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131	Avaliação do teste de imunodifusão dupla em gel de agar e do ensaio imunoenzimático - ELISA no diagnóstico e seguimento de pacientes com bola fúngica aspergilar Azevedo, Priscila Zacarias de [UNESP] 26 February 2015 (has links) (PDF) Made available in DSpace on 2016-06-07T17:12:08Z (GMT). No. of bitstreams: 0 Previous issue date: 2015-02-26. Added 1 bitstream(s) on 2016-06-07T17:16:41Z : No. of bitstreams: 1 000860294.pdf: 1568094 bytes, checksum: 044319797056c4a704a1822a33bee13d (MD5) / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) Aspergilose pulmonar Imunodifusão Ensaio de imunoadsorção enzimática Polissacarideos Sorologia Enzyme-linked immunosorbent assay
132	Validation and application of the ELISA technique for the detection of fish aero-antigens George, Dashwill Anton January 2003 (has links) Thesis (MTech (Biomedical Technology))--Peninsula Technikon, 2003 / Increased seafood consumption due to its nutrition and promotion of a healthy diet has lead to more frequent reports of allergic reactions. In the seafood industry, workers are exposed to the antigens through inhalation of the vapours created during the seafood processing and cooking. Most seafood allergens are stable molecules, which are resistant to the effect of cooking and processing. The prevalence of occupational asthma varies from 7-36% among different groups of workers including seafood processing and fishmeal workers, fishermen and restaurant cooks (Jeebhay et al 2001). Purpose of Study: The purpose of the study is to determine total protein and the specific fish antigen concentrations in the environment by means of personal air sampling filters obtained from various categories of workers in the seafood processing industry. Objectives: • To determine the correlation between total protein concentrations and specific fish (pilchard and anchovy) antigen concentrations on personal air sampling filters using the linear response model of the standard curve. • To determine the correlation between total protein concentrations and specific fish (pilchard and anchovy) antigen concentrations on personal air sampling filters using the sigmoidal response model with a variable slope of the standard curve. • To identify the most efficient standard curve response model for fish antigen detection by comparing the percentage recovery of the linear standard curve response model and the sigmoidal standard curve response model. Methodology: A sample population of 195 samples was taken from workers in the seafood industry at the St. Helena Bay Fisheries and West Point Processors using personal air sampling pumps. Antigen-antibody reactions Enzyme-linked immunosorbent assay
133	Mediadores inflamatorios sericos na paracoccidioidomicose humana / Serum levels of inflammatory mediators in human paracoccidioidomycosis Corvino, Claudia Tres 17 August 2006 (has links) Orientador: Maria Heloisa Souza Lima Blotta / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Ciencias Medicas / Made available in DSpace on 2018-08-07T06:51:40Z (GMT). No. of bitstreams: 1 Corvino_ClaudiaTres_M.pdf: 633875 bytes, checksum: 46aff21f882b64dcbb4eefa73f93a232 (MD5) Previous issue date: 2005 / Resumo: A interleucina 18 (IL-18) é uma citocina pró-inflamatória com importante participação tanto na resposta inata como adquirida. Concentrações elevadas de IL-18 são encontradas em várias doenças inflamatórias e infecciosas. A expressão aumentada de IL-18 pode contribuir para a resolução de processos infecciosos, mas também pode promover uma resposta inflamatória exagerada, prejudicial ao hospedeiro. O objetivo deste estudo foi determinar as concentrações séricas de IL-18 e outros mediadores inflamatórios (IL-12, sICAM-1, sTNFRI, sTNFRII, CXCL9, CXCL10), antes e após tratamento antifúngico, em pacientes com a forma juvenil (FJ) e adulta (FA) da paracoccidioidomicose (PCM), assim como em indivíduos normais saudáveis e relacionar com a atividade e gravidade da doença. Também foram avaliadas as concentrações de IgG total, subclasses de IgG e IgE anti-gp43 de P. brasiliensis. Todas as dosagens foram realizadas por método imunoenzimático (ELISA). Os níveis séricos basais de IL-18, IL-12, sICAM-1, sTNFRI, sTNFRII, CXCL9, CXCL10 estavam mais elevados em pacientes com PCM em relação ao grupo controle. Pacientes com a FJ apresentaram concentrações mais elevadas de IL-18 e sTNFRII em relação aqueles com a FA da PCM, enquanto estes mostraram maiores concentrações de sTNFRI em relação aos pacientes com a FJ. Houve correlação positiva entre as concentrações de IL-18 e sICAM-1 (r=0.62, p<0.0001), sTNFRI (r=0.61, p<0.0001), sTNFRII (r=0.64, p=0.002) e também em relação a gravidade da doença nos pacientes com a FJ. A terapia anti-fúngica resultou em significante diminuição das concentrações séricas de todos os mediadores inflamatórios analisados que, de maneira geral, atingiram os valores encontrados no grupo controle ao final de 2 anos de tratamento. A pesquisa de anticorpos mostrou níveis basais maiores de IgG4 e IgE nos pacientes com a FJ, enquanto que a IgG1 estava mais elevada naqueles com a FA. Em conjunto os resultados mostraram que uma forte resposta inflamatória marca a fase inicial da PCM humana e que mediadores como a IL-18 e o sTNFRII parecem contribuir em particular para uma forma mais grave da doença / Abstract: IL-18 is a pro-inflammatory cytokine of the IL-1 superfamily that exhibits broad functional effects in innate and acquired immune responses and which has been found in high levels in several chronic inflammatory and autoimmune diseases. Over-expression of IL-18 may promote early resolution of infection or could induce a detrimental exaggerated immune response. The aim of this study was to determine serum levels of IL-18 and other inflammatory mediators (IL-12, sICAM-1, sTNFRI, sTNFRII, CXCL9, CXCL10) at baseline and after antifungal therapy in serum from patients with juvenil (JF) and adult form (AF) of paracoccidioidomycosis (PCM) as well as in healthy controls (C), and to assess their possible relationships to the severity of disease. IL-18 and sTNFRII levels in patients with the JF of PCM were significantly higher than in the AF and controls. In relation to sICAM-1, no difference was observed between JF and AF but both presented higher levels than controls. sTNFRI levels were higher in patients with PCM than in controls, and significant higher concentrations were detected in AF patients as compared to JF ones. Moreover IL-12 and chemokines CXCL9 and CXCL10 were also higher in patients than in controls. In JF patients IL-18 levels significantly correlated with sICAM-1 (r=0.62, p<0.0001), sTNFRI (r=0.61, p<0.0001), sTNFRII (r=0.64, p=0.002), as well as with clinical severity. The results suggest the value of serum IL-18 and sTNFRs levels as a parameter of PCM severity and may support a possible role for them in the pathogenesis of the disease / Mestrado / Ciencias Biomedicas / Mestre em Ciências Médicas Paracoccidioides Citocinas Inflamação Teste imunoenzimatico Ensaio de imunoadsorção enzimática Paracoccidioidomycosis Cytokines Inflammation Enzyme-linked immunosorbent assay
134	"Pesquisa do anticorpo antitransglutaminase tissular avaliando as interações da transglutaminase com a fibronectina e comparação com os resultados de dois ensaios comerciais" / Standardization of anti-tissue transglutaminase antibody detection and assessment of transglutaminase interactions with fibronectin : comparison of the results with two commercially available essays Clarice Pires Abrantes Lemos 24 August 2005 (has links) Os objetivos desse estudo foram: 1) Padronizar a pesquisa do anti-tTg, comparando-o com o anticorpo antiendomísio (AAE) e 2) Avaliar as interações da tTg com a fibronectina. 49 celíacos e 124 controles com AAE negativo foram avaliados. O AAE foi pesquisado por imunofluorescência indireta e a reatividade contra a tTg e a fibronectina por ELISA in house e com kits comerciais. O antitTg foi positivo em 46,9% e 100% dos celíacos com o ELISA in house e com kits comerciais, respectivamente. A adição de fibronectina não melhorou a sensibilidade do ELISA. Em conclusão: a detecção do antitTg por ELISA apresenta percentual elevado de falso-positivos, não podendo substituir a pesquisa do AAE / The aims of the current study were: to standardize the detection of anti-tTg antibodies, comparing them with antiendomysial antibodies (EMA) and to assess the interaction of tTg with fibronectin. 49 celiac patients and 124 controls were enrolled. EMA was detected by indirect immunofluorescence reaction and tTg and fibronectin reactivity by in house ELISA and with commercially available kits. Seropositivity to anti-tTG was found in 46.9% and 100% of patients by the in house technique and by commercial kits, respectively. Fibronectin addition did not improve the ELISA sensibility. In conclusion, ELISA for anti-tTG detection has a high rate of false positive results and does not replace EMA DOENÇA CELÍACA/diagnóstico ELISA FIBRONECTINAS TRANSGLUTAMINASE CELIAC DISEASE/diagnosis ENZYME-LINKED IMMUNOSORBENT ASSAY FIBRONECTINS TRANSGLUTAMINASES
135	Infecções endodônticas primária x secundária : perfil microbiano, níveis de endotoxinas e ácido lipoteicóico, sinais e sintomas / Machado, Felipe Paiva. January 2018 (has links) Orientador: Marcia Carneiro Valera / Banca: Cláudio Antonio Talge Carvalho / Banca: Flaviana Bombarda de Andrade / Resumo: Esta pesquisa clínica teve como objetivo comparar a carga e composição microbiana bem como as concentrações de LPS e LTA encontradas na infecção endodôntica primária (IEP) e na infecção endodôntica secundária (IES). Além disso, a correlação desses achados com características clínicas e tomográficas também foram investigadas. Sessenta dentes de pacientes com IEP (31) e IES (29) foram submetidos à avaliação clínica e tomográfica, seguido do tratamento endodôntico ou retratamento. Amostras foram coletadas de cada canal radicular utilizando cones de papel. Logo após a abertura coronária (IEP) ou após a desobturação dos canais (IES) o conteúdo coletado foi submetido à técnica de cultura microbiológica para determinar a carga microbiana de bactérias anaeróbias e ao método Checkerboard DNA-DNA hybridization para investigação de espécies bacterianas presentes. O teste de Lisado de Amebócito de Limulus e o Ensaio de Imunoabsorção Enzimática foram utilizados para quantificar os níveis de LPS e LTA. Os dados obtidos foram correlacionados com os achados clínicos e tomográficos. Maiores quantidades de bactérias cultiváveis e de LPS foram encontradas na IEP (p < 0,05). Não houve diferença nos níveis de LTA entre IEP e IES (p > 0,05). A mediana de espécies por canal radicular encontrada na IEP foi de 9 espécies e na IES foi de 22 (p < 0,05). As espécies bacterianas mais prevalentes detectadas na IEP foram P. gingivalis (14/31) e S. intermedius (14/31). Na IES, as espécies mais prevalentes f... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: This clinical research aimed to compare the microbial load and composition as well as the LPS and LTA concentrations found in Primary Endodontic Infection (PEI) and Secondary Endodontic Infection (SEI). In addition, the correlation of these findings with clinical and tomographic features was also investigated. Sixty patients' teeth with PEI (31) and SEI (29) were submitted to clinical and tomographic assessment, followed by endodontic treatment or retreatment. Samples were taken from each root canal using paper points. After the coronary opening (PEI) or after the removal of root filling material (SEI), the collected samples were submitted to the microbiological culture technique to determine the microbial load of anaerobic bacteria and to the Checkerboard DNA-DNA hybridization method for investigation of present bacterial species. The Limulus amebocyte lysate assay and enzyme-linked immunosorbent assay were used to quantify LPS and LTA levels. The data obtained were correlated with clinical and tomographic findings. A higher number of cultivable bacteria and LPS was found in PEI (p < 0.05). There was no difference in LTA levels between PEI and SEI (p> 0.05).The median number of species per root canal found in PEI was 9 and 22 in SEI (p < 0.05). The most prevalent bacterial species detected in PEI were P. gingivalis (14/31) and S. intermedius (14/31). In SEI, the most prevalent species were P. gingivalis (21/29) and C. rectus (20/29). LPS was positively correlated with a larg... (Complete abstract click electronic access below) / Mestre Periodontite periapical. Microbiota. Endotoxina. Ensaio de imunoadsorção enzimática. Adesivos dentinários. Periapical periodontitis Microbiota. Enzyme-linked immunosorbent assay
136	Innervation of Guinea Pig Heart by Neurons Sensitive to Capsaicin Hougland, Margaret W., Durkee, Kristine H., Hougland, Arthur E. 01 January 1986 (has links) To determine the origin of non-vagal afferent fibers innervating the heart of guinea pigs, capsaicin was injected into the ventricular myocardium to induce depletion of substance P (SP). The lower cervical, upper thoracic and lumbar spinal ganglia, as well as the left atrium and base of ventricles, were assayed for SP depletion by using the enzyme-linked immunosorbent assay (ELISA) and immunohistochemical procedures. Capsaicin affected spinal ganglia from the 3 regions differently. The substance P level in lumbar spinal ganglia remained fairly constant, while the level of SP from cervical and thoracic regions declined significantly. At the maximal depletion dosage (173 μg of capsaicin/kg), SP concentration decreased 72.3% in cervical spinal ganglia, 45.5% in thoracic ganglia and 56.1% in the atrium. The lack of SP depletion in lumbar ganglia indicates that capsaicin acted locally on cardiac afferents rather than systemically. Data from this study suggest that capsaicin-sensitive neurons of the heart have cell bodies in the lower cervical spinal ganglia as well as in the upper thoracic spinal ganglia. capsaicin guinea pig heart immunohistochemistry spinal ganglia substance P Biomedical Sciences
137	Lipid Transfer Inhibitor Protein (Apolipoprotein F) Concentration in Normolipidemic and Hyperlipidemic Subjects Morton, Richard, Gnizak, Hannah M., Greene, Diane J., Cho, Kyung Hyun, Paromov, Victor M. 01 January 2008 (has links) Lipid transfer inhibitor protein (LTIP) is an important regulator of cholesteryl ester transfer protein function. We report the development of an immunoassay for LTIP and its use to quantify LTIP in plasma of varying lipid contents. A rabbit antibody against bacterially produced recombinant LTIP detected two LTIP isoforms in plasma differing in carbohydrate content. This antibody was used in a competitive, enzyme-linked immunoassay that uses partially purified LTIP bound to microtiter plates. To optimize LTIP immunoreactivity, plasma samples required preincubation in 1% Tween-20 and 0.5% Nonidet P-40. In normolipidemic plasma, LTIP averaged 83.5 mg/ml. LTIP was 31% higher in males than in females. LTIP was positively associated with HDL cholesterol in normolipidemic males but not in females. In hypertriglyceridemic males, LTIP was only 56% of control values, whereas in hypertriglyceridemic females, LTIP tended to increase. Additionally, in males with normal cholesterol and triglyceride (TG) ≤ 200 mg/dl, LTIP varied inversely with plasma TG. Overall, we have confirmed the negative association between plasma TG levels and LTIP previously suggested by a small data set, but now we demonstrate that this effect is seen only in males. The mechanisms underlying this gender-specific response to TG, and why LTIP and HDL levels correlate in males but not in females, remain to be determined. cholesteryl ester transfer protein enzyme-linked immunosorbent assay glycoprotein
138	A new mass spectrometric assay of N8-acetylspermidine deacetylase and partial purification of the enzyme Zhao, YongYuan 01 January 2007 (has links) A new enzyme activity assay has been developed for the target N8-acetylspermidine deacetylase, a not-well-studied but essential enzyme in the polyamine interconversion and reutilization pathway. The enzyme assay, based on mass spectrometric detection of a specific reaction product following sample introduction by flow injection, was shown to have a sensitivity of smaller than 1 micromolar and typical RSD of 3-10%. The linear range for analyte was from 1 μM to 100 μM, with R2 > 0.992. The new assay avoids the use of radio labels. Sample preparation is straightforward, and high specificity is provided by the selected reaction monitoring, SRM, using a triple quadrupole mass spectrometer. Acetylputrescine was used for the first time as the substrate for the assay of N8-acetylspermidine deacetylase in lieu of N8 -acetylspermidine. The crude enzyme extracted from rat liver had an apparent Km value of 80.6 μM for acetylputrescine and a Vmax of 1.1 nmol mg-1 min-1. Enzyme extracted from frozen rat liver was compared with that from fresh rat liver. Frozen rat liver extraction had similar kinetics parameters with the fresh preparation and had a specific activity of 0.8 nmol mg-1 min-1. N8-acetylspermidine deacetylase was partially purified by protein precipitation and gell filtration chromatography. Affinity chromatography was tentatively applied for further isolation of the enzyme, but was not yet successful. Enzyme-linked immunosorbent assay Enzymatic analysis Mass spectrometry Chemistry Medicinal-Pharmaceutical Chemistry Physical Sciences and Mathematics
139	Studies on the safety of food and feed, and on the effects of plant derivedanti-inflammatory components / 食品および飼料の安全性と植物由来抗炎症成分に関する研究 Yamamoto, Takayuki 23 March 2016 (has links) 京都大学 / 0048 / 新制・課程博士 / 博士(農学) / 甲第19770号 / 農博第2166号 / 新制\|\|農\|\|1040(附属図書館) / 学位論文\|\|H28\|\|N4986(農学部図書室) / 32806 / 京都大学大学院農学研究科食品生物科学専攻 / (主査)教授河田照雄, 教授保川清, 教授橋本渉 / 学位規則第4条第1項該当 / Doctor of Agricultural Science / Kyoto University / DGAM bovine spongiform encephalopathy (BSE) food allergy anti-inflammtory polyphenol 610
140	DEVELOPMENT OF A LC/MS/MS ENZYME METHOD FOR N8 - ACETYLSPERMIDINE MEASUREMENTS IN ENZYME ASSAYS Tang, Jennifer Huiqin 01 January 2005 (has links) (PDF) This thesis describes the development of a way to study the N8 - acetylspermidine deacetylase enzyme activity. The method created in this thesis emphasizes sensitivity, accuracy and safety. In this study, HeLa cells were cultured and extracted to yield a crude N8 - acetylspermidine deacetylase enzyme mixture. By measuring the decrease of N8 - acetylspermidine and the increase of spetmidine, N8 -acetylspermidine deacetylase enzyme activity can be determined using either a Varian 1200L LC/MS/MS or an API 3000 LC-ES (+)/MS/MS. An acetylation-derivatization method was developed because N8 -acetylspermidine and spermidine are hard to purify from a biological sample since they are not retained on a CIS solid phase extraction column or on a RP HPLC (high performance liquid chromatography) reverse phase column due to their small molecular weight and high polarity. The quantitation of N8 -acetylspem1indine over the range 2ng/ul to 5pg/ul was fit by linear regression as y = 1.064x + 0.218 with an R-squared value of 0.9996, where y is the peak area of the fragment-ion SRM (selected reaction monitoring: m/z: 188/114) chromatograms from N8 -acetylspermindine and x is the concentration of N8 - acetylspermindine. Acetylation of spermidine (SPD) and N8-acetylspermidine (N8AcSPD) with d6-acetic anhydride produces the d9 labeled triacetylated derivative of SPD and d6 labled triacetylated spermidine derivative of N8AcSPD. These triacetylated forms are retained on a C18 column. MS/MS gives characteristic m/z fragment ions for the derivatized species: N8AcSPD (278 to 215), NlAcSPD (278 to 218) and SPD (281 to 218). The fragment-ion SRM (selected reaction monitoring) chromatograms are used for the quantitation. A plot of peak area ratios for known mixtures of N8AcSPD and total SPD versus the molar ratios of N8AcSPD and total SPD was found to fit a linear regression line withy= 0.705x + 0.035 with an R-squared value of 0.9919. Quantitation of d6- and dg-tri-acetylspermidine by LC/MS/MS is possible at the low levels of materials found in cell extracts since the separation method results in a lower limit of quantitation. This approach enables the study of N8 - acetylspermidine deacetylase enzyme activity. Enzyme-linked immunosorbent assay Enzymatic analysis Medicinal and Pharmaceutical Chemistry Medicine and Health Sciences Pharmacy and Pharmaceutical Sciences

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