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Avaliação da Proteína C Reativa como marcador inflamatório e de seu potencial para monitoração terapêutica em casos de pênfigo foliáceo e de piodermite superficial na espécie canina / Evaluation of C- Reactive Protein as an inflammatory marker and its potential for therapeutic monitoring in cases of canine pemphigus foliaceus and superficial pyoderma in dogsSevero, Júlia Só 19 August 2015 (has links)
O pênfigo foliáceo inclui-se em um grupo de dermatoses autoimunes vésico-bolhosas da pele e mucosas reconhecido em alguns mamíferos, incluíndo os cães. Muitos autores acreditam que o pênfigo foliáceo (PF) é a dermatopatia autoimune mais frequentemente observada em caninos. Muitas podem ser as enfermidades caninas que devem ser incluídas no diagnóstico diferencial do pênfigo foliáceo, principalmente, a piodermite superficial (PS). A Proteína C Reativa (PCr) é conhecida como a principal proteína de fase aguda em cães. Nesses espécimes, a elevação da PCr tem sido observada em ampla variedade de condições mórbidas. A determinação da PCr tem sido proposta como um marcador inflamatório de algumas doenças autoimunes. O objetivo deste estudo foi determinar se a Proteína C Reativa pode ser utilizada como um marcador biológico precoce para diferenciar o pênfigo foliáceo da piodermite superficial em cães. Esta pesquisa constituiu um estudo clínico observacional prospectivo longitudinal, realizada em cães acometidos pelo PF ou PS. Foram incluídos 59 cães divididos em três Grupos I (Controle) com 31 animais, II (PF) e III (PS), cada um constituído por 14 cães. Submeteram-se, respectivamente, fragmentos cutâneos e soros de caninos, acometidos por PF ou PS, a exames histopatologicos e imunofluorescência direta (IFD) e à determinação de PCr e, também, a imunofluorescência indireta (IFI), utilizando-se para essa última coxins palmo-plantares a título de substrato. O grau de acometimento dos pacientes penfigosos (Grupo II) foi avaliado pelo PEFESI, durante período de até 90 dias, em diferentes momentos em que se realizou a IFI e a avaliação da PCr. Comparando-se os valores de IFD com aqueles da histopatologia obtiveram-se valores geral de concordância de 75% (9/12) e Índice Kappa de 0,77 (p<0,001) e, também, concordância dita substancial entre os dois métodos. Já, na IFI o valor de concordância foi de 100% (14/14), o de Kappa de 1,0 (p<0,001), com concordância considerada perfeita entre a IFI e a histopatologia. O Grupo II apresentou maior valor de mediana de PCr (37,4µg/mL) quando comparado aos Grupos I, com 2,9 µg/mL (p<0,0001) e III, com 3,8 µg/mL (p=0,008). Não houve diferença entre os Grupos I e III (p=0,178). Considerando-se como ponto de corte um valor de PCr > 10,6µg/mL, a chance de um animal estar acometido pelo PF é 5,5 vezes maior àquela de um cão não afetado, o que equivale a uma probabilidade pós-teste de 84,6%, conferindo um acréscimo de 34,6% na capacidade de diagnóstico do PF. Conclui-se que determinação de PCr é de inequívoca valia para o estabelecimento de diferenciação diagnóstica entre a casuística da contumaz piodermite superficial com quadros do pênfigo foliáceo canino / Pemphigus is included in a group of skin and mucous autoimmune vesicobullous dermatoses recognized in some mammals, including dogs. Many authors believe that pemphigus foliaceus (PF) is the autoimmune skin disease most often observed in dogs. Many must be the canine diseases considered in the pemphigus foliaceus differential diagnosis, especially the superficial pyoderma (SP). The C-Reactive Protein (CRP) is known as a major acute phase protein in dogs. The CRP increase has been observed in a wide variety of morbid conditions in dogs. The determination of CRP has been proposed as an inflammatory marker of some autoimmune diseases. This study aimed to determine whether C-Reactive Protein can be used as an early biomarker to differentiate pemphigus foliaceus of superficial pyoderma in dogs. An observational prospective longitudinal clinical study was undertaken including dogs affected by PF or PS. Fifth nine dogs were divided into three groups: Group I (Control) with 31 animals and II (PF) and III (SP), consisting of 14 dogs each. Dogs affected by PF or SP had skin fragments submitted to histopathological examination and direct immunofluorescent reaction (DIF). The blood sera were used to determine the CRP concentration, and also to perform the indirect imunofluorescent reaction (IIF) using canine footpad as substrate. The pemphigus patients (Group II) clinical involvement degree was evaluated by PEFESI, over a period of 90 days, moments in which IFI and evaluation of CRP took place. Comparing the DIF values with the histopathology there was an agreement of 75% (9/12) with a Kappa index of 0.77 (p <0.001) which means a degree of substantial arrangement between the two methods. Considering IIF, the agreement value was 100% (14/14) with Kappa index of 1.0 (p<0.001), showing perfect arrangement between the IIF and the histopathology. Group II showed higher CRP median (37.4 mg / mL) compared to Groups I, with 2.9 mg / mL (p <0.0001) and III with 3.8 mg / mL (p = 0.008 ). There was no statistic difference between groups I and III (p = 0.178). Considering CRP> 10,6µg / mL as a cutoff value, the chance of an animal having PF is 5.5 times higher than not to be, which is equivalent to a post-test probability of 84,6%, giving a 34.6% increase in the PF diagnostic capability. It concludes that determination of CRP is unequivocal asset for the establishment of diagnostic differentiation between the common superficial pyoderma to canine pemphigus foliaceus
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Avaliação da Proteína C Reativa como marcador inflamatório e de seu potencial para monitoração terapêutica em casos de pênfigo foliáceo e de piodermite superficial na espécie canina / Evaluation of C- Reactive Protein as an inflammatory marker and its potential for therapeutic monitoring in cases of canine pemphigus foliaceus and superficial pyoderma in dogsJúlia Só Severo 19 August 2015 (has links)
O pênfigo foliáceo inclui-se em um grupo de dermatoses autoimunes vésico-bolhosas da pele e mucosas reconhecido em alguns mamíferos, incluíndo os cães. Muitos autores acreditam que o pênfigo foliáceo (PF) é a dermatopatia autoimune mais frequentemente observada em caninos. Muitas podem ser as enfermidades caninas que devem ser incluídas no diagnóstico diferencial do pênfigo foliáceo, principalmente, a piodermite superficial (PS). A Proteína C Reativa (PCr) é conhecida como a principal proteína de fase aguda em cães. Nesses espécimes, a elevação da PCr tem sido observada em ampla variedade de condições mórbidas. A determinação da PCr tem sido proposta como um marcador inflamatório de algumas doenças autoimunes. O objetivo deste estudo foi determinar se a Proteína C Reativa pode ser utilizada como um marcador biológico precoce para diferenciar o pênfigo foliáceo da piodermite superficial em cães. Esta pesquisa constituiu um estudo clínico observacional prospectivo longitudinal, realizada em cães acometidos pelo PF ou PS. Foram incluídos 59 cães divididos em três Grupos I (Controle) com 31 animais, II (PF) e III (PS), cada um constituído por 14 cães. Submeteram-se, respectivamente, fragmentos cutâneos e soros de caninos, acometidos por PF ou PS, a exames histopatologicos e imunofluorescência direta (IFD) e à determinação de PCr e, também, a imunofluorescência indireta (IFI), utilizando-se para essa última coxins palmo-plantares a título de substrato. O grau de acometimento dos pacientes penfigosos (Grupo II) foi avaliado pelo PEFESI, durante período de até 90 dias, em diferentes momentos em que se realizou a IFI e a avaliação da PCr. Comparando-se os valores de IFD com aqueles da histopatologia obtiveram-se valores geral de concordância de 75% (9/12) e Índice Kappa de 0,77 (p<0,001) e, também, concordância dita substancial entre os dois métodos. Já, na IFI o valor de concordância foi de 100% (14/14), o de Kappa de 1,0 (p<0,001), com concordância considerada perfeita entre a IFI e a histopatologia. O Grupo II apresentou maior valor de mediana de PCr (37,4µg/mL) quando comparado aos Grupos I, com 2,9 µg/mL (p<0,0001) e III, com 3,8 µg/mL (p=0,008). Não houve diferença entre os Grupos I e III (p=0,178). Considerando-se como ponto de corte um valor de PCr > 10,6µg/mL, a chance de um animal estar acometido pelo PF é 5,5 vezes maior àquela de um cão não afetado, o que equivale a uma probabilidade pós-teste de 84,6%, conferindo um acréscimo de 34,6% na capacidade de diagnóstico do PF. Conclui-se que determinação de PCr é de inequívoca valia para o estabelecimento de diferenciação diagnóstica entre a casuística da contumaz piodermite superficial com quadros do pênfigo foliáceo canino / Pemphigus is included in a group of skin and mucous autoimmune vesicobullous dermatoses recognized in some mammals, including dogs. Many authors believe that pemphigus foliaceus (PF) is the autoimmune skin disease most often observed in dogs. Many must be the canine diseases considered in the pemphigus foliaceus differential diagnosis, especially the superficial pyoderma (SP). The C-Reactive Protein (CRP) is known as a major acute phase protein in dogs. The CRP increase has been observed in a wide variety of morbid conditions in dogs. The determination of CRP has been proposed as an inflammatory marker of some autoimmune diseases. This study aimed to determine whether C-Reactive Protein can be used as an early biomarker to differentiate pemphigus foliaceus of superficial pyoderma in dogs. An observational prospective longitudinal clinical study was undertaken including dogs affected by PF or PS. Fifth nine dogs were divided into three groups: Group I (Control) with 31 animals and II (PF) and III (SP), consisting of 14 dogs each. Dogs affected by PF or SP had skin fragments submitted to histopathological examination and direct immunofluorescent reaction (DIF). The blood sera were used to determine the CRP concentration, and also to perform the indirect imunofluorescent reaction (IIF) using canine footpad as substrate. The pemphigus patients (Group II) clinical involvement degree was evaluated by PEFESI, over a period of 90 days, moments in which IFI and evaluation of CRP took place. Comparing the DIF values with the histopathology there was an agreement of 75% (9/12) with a Kappa index of 0.77 (p <0.001) which means a degree of substantial arrangement between the two methods. Considering IIF, the agreement value was 100% (14/14) with Kappa index of 1.0 (p<0.001), showing perfect arrangement between the IIF and the histopathology. Group II showed higher CRP median (37.4 mg / mL) compared to Groups I, with 2.9 mg / mL (p <0.0001) and III with 3.8 mg / mL (p = 0.008 ). There was no statistic difference between groups I and III (p = 0.178). Considering CRP> 10,6µg / mL as a cutoff value, the chance of an animal having PF is 5.5 times higher than not to be, which is equivalent to a post-test probability of 84,6%, giving a 34.6% increase in the PF diagnostic capability. It concludes that determination of CRP is unequivocal asset for the establishment of diagnostic differentiation between the common superficial pyoderma to canine pemphigus foliaceus
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Immunological assays relevant to definition of bovine theileria parva-specific cytotoxic CD8+ T cell responsesMusembi, Susan Mbithe January 2012 (has links)
A major objective in Theileria parva subunit vaccine development is to induce a vaccine antigen specific response mediated by cytotoxic CD8+ T cells (CTL). Therefore it is essential to be able to measure the frequency of the responding CD8+ T cells after vaccination and correlate it with a clinical outcome on challenge. Recently concluded immunogenicity and efficacy studies of T. parva specific CTL antigens showed successful induction of CTL responses in some animals, which correlated with reduced disease severity after challenge. To provide correlates of immunity antigen-specific CD8+ T cell mediated IFN-γ responses and CTL lytic responses were measured over the course of the experiments. Several challenges presented in these trials aimed at optimising vaccine efficacy. While the IFN-γ ELISPOT is a sensitive and reliable assay widely used in vaccine research, the use of chromium/indium release assay remains to be the only assay in use that measures T. parva-specific CTL activity. Hence the overall goal of the study was to develop novel reagents and novel assays to identify parasite-specific CD8+ T lymphocytes with lytic potential. To address this objective, bovine perforin, granzymes A and B, as specific effector proteins expressed in activated CTL were cloned and expressed using a baculovirus expression system. Sequence analysis of the cloned cDNAs showed the isolated cDNA belonged to the perforin and granzyme sub-families respectively. Perforin cDNA demonstrated 85% homology to human perforin with presence of conserved regions resembling calcium binding motif, membrane attack complex component as well complement protein. The sequences encoded by the cloned granzyme A and B cDNAs have the features of a trypsin like serine protease and demonstrates over 70% homology to the human cDNA over the active enzyme region as well catalytic residues characteristic of serine proteases. The expressed polypeptides of all three proteins were used to produce specific antibodies for use as reagents in immunoassays including ELISpot and intracellular staining for flow cytometric analysis. While the antibodies showed reactivity to the recombinant proteins, these reagents displayed different functionality in the recognition of the native protein. Peptide-major histocompatibility complexes (MHC) class I tetrameric complexes (tetramers) are proving invaluable as fluorescent reagents for enumeration, characterisation and isolation of peptide-specific CD8+ T cells and have afforded advantages to phenotype antigen-specific T cells with minimal in vitro manipulation. Fluorescent bovine tetramers were shown to specifically stain antigen-specific CTL by directly binding the T cell receptor (TCR). Analyses of CD8 T-cell responses in live-vaccine immunised cattle also showed that this method is robust and demonstrates changes in the kinetics and specificity of the CD8+ T cell response in primary and secondary infections with T. parva. On average, results of functional assays and tetramer staining followed parallel trends, measured roughly the same populations and allowed for surface and intracellular staining for CD8 T cell marker and perforin, respectively, demonstrating a method that reliably quantifies the frequency, phenotype and function of specific CD8+ T cells. The technical simplicity, rapidity and ability of the flow cytometric technique described in this thesis to measure low frequency antigen-specific responses suggests that tetramer staining, combined with functional assays could be broadly applicable to the valuation of vaccination efficacy to determine which protocols are most successful in inducing CTL responses.
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