação de bacteriófagos do tipo DNA e RNA sem invólucro, a qual pode ser considerada como uma alternativa ao tratamento convencional com agentes antivíricos, mesmo com intensidades luminosas baixas, sem o risco associado de desenvolvimento de mecanismos de resistência.
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Photodynamic inactivation (PDI) is defined as the process of cell destruction by oxidative stress resulting from the interaction between light and a photosensitizer (PS), in the presence of molecular oxygen. PDI of bacteria has been extensively studied in recent years, proving to be a promising alternative to conventional antimicrobial agents for the treatment of superficial and localized infections. Moreover, the applicability of PDI goes far beyond the clinical field, as its potential use in water disinfection, using PS immobilized on solid supports, is currently under study. The aim of the first part of this work was to study the oxidative modifications in phospholipids, nucleic acids and proteins of Escherichia coli and Staphylococcus warneri, subjected to photodynamic treatment with cationic porphyrins. The aims of the second part of the work were to study the efficiency of PDI in aquaculture water and the influence of different physicalchemical parameters in this process, using the Gram-negative bioluminescent bacterium Vibrio fischeri, and to evaluate the possibility of recycling cationic PS immobilized on magnetic nanoparticles. To study the oxidative changes in membrane phospholipids, a lipidomic approach has been used, combining chromatographic techniques and mass spectrometry. The FOX2 assay was used to determine the concentration of lipid hydroperoxides generated after treatment. The oxidative modifications in the proteins were analyzed by one-dimensional polyacrylamide gel electrophoresis (SDS-PAGE). Changes in the intracellular nucleic acids were analyzed by agarose gel electrophoresis and the concentration of doublestranded DNA was determined by fluorimetry. The oxidative changes of bacterial PDI at the molecular level were analyzed by infrared spectroscopy. In laboratory tests, bacteria (108 CFU mL-1) were irradiated with white light (4.0 mW cm-2) after incubation with the PS (Tri-Py+-Me-PF or Tetra-Py+-Me) at concentrations of 0.5 and 5.0 μM for S. warneri and E. coli, respectively. Bacteria were irradiated with different light doses (up to 9.6 J cm-2 for S. warneri and up to 64.8 J cm-2 for E. coli) and the changes were evaluated throughout the irradiation time. In the study of phospholipids, only the porphyrin Tri-Py+-Me-PF and a light dose of 64.8 J cm-2 were tested. The efficiency of PDI in aquaculture has been evaluated in two different conditions: in buffer solution, varying temperature, pH, salinity and oxygen concentration, and in aquaculture water samples, to reproduce the conditions of PDI in situ. The kinetics of the process was determined in realtime during the experiments by measuring the bioluminescence of V. fischeri (107 CFU mL-1, corresponding to a level of bioluminescence of 105 relative light units). A concentration of 5.0 μM of Tri-Py+-Me-PF was used in the experiments with buffer solution, and 10 to 50 μM in the experiments with aquaculture water. Artificial white light (4.0 mW cm-2) and solar irradiation (40 mW cm-2) were used as light sources.
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Helicobacter pylori is a bacterial pathogen that affects more than half of the world’s population with gastro-intestinal diseases and is associated with gastric cancer. The cell surface of H. pylori is decorated with lipopolysaccharides (LPSs) composed of three distinct regions: a variable polysaccharide moiety (O-chain), a structurally conserved core oligosaccharide, and a lipid A region that anchors the LPS to the cell membrane. The O-chain of H. pylori LPS, exhibits unique oligosaccharide structures, such as Lewis (Le) antigens, similar to those present in the gastric mucosa and are involved in interactions with the host. Glucan, heptoglycan, and riban domains are present in the outer core region of some H. pylori LPSs. Amylose-like glycans and mannans are also constituents of some H. pylori strains, possibly co-expressed with LPSs. The complexity of H. pylori LPSs has hampered the establishment of accurate structure-function relationships in interactions with the host, and the design of carbohydrate-based therapeutics, such as vaccines. Carbohydrate microarrays are recent powerful and sensitive tools for studying carbohydrate antigens and, since their emergence, are providing insights into the function of carbohydrates and their involvement in pathogen-host interactions. The major goals of this thesis were the structural analysis of LPSs from H. pylori strains isolated from gastric biopsies of symptomatic Portuguese patients and the construction of a novel pathogen carbohydrate microarray of these LPSs (H. pylori LPS microarray) for interaction studies with proteins. LPSs were extracted from the cell surface of five H. pylori clinical isolates and one NCTC strain (26695) by phenol/water method, fractionated by size exclusion chromatography and analysed by gas chromatography coupled to mass spectrometry. The oligosaccharides released after mild acid treatment of the LPS were analysed by electrospray mass spectrometry. In addition to the conserved core oligosaccharide moieties, structural analyses revealed the presence of type-2 Lex and Ley antigens and N-acetyllactosamine (LacNAc) sequences, typically found in H. pylori strains. Also, the presence of O-6 linked glucose residues, particularly in LPSs from strains 2191 and NCTC 26695, pointed out to the expression of a 6-glucan. Other structural domains, namely ribans, composed of O-2 linked ribofuranose residues were observed in the LPS of most of H. pylori clinical isolates. For the LPS from strain 14382, large amounts of O-3 linked galactose units, pointing to the occurrence of a galactan, a domain recently identified in the LPS of another H. pylori strain. A particular feature to the LPSs from strains 2191 and CI-117 was the detection of large amounts of O-4 linked N-acetylglucosamine (GlcNAc) residues, suggesting the presence of chitin-like glycans, which to our knowledge have not been described for H. pylori strains. For the construction of the H. pylori LPS microarray, the structurally analysed LPSs, as well as LPS-derived oligosaccharide fractions, prepared as neoglycolipid (NGL) probes were noncovalently immobilized onto nitrocellulosecoated glass slides. These were printed together with NGLs of selected sequence defined oligosaccharides, bacterial LPSs and polysaccharides. The H. pylori LPS microarray was probed for recognition with carbohydratebinding proteins (CBPs) of known specificity. These included Le and blood group-related monoclonal antibodies (mAbs), plant lectins, a carbohydratebinding module (CBM) and the mammalian immune receptors DC-SIGN and Dectin-1. The analysis of these CBPs provided new information that complemented the structural analyses and was valuable in the quality control of the constructed microarray. Microarray analysis revealed the occurrence of type-2 Lex and Ley, but not type-1 Lea or Leb antigens, supporting the results obtained in the structural analysis. Furthermore, the H. pylori LPSs were recognised by DC-SIGN, a mammalian lectin known to interact with this bacterium through fucosylated Le epitopes expressed in its LPSs. The -fucose-specific lectin UEA-I, showed restricted binding to probes containing type-2 blood group H sequence and to the LPSs from strains CI-117 and 14382. The presence of H-type-2, as well Htype- 1 in the LPSs from these strains, was confirmed using specific mAbs. Although H-type-1 determinant has been reported for H. pylori LPSs, this is the first report of the presence of H-type-2 determinant. Microarray analysis also revealed that plant lectins known to bind 4-linked GlcNAc chitin oligosaccharide sequences bound H. pylori LPSs. STL, which exhibited restricted and strong binding to 4GlcNAc tri- and pentasaccharides, differentially recognised the LPS from the strain CI-117. The chitin sequences recognised in the LPS could be internal, as no binding was detected to this LPS with WGA, known to be specific for nonreducing terminal of 4GlcNAc sequence. Analyses of the H. pylori LPSs by SDS-PAGE and Western blot with STL provided further evidence for the presence of these novel domains in the O-chain region of this LPS. H. pylori LPS microarray was also applied to analysis of two human sera. The first was from a case infected with H. pylori (H. pylori+ CI-5) and the second was from a non-infected control.The analysis revealed a higher IgG-reactivity towards H. pylori LPSs in the H. pylori+ serum, than the control serum. A specific IgG response was observed to the LPS isolated from the CI-5 strain, which caused the infection. The present thesis has contributed to extension of current knowledge on chemical structures of LPS from H. pylori clinical isolates. Furthermore, the H. pylori LPS microarray constructed enabled the study of interactions with host proteins and showed promise as a tool in serological studies of H. pyloriinfected individuals. Thus, it is anticipated that the use of these complementary approaches may contribute to a better understanding of the molecular complexity of the LPSs and their role in pathogenesis.
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Tese dout., Ciências e Tecnologias do Ambiente, 2009, Universidade do Algarve
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Tese de dout., Bioquímica (Biologia Celular e Molecular), Faculdade de Ciências e Tecnologia, Univ. do Algarve, 2010
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O folding oxidativo de proteínas consiste na formação de pontes dissulfureto intramoleculares envolvendo a oxidação de grupos tiol no sentido da criação de uma ligação entre duas cisteínas. Esta modificação postransducional é essencial para a estabilidade das proteínas, principalmente em proteínas secretadas para o meio extracelular. In vivo, o folding oxidativo ocorre no retículo endoplasmático e é assistido por uma série de proteínas que atuam como catalisadores. Estas reações em cadeia necessitam da presença de um aceitador final de eletrões. No presente trabalho foram estudadas duas vias que atuam no reticulo endoplasmático para o refolding oxidativo da proteína modelo Ribonuclease A: Uma via envolve a interação entre duas proteínas, a Endoplasmic Recticulum Oxireductase 1 (Ero1) e a Protein Disulfide Isomerase (PDI); A outra via envolve a interação da PDI com a Peroxiredoxin IV (PRDX4). Foi igualmente estudado o refolding oxidativo com uma enzima homóloga da PRDX4, a PRDX2, no sentido de compreender se existe especificidade na interação entre a PRDX4 e a PDI. O estudo do refolding oxidativo da Ribonuclease foi realizado in vitro e avaliado em géis SDS-PAGE-Tricina com o objetivo de verificar a diferença de mobilidades entre a Ribonuclease reduzida e oxidada no gel. Na via da PRDX4/PDI e PRDX2/PDI é necessária a introdução de Glucose e Glucose Oxidase, responsáveis pela produção de peróxido de hidrogénio que atua como aceitador final de eletrões desta via. Em todas as vias foi observado refolding oxidativo da RNase. Na via da Ero1/PDI este foi substancialmente mais rápido e ocorre, embora em muito menor grau, mesmo na ausência da PDI. Na via da PRDX4/PDI o refolding é mais lento e foi constatado que não existe especificidade da PRDX4 para a PDI visto que, na presença da PRDX2, os resultados foram semelhantes aos resultados obtidos com a PRDX4.
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It is widely recognized that protein restriction in utero may cause metabolic and endocrine adaptations, which may be of benefit to the neonate on a short-term basis but may cause adverse long-term conditions such as obesity, Type 2 diabetes, metabolic syndrome, hypertension and cardiovascular diseases. Adequate foetal and early post natal nutrient and energy supply is therefore essential for adult animal health, performance and life span. In this project it was investigated the progressive adaptations of the hepatic proteome in male mink offspring exposed to either a low protein (FL) or an adequate protein (FA) diet in utero fed either on a low protein (LP) or on an adequate (AP) diet from weaning until sexual maturity. Specifically, the aim was to determine the metabolic adaptations at selected phases of the animal’s first annual cycle and establish the metabolic priorities occurring during those phases. The three different morphological stages studied during the first year of development included, end of bone growth at 4 months of age, maximal fat accretion at 6 months of age and sexual maturity at 12 months of age. A reference proteome of mink liver coming from these different animal groups were generated using 2D electrophoresis coupled to MALDI-TOF analysis and the way in which dietary treatment affect their proteome was established. Approximately 330 proteins were detected in the mink liver proteome. A total of 27 comparisons were carried out between all different animal groups which resulted in 20 differentially expressed proteins. An extensive survey was conducted towards the characterization of these proteins including their subcellular localization, the biological processes in which they are involved and their molecular functions. This characterization allowed the identification of proteins in various processes including the glycolysis and fatty acid metabolism. The detailed analysis of the different dietary treatment animal groups was indicative of differences in metabolism and also to changes associated with development in mink.
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O objectivo primordial deste trabalho foi efectuar a extracao e o estudo das proteinas da Goma da Alfarroba ou Locust Bean Gum (LBG) com vista a sua clarificacao e purificacao. Para atingir este objectivo em primeiro lugar estudou-se o teor de etanol que se deveria utilizar numa suspensao aquosa de LBG, uma vez que a LBG e um polissacarido que hidrata facilmente com agua e consequentemente origina solucoes altamente viscosas que impossibilitam a realizacao de tecnicas de extracao de proteinas. Para isso estudou-se o comportamento da LBG em suspensoes aquosas com 10% (p/v) de LBG e diferentes concentracoes de etanol, designadamente 10% (v/v), 20% (v/v), 30% (v/v) e 40% (v/v). Com este estudo concluiu-se que seria necessario utilizar uma concentracao de 40% (v/v) de etanol a 96% em cada suspensao de LBG a 10% (p/v) para conseguir evitar a sua hidratacao excessiva. Assim, todas as extracoes neste trabalho foram realizadas de acordo com estas condicoes. Posteriormente com vista a extracao das proteinas da LBG testaram-se diferentes tratamentos, designadamente tratamentos alcalinos, acidos e com detergentes. Segundo a bibliografia consultada para os tratamentos alcalinos, realizaram-se estas extracoes com hidroxido de sodio (NaOH) com concentracoes de 0,025 M, 0,05M, 0,1M e 0,2M. Estes tratamentos foram iniciados com uma concentracao de NaOH a 0,2M, contudo apos analise dos resultados verificou-se que esta originou uma LBG com uma coloracao mais amarela do que a LBG bruta (inicial) apresentava. Sendo a ideia final a clarificacao da goma este nao foi um resultado desejavel e como tal testaram-se concentracoes inferiores de NaOH, acima referidas. No final concluiu-se que todas estas extracoes efetuadas com NaOH originavam uma LBG mais amarela do que a LBG bruta e que assim este nao seria o tratamento mais adequado para o objectivo pretendido. Como tal prosseguiram-se os estudos com um tratamento acido, que atraves de consulta bibliografica se iniciou com acido sulfurico (H2SO4). O tratamento acido iniciou-se com uma concentracao de H2SO4 de 0,1M, testando-se posteriormente tambem uma extracao com H2SO4 com concentracao de 0,05M. No final destas extracoes verificou-se que a LBG obtida em ambas apresentava uma coloracao mais clara do que a LBG bruta, o que representava, numa primeira analise, um bom resultado. Por fim efectuaram-se extracoes solido-liquido com diferentes detergentes, designadamente com Tween 20, Tween 40, Tween 60, Tween 65, Tween 80, Tween 85, Triton X-100, Triton X-114 e SDS todos a uma concentracao de 0,1% (v/v) a excepcao do Tween 65 em que foi utilizada uma concentracao de 0,1% (p/v), porque a temperatura ambiente este detergente e solido. No final destas extracoes concluiu-se que na maioria dos casos a LBG apresentava uma coloracao mais clara do que a LBG bruta. Para quantificar as proteinas extraidas atraves de cada um dos tratamentos acima mencionados utilizaram-se dois metodos, o metodo de Bradford para quantificar as proteinas presentes nos sobrenadantes das extracoes e o metodo de Kjeldahl para quantificar as proteinas ainda presentes na LBG apos as extracoes. Analisando os resultados obtidos por estes metodos concluiu-se que a extracao efetuada com Tween 80, em que se efectuou uma lavagem adicional a LBG durante a filtracao com uma solucao de agua destilada e etanol a 40% (v/v), foi a que apresentou melhores resultados. Assim, foi com esta amostra proteica que se prosseguiram os estudos as proteinas. Para realizar os estudos as proteinas extraidas efectuou-se uma eletroforese em SDS-PAGE (sodium dodecyl sulfate polyacrylamide gel electrophoresis) com o intuito de verificar o estado da amostra. Analisando os geles obtidos constatou-se que a amostra se encontrava em boas condicoes. Deste modo realizou-se uma eletroforese bidimensional (2 – D) das proteinas extraidas da LBG. Nesta tecnica, como se desconheciam que tipo de proteinas se encontravam presentes na amostra utilizou-se uma banda de pH para a Focagem Isoelectrica (1a Dimensao) entre 3 e 10 e a separacao por Peso Molecular (2a Dimensao) foi efetuada em SDS-PAGE. Analisando os geles obtidos concluiu-se que a maioria das proteinas presentes nesta amostra apresentam pontos isoelectricos na gama de pH entre 5 e 6 e tem pesos moleculares entre 40 e 60 kDa. Pode-se entao concluir que o objectivo deste trabalho foi apenas parcialmente atingido uma vez que se conseguiu extrair e estudar algumas das caracteristicas das proteinas presentes na LBG, mas nao se alcancou a sua clarificacao.
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Exposure to allergens is pivotal in determining sensitization and allergic symptoms in individuals. Pollen grain counts in ambient air have traditionally been assessed to estimate airborne allergen exposure. However, the exact allergen content of ambient air is unknown. We therefore monitored atmospheric concentrations of birch pollen grain and the matched major birch pollen allergen Bet v 1 simultaneously across Europe within the EU-funded project HIALINE (Health Impacts of Airborne Allergen Information Network). Pollen count was assessed with Hirst type pollen traps at 10 l/min at sites in France, United Kingdom, Germany, Italy and Finland. Allergen concentrations in ambient air were sampled at 800l/min with a Chemvol high-volume cascade impactor equipped with stages PM>10μm, 10 μm>PM>2.5μm, and in Germany also 2.5 μm>PM>0.12μm. The major birch pollen allergen Bet v 1 was determined with an allergen specific ELISA. Bet v 1 isoform patterns were analyzed by 2D-SDS-PAGE blots and mass spectrometric identification. Basophil activation was tested in an FcεR1-humanized rat basophil cell line passively sensitized with serum of a birch pollen lmptomatic patient. Compared to 10 previous years, 2009 was a representative birch pollen season for all stations. About 90% of the allergen was found in the PM>10μm fraction at all stations. Bet v 1 isoforms pattern did not varied substantially neither during ripening of pollen nor between different geographical locations. The average European allergen release from birch pollen was 3.2 pg Bet v 1/pollen and did not vary much between the European countries. However, in all countries a >10-fold difference in daily allergen release per pollen was measured which could be explained by long range transport of pollen with a deviating allergen release. Basophil activation by ambient air extracts correlated better with airborne allergen than with pollen concentration. Although Bet v 1 is a mixture of different isoforms, its fingerprint is constant across Europe. Bet v 1 was also exclusively linked to pollen. Pollen from different days varied >10-fold in allergen release. Thus exposure to allergen is inaccurately monitored by only monitoring birch pollen grains. Indeed, a humanized basophil activation test correlated much better with allergen concentrations in ambient air than with pollen count. Monitoring the allergens themselves together with pollen in ambient air might be an improvement in allergen exposure assessment.
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Dissertação de Mestrado, Biotecnologia em Controlo Biológico, 27 de Junho de 2013, Universidade dos Açores.
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Presence of surface glycoprotein in Piptocephalis virginiana that recognizes the host glycoproteins band c, reported earlier from our laboratory, was detected by immunofluorescence microscopy. Germinated spores of P. virginiana treated with Mortierella pusilla cell wall protein extract, primary antibodies prepared against glycoproteins band c and FITC-goat anti-rabbit IgG conjugate showed fluorescence. This indicated that on the surfaces of the biotrophic mycoparasite P. virginiana , there might be a complementary molecule which recognizes the glycoproteins band c from M. pusilla. Immunobinding analysis identified a glycoprotein of Mr 100 kDa from the mycoparasite which binds with the host glycoproteins band c, separately as well as collectively. Purification of this glycoprotein was achieved by (i) 60% ammonium sulfate precipitation, (ii) followed by heat treatment, and (iii) Sephadex G-IOO gel filtration. The glycoprotein was isolated by preparative polyacrylamide gel electrophoresis by cutting and elution. The purity of the protein ·was ascertained by SDS-PAGE and Western blot analysis. Positive reaction to periodic acid-Schiff reagent revealed the glycoprotein nature of this 100 kDa protein. Mannose was identified as a major sugar component of this glycoprotein by using a BoehringerMannheim Glycan Differentiation Kit. Electrophoretically purified glycoprotein was used to raIse polyclonal antibody in rabbit. The specificity of the antibody was determined by dot-immunobinding test and western-blot analysis. Immunofluorescence mIcroscopy revealed surface localization of the protein on the germ tube of Piptocephalis virginiana. Fluorescence was also observed at the surfaceJ of the germinated spores and hyphae of the host, M. pusilla after treatment with complementary protein from P. virginiana, primary antibody prepared against the complementary protein and FITC-goat anti-rabbit IgG conjugate.
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This project aimed to determine the protein prof i les and concent rat ion in honeys, ef fect of storage condi t ions on the protein content and the interact ion between proteins and polyphenols. Thi r teen honeys f rom di f ferent botanical or igins were analyzed for thei r protein prof i les using SDS-PAGE, protein concent rat ion and phenol ic content , using the Pierce Protein Assay and Fol in-Ciocal teau methods, respectively. Protein-polyphenol interact ions were analyzed by a combinat ion of the ext ract ion of honeys wi th solvents of di f ferent polar i t ies fol lowed by LCjMS analysis of the obtained f ract ions. Results demonst rated a di f ferent protein content in the tested honeys, wi th buckwheat honey possessing the highest protein concent rat ion. We have shown that the reduct ion of proteins dur ing honey storage was caused, partially, by the protein complexat ion wi th phenolics. The LCjMS analysis of the peak elut ing at retent ion t ime of 10 to 14 min demonst rated that these phenolics included f lavonoids such as Pinobanksin, Pinobanksin acetate, Apigenin, Kaemferol and Myricetin and also cinnamic acid.
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Black fly (Simuliidae) silk is produced by the larvae and pharate pupae and is used for anchorage and cocoon production. There exists limited information on simuliid silks, including protein composition and genetic sequences encoding such proteins. The present study aimed to expand what is known about simuliid silks by examining the silks of several simuliid species and by making comparisons to the silk of non-biting midges (Chironomidae). Silk glands were dissected out of larval and pupal simuliids, and protein contents were separated by sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE) and visualized with silver stain. Protein contents were compared by mass in kilodaltons (kDa) between life stages and among species. Polymerase chain reaction (PCR) was used to expand upon known gene sequence information, and to determine the presence of genes homologous to chironomid silk. SDS-PAGE of cocoons revealed the presence of a 56 kDa and a 67 kDa protein. Silk gland contained as many as 28 different proteins ranging from 319 kDa to 8 kDa. Protein profiles vary among species, and group into large (>200), intermediate(>100), and small (<100) protein classes as is found in chironomids. It is likely that silk evolved in a common ancestor of simuliids and chironomids
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Les infections à Salmonella Typhimurium constituent un problème de taille pour l’industrie porcine et la santé publique car cet animal est un réservoir pour les infections chez l’homme. De plus, on observe, chez des souches appartenant au lysotype (LT) 104, des résistances multiples aux antimicrobiens associées à des septicémies chez les porcs en engraissement, ce qui peut contribuer à la contamination des carcasses. Il faut donc contrôler l’infection au niveau du troupeau. Pour ce faire, il importe donc de mieux caractériser ces souches, comprendre la pathogénie de l’infection et identifier des facteurs de virulence. L’objectif principal de cette étude était de caractériser des isolats de S. Typhimurium provenant de porcs septicémiques et de les comparer avec ceux de porcs sains. Une banque d’isolats provenant de porcs septicémiques (ASC) et de porcs sains à l’abattoir (SSC) était constituée. Le lysotype des isolats a été identifié et ceux-ci ont été caractérisés selon le profil de résistance aux antimicrobiens, le SDS-PAGE et l’immunobuvardage et le PFGE. Chez les isolats ASC, LT 104 représentait 36.4% des isolats et chez les isolats SSC la proportion était de 51.5%. Les isolats pouvaient être résistants jusqu’à douze antimicrobiens, peu importe leur origine. Il n’a toutefois pas été possible d’associer une protéine spécifique au groupe d’isolats ASC. Parmi les souches LT 104, plusieurs groupes génétiques ont été identifiés. Les différentes étapes de la pathogénie de Salmonella ont ensuite été évaluées, dont l’adhésion et l’invasion des isolats des deux banques sur des cellules intestinales humaines. Nos résultats ont démontré que les isolats ASC avaient un pouvoir accru d’invasion comparés aux isolats SSC (P=0.003). Pour un sous-groupe d’isolats sélectionnés selon leur taux d’invasion, des tests de phagocytose, d’apoptose et d’adhésion au mucus intestinal ont été effectués en utilisant la cytométrie en flux. La survie des bactéries après la phagocytose a aussi été évaluée et la méthode MATS a été utilisée pour évaluer l'adhésion aux solvants. Les pourcentages de phagocytose chez les isolats SSC par les monocytes porcins étaient plus élevés que chez les isolats ASC à 15 minutes (P=0.02). Nous n’avons trouvé aucune différence significative pour les autres méthodes utilisées. Nous avons ensuite comparé le génome d’un isolat ASC (#36) à celui d’un isolat SSC (#1) par le SSH pour identifier des facteurs de virulence potentiels. Des clones correspondant à des gènes retrouvés sur le chromosome ainsi que sur des plasmides ont été identifiés. Ces résultats nous ont dirigés vers l’analyse des profils plasmidiques de tous les isolats. Les différents profils étaient retrouvés autant chez les isolats ASC que chez les isolats SSC. Deux profils (PL14 et PL20) étaient observés plus fréquemment chez les isolats LT 104 que chez les isolats d’autres lysotypes (P=0.01 et P=0.01, respectivement). Le séquençage d’un des plasmides de l’isolat ASC, démontrait la présence d’informations génétiques codant pour la réplication et une bêta-galactosidase-α. Il serait intéressant de préciser le rôle exact de ces gènes dans l’infection. Nos travaux suggèrent que les isolats de S. Typhimurium provenant de porcs septicémiques se distinguent par un pouvoir d’invasion accru ainsi que par des taux de phagocytose plus faibles dans les phases initiales de l’infection. Cette étude aura donc permis d’accroître les connaissances sur la pathogénie des infections à S. Typhimurium chez le porc.
