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Detection of the fluorescing group of Pseudomonas by enzyme-linked immunosorbent assay (ELISA) for the prediction of shelf-life of dairy productsDishart, Katy Johanna 04 August 2009 (has links)
An enzyme-linked immunosorbent assay (ELISA) using polyclonal antibodies has been developed for the detection of the fluorescing group of Pseudomonas. The assay was used as a rapid test (6h) for predicting the shelf-life of pasteurized fluid milk. Milk samples were held at 7°C and tested weekly until determined to be unacceptable by daily sensory evaluation. Sterile milk samples were inoculated with target concentrations of 0 (control), 100, and 1000 cells/ml of Pseudomonas fluorescens on day 0. Samples were tested before and after preliminary incubations. Preliminary incubations conducted include milk alone and milk with broth (1:1) for 18h at 21°C. ELISA and plate counts were performed before and after preliminary incubation to determine the number of pseudomonads present and the relationship between ELISA and plate counts. These numbers were correlated to the shelf-life of each sample, as determined by sensory evaluation. Samples undergoing a preliminary incubation with only milk gave the best correlation to shelf-life (R=0.86). / Master of Science
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Effects of using an enzyme-linked immunosorbent assay to monitor the control of Staphylococcus aureus mastitis in dairy herdsGrove, Tina Moler 14 April 2009 (has links)
Bovine mastitis is the most important economic disease to the dairy industry with losses estimated at 2 billion dollars per year in the United States. Staphylococcus aureus (.§.. aureus) is the primary cause of contagious mastitis. Conventional culture methods (National Mastitis Council) were used as a basis for comparing the ability of the enzyme linked immunosorbent assay. ProStaph Iâ ¢, to identify s. aureus. The test had an accuracy of 96%, with a sensitivity of 90% and a specificity of 97%. Results indicated that rinsing teat-cup liners with a 25 ppm iodophor or 100 ppm chlorine solution reduced the presence of S. aureus on the liners by 97%. ProStaph I was used to rapidly screen DHIA preserved milk samples in 10 Virginia cooperator herds. Herds were classified as high (>10% infected) or low prevalence (<10% infected). There were six high prevalence herds after the first test. Average prevalence of cows scoring Ab +2 and +3 was 11.9% ± 7.9. Over the seven month study, prevalence of positive cows declined significantly (P<.OI), but somatic cell count remained relatively unchanged (P>.lO). Four herds continued to have >10% of the animals infected. Incidence of new infection averaged 3.6% ± 2.8 from the first to the last test. Chronic cows averaged 6.9% ± 4.8 over the seven month study. Analysis of variance showed significant (P<.Ol) effects of herd on ProStaph I score J milk yield, and see. Elevated ProStaph I scores were highly correlated (P <.01) with increases in lactation number. ProStaph I changed quadratically (P<.Ol) with increasing SCC. Somatic cell count increased (P<.OI) as ProStaph I score increased. / Master of Science
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Release kinetics of tumor necrosis factor-α and interleukin-1 receptor antagonist in the equine whole bloodRütten, Simon, Schusser, Gerald F., Abraham, Getu, Schrödl, Wieland 21 June 2016 (has links) (PDF)
Background: Horses are much predisposed and susceptible to excessive and acute inflammatory responses that cause the recruitment and stimulation of polymorphnuclear granulocytes (PMN) together with peripheral blood mononuclear cells (PBMC) and the release of cytokines. The aim of the study is to develop easy, quick, cheap and reproducible methods for measuring tumor necrosis factor alpha (TNF-α) and interleukin-1 receptor antagonist (IL-1Ra) in the equine whole blood cultures ex-vivo time- and concentration dependently. Results: Horse whole blood diluted to 10, 20 and 50 % was stimulated with lipopolysaccharide (LPS), PCPwL (a combination of phytohemagglutinin E, concanavalin A and pokeweed mitogen) or equine recombinant TNF-α (erTNF-α). TNF-α and IL-1Ra were analyzed in culture supernatants, which were collected at different time points using specific enzyme-linked immunosorbent assays (ELISA). Both cytokines could be detected optimal in stimulated 20 % whole blood cultures. TNF-α and IL-1Ra releases were time-dependent but the kinetic was different between them. PCPwL-induced TNF-α and IL-1Ra release was enhanced continuously over 24–48 h, respectively. Similarly, LPS-stimulated TNF-α was at maximum at time points between 8–12 h and started to decrease thereafter, whereas IL-1Ra peaked later between 12–24 h and rather continued to accumulate over 48 h. The equine recombinant TNF-α could induce also the IL-1Ra release. Conclusions: Our results demonstrate that similar to PCPwL, LPS stimulated TNF-α and IL-1Ra production time-dependently in whole blood cultures, suggesting the suitability of whole blood cultures to assess the release of a variety of cytokines in health and diseases of horse.
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Release kinetics of tumor necrosis factor-α and interleukin-1 receptor antagonist in the equine whole bloodRütten, Simon, Schusser, Gerald F., Abraham, Getu, Schrödl, Wieland January 2016 (has links)
Background: Horses are much predisposed and susceptible to excessive and acute inflammatory responses that cause the recruitment and stimulation of polymorphnuclear granulocytes (PMN) together with peripheral blood mononuclear cells (PBMC) and the release of cytokines. The aim of the study is to develop easy, quick, cheap and reproducible methods for measuring tumor necrosis factor alpha (TNF-α) and interleukin-1 receptor antagonist (IL-1Ra) in the equine whole blood cultures ex-vivo time- and concentration dependently. Results: Horse whole blood diluted to 10, 20 and 50 % was stimulated with lipopolysaccharide (LPS), PCPwL (a combination of phytohemagglutinin E, concanavalin A and pokeweed mitogen) or equine recombinant TNF-α (erTNF-α). TNF-α and IL-1Ra were analyzed in culture supernatants, which were collected at different time points using specific enzyme-linked immunosorbent assays (ELISA). Both cytokines could be detected optimal in stimulated 20 % whole blood cultures. TNF-α and IL-1Ra releases were time-dependent but the kinetic was different between them. PCPwL-induced TNF-α and IL-1Ra release was enhanced continuously over 24–48 h, respectively. Similarly, LPS-stimulated TNF-α was at maximum at time points between 8–12 h and started to decrease thereafter, whereas IL-1Ra peaked later between 12–24 h and rather continued to accumulate over 48 h. The equine recombinant TNF-α could induce also the IL-1Ra release. Conclusions: Our results demonstrate that similar to PCPwL, LPS stimulated TNF-α and IL-1Ra production time-dependently in whole blood cultures, suggesting the suitability of whole blood cultures to assess the release of a variety of cytokines in health and diseases of horse.
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Analys av antikroppar mot <em>Moraxella catarrhalis</em> hos patienter med multipelt myelom, Waldenströms makroglobulinemi och monoklonal gammopati av oklar signifikans med ”enzyme-linked immunosorbent assay”Erman, Evelina January 2010 (has links)
<p>Försämrat immunförsvar och ökad risk att drabbas av bakterie- och virusinfektioner förekommer hos patienter med blodsjukdomarna multipelt myelom, Waldenströms makroglobulinemi samt hos vissa patienter med blodsjukdomen monoklonal gammopati av oklar signifikans. Infektionerna kräver ofta antibiotikabehandling och behandling med antivirala medel. I dagsläget är det svårt att förutsäga vilka av patienterna som kommer att drabbas av svåra och ibland livshotande infektioner. Därför ges många av patienterna förebyggande antibiotikabehandling.</p><p>I studiens början sattes en enzyme-linked immunosorbent assay (ELISA) för detektion av antikroppar mot <em>Moraxella catarrhalis </em>upp. I studien undersöktes om antikroppstitrar i serum mot bakterien <em>Moraxella catarrhalis</em> var lägre hos patientgrupperna än hos friska kontrollpersoner i samma ålder och om variationer förekom mellan patientgrupperna samt hur kontrollgrupper i olika åldrar skiljde sig från varandra. Kontrollgrupperna som undersöktes var mellan 20-40 år, 40-60 år samt 60 år och äldre.</p><p>Resultatet var att patienterna med multipelt myelom hade lägst antikroppstitrar, patienter med monoklonal gammopati av oklar signifikans hade något högre och patienter med Waldenströms makroglobulinemi hade ännu högre antikroppstitrar. Kontrollgruppen äldre än 60 år hade högre antikroppstitrar än både kontrollgruppen 20-40 år och 40-60 år. Lägst antikroppstitrar hade kontrollgrupp 40-60 år men ingen signifikant skillnad påvisades mellan kontrollgrupp 20-40 år och 40-60 år.</p>
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Identificação de fonte sanguínea em dípteros da Família Culicidae, em áreas de epizootia da febre amarela silvestre / Identification of blood source in the family Culicidae flies, in areas of outbreak of jungle yellow feverMarassa, Ana Maria 16 June 2009 (has links)
A importância em conhecer o padrão alimentar em mosquitos da Família Culicidae permite esclarecer alguns aspectos relacionados à transmissão de zoonoses e estimar o grau de contato humano-vetor que é fator relevante em estudos epidemiológicos. Com o objetivo de explorar o comportamento alimentar dessa Família, em área epizoótica de febre amarela silvestre, foram coletados exemplares nos municípios de Santo Antônio das Missões e Garruchos, Estado do Rio Grande do Sul. Fêmeas ingurgitadas foram obtidas por aspiração em ambiente de mata, no período de setembro de 2005 a abril de 2007 e identificadas segundo fonte de sangue ingerido através da técnica imunoenzimática ELISA de captura no sistema avidinabiotina. Foram testadas seis fontes de alimento: ave, bovino, eqüino, humano, macaco e rato. Os resultados obtidos mediante a padronização de anticorpos monoclonais possibilitaram demonstrar pela primeira vez o reconhecimento de sangue humano ingerido nesses mosquitos pelo emprego da subclasse IgG1 e comprovar a sensibilidade e especificidade da técnica ELISA de captura. No município de Santo Antônio das Missões, de um total de 190 amostras, 60,9% reagiram para sangue de boi, 23,6% para humano, 9,9% para ave, 1,9% para macaco e 3,7% para combinações de dois hospedeiros. Quanto às amostras referentes ao município de Garruchos, das 158 fêmeas capturadas na área Cachoeirinha pode-se observar reatividade para ave (16%), boi (29,6%), humano (36,8%), cavalo (4%), macaco (0,8%) e combinações de hospedeiros (12,8%), enquanto que para as 149 fêmeas pertencentes à área de São José, detectou-se sangue ingerido de boi em (51,5%), ave e humano (11,5%), macaco (6,2%), cavalo (0,8%) e mistos (18,5%). Aedes scapularis, Aedes crinifer, Culex (Culex) spp., Haemagogus leucocelaenus apresentaram maior número de fêmeas ingurgitadas nos dois municípios. Os resultados obtidos com Aedes scapularis sugerem ecletismo, conforme combinações detectadas em amostras de sangue de diferentes fontes. Haemagogus leucocelaenus apresentou a maior proporção de amostras contendo sangue humano em relação às demais fontes e essa característica traz implicações, por ser espécie incriminada na transmissão e por se tratar de área de ocorrência de epizootias de febre amarela. / The knowledge of mosquitoes Culicidae host feeding patterns permits to clarify some aspects related to zoonosis transmission and to estimate the degree of human-vector contact which is relevant in epidemiological studies. Aiming to explore the feeding behavior of these mosquitoes, specimens were collected in the municipalities of Santo Antônio das Missões and Garruchos, Rio Grande do Sul, an epizootic area of sylvatic yellow fever. Engorged females were collected by aspiration from forested areas from September 2005-April 2007 and their blood meals were identified using the avidin-biotin system of immunoenzymatic ELISA capture. Six blood meal sources were tested: bird, cattle, horse, human, monkey and rat. The result achieved with the species-specific IgG1 mAb was unprecedented for mosquito blood meal identification and reinforced the sensibility and specificity of the immunoenzymatic ELISA capture. Of the 190 samples from Santo Antônio das Missões, 60.9% reacted to cattle, 23.6% to human, 9.9% to bird, 1.9% to monkey and 3.7% to mixed blood meals. In Garruchos, of the 158 females collected in Cachoeirinha, 16.0% reacted to bird, 29.6% to cattle, 36.8% to human, 4.0% to horse, 0.8% to monkey and 12.8% to mixed blood, while of the 149 engorged females from São José, blood from cattle accounted for 51.5%, of blood identified, bird and human 11.5%, monkey 6.2%, horse 0.8% and mixed blood 18.5%. Blood engorged females of Aedes scapularis, Aedes crinifer, Culex (Culex) spp., Haemagogus leucocelaenus predominated in the two municipalities. The results obtained with Aedes scapularis suggests its eclecticism, according to the combinations of blood which were detected from different sources. Haemagogus leucocelaenus was found to have the highest proportion of samples containing human blood in comparison with other sources, which has implications, on account of being incriminated in the transmission and also for taking into consideration the outbreaks reported that underline the risk of yellow fever.
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Alpha Glutationa S Transferase: marcador de lesão hepática em pacientes com hepatite pelo vírus C? / Alpha Glutathione S Transferase: a marker of liver damage in hepatitis C virus patients?Oliveira Júnior, Evandro Antônio Bentes de 07 January 2005 (has links)
INTRODUÇÃO E OBJETIVOS: A a-Glutathiona-S-transferase (aGST) vem sendo proposta como um marcador sensível e não-invasivo de lesão hepática em pacientes com Hepatite pelo vírus C. Avaliamos neste trabalho como a (aGST) se correlaciona com características bioquímicas e histológicas em pacientes com HCV. MATERIAL E MÉTODOS: Realizamos a determinação da concentração plasmática das aGST, alanina aminotransferase (ALT), aspartato aminotransferase (AST) e gama-glutamyltransferase (gGT) em 114 pacientes com HCV, dos quais 97 foram submetidos à biópsia hepática em até 6 meses da realização dos testes bioquímicos. Avaliamos também os níveis de aGST em 66 doadores de sangue sadios, que serviram como controles. Comparamos os níveis de aGST com as demais provas bioquímicas e a histologia hepática. RESULTADOS: A aGST estava elevada em 85.96% dos pacientes com HCV e mostrou associação com a elevação das aminotransferases (p<0.01). O valor de 4mg/dL mostrou as melhores sensibilidade (85,96%) e especificidade (92,42%) para determinar a normalidade do teste aGST. aGST ³ 8mg/dL mostrou a melhor especificidade para determinar lesão histológica hepática mais agressiva e o melhor valor preditivo positivo e razão de verossimilhança positiva para inflamação portal e atividade parenquimatosa mais agressiva nos pacientes com HCV. CONCLUSÕES: A aGST está relacionada à lesão hepática na infecção pelo HCV (valor de corte = 4mg/dL) e lesões histológicas hepáticas mais agressivas (valor de corte = 8mg/dL). Neste contexto, a aGST poderia ser utilizada em pacientes com Hepatite pelo HCV com ALT elevada, como um indicador complementar de lesão histopatológica mais agressiva. Entretanto, seu valor preditivo positivo não é suficientemente elevado para evitar a necessidade de realizar a biópsia hepática, mesmo quando está acima de 8mg/dL. / BACKGROUND/AIMS: a-Glutathione-S-transferase (aGST) has been proposed as a sensitive non-invasive indicator of hepatocellular injury due to Hepatitis C virus (HCV) infection. In this work, we evaluate how alpha-GST concentration correlates with biochemical and histological features in HCV patients. METHODS: We assayed plasma aGST, alanine aminotransferase (ALT), spartate aminotransferase (AST) and gama-glutamyl-transferase (gGT) in 114 HCV+ patients, among whom liver biopsy was performed in 97, within 6 months of the biochemical evaluation. We also assessed aGST levels in 66 health blood donors, aimed to serve as control. We compared aGST levels with other biochemical tests and liver histology. RESULTS: In 85.96% of HCV patients aGST was elevated and showed association with serum aminotransferases (p<0.01). The value of 4mg/dL (or lower) showed the best sensitivity (85.96%) and specificity (92.42%) to determine normality on the aGST test. aGST levels 8mg/dL and higher showed the best specificity to determine the presence of more aggressive liver histological damage among HCV patients and the best predictive positive value and positive likelihood for more aggressive portal inflammation and lobular activity. CONCLUSION: aGST is related to HCV infection (cut-off = 4mg/dL) and more aggressive liver histological damage (cut-off = 8mg/dL). In this sense, aGST could be used in HCV patients with altered ALT levels as an indicator of more aggressive hystopathological damage. However, its positive predictive value (PPV) is not high enough to preclude the decision of performing hepatic biopsy, even when it is above 8mg/dL.
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Identificação de fonte sanguínea em dípteros da Família Culicidae, em áreas de epizootia da febre amarela silvestre / Identification of blood source in the family Culicidae flies, in areas of outbreak of jungle yellow feverAna Maria Marassa 16 June 2009 (has links)
A importância em conhecer o padrão alimentar em mosquitos da Família Culicidae permite esclarecer alguns aspectos relacionados à transmissão de zoonoses e estimar o grau de contato humano-vetor que é fator relevante em estudos epidemiológicos. Com o objetivo de explorar o comportamento alimentar dessa Família, em área epizoótica de febre amarela silvestre, foram coletados exemplares nos municípios de Santo Antônio das Missões e Garruchos, Estado do Rio Grande do Sul. Fêmeas ingurgitadas foram obtidas por aspiração em ambiente de mata, no período de setembro de 2005 a abril de 2007 e identificadas segundo fonte de sangue ingerido através da técnica imunoenzimática ELISA de captura no sistema avidinabiotina. Foram testadas seis fontes de alimento: ave, bovino, eqüino, humano, macaco e rato. Os resultados obtidos mediante a padronização de anticorpos monoclonais possibilitaram demonstrar pela primeira vez o reconhecimento de sangue humano ingerido nesses mosquitos pelo emprego da subclasse IgG1 e comprovar a sensibilidade e especificidade da técnica ELISA de captura. No município de Santo Antônio das Missões, de um total de 190 amostras, 60,9% reagiram para sangue de boi, 23,6% para humano, 9,9% para ave, 1,9% para macaco e 3,7% para combinações de dois hospedeiros. Quanto às amostras referentes ao município de Garruchos, das 158 fêmeas capturadas na área Cachoeirinha pode-se observar reatividade para ave (16%), boi (29,6%), humano (36,8%), cavalo (4%), macaco (0,8%) e combinações de hospedeiros (12,8%), enquanto que para as 149 fêmeas pertencentes à área de São José, detectou-se sangue ingerido de boi em (51,5%), ave e humano (11,5%), macaco (6,2%), cavalo (0,8%) e mistos (18,5%). Aedes scapularis, Aedes crinifer, Culex (Culex) spp., Haemagogus leucocelaenus apresentaram maior número de fêmeas ingurgitadas nos dois municípios. Os resultados obtidos com Aedes scapularis sugerem ecletismo, conforme combinações detectadas em amostras de sangue de diferentes fontes. Haemagogus leucocelaenus apresentou a maior proporção de amostras contendo sangue humano em relação às demais fontes e essa característica traz implicações, por ser espécie incriminada na transmissão e por se tratar de área de ocorrência de epizootias de febre amarela. / The knowledge of mosquitoes Culicidae host feeding patterns permits to clarify some aspects related to zoonosis transmission and to estimate the degree of human-vector contact which is relevant in epidemiological studies. Aiming to explore the feeding behavior of these mosquitoes, specimens were collected in the municipalities of Santo Antônio das Missões and Garruchos, Rio Grande do Sul, an epizootic area of sylvatic yellow fever. Engorged females were collected by aspiration from forested areas from September 2005-April 2007 and their blood meals were identified using the avidin-biotin system of immunoenzymatic ELISA capture. Six blood meal sources were tested: bird, cattle, horse, human, monkey and rat. The result achieved with the species-specific IgG1 mAb was unprecedented for mosquito blood meal identification and reinforced the sensibility and specificity of the immunoenzymatic ELISA capture. Of the 190 samples from Santo Antônio das Missões, 60.9% reacted to cattle, 23.6% to human, 9.9% to bird, 1.9% to monkey and 3.7% to mixed blood meals. In Garruchos, of the 158 females collected in Cachoeirinha, 16.0% reacted to bird, 29.6% to cattle, 36.8% to human, 4.0% to horse, 0.8% to monkey and 12.8% to mixed blood, while of the 149 engorged females from São José, blood from cattle accounted for 51.5%, of blood identified, bird and human 11.5%, monkey 6.2%, horse 0.8% and mixed blood 18.5%. Blood engorged females of Aedes scapularis, Aedes crinifer, Culex (Culex) spp., Haemagogus leucocelaenus predominated in the two municipalities. The results obtained with Aedes scapularis suggests its eclecticism, according to the combinations of blood which were detected from different sources. Haemagogus leucocelaenus was found to have the highest proportion of samples containing human blood in comparison with other sources, which has implications, on account of being incriminated in the transmission and also for taking into consideration the outbreaks reported that underline the risk of yellow fever.
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Alpha Glutationa S Transferase: marcador de lesão hepática em pacientes com hepatite pelo vírus C? / Alpha Glutathione S Transferase: a marker of liver damage in hepatitis C virus patients?Evandro Antônio Bentes de Oliveira Júnior 07 January 2005 (has links)
INTRODUÇÃO E OBJETIVOS: A a-Glutathiona-S-transferase (aGST) vem sendo proposta como um marcador sensível e não-invasivo de lesão hepática em pacientes com Hepatite pelo vírus C. Avaliamos neste trabalho como a (aGST) se correlaciona com características bioquímicas e histológicas em pacientes com HCV. MATERIAL E MÉTODOS: Realizamos a determinação da concentração plasmática das aGST, alanina aminotransferase (ALT), aspartato aminotransferase (AST) e gama-glutamyltransferase (gGT) em 114 pacientes com HCV, dos quais 97 foram submetidos à biópsia hepática em até 6 meses da realização dos testes bioquímicos. Avaliamos também os níveis de aGST em 66 doadores de sangue sadios, que serviram como controles. Comparamos os níveis de aGST com as demais provas bioquímicas e a histologia hepática. RESULTADOS: A aGST estava elevada em 85.96% dos pacientes com HCV e mostrou associação com a elevação das aminotransferases (p<0.01). O valor de 4mg/dL mostrou as melhores sensibilidade (85,96%) e especificidade (92,42%) para determinar a normalidade do teste aGST. aGST ³ 8mg/dL mostrou a melhor especificidade para determinar lesão histológica hepática mais agressiva e o melhor valor preditivo positivo e razão de verossimilhança positiva para inflamação portal e atividade parenquimatosa mais agressiva nos pacientes com HCV. CONCLUSÕES: A aGST está relacionada à lesão hepática na infecção pelo HCV (valor de corte = 4mg/dL) e lesões histológicas hepáticas mais agressivas (valor de corte = 8mg/dL). Neste contexto, a aGST poderia ser utilizada em pacientes com Hepatite pelo HCV com ALT elevada, como um indicador complementar de lesão histopatológica mais agressiva. Entretanto, seu valor preditivo positivo não é suficientemente elevado para evitar a necessidade de realizar a biópsia hepática, mesmo quando está acima de 8mg/dL. / BACKGROUND/AIMS: a-Glutathione-S-transferase (aGST) has been proposed as a sensitive non-invasive indicator of hepatocellular injury due to Hepatitis C virus (HCV) infection. In this work, we evaluate how alpha-GST concentration correlates with biochemical and histological features in HCV patients. METHODS: We assayed plasma aGST, alanine aminotransferase (ALT), spartate aminotransferase (AST) and gama-glutamyl-transferase (gGT) in 114 HCV+ patients, among whom liver biopsy was performed in 97, within 6 months of the biochemical evaluation. We also assessed aGST levels in 66 health blood donors, aimed to serve as control. We compared aGST levels with other biochemical tests and liver histology. RESULTS: In 85.96% of HCV patients aGST was elevated and showed association with serum aminotransferases (p<0.01). The value of 4mg/dL (or lower) showed the best sensitivity (85.96%) and specificity (92.42%) to determine normality on the aGST test. aGST levels 8mg/dL and higher showed the best specificity to determine the presence of more aggressive liver histological damage among HCV patients and the best predictive positive value and positive likelihood for more aggressive portal inflammation and lobular activity. CONCLUSION: aGST is related to HCV infection (cut-off = 4mg/dL) and more aggressive liver histological damage (cut-off = 8mg/dL). In this sense, aGST could be used in HCV patients with altered ALT levels as an indicator of more aggressive hystopathological damage. However, its positive predictive value (PPV) is not high enough to preclude the decision of performing hepatic biopsy, even when it is above 8mg/dL.
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Determination of the Expression Patterns of Bovine Non-Classical Major Histocompatibility Complex (MHC) Class I ProteinsParasar, Parveen 01 December 2013 (has links)
My dissertation hypothesis is that bovine trophoblast cells express cell-surface and secreted non-classical major histocompatibility complex class I (MHC-Ib) proteins which inhibit NK cells and other leukocytes by binding to inhibitory receptors (e.g., LILRB1, LILRB2, KIR2DL4, and/or CD94/NKG2A).
Extremely polymorphic and ubiquitously expressed classical MHC class I (MHC-Ia) proteins, which present foreign antigenic peptides to CD8+ T lymphocytes, are involved in acceptance or rejection of tissue grafts. Non-classical MHC class I (MHC-Ib) glycoproteins, such as Human Leukocyte Antigen-G (HLA-G) and murine Qa-2, are important modulators of the maternal immune system during pregnancy. MHC-Ib proteins are: (a) oligomorphic or monomorphic, (b) expressed in specific tissues under specific condtions, and (c) produced as surface and/or soluble isoforms due to alternative splicing.
Third trimester-bovine trophoblast cells express both MHC-Ia and MHC-Ib proteins. The MHC-Ib proteins expressed by trophoblast cells during the third trimester of pregnancy are encoded by four bovine leukocyte antigen (BoLA) loci: BoLA-NC1, BoLA-NC2, BoLA-NC3, and BoLA-NC4.
Two MHC-Ia (N*01701 and N*01802) and three MHC-Ib (NC1*00501, NC3*00101 and NC4*00201) proteins showed cell-surface expression in transfection studies performed in murine P815 and human K562 cells. Two additional isoforms, NC1*00401 and NC2*00102, were not detected on the surface of these cells. Nevertheless, both class Ia proteins, N*01701 and N*01802, and five class Ib proteins, NC1*00401, NC1*00501, NC2*00102, NC3*00101, and NC4*00201, were detected in crude cell lysates on Western blots. Precipitation of proteins from culture supernatants showed that cell-surface MHC-Ia (N*01701 and N*01802) and MHC-Ib proteins (NC1*00501, NC3*00101, and NC4*00201) are shed from the surface of these cells into the media. The mechanism of shedding of these proteins is, however, not known.
Monoclonal antibodies W6/32, IL-A88, H1A, H6A, H11A, H58A, and PT-85A recognized surface MHC-I isoforms with varying affinity. We were able to develop a sandwich enzyme-linked immunosorbent assay (ELISA) using either H1A or IL-A88 antibody as the capture antibody and the W6/32 antibody for detection. We produced monoclonal antibodies against cattle NC1*00501 and NC3*00101 proteins. One monoclonal antibody generated against BoLA-NC3*00101 was highly specific. Unfortunately, due to failure to clone the NC3*00101- hybridoma, we no longer have an infinite source of this monoclonal antibody for NC3*00101. We eluted peptides from NC3*00101-transfected MHC-null K562 cells and identified peptides using liquid chromatography-mass spectrum (LC-MS) analysis. Analysis of peptide binding data using the SAS Proc mixed statistical program, suggested that the peptide EVTNQLVVL is a potential peptide ligand, which can be used to make tetramers for enumeration of antigen-specific leukocytes.
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