Global ETD Search

221	Identification of differentially expressed genes in fibroblasts from human hypertrophic scars by using differential display RT-PCR technique. January 1998 (has links) by Cheng Chi Wa. / Thesis (M.Phil.)--Chinese University of Hong Kong, 1998. / Includes bibliographical references (leaves 110-120). / Abstract also in Chinese. / Title --- p.i / Abstract --- p.ii / Acknowledgement --- p.iv / Abbreviations --- p.v / Abbreviation Table for Amino Acids --- p.vi / Table of Contents --- p.vii / List of Figures --- p.xii / List of Tables --- p.xv / Chapter Chapter 1 --- Introduction --- p.1 / Chapter Chapter 2 --- Literature review --- p.2 / Chapter Part I --- Hypertrophic Scar / Chapter 2.1 --- Definition of hypertrophic scar --- p.2 / Chapter 2.2 --- Pathology --- p.2 / Chapter 2.3 --- Epidemiology findings --- p.3 / Chapter 2.3.1 --- Ethnicity --- p.3 / Chapter 2.3.2 --- Age --- p.3 / Chapter 2.3.3 --- Body location --- p.3 / Chapter 2.4 --- Mechanism of cutaneous wound healing --- p.4 / Chapter 2.4.1 --- Phase I - Haemostasis and inflammation --- p.4 / Chapter 2.4.1.1 --- Haemostasis --- p.6 / Chapter 2.4.1.2 --- Early phase of inflammation --- p.6 / Chapter 2.4.1.3 --- Late phase of inflammation --- p.7 / Chapter 2.4.2 --- Phase II - Re-epithelialization --- p.7 / Chapter 2.4.2.1 --- Migration of epidermal keratinocytes --- p.8 / Chapter 2.4.2.2 --- Migration of fibroblasts --- p.8 / Chapter 2.4.2.3 --- Angiogenesis --- p.9 / Chapter 2.4.3 --- Phase III - Tissue remodeling --- p.10 / Chapter 2.4.3.1 --- Cell maturation and apoptosis --- p.10 / Chapter 2.4.3.2 --- Exrtracellular matrix remodeling --- p.10 / Chapter 2.5 --- Alteration of wound healing - Possible pathogenic factors of hypertrophic scar --- p.11 / Chapter 2.5.1 --- Changes in Phase I-Inflammation --- p.13 / Chapter 2.5.2 --- Changes in Phase II - Re-epithelialization/ tissue formation --- p.14 / Chapter 2.5.3 --- Changes in Phase III - Tissue remodeling --- p.15 / Chapter 2.6 --- The Role of fibroblasts in the formation of hypertrophic scar --- p.16 / Chapter 2.6.1 --- Functions of fibroblasts in wound healing --- p.16 / Chapter 2.6.2 --- Suggested aetiological role in the formation of hypertrophic scar fibroblasts --- p.16 / Chapter 2.6.2.1 --- Fibroproliferation disorder --- p.18 / Chapter 2.6.2.2 --- Extracellular Matrix remodeling disorder --- p.18 / Chapter a) --- CoUaqen --- p.18 / Chapter b) --- Proteoglycan --- p.19 / Chapter 2.6.2.3 --- Other differentially expressed factors --- p.20 / Chapter 2.7 --- Treatment of hypertrophic scar --- p.21 / Chapter Part II --- Differential Display / Chapter 2.8 --- Current approaches for the studies of differential gene expression --- p.23 / Chapter 2.9 --- Comparison amongst different approaches --- p.23 / Chapter 2.10 --- The strategy of Differential Display RT-PCR (DDRT-PCR) --- p.24 / Chapter 2.11 --- The application of DDRT-PCR to identify differentially expressed genes --- p.26 / Chapter Chapter 3 --- Aims and Strategies --- p.27 / Chapter Chapter 4 --- Methods and Materials --- p.29 / Chapter 4.1 --- Materials --- p.29 / Chapter 4.2 --- Clinical specimen collection --- p.31 / Chapter 4.3 --- Primary explant culture --- p.31 / Chapter 4.4 --- Immunohistochemical staining --- p.32 / Chapter 4.5 --- Total RNA extraction --- p.32 / Chapter 4.6 --- DNase I digestion --- p.33 / Chapter 4.7 --- Differential display-RTPCR (DD-RTPCR) --- p.33 / Chapter 4.8 --- Polyacrylamide gel electrophoresis --- p.34 / Chapter 4.9 --- Reamplification of the differentially expressed fragments --- p.35 / Chapter 4.10 --- Molecular cloning of the DNA fragments --- p.35 / Chapter 4.11 --- Screening and miniprep of the plasmid DNA --- p.36 / Chapter 4.12 --- Cycle sequencing --- p.38 / Chapter 4.13 --- Data analysis --- p.38 / Chapter 4.14 --- RT-PCR --- p.39 / Chapter 4.15 --- Probe labeling by PCR with DIG-dUTP --- p.40 / Chapter 4.16 --- Southern blotting --- p.41 / Chapter Chapter5 --- p.42 / Chapter 5.1 --- Clinical Specimen --- p.42 / Chapter 5.2 --- Primary explant culture --- p.42 / Chapter 5.3 --- The total RNA extraction from the cultured fibroblast --- p.45 / Chapter 5.4 --- Differential display RT-PCR --- p.47 / Chapter 5.5 --- Reamplification of the DNA fragments --- p.49 / Chapter 5.6 --- Molecular cloning of the DNA fragment --- p.53 / Chapter 5.7 --- DNA sequencing of the inserts --- p.58 / Chapter 5.8 --- Analysis and identification of the DNA sequences --- p.62 / Chapter 5.9 --- Semi-quantitative RT-PCR analysis of the differentially expressed genes --- p.76 / Chapter Chapter6 --- p.87 / Chapter Part I --- Validity of the Findings / Chapter 6.1 --- The Limitation of Tissue Sampling --- p.87 / Chapter 6.2 --- Tissue Culture model --- p.88 / Chapter 6.3 --- Differential Display RT-PCR --- p.89 / Chapter 6.3.1 --- Identification of the differentially expressed genes --- p.89 / Chapter 6.3.2 --- Confirmation of the differentially expressed genes --- p.91 / Chapter 6.4 --- Technical difficulties and Limitations --- p.92 / Chapter 6.4.1 --- Sampling --- p.92 / Chapter 6.4.2 --- Primary tissue culture --- p.93 / Chapter Part II --- Significance and Future Studies / Chapter 6.5 --- Down-regulation of thrombospondin 1 (TSP 1) in the hypertrophic scar fibroblasts --- p.94 / Chapter 6.6 --- Biochemical and biological functions of TSP1 --- p.96 / Chapter 6.6.1 --- The biochemical functions of TSP1 --- p.96 / Chapter 6.6.2 --- The biochemical functions of TSP1 --- p.97 / Chapter 6.7 --- The role of TSP 1 in the pathogenesis of hypertrophic scar --- p.98 / Chapter 6.7.1 --- Down-regulation of TSP 1 may be responsible for the excessive microvessels in hypertrophic scar --- p.98 / Chapter 6.7.2 --- Down-regulation of TSP 1 may be responsible for the failure of the apoptosis of the fibroblasts in the hypertrophic scar --- p.101 / Chapter 6.8 --- Expression of TSP 1 during wound healing --- p.103 / Chapter 6.9 --- Expression of TSP 1 in hypertrophic scarring --- p.107 / Chapter 6.10 --- Cytochrome b561 and its biological function --- p.109 / Chapter 6.11 --- Future studies --- p.108 / Chapter 6.11.1 --- The expression of TSP 1 in hypertrophic scarring and normal wound healing --- p.108 / Chapter 6.11.2 --- The expression of cytochrome b561 --- p.109 / Chapter 6.11.3 --- A full scale study of differential display RT-PCR --- p.109 / References --- p.110 / Appendices --- p.121 / Chapter I --- The complete mRNA sequence of thrombospondin1 precursor --- p.121 / Chapter II --- The mRNA sequence of cytochrome b561 --- p.123 Cicatrix, Hypertrophic--genetics Cicatrix, Hypertrophic--therapy Fibroblasts Polymerase Chain Reaction Transcription, Genetic
222	Quantitative detection of water-borne bacterial pathogens by filtration, immunomagnetic separation (IMS) and real-time PCR. January 2001 (has links) Lui Yuk Sun. / Thesis (M.Phil.)--Chinese University of Hong Kong, 2001. / Includes bibliographical references (leaves 138-148). / Abstracts in English and Chinese. / Abstract (English) --- p.i / Abstract (Chinese) --- p.iii / Acknowledgements --- p.iv / Abberviations --- p.v / Table of Contents --- p.vii / List of Tables --- p.xiv / List of Figures --- p.xvi / Chapter 1. --- Introduction --- p.1 / Chapter 1.1. --- Bacteriological evaluation of water --- p.1 / Chapter 1.1.1. --- Indicator organisms for water quality monitoring --- p.2 / Chapter 1.1.2. --- Properties defined for indicator organisms --- p.3 / Chapter 1.1.3. --- Example of common indicator organisms --- p.3 / Chapter 1.1.3.1. --- Total coliform group --- p.3 / Chapter 1.1.3.2. --- "Fecal coliform, Escherichia coli" --- p.4 / Chapter 1.1.3.3. --- Fecal Streptococcus --- p.5 / Chapter 1.1.3.4. --- Klebsiella --- p.5 / Chapter 1.2. --- The need for specific detection of waterborne pathogenic organisms --- p.6 / Chapter 1.3. --- Common water-borne pathogenic organisms --- p.7 / Chapter 1.3.1. --- Bacteria --- p.7 / Chapter 1.3.1.1. --- Escherichia coli 0157:H7 --- p.7 / Chapter 1.3.1.2. --- Salmonella typhimurium --- p.11 / Chapter 1.3.1.3 --- Legionella pneumophila --- p.12 / Chapter 1.3.2. --- Protozoa --- p.14 / Chapter 1.3.3. --- Viruses --- p.15 / Chapter 1.4. --- Conventional approaches for pathogens detection --- p.16 / Chapter 1.4.1. --- Examples of conventional detection methods --- p.17 / Chapter 1.4.2. --- Problems related to the conventional detection methods --- p.18 / Chapter 1.5. --- Novel approaches for pathogens detection --- p.19 / Chapter 1.5.1. --- Modifications of media --- p.19 / Chapter 1.5.2. --- Antibody-based methods --- p.20 / Chapter 1.5.3. --- Nucleic acid-based methods --- p.21 / Chapter 1.6. --- Principles of pathogens concentration by filtration and immunomagnetic separation --- p.22 / Chapter 1.7. --- Principles of pathogens detection by polymerase chain reaction --- p.24 / Chapter 1.8. --- Principles of quantitative assay of water-borne pathogens using real-time PCR --- p.26 / Chapter 1.9. --- Aims of this study --- p.28 / Chapter 2. --- Detection of water-borne bacteria by polymerase chain reaction --- p.31 / Chapter 2.1. --- Introduction --- p.31 / Chapter 2.2. --- Materials and Methods --- p.35 / Chapter 2.2.1 --- Bacterial strains --- p.35 / Chapter 2.2.2. --- Bacterial enumeration --- p.35 / Chapter 2.2.3. --- DNA extraction and purification --- p.36 / Chapter 2.2.3.1. --- Boiling method --- p.36 / Chapter 2.2.3.2. --- Protinesae K extraction method --- p.36 / Chapter 2.2.3.3. --- Chelex extraction method --- p.37 / Chapter 2.2.4. --- Targeted sequences --- p.38 / Chapter 2.2.4.1. --- eaeA gene --- p.38 / Chapter 2.2.4.2. --- mdh gene --- p.39 / Chapter 2.2.4.3. --- flaR gene --- p.39 / Chapter 2.2.5. --- PCR amplification --- p.40 / Chapter 2.2.6. --- Gel electrophoresis --- p.41 / Chapter 2.3. --- Results --- p.42 / Chapter 2.3.1. --- Optimization of the PCR --- p.42 / Chapter 2.3.2. --- Sensitivity of PCR detection --- p.42 / Chapter 2.3.2.1. --- Boiling method --- p.42 / Chapter 2.3.2.2. --- Proteinease K method --- p.43 / Chapter 2.3.2.3. --- Chelex method --- p.43 / Chapter 2.3.3. --- Specificity of PCR detection --- p.43 / Chapter 2.3.3.1. --- primers targeted uidA gene --- p.44 / Chapter 2.3.3.2. --- primers targeted mdh gene --- p.44 / Chapter 2.3.3.3. --- primers targeted flaR gene --- p.44 / Chapter 2.4. --- Discussion --- p.57 / Chapter 3. --- Concentration and separation of water-borne bacteria by two-step-filtration and immunomagnetic separation --- p.61 / Chapter 3.1. --- Introduction --- p.61 / Chapter 3.2. --- Materials and Methods --- p.66 / Chapter 3.2.1. --- Bacterial strains --- p.66 / Chapter 3.2.2. --- Bacterial enumeration --- p.66 / Chapter 3.2.3. --- Filtration --- p.67 / Chapter 3.2.4. --- Immunomagnetic separation (IMS) --- p.68 / Chapter 3.2.4.1. --- Antibodies and Magnetic beads --- p.68 / Chapter 3.2.4.2. --- Binding of antibodies to magnetic beads --- p.68 / Chapter 3.2.4.3. --- Immunomagnetic separation of bacteria in seeded samples --- p.70 / Chapter 3.2.5. --- Determine the efficiency of filtration and immunomagnetic separation --- p.70 / Chapter 3.2.6. --- DNA extraction --- p.71 / Chapter 3.2.7. --- Multiplex PCR --- p.71 / Chapter 3.2.8. --- PCR amplification --- p.72 / Chapter 3.2.9. --- Gel electrophoresis --- p.72 / Chapter 3.3. --- Results --- p.73 / Chapter 3.3.1. --- Efficiency of filtration and immunomagnetic separation --- p.73 / Chapter 3.3.2. --- Detection limit of PCR --- p.73 / Chapter 3.3.2.1. --- Filtration and immunomagnetic separation --- p.73 / Chapter 3.3.2.2. --- Influence of background flora --- p.73 / Chapter 3.3.2.3 --- Shing Mun River and Lam Tsuen River --- p.77 / Chapter 3.3.3. --- Multiplex PCR --- p.77 / Chapter 3.4. --- Discussion --- p.91 / Chapter 4. --- Quantitative assay of water-borne pathogens using real-time PCR --- p.94 / Chapter 4.1. --- Introduction --- p.94 / Chapter 4.2. --- Materials and Methods --- p.99 / Chapter 4.2.1. --- Bacteria strains --- p.99 / Chapter 4.2.2. --- Bacterial enumeration --- p.99 / Chapter 4.2.3. --- Primers and Probes --- p.100 / Chapter 4.2.3.1. --- eaeA gene --- p.101 / Chapter 4.2.3.2. --- mdh gene --- p.102 / Chapter 4.2.3.3. --- flaR gene --- p.102 / Chapter 4.2.4. --- Targeted sequences cloning and sequencing --- p.103 / Chapter 4.2.4.1. --- Amplication of targeted sequence by PCR --- p.103 / Chapter 4.2.4.2. --- Purification of PCR product --- p.104 / Chapter 4.2.4.3. --- Ligation with cloning vector --- p.105 / Chapter 4.2.4.4. --- Transformation of E.coli DH5a cells --- p.105 / Chapter 4.2.4.5. --- Plasmid DNA isolation --- p.106 / Chapter 4.2.4.6. --- DNA quantitation and sequencing --- p.107 / Chapter 4.2.5. --- Quantitation determination using real-time PCR --- p.108 / Chapter 4.3. --- Results --- p.110 / Chapter 4.3.1. --- Determination of targeted sequences --- p.110 / Chapter 4.3.2. --- Reading of fluorescence intensity and data analysis --- p.110 / Chapter 4.3.3. --- Sensitivity of real-time PCR --- p.114 / Chapter 4.3.4. --- Specificity of real-time PCR --- p.121 / Chapter 4.3.5. --- Quantitation analysis in seeded samples --- p.121 / Chapter 4.4. --- Discussion --- p.131 / Chapter 5. --- Conclusion and future perspectives --- p.133 / Chapter 6. --- References --- p.138 Water Microbiology Bacteriological Techniques Immunomagnetic Separation Polymerase Chain Reaction Bacteria--pathogenicity
223	Infecção experimental para avaliar a excreção do vírus da diarreia viral bovina por leitões desmamados e transmissão viral por via aerógena / Santos, Anne Caroline Ramos dos January 2016 (has links) Orientador: Luís Guilherme de Oliveira / Coorientador: Andressa de Souza Pollo / Banca: João Pessoa Araújo Junior / Banca: Hélio José Montassier / Resumo: O vírus da Diarreia Viral Bovina (BVDV), do gênero Pestivírus, pode ocasionar significativas perdas econômicas em bovinos. No entanto, este vírus também pode infectar os suínos, nos quais a infecção por BVDV poderá ocasionar sinais clínicos, afetar a diagnose da PSC (Peste Suína Clássica), além de torná-los fonte de disseminação viral. Tendo em vista esta problemática, este trabalho teve por objetivo verificar se leitões infectados experimentalmente por BVDV podem passar a excretar o vírus e se a disseminação viral pode ocorrer por via aerógena. Para tanto, foram realizados dois experimentos. Em cada experimento, seis leitões foram distribuídos em duplas em três câmaras de isolamento, ligadas por tubos com fluxo de ar contínuo, nas quais os animais introduzidos corresponderam ao controle, infectado e sentinela, respectivamente. Os animais da segunda câmara foram inoculados pela administração de inóculo de BVDV-1 estirpe Singer citopático por via nasal e oral. Foram avaliadas amostras de sangue, suabe nasal e retal, e no último dia foi realizada eutanásia e necropsia dos animais e coletada amostras de tecidos. No primeiro experimento, ambos os animais inoculados soroconverteram e apresentaram sinais clínicos da infecção, mas somente em um animal foi detectada excreção do vírus por via nasal e presença de RNA viral nos rins, baço e fígado, avaliadas por RT-PCR. Neste caso, a transmissão do vírus por via aerógena não foi comprovada, uma vez que o experimento foi finalizado um di... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: The virus of Bovine Viral Diarrhea (BVDV), belonging to the Pestivirus genus, can cause significant economic losses in cattle. However, this virus can also infect swine, in which infection by BVDV may cause clinical signs, affect the diagnosis of CSF (Classical Swine Fever), and makes them a source of viral spread. Based on these issues, this study aimed to verify whether piglets experimentally infected by BVDV can shed the virus and whether viral airborne transmission is possible. For this, two experiments were carried out. In each experiment, six piglets were distributed in pairs in three isolation chambers, connected by continuous air flow tubes, in which the animals introduced corresponded to control, infected and sentinel, respectively. The animals present in the second chamber were inoculated with BVDV-1 strain Singer cytopathic inoculum by nasally and orally administration. Samples of blood, nasal and rectal swabs, and the last day was conducted euthanasia and necropsy of the animals and tissue samples were evaluated. In the first experiment, both inoculated animals seroconverted and showed clinical signs of infection, but only in one animal nasally virus shedding was detected, as well as, viral RNA presence in kidney, spleen and liver, both identified by RT-PCR. In this case, viral airborne transmission has not been confirmed, since the experiment was finalized one day after the viral shedding. In the second experiment, the two infected animals seroconverted with nine... (Complete abstract click electronic access below) / Mestre Suínos - Doenças. Diarréia. Reação em cadeia da polimerase. Virus. Leitão (Suino) Viruses Polymerase chain reaction
224	Avaliação de diferentes protocolos de extração de DNA para detecção de Brucella abortus a partir de materiais colhidos de feto abortado ou bezerros nascidos de vacas experimentalmente infectadas com a cepa 2308 / Evaluation of differents protocols of DNA extraction for Brucella abortus detection from aborted featus materials or from calves born from experimentally infected cows with 2308 strain Marianna Matrone 10 June 2008 (has links) A Brucella abortus causa diminuição da eficiência reprodutiva em bovinos e é também o agente de uma das zoonoses mais difundidas no mundo. A doença é alvo de programas de controle em muitos países e, no Brasil, seu combate foi melhor organizado a partir de 2001, com o lançamento de programa nacional pelo MAPA. O objetivo do presente estudo foi aperfeiçoar a detecção de B. abortus em homogeneizados de órgãos de fetos abortados por vacas infectadas. Assim, foram comparados diferentes protocolos de extração de DNA, visando à detecção de B. abortus pela PCR em amostras clínicas colhidas de fetos abortados ou bezerros oriundos de vacas experimentalmente desafiadas com B. abortus cepa 2308. Para tanto, foram construídos dois grupos padrão ouro com base na bacteriologia clássica, constituídos por: 32 pulmões (17 positivos ao isolamento), 26 baços (11 positivos ao isolamento), 23 fígados (8 positivos ao isolamento) e 22 linfonodos bronquiais (7 positivos ao isolamento). Todas essas amostras foram submetidas a três distintos protocolos de extração de DNA, seguidos do mesmo processo de amplificação com os primers B4 e B5. A análise dos resultados consolidados mostrou uma sensibilidade de 95% para o protocolo da proteinase K (PK), 86% para o do isotiocianato de guanidina (GT) e de 88% para o de Boom. Os valores encontrados de Sensibilidade para pulmão, baço, fígado e linfonodo foram, respectivamente, 100%, 100%, 100% e 71% (PK), 82%, 100%, 88% e 71% (GT) e 94%, 100%, 63% e 86% (Boom). No grupo dos animais dos quais não foi possível isolar brucellas (gold standard negativo), a PCR resultou positiva em 8 amostras para o protocolo de extração PK (4 pulmões, 1 fígado e 3 linfonodos), em 6 amostras para o protocolo de extração GT (1 pulmão, 3 fígados e 2 linfonodos) e em 37 amostras para o protocolo de extração Boom (10 pulmões, 10 baços, 10 fígados e 7 linfonodos). Esses resultados permitem afirmar que o protocolo de extração PK apresentou a melhor sensibilidade diagnóstica e que o protocolo de extração de Boom apresentou o melhor desempenho nas amostras onde o isolamento foi negativo. Dentre os órgãos estudados, o baço apresentou a maior probabilidade de detecção de B. abortus. Assim, a melhor estratégia para detecção de B. abortus em homogeneizados de órgãos de fetos abortados é a utilização do isolamento e da PCR em paralelo. / Infection by Brucella abortus diminishes the reproductive efficiency in bovines and it is also the agent of one of the most spread zoonosis in the world. In many countries control programs aim this disease, and in Brazil its combat was better organized since 2001 with the creation of the national program by the Ministry of Agriculture, Livestock and Supplies (MAPA). The objective of the present study was to improve the detection of B. abortus in aborted fetus homogenates from infected cows. For that reason, different DNA extraction protocols were compared, focusing the PCR detection of B. abortus in clinical samples collected from aborted fetus or calves obtained from cows experimentally defied with the 2308 B. abortus strain. Therefore, two gold standard groups were built based on classical bacteriology, formed by: 32 lungs (17 isolation positives samples), 26 spleens (11 isolation positives samples), 23 livers (8 isolation positives samples) and 22 bronchial lymph nodes (7 isolation positives samples). All samples were submitted to three distinct DNA extraction protocols, followed by the same amplification process with the primers B4 and B5. The analysis of the consolidated results showed a 95% sensibility for the proteinase K protocol (PK), 86 % for the guanidine isotiocianate (GT) and 88% for the Boom. The sensibility values obtained for lungs, spleen, liver and lymph node were, respectively, 100%, 100%, 100% and 71% (PK), 82%, 100%, 88% and 71% (GT) and 94%, 100%, 63% and 86% (Boom). In the group of animals in which it was not possible to isolate brucellas (negative gold standard), the PCR resulted positively in 8 samples for the PK extraction protocol (4 lungs, 1 liver and 3 lymph nodes), in 6 samples for the GT extraction protocol (1 lung, 3 livers and 2 lymph nodes) and in 37 samples for the Boom extraction protocol (10 lungs, 10 spleens, 10 livers and 7 lymph nodes). These results permit affirming that the PK extraction protocol showed the best diagnostic sensibility and that the Boom extraction protocol showed the best performance in negative isolation samples. Within the studied organs, the spleen showed the highest probability of B. abortus detection. Therefore, the best strategy for B. abortus detection in organs homogenates from aborted fetus is the utilization of isolation and in parallel, the PCR. Brucella abortus Bovinos Brucelose Reação em Cadeia pela Polimerase Brucella abortus Bovine Brucellosis Polymerase Chain Reaction
225	Estudo do nível de infecção por Babesia bovis e Babesia bigemina em bovinos da raça Canchim naturalmente infestados com o carrapato Rhipicephalus (Boophilus) microplus / Bilhassi, Talita Barban. January 2016 (has links) Orientador: Henrique Nunes Oliveira / Coorientador: Márcia Cristina de Sena Oliveira / Banca: Marcos Rogério André / Banca: Janete Aparecida Desidério / Banca: Wilson Malago Junior / Banca: Fernanda de Freitas Anibal / Resumo: Entre as principais causas de perdas produtivas em bovinos criados nos trópicos está a infestação pelo carrapato Rhipicephalus (Boophilus) microplus e, consequentemente, dos hemoparasitas transmitidos por ele. A resistência dos zebuínos e de animais cruzados com raças taurinas à infestação por esse ácaro é amplamente conhecida. Entretanto, no que se refere à suscetibilidade às babesioses bovinas, existem evidências de que o grupo genético também pode interferir na resistência, seguindo o mesmo padrão observado para o carrapato vetor, com os taurinos apresentando maior sensibilidade. Assim, este estudo teve por objetivo avaliar a parasitemia porBabesia bovis e Babesia bigemina em 50 novilhas da raça Canchim ( Charolês + Zebu) naturalmente infestadas pelo R. (B.) microplus nas quatro estações do ano durante 24 meses, além de caracterizar o perfil de citocinas que podem estar associados ao fenótipo de resistência e suscetibilidade aos hemoparasitas do gênero Babesia spp. Foram realizadas contagens de fêmeas adultas de carrapatos com tamanho igual ou superior a 4,5 mm de diâmetro, presentes no lado esquerdo de cada bovino. As amostras de DNA extraídas foram submetidas à amplificação por meio da Reação em Cadeia daPolimerase Quantitativa em Tempo Real (qPCR), utilizando iniciadores que flanqueiam fragmentos dos genes mitocondriais do citocromo b (mt-cyt B), específicos para B. bovis e B. bigemina. O RNA extraído do sangue, foi usado para sintetizar o DNA complementar (cDNA) ... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Among the main causes of production losses in cattle is in the tropics infestation by Rhipicephalus (Boophilus) microplus, and consequently the hemoparasites transmitted by it. The resistance of zebu and crossbred with European breeds to infestation by this mite is widely known. However, as regards susceptibility to bovine babesiosis, there is evidence that genetic group can also interfere in resistance following the same pattern observed in the tick vector, with the taurine presenting greater sensitivity. This study aimed to evaluate parasitaemia by Babesia bovis and Babesia bigemina in 50 heifers Canchim (⅝ Charolais + ⅜ Zebu) naturally infested by R. (B.) microplus in four seasons for 24 months, and characterize the profile of cytokines that may be associated with phenotype resistance and susceptibility by gender hemoparasites Babesia spp. Adult female ticks counts with size equal to or greater than 4.5 mm in diameter, present in the left side of each calf were performed. The extracted DNA samples were subjected to amplification by Reaction Polymerase Chain Quantitative Real Time (qPCR), using primers flanking fragments of mitochondrial gene cytochrome B (mt-cyt B) specific for B. bovis and B. bigemina. The RNA extracted from the blood was used to synthesize complementary DNA (cDNA) for expression analysis of genes IFN-γ, TNF-α, IL-10 and IL-12B by relative quantification (RT-qPCR). Significant differences were observed (P <0.05) between the months of reviews for the tick ... (Complete abstract click electronic access below) / Doutor Babesia. Bovinos. Infecção. Citocinas. Carrapato como transmissor de doenças. Reação em cadeia da polimerase. Polymerase chain reaction Cytokines
226	Detecção e caracterização molecular de cryptosporidium spp. em canários (serinus canaria) mantidos em cativeiro por meio de diferentes métodos de diagnóstico / Camargo, Vinicius da Silva January 2017 (has links) Orientador: Marcelo Vasconcelos Meireles / Banca: Sérgio Diniz Garcia / Banca: Weslen Fabrício Pires Teixeira / Resumo: Este trabalho teve como objetivos determinar a ocorrência e realizar a caracterização molecular de Cryptosporidium spp. e comparar três métodos de detecção deste protozoário em amostras fecais de canários (Serinus canaria) criados em cativeiro nas regiões Sul e Sudeste do Brasil. Um total de 498 amostras foi purificado por centrífugo-flutuação em solução de Sheather. A detecção de Cryptosporidium spp. foi realizada utilizando três métodos de diagnóstico: análise microscópica pela coloração negativa com verde malaquita, nested PCR (gene 18S rRNA), seguida de sequenciamento dos fragmentos amplificados, e PCR em duplex em tempo real (gene 18S rRNA) específica para detecção de Cryptosporidium galli e Cryptosporidium genótipo III de aves. A positividade para Cryptosporidium spp. (total de amostras positivas em pelo menos um método de diagnóstico) obtida pela análise microscópica, nested PCR e PCR duplex em tempo real foi de 13,3% (66/498). As taxas de positividade para Cryptosporidium spp. foram 2,0% (10/498) e 4,6% (23/498) por microscopia e nested PCR, respectivamente. O sequenciamento de 20 amostras amplificadas pela nested PCR identificou C. galli (3,0%;15/498), Cryptosporidium genótipo I de aves (0,8%; 4/498) e Cryptosporidium avium (0,2%; 1/498). A PCR duplex em tempo real revelou positividade de 7,8% (39/498) para C. galli e 2,4% (12/498) para Cryptosporidium genótipo III de aves. A análise microscópica diferiu significativamente da nested PCR para detecção de Cryptosporidi... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: This study used several diagnostic methods to examine the occurrence of and molecularly characterize Cryptosporidium spp. in captive canaries (Serinus canaria) in southern and southeastern Brazil. A total of 498 samples were purified by centrifugal-flotation using Sheather's solution. Cryptosporidium spp. diagnosis was performed using three diagnostic methods: malachite green negative staining, nested PCR targeting the 18S rRNA gene, followed by sequencing the amplified fragments, and duplex real-time PCR targeting the 18S rRNA specific to detect Cryptosporidium galli and Cryptosporidium avian genotype III. The overall positivity for Cryptosporidium spp. (total samples positive in at least one protocol) from the microscopic analysis, nested PCR and duplex real-time PCR protocol results was 13.3% (66/498). The positivity rates were 2.0% (10/498) and 4.6% (23/498) for Cryptosporidium spp. by microscopy and nested PCR, respectively. Sequencing of 20 samples amplified by nested PCR identified C. galli (3.0%; 15/498), Cryptosporidium avian genotype I (0.8%; 4/498) and Cryptosporidium avium (0.2%; 1/498). Duplex real-time PCR revealed a positivity of 7.8% (39/498) for C. galli and 2.4% (12/498) for avian genotype III. Malachite green negative staining differed significantly from nested PCR in detecting Cryptosporidium spp.. Duplex real-time PCR was more sensitive than nested PCR/sequencing for detecting gastric Cryptosporidium in canaries. / Mestre Criptosporidiose. Aves. Reação em cadeia da polimerase. Epidemiologia. Birds cryptosporidiosis Polymerase chain reaction epidemiology
227	Integrated CMOS Polymerase Chain Reaction Lab-on-chip Norian, Haig January 2014 (has links) Considerable effort has recently been directed toward the miniaturization of quantitative-polymerase-chain-reaction [QPCR] instrumentation in an effort to reduce both cost and form factor for point-of-care applications. Notable gains have been made in shrinking the required volumes of PCR reagents, but resultant prototypes retain their bench-top form factor either due to heavy heating plates or cumbersome optical sensing instrumentation. In this thesis, we describe the use of complementary-metal-oxide semiconductor (CMOS) integrated circuit (IC) technology to produce a fully integrated qPCR lab-on-chip. Exploiting a 0.35-µm high-voltage CMOS process, the IC contains all of the key components for performing qPCR. Integrated resistive heaters and temperature sensors regulate the surface temperature of the chip to 0.45°C. Electrowetting-on-dielectric microfluidic pixels are actively driven from the chip surface, allowing for droplet generation and transport down to volumes of less than 1.2 nanoliters. Integrated single-photon avalanche diodes [SPAD] are used for fluorescent monitoring of the reaction, allowing for the quantification of target DNA with more than four-orders-of-magnitude of dynamic range with sensitivities down to a single copy per droplet. Using this device, reliable and sensitive real-time proof-of-concept detection of Staphylococcus aureus (S. aureus) is demonstrated. Molecular diagnosis Labs on a chip Microelectromechanical systems Polymerase chain reaction Electrical engineering
228	Caracterização de protozoários pertencentes à sub-família Toxoplasmatinae pela análise molecular do gene codificador de proteína do choque térmico (HSP70) e do espaçador interno transcrito 1 (ITS-1) / Characterization of protozoan belonging to sub-family Toxoplasmatinae through the molecular analysis from of heat shock protein (HSP70) coding gene and internal transcript spacer 1 (ITS-1) Monteiro, Renata Molina 29 November 2006 (has links) Os membros da sub-famíla Toxoplasmatinae conhecidos são Hammondia hammondi, Toxoplasma gondii, Neospora hughesi, Neospora caninum e Hammondia heydorni. As duas primeiras espécies têm os felídeos como hospedeiro definitivo, enquanto as duas últimas têm desenvolvimento sexual em carnívoros da família dos canídeos. O ciclo biológico de N. hughesi é pouco conhecido. Foi estudado a variabilidade nucleotídica de seqüências intercaladas entre os genes codificadores das frações ribossômicas 18S, 5.8S (ITS-1). No entanto, como estas não permitem reconstruções filogenéticas com o uso de grupo externo, em virtude da inconsistência dos alinhamentos produzidos, pesquisamos uma seqüência codificadora de proteína sendo o marcador escolhido, o gene codificador da proteína de choque térmico HSP70 (heat shock protein 70KDa). Este gene é bastante utilizado para resolução de filogenias de outros organismos como, por exemplo, aqueles pertencentes ao gênero Cryptosporidium. No presente trabalho, amplificamos por PCR e seqüenciamos 951 pares de bases (pb) do gene codificador de HSP70 de oocistos T. gondii-like (oriundos de fezes gatos), de oocistos Neospora-like (de fezes de cães) e de taquizoitos de N. caninum, N. hughesi e T. gondii mantidos em laboratório. Os primers foram desenhados a partir de seqüências consenso obtidas em pesquisa de bancos de dados de seqüências EST de N. caninum e seqüências de RNAm de T. gondii. Seqüências ITS-1 destes oocistos também foram determinadas para a confirmação da espécie de parasito estudada. Os resultados mostram que os táxons H. hammondi e T. gondii são monofiléticos e geneticamente muito próximos, mas contrariando resultados anteriores, não foi demonstrada a monofilia entre os táxons H. heydorni e N. caninum. De fato, a análise de diversidade nucleotídica de gene codificador HSP70 mostra que a distância evolutiva entre H. heydorni e N. caninum é tão grande quanto a distância de cada uma destas espécies com T. gondii. Em adição, foi possível identificar dentre as amostras de oocistos, duas linhagens divergentes de H. heydorni. Paralelamente ao estudo filogenético também foi possível desenvolver um método diagnostico diferencial para oocistos tipo Hammondia. As seqüências de gene HSP70 obtidas foram alinhadas e dois pares de primers internos a estas seqüências foram desenhados. O primeiro par amplifica 771 pb de oocistos T. gondii-like e o segundo 400 pb de oocistos Neospora-like. A clivagem do fragmento de 771 pb com enzima de restrição Hin6I produz perfis eletroforéticos distintos para amostras de T. gondii e H. hammondi. A clivagem do fragmento de 400pb com a enzima de restrição MunI também produz perfis eletroforéticos distintos entre amostras de N. caninum e H. heydornii. A diferenciação dos perfis de restrição pode ser feita em eletroforese em gel de agarose a 2,5%. / Hammondia hammondi, Toxoplasma gondii, Neospora huguesi, Neospora caninum and Hammondia heydorni are the known members of the sub-family Toxoplasmatinae. H. heydorni and N. caninum use canids as definitive hosts whereas felids are the definitive hosts from T. gondii and H. hammondi. The definitive host of N. hughesi is unknown. Here, the nucleotide diversity at internal transcribed spacer (ITS-1) and heat shock protein (HSP70 kDa) loci in the subfamily toxoplasmatinae were studied. The HSP70 coding genes are widely used for phylogenetic studies in a number of other organisms specially within the genus Cryptosporidium. In the present study, it was amplified by PCR and sequenced 951 bases pairs (bp) from HSP70 coding gene from oocysts T.gondii-like (from cat), from oocysts N. caninum-like (from dog) and tachyzoites of N. hughesi grown on cell cultures. The primers were designed based on consensus sequences within EST sequences of N. caninum sequences and RNAm sequences of T. gondii. ITS-1 sequences amplified from oocysts were also obtained in order to confirm the species of the parasites. The results showed that T. gondii and H. hammondi are monophyletic and genetically very close, but the monophyletic status of H. heydorni N. caninum was not demonstrated. In fact, the nucleotide diversity at the HSP70 locus has shown that the evolutionary distance between H. heydorni and N. caninum is as high as that observed between either H. heydorni or N. caninum and T. gondii., In addition, it was possible to identify two distinct groups among the H. heydorni oocysts. Concomitantly to the phylogenetic study it was also possible to standardize a diagnostic test capable of differentiate the oocysts Hammondia-like was development a diagnostic method that differ oocysts T. gondii-like and N. caninum-like. The sequences obtained from HSP70 coding gene were aligned and two new pair of PCR primers was designed. The first pair amplifies 771bp from T. gondii-like oocysts, whereas the second pair amplifies 400 bp from N. caninum-like oocysts. The restriction enzyme Hin6I used to cleave the 771 bp amplicons generated distinct profiles with samples from H. hammondi and T. gondii. The same occurred with the restriction of the fragments of 400bp cleaved by the enzyme MunI used in N. caninum e H. heydorni samples. The profiles can be differentiated by 2.5% agarose gel electrophoresis. diagnostic diagnóstico feaces fezes polymerase chain reaction reação em cadeia pela polimerase
229	Detecção de microrganismos, quantificação de endotoxinas e avaliação in vivo do extrato glicólico de própolis em dentes com necrose pulpar e lesão periapical / Xavier, Ana Claudia Carvalho. January 2011 (has links) Orientador: Cláudio Antonio Talge Carvalho / Banca: Flaviana Bombarda de Andrade / Banca: Marcia Carneiro Valera / Resumo: Este estudo avaliou in vivo a ação do extrato glicólico de própolis 12%, como substância química auxiliar em tratamentos endodônticos de dentes com necrose pulpar e lesão periapical. A avaliação foi realizada através da cultura e detecção de microrganismos por Reação em Cadeia Polimerase (PCR) e da quantificação de endotoxinas. Além disso, foi avaliada a correlação entre o tamanho da lesão periapical e a quantidade de endotoxinas presente. Foram selecionados 30 dentes, os quais foram divididos em 3 grupos (n=10), de acordo com a substância química auxiliar utilizada para a instrumentação: NaOCl) Hipoclorito de sódio 1%; CLX) Clorexidina gel 2%, intercalada com solução salina; PRO) Extrato glicólico de própolis 12%, intercalado com solução salina. As radiografias iniciais foram digitalizadas e as lesões periapicais foram medidas através de software específico. Foram realizadas 3 coletas do conteúdo do canal radicular: após a abertura coronária, após instrumentação e após 14 dias da medicação intracanal. A medicação intracanal utilizada foi o hidróxido de cálcio com propilenoglicol. Em todas as coletas realizou-se: detecção de microrganismos por PCR; avaliação do crescimento microbiológico em diferentes meios de cultura e quantificação de endotoxinas através do teste cinético cromogênico (LAL). Os resultados foram analisados através dos testes de Kruskal Wallis, Dunn (nível de significância 5%) e correlação linear de Pearson. A quantidade de microrganismos e endotoxinas, nas 2ª e 3ª coletas, diminuiu em relação à 1ª coleta, em todas as soluções avaliadas (p<0,05). Os canais apresentaram diversidade microbiana, com predominância de Parvimonas micra, Tanerella forsythia e Prevotella nigrescens. Concluiu-se que o extrato glicólico de própolis 12% apresentou atividade antimicrobiana e antiendotóxica semelhante aos demais ... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: The aim of this study was in vivo evaluated of 12% propolis glycolic extract action in root canal treatments, through the culture of microorganisms, quantification of endotoxins and detection of microorganisms by molecular method of polymerase chainreaction (PCR). A total of 30 human teeth were divided into 3 groups (n=10) according to the auxiliary chemical solution used for biomechanical preparation: NaOCl) sodium hypoclorite 1%; CLX) 2% chlorhexidine gel; PRO) 12% propolis glycolic extract. Collections were performed immediately after coronary open, after instrumentation and after 14 days with intracanal medication. For all collections were performed the following tests: microorganisms detection by PCR; assessment of microbiological growth and analyzing the amount of endotoxi (Limulus amoebocyte lysate). The results showed a decrease in the amount of microorganisms and endotoxins in the 2nd and 3rd collections of all irrigation solutions. The canals showed microbial diversityy, but Parvimonas micra was predominantly. It was concluded thar all solutions are evaluated antimicrobial and anti-endotoxic similar. The most common microorganism present in root canals with pulp necrosis and periapical lesion was Parvimonas microns. There is a evidence that the higher amount of endotoxins is in the biggest lesions / Mestre Própole. Tratamento do canal radicular. Root canals irrigants. eng Polymerase chain reaction. eng Endotoxins. eng Propolis. eng
230	Genes de virulência e perfil de susceptibilidade a extratos vegetais de isolados de Escherichia coli enterotoxigênicas (ETEC), shigatoxigênicas (STEC) e enteropatogênicas (EPEC) em bezerros / Azola, Juliana da Silva Menezes. January 2016 (has links) Orientador: Fernando Antônio de Ávila / Banca: Luiz Carlos do Nascimento / Banca: Roberta Hilsdorf Piccoli / Banca: Hélio José Montassier / Banca: Karina Paes Bürger / Resumo: A diarreia neonatal é uma das mais recorrentes enfermidades que acometem bezerros, acarretando prejuízos à pecuária leiteira. Nestes casos, um dos micro-organismos mais prevalentes é Escherichia coli, relacionada à contaminação fecal e a surtos alimentares. Para o tratamento, a crescente resistência bacteriana a antimicrobianos leva à busca por novas alternativas farmacológicas. O presente trabalho teve como objetivo geral testar a susceptibilidade de isolados de E. coli oriundos de bezerros neonatos diarreicos e sem diarreia a extratos vegetais. Os animais pertenceram a fazendas destinadas à produção leiteira no Estado de Minas Gerais, Brasil. As amostras foram submetidas ao isolamento microbiológico, à sorologia, à identificação genética por PCR e a testes antimicrobianos. Em relação aos antissoros polivalentes, houve isolados positivos a sorogrupos de importância clínica em humanos, como O26 e O111. Foram isoladas 36 estirpes oriundas de animais acometidos, positivas para pelo menos um gene testado, sendo eles stx1, stx2, eae, bfp e Sta. Relacionadas ao isolamento de animais sem diarreia, 9 estirpes foram carreadoras dos genes stx1, stx2 ou ambos, caracterizando os bovinos como reservatórios do patótipo STEC. O gene LT-II não foi encontrado. Quanto aos testes de susceptibilidade, encontrou-se isolados resistentes a diferentes classes de antimicrobianos. Entre os extratos testados, houve sensibilidade frente à planta Salvia officinalis L. (sálvia). Assim, esta vertente de e... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Neonatal diarrhea is one of the most recurrent illnesses that affect calves, resulting in losses to dairy farming. In these cases, one of the most prevalent microorganisms is Escherichia coli that is related to fecal contamination and food outbreaks. For the treatment, the increase bacterial resistance to antimicrobials leads to the search for new pharmacological alternatives. The main aim of this study was to test the susceptibility of E. coli isolated from neonatal calves with diarrhea and healthy to plant extracts. The animals were found in farms which are dairy-producing in the State of Minas Gerais, Brazil. The samples were subject to microbiological isolation, serology, PCR genetic identification and antimicrobial testing. In relation to polyvalent antiserum, there were positive isolates of clinical importance of serogroups in humans, such as O26 and O111. Thirty six strains were isolated from affected animals and they were positive to at least one gene tested, such as stx1, stx2, eae, bfp and Sta. Related to the healthy animals, 9 strains were carriers of the genes stx1, stx2 or both, characterizing the cattles as reservoirs of pathotype STEC. The gene LT-II was not found. In relation to susceptibility tests, resistant isolates to different classes of antimicrobials were found. Among the extracts that were tested, there was sensitivity to the Salvia officinalis L. plant (sálvia). Thus, this aspect of study can be alternative to combat the bacterial pathogens, valid for future tests as to the discovery of new chemical compounds with antimicrobial activity / Doutor Colibacilose. Reação em cadeia da polimerase. Bovino - Doenças. Bezerro. Enterobacterias. Polymerase chain reaction.

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