379 resultados para Doenca infecciosa bursal
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O enrolamento do arroz é uma doença viral emergente no Brasil causada pelo Rice stripe necrosis virus (RSNV) que é transmitido pelo protozoário Polymyxa graminis. RSNV é um membro do gênero Benyvirus com genoma dividido em 4 RNAs de fita simples no sentido positivo (ssRNA +). Em função da falta de conhecimento sobre a seqüência de nucleotídeos do seu genoma, a detecção de RSNV através de métodos moleculares não é utilizada. O objetivo deste trabalho foi identificar seqüências do genoma de RSNV que possibilitassem sua detecção em plantas de arroz através da técnica de transcrição reversa seguida da reação em cadeia da polimerase (RT-PCR). As seqüências do genoma foram identificadas a partir de clones de uma biblioteca de cDNAs obtidos de uma amostra do vírus parcialmente purificado. Os clones que hibridizaram com sondas sintetizadas a partir de RNA de plantas infectadas com RSNV foram seqüenciados e comparados às seqüências do GenBank. Um fragmento de 957 nt da extremidade 3’ da fita de um dos 4 RNAs genômicos de RSNV foi obtido. A análise da seqüência nucleotídeos desse fragmento não revelou qualquer similaridade com seqüências conhecidas, tampouco indicou uma possível função. Um par de oligonucleotídeos iniciadores foi desenhado a partir de um clone que potencialmente contém uma seqüência de RSNV. A especificidade e a sensibilidade da RT-PCR utilizando esse par de oligonucleotídeos iniciadores, bem como sua eficiência na detecção do vírus em diferentes partes da planta de arroz, foram avaliadas. Os resultados indicam que a RT-PCR é específica para RSNV e pode detectar o vírus em tecido oriundo das raízes, do colo e de folhas com distorção. Comparada ao diagnóstico da doença através da observação de sintomas e de estruturas do vetor, a RT-PCR é uma ferramenta confiável para a diagnose do enrolamento do arroz.
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A brusone, causada pelo fungo Magnaporthe grisea (Hebert) Barr, é uma das mais importantes doenças da cultura do arroz. A resistência genética é a forma mais efetiva para o controle da doença. Os objetivos do presente trabalho foram: identificar genes envolvidos na resposta de resistência à infecção de M. grisea em arroz através das técnicas de expressão diferencial; obter e caracterizar uma biblioteca de cDNAs utilizando como modelo linhas quase-isogênicas de arroz (NILs = Near Isogenic Lines), contendo os genes de resistência Pi-1 e Pi-2; e avaliar e comparar a expressão diferencial de mRNAs, através dos cDNAs isolados em uma série de cultivares com resposta distinta à infecção de M. grisea. Foram identificados dois isolados com virulência diferencial para as NILs e um isolado para os cultivares. Os cDNAs relacionados à resistência do arroz à M. grisea foram identificados a partir de mRNAs isolados das NILs. Foram obtidos 30 fragmentos de cDNAs e 232 clones de cDNAs pelas técnicas de cDNA-AFLP e SSH, respectivamente. A análise das seqüências permitiu identificar genes envolvidos nos processos de metabolismo, transporte de íon inorgânico; transdução de sinais; fatores de transcrição; metabolismo de coenzima; conversão e produção de energia; metabolismo e transporte de carboidrato e biossíntese de proteína. Noventa clones isolados através da técnica de SSH foram selecionados e a expressão diferencial foi avaliada via hibridização em macroarranjos de cDNAs. A ausência de conservação entre os mRNAs diferencialmente expressos nas interações analisadas e a diversidade dos grupos de genes reflete a complexidade das respostas. A análise funcional in vivo desses genes poderá contribuir para utilização dos mesmos na obtenção de uma resistência de espectro amplo à brusone do arroz.
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A doença de Marek (MD), causada por um alfaherpesvírus, é uma enfermidade linfoproliferativa que acomete principalmente galinhas. Como não existe tratamento, a melhor forma de prevenção e controle da MD é através do uso de vacinas atenuadas, que vêm sendo usadas desde 1970. Este trabalho descreve a análise de vacinas vivas congeladas contra o sorotipo 3 do vírus da doença de Marek (herpesvírus de peru – HVT) por PCR em tempo real (qPCR) e por cultivo em células de embrião de galinha. Foram avaliadas três vacinas (cepa FC126) provenientes de distintos fabricantes. As análises da homogeneidade inter e intra-lote apresentaram, respectivamente, média ± desvio padrão de 2,6 ± 1,7%, 2,1 ± 1,1% e 1,2 ± 0,1% e média ± desvio padrão de 1,5 ± 0,1%, 1,2 ± 0,8% e 1,0 ± 0,3% para A, B e C, respectivamente. A qPCR subestimou os títulos das vacinas concentradas 4x e superestimou os títulos das vacinas diluídas 8x, enquanto o cultivo celular superestimou os títulos das vacinas concentradas. As vacinas apresentaram quantidades diferentes de células/dose e unidade formadoras de placa/dose. Conseqüentemente, a relação PFU/célula também foi diferente, o que demonstra a necessidade de construção de curvas diferentes, para cada fabricante, para a titulação por qPCR.
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Ornithobacterium rhinotracheale é uma bactéria associada com doença respiratória, decréscimo no crescimento, condenação de carcaças e mortalidade em galinhas e perus. Esta bactéria tem sido isolada em vários países e, recentemente, foi isolada no Brasil pelo nosso grupo que também estabeleceu um protocolo de reação em cadeia da polimerase (PCR) para a sua detecção e identificação e determinou a prevalência de anticorpos contra esta bactéria em plantéis comerciais de frangos e de matrizes da Região Sul do Brasil. O presente trabalho teve o objetivo de caracterizar isolados de O. rhinotracheale através de sorotipificação, resistência a antimicrobianos e single-enzyme amplified fragment length polymorphism (SAFLP). Vinte e sete isolados foram compatíveis com esta espécie através de isolamento em ágar sangue com gentamicina, coloração de Gram, teste de aglutinação em lâmina e reação em cadeia da polimerase. Dezenove isolados foram classificados como sorotipo A, seis não puderam ser sorotipificados com o painel de soros existentes e dois pertenceram ao sorotipo C. Vinte e cinco isolados foram sensíveis à norfloxacina, amoxicilina, doxiciclina, lincomicina e cefalotina, dois isolados foram resistentes à neomicina e 18 foram resistentes à sulfametoxazol/trimetoprima. Na análise de SAFLP, 22 isolados apresentaram padrão idêntico e os cinco isolados restantes foram classificados em cinco padrões distintos. Os resultados da sorotipificação indicaram que o sorotipo A de O. rhinotracheale é predominante em criações comerciais no Brasil. Os isolados brasileiros foram sensíveis à maioria dos antimicrobianos testados. O poder discriminatório do teste de suscetibilidade a antimicrobianos foi maior do que a sorotipificação e SAFLP, porém o método de SAFLP gerou um maior número de padrões, sugerindo que possa ser utilizado como ferramenta em estudos epidemiológicos.
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O desenvolvimento de materiais tipo Burley resistente a Murcha Bacteriana é de suma importância para a fumicultura brasileira. Em fumo tipo Burley não existem variedades comerciais com boa adaptação resistentes à R. solanacearum. O objetivo desse trabalho foi determinar o efeito da seleção artificial para resistência à murcha bacteriana na população Burley x Virgínia em diferentes gerações segregantes. Este estudo foi realizado em um infectário de R. solanacearum, localizado em Santa Cruz do Sul, RS. Foi realizado cruzamento entre um cultivar tipo Burley moderadamente resistente (BY 26) e um material tipo Virgínia resistente à murcha (Oxford 207). Foram comparados quatro gerações F1, F3, F5, F7, pai moderadamente resistente (BY 26), pai resistente (OX 207) e uma testemunha suscetível (01528). O delineamento experimental utilizado foi de blocos ao acaso, com quatro repetições e 10 plantas em cada parcela, para uniformizar e aumentar o nível de severidade da moléstia, as plantas foram inoculadas através da deposição de 20 mL de uma suspensão (108 UFC/mL) de R. solanacearum. Para a murcha bacteriana não houve diferença significativa entre as médias das quatro gerações e nem destas com o genitor resistente, já que provavelmente a seleção efetuada em todas as gerações foi suficiente para manter os níveis de resistência observados na geração F1. Observou-se em F7 que várias linhas já estavam fixas com níveis de resistência à murcha semelhante ao genitor resistente. Portanto, os resultados finais mostraram que a seleção artificial foi eficiente para selecionar a resistência à murcha bacteriana, e que é possível transferir resistência a R. solanacearum de fumo Virgínia para fumo tipo Burley – mantendo as características desejadas de cor e tipo do fumo Burley com a resistência similar a do pai resistente.
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No estudo da propagação de uma doença infecciosa, diz-se que sua transmissão ocorre horizontalmente, quando um indivíduo suscetível tem um contato direto ou indireto com um indivíduo infeccioso. Algumas doenças, entretanto, também podem ser transmitidas verticalmente, entendendo-se que, neste caso, a doença é transmitida a um indivíduo, ao ser gerado por uma mãe infecciosa. Fazendo uso de modelos epidemiológicos determinísticos básicos, envolvendo sistemas de equações diferenciais ordinárias, nosso principal objetivo, neste trabalho, consiste em investigar qual o papel da transmissão vertical na propagação de doenças causadas por microparasitas. Diversas formas de inclusão de transmissão vertical são apresentadas e, em cada modelo estudado, investigamos a existência e a estabilidade local dos estados de equilíbrio da população hospedeira, identificamos os parâmetros e limiares que caracterizam a dinâmica do sistema, e completamos as informações decorrentes dos resultados analíticos com a apresentação de soluções numéricas do mesmo. Por fim, comparamos os efeitos da transmissão horizontal com aqueles decorrentes da transmissão vertical.
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Despite advances in antibiotic therapy, bacterial meningitis (BM) remains with high mortality and morbidity rates in worldwide. One important mechanism associated to sequels during disease is the intense inflammatory response which promotes an oxidative burst and release of reactive oxygen species, consequently leading to cell death. Activation of DNA repair enzymes during oxidative stress has been demonstrated in several neurological disorders. APE1/Ref-1 is a multifunctional protein involved in DNA repair and plays a redox function on transcription factors such as NFkB and AP-1.The aim of this study was assess the role of APE1/Ref-1 on inflammatory response and the possibility of its modulation to reduce the sequels of the disease. Firstly it was performed an assay to measure cytokine in cerebrospinal fluid of patients with BM due to Streptococcus pneumoniae and Neisseriae meningitides. Further, a cellular model of inflammation was used to observe the effect of the inhibition of the endonuclease and redox activity of APE1/Ref-1 on cytokine levels. Additionally, APE1/Ref-1 expression in cortex and hippocampus of rat with MB after vitamin B6 treatment was evaluated. Altogether, results showed a similar profile of cytokines in the cerebrospinal fluid of patients from both pathogens, although IFNy showed higher expression in patients with BM caused by S. pneumoniae. On the other hand, inhibitors of APE1/Ref-1 reduced cytokine levels, mainly TNF-α. Reduction of oxidative stress markers was also observed after introduction of inhibitors in the LPS-stimulated cell. In the animal model, BM increased the expression of the protein APE1/Ref-1, while vitamin B6 promoted reduction. Thereby, this data rise important factors to be considered in pathogenesis of BM, e.g., IFNy can be used as prognostic factor during corticosteroid therapy, APE1/Ref-1 can be an important target to modulate the level of inflammation and VIII oxidative stress, and vitamin B6 seems modulates several proteins related to cell death. So, this study highlights a new understanding on the role of APE1/Ref-1 on the inflammation and the oxidative stress during inflammation condition
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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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The main problem faced by the shrimp industry are the infectious diseases. The hypodermal and hematopoietic necrosis infection (IHHN) is one of the major cause of disease in the cultured shrimp, Litopenaeus vannamei. Environmental changes involving water quality, oxygen concentration, salinity, temperature, stocking density, presence of pathogens, among others, triggering a stressing condition for the cultured shrimp, weakening them and allowing the outbreak of diseases. The stress on the animal leads to a change in the molecules immune response components, which can be used as indicators of shrimp health. Thus, the objective of the present study was to evaluate the effect of salinity, stocking density and IHHNV infection on the L. vannamei shrimp. The immune parameters used to check the shrimp health were the total hemocytes counts (THC), the agglutinating activity (AA) and the clotting time (CT) of the serum of shrimp. These parameters were analyzed in healthy and IHHNV-infected shrimp, grown in low (0-0.5 ), medium (19-24 ) and high (> 38 ) salinity, and extensive (7-12 cam.m-2), semi-intensive (15-25 cam.m-2) and intensive (33-45 cam.m -2) stocking density. The IHHNV infection rate was significantly higher in low salinity (P<0.005) and intensive density (P<0.005), both stressful conditions for L. vannamei. Low salinity significantly increased THC (P<0.05) and decreased and CT (P<0.05) in healthy and infected shrimp, but AA (P<0.05) significantly decreased in healthy shrimp at medium salinity. Culture intensification did not affect the THC, AA and CT of healthy and infected shrimp (P>0.05). The IHHNV infection did not affect any immune parameters of shrimp cultured at different salinities and stocking densities. It is necessary to emphasize that this study was conducted in shrimp grown in ponds, where several environmental factors are acting simultaneously. Thus, further studies are needed about the influence of other environmental factors on the immune parameters of shrimp cultured in pond
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Malaria, also popularly known as maleita , intermittent fever, paludism, impaludism, third fever or fourth fever, is an acute infectious febrile disease, which, in human beings, is caused by four species: Plasmodium falciparum, P. vivax, P. malariae and P. ovale. Malaria, one of the main infectious diseases in the world, is the most important parasitoses, with 250 million annual cases and more than 1 million deaths per year, mainly in children younger than live years of age. The prophylactic and therapeutic arsenal against malaria is quite restricted, since all the antimalarials currently in use have some limitation. Many plant species belonging to several families have been tested in vivo, using the murine experimental model Plasmodium berghei or in vitro against P. falciparum, and this search has been directed toward plants with antithermal, antimalarial or antiinflammatory properties used in popular Brazilian bolk medicine. Studies assessing the biological activity of medicinal plant essential oils have revealed activities of interest, such as insecticidal, spasmolytic and antiplasmodic action. It has also been scientifically established that around 60% of essential oils have antifungal properties and that 35% exhibit antibacterial properties. In our investigation, essential oils were obtained from the species Vanillosmopsis arborea, Lippia sidoides and Croton zethneri which are found in the bioregion of Araripe-Ceará. The chemical composition of these essential oils was partially characterized and the presence of monoterpenes and sesquiterpenes. The acute toxicity of these oils was assessed in healthy mice at different doses applied on a single day and on four consecutive days, and in vitro cytotoxicity in HeLa and Raw cell lines was determined at different concentrations. The in vivo tests obtained lethal dose values of 7,1 mg/Kg (doses administered on a single day) and 1,8 mg/Kg (doses administered over four days) for 50% of the animals. In the in vitro tests, the inhibitory concentration for 50% of cell growth in Hela cell lines was 588 μg/mL (essential oil from C. zethneri after 48 h), from 340-555 μg/mL (essential oil from L. sidoides, after 24 and 48 h). The essential oil from V. arborea showed no cytotoxicity and none of the essential oils were cytotoxic in Raw cell lines. These data suggest a moderate toxicity in the essential XVIII oils under study, a finding that does not impede their testing in in vivo antimalarial assays. Was shown the antimalarial activity of the essential oils in mice infected with P. berghei was assessed. The three species showed antimalarial activity from 36%-57% for the essential oil from the stem of V. arborea; from 32%-82% for the essential oil from the leaves of L. sidoides and from 40%-70% of reduction for the essential oil from the leaves of C. zethneri. This is the first study showing evidence of antimalarial activity with these species from northeast Brazil. Further studies to isolate the active ingredients of these oils are needed to determine if a single active ingredient accounts for the antimalarial activity or if a complex integration of all the compounds present occurs, a situation reflected in their biological activity
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Known for thousands of years, tuberculosis (TB) is the leading cause of mortality by a single infectious disease due to lack of patient adherence to available treatment regimens, the rising of multidrug resistant strains of TB (MDR-TB) and co-infection with HIV virus. Isoniazid and rifampicin are the most powerful bactericidal agents against M. tuberculosis. Because of that, this couple of drugs becomes unanimity in anti-TB treatment around the world. However, the rifampicin in acidic conditions in the stomach can be degraded rapidly, especially in the presence of isoniazid, which reduces the amount of available drug for absorption, as well as its bioavailability, contributing to the growing resistance to tuberculostatic drugs. Rifampicin is well absorbed in the stomach because of its high solubility between pH 1 and 2 and the gastric absorption of isoniazid is considered poor, therefore it is mostly intestinal. This work has as objective the development of gastro-resistant multiple-systems (granules and pellets) of isoniazid aiming to prevent the contact with rifampicin, with consequent degradation in acid stomach and modulate the release of isoniazid in the intestine. Granules of isoniazid were obtained by wet method using both alcoholic and aqueous solutions of PVP K-30 as aggregating and binder agent, at proportions of 5, 8 and 10%. The influence of the excipients (starch, cellulose or filler default) on the physical and technological properties of the granules was investigated. The pellets were produced by extrusionesferonization technique using isoniazid and microcrystalline cellulose MC 101 (at the proportion of 85:15) and aqueous solution of 1% Methocel as platelet. The pellets presented advantages over granular, such as: higher apparent density, smaller difference between apparent and compaction densities, smoother surface and, especially, smaller friability, and then were coated with an organic solution of Acrycoat L 100 ® in a fluidized bed. Different percentages of coating (15, 25 and 50%) were applied to the pellets which had their behavior evaluated in vitro by dissolution in acidic and basic medium. Rifampicin dissolution in the presence of uncoated and coated isoniazid pellets was evaluated too. The results indicate that the gastro resistance was only achieved with the greatest amount of coating and isoniazid is released successfully in basic step. The amount of rifampicin in the dissolution medium when the isoniazid pellets were not coated was lower than in the presence of enteric release pellets. Therefore, the polymer Acrycoat L 100 ® was efficient for coating with gastro-resistant function and can solve the problem of low bioavailability of rifampicin and help to reduce its dosage
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The Chagas disease is a infectious and parasite disease that has as the causative agent a Trypanosoma cruzi, a protozoan parasite that can be transmitted to humans by the faeces of triatomines ( barbeiros ) in the blood-sucking. To understand the relationship between factors associated with chagasic infection and the risk of transmission of Trypanosoma cruzi, this work aimed to make a correlation between the results of serology, obtained by different immunological techniques, used for diagnosis of Chagas disease and risk factors to which the population of the city of Apodi-RN is exposed, to be considered a endemic area. The case-control study was conducted with 199 individuals, which initially was applied a questionary about socio-economic questions and some risk factors which they were exposed and also favor the spread of disease. Then was given the diagnosis by immunological techniques of serology by indirect hemagglutination, ELISA and indirect immunofluorescence. From the diagnosis, the subjects were divided into case group (presence of infection) and control group (no infection). Regarding the descriptive characteristics of the sample, were found a higher frequency of female individuals (59.3%), between 36 and 50 years of age (36.7%), with low education level (91%) and income monthly up to 1 minimum wage (67.8%). The serology, performed by three techniques of different principles, had a reactivity of 38.9% by Indirect Hemagglutination, 39.7% by ELISA and 38.7% by Indirect Immunofluorescence. As the result of the serology, 71 of samples showed reactivity in 2 or more techniques. On some risk variables, was found a significant relationship between individuals who had been bitten by the triatomines and had positive serology for Chagas disease (93.3%). Other variables of risk revealed individuals who had positive serology and had domestic animal (80.3%), lived in poorly maintained homes (97.2%) and near the forest (84.5%). A better understanding of the dynamics of transmission of T. cruzi and the risk factors that contribute to its occurrence in a region are needed to develop effective strategies for control of Chagas disease in these áreas
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Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
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Several studies demonstrate that environmental temperature can influence the immune response of poultry. The objective of this research was to determine at which stage in the life of a bird this effect is greatest. In experiment 1, broiler breeder eggs were incubated at three different temperatures (36.8+/-0.2, 37.8+/-0.2, and 38.8+/-0.2degreesC from the 13th day of incubation to hatching. After hatching, birds were raised in thermoneutral temperature. In experiment 2, 144 1-d-old broiler chicks were distributed into three environmental chambers with different temperatures (18+/-2, 24+/-2, and 32+/-2degreesC). In both experiments, the humoral immune responses to Newcastle disease virus (NDV) and infectious bursal disease (IBDV) were evaluated. NDV and IBDV antibody titers were not significantly different (P > 0.05) among treatments.
