Global ETD Search

51	Cellular and molecular characterization of inflammation in the injured spinal cord Ghasemlou, Nader. January 2008 (has links) Spinal cord injury (SCI) results in a well-orchestrated inflammatory response which causes secondary tissue damage. Activated macrophages contribute to this cytotoxic response, which includes damage to neurons, glia and myelin, and tissue loss that worsens functional outcomes after SCI. However, activated macrophages in the spinal cord under other conditions are not cytotoxic, such as after intraspinal injection of lysophosphatidylcholine (LPC), a potent demyelinating agent. Recovery from SCI may be optimized by reducing the detrimental effects of macrophages while promoting their beneficial ones. Therefore, I compared spinal cord tissue, as well as purified macrophages, from mice after SCI (cytotoxic response) and intraspinal LPC injection (non-cytotoxic response). As a first step to carry out this work, I characterized the injury parameters for SCI contusion injury (i.e. injury force and spinal cord displacement) in mice using the Infinite Horizons impactor (Chapter 2). This lesioning model was used in other work for the thesis. The role T cells may play in mediating macrophage activation after LPC microinjection and SCI was also assessed using Nude mice (Chapter 3). Next, Affymetrix GeneChip analysis was carried out on spinal cord tissue obtained at the peak of the macrophage response after SCI and intraspinal LPC injection to identify potential candidate genes that may control the divergent inflammatory responses (Chapter 4). Several potential genes were identified. I next characterized the expression and role of one of these genes, MAPK activated protein kinase 2 (MK2), and showed that it mediates secondary tissue damage after SCI via several mechanisms (Chapter 5). The differences in gene expression profiles of macrophages purified from the spinal cord after SCI and LPC-injection were also assessed (Chapter 6). This microarray analysis of macrophages led to the identification of 10 novel candidate genes, two of which were validated at the protein level. Finally, I also examined the expression and role of secretory leukocyte protease inhibitor (SLPI) in SCI (Chapter 7). Using a combination of knockout/overexpressing transgenic mice and recombinant SLPI, I found that SLPI mediates protective anti-inflammatory effects after SCI. In conclusion, work done for this thesis has led to the identification of several novel molecules that influence the inflammatory response after injury and thus have led to the identification of potentially novel targets for the development of pharmacological approaches to treat acute SCI. Spinal Cord Injuries -- complications. Inflammation -- etiology. Lysophosphatidylcholines. Mice. Mice, Inbred BALB C.
52	Cannabinoids suppress dendritic cell-induced T helper cell polarization / Lu, Tangying (Lily). January 2006 (has links) Dissertation (Ph.D.)--University of South Florida, 2006. / Includes vita. Includes bibliographical references (leaves 86-105). Also available online.
53	Sono e imunidade: evidências em voluntários saudáveis e em modelo murino de transplante de pele / Sleep and immunity: evidence in healthy volunteers and mice skin allograft model Silva, Francieli Ruiz da [UNIFESP] January 2011 (has links) (PDF) Made available in DSpace on 2015-12-06T23:45:03Z (GMT). No. of bitstreams: 0 Previous issue date: 2011 / BV UNIFESP: Teses e dissertações Privação do Sono Linfócitos Citocinas Imunidade Transplante de Pele Camundongos Endogâmicos BALB C Camundongos Endogâmicos C57BL Animais Adulto Humanos
54	On the expression and deficiency of 5,10-methylenetetrahydrofolate reductase in murine sperm development Cushnie, Duncan Wells. January 2008 (has links) No description available. Mice, Inbred C57BL. Mice. Mice, Inbred BALB C. Spermatogenesis -- genetics.
55	Long-term dietary folate deficiency and intestinal tumor development in mice Knock, Erin Heather, 1981- January 2008 (has links) No description available. Folic Acid Deficiency -- complications. Mice, Inbred C57BL. Mice. Mice, Inbred BALB C. Colorectal Neoplasms -- metabolism.
56	Cellular and molecular characterization of inflammation in the injured spinal cord Ghasemlou, Nader. January 2008 (has links) No description available. Inflammation -- etiology. Spinal Cord Injuries -- complications. Mice, Inbred BALB C. Mice. Lysophosphatidylcholines.
57	Emprego da citotoxicidade basal in vitro na redução do número de animais em ensaios de avaliação da toxicidade oral aguda: a grandisina e seu metabólito majoritário como protótipos / Use of basal cytotoxicity in vitro in reducing the number of animals tests in the evaluation of acute oral toxicity: a grandisin and its major metabolite as prototypes VIEIRA, Marcelo de Sousa 14 April 2009 (has links) Made available in DSpace on 2014-07-29T15:29:08Z (GMT). No. of bitstreams: 1 Marcelo de sousa Vieira.pdf: 1862129 bytes, checksum: 7cc8be40ceb11c75c5ec56b362ffec29 (MD5) Previous issue date: 2009-04-14 / The animal replacement in expirements has been very encouraged by government and other institutions. However, in drugs development the animal replacement is not yet a reality, like at oral acute systemic tests. The validation of in vitro protocols is necessary for data generation with reproducibility, repetability and accuracy. In this study was validated at the Laboratório de Farmacologia e Toxicologia Celular- Faculdade de Farmácia/Universidade Federal de Goiás the protocol already validated by three laboratories (two in the USA and one at United Kingdom) and coordinated by ICCVAM: In Vitro Cytotoxicity Methods for Estimating Starting Doses for Acute Systemic Toxicity Tests, using the neutral red uptake in BAL/c 3T3-A31 cell line. It was used the grandisine, a lignan, and its major metabolite taken by fungi biodegradation. Our research group has identified a potential anti-tumoral action of grandisine, data not yet published. After in house validation we estimated the LD50 of grandisin and 4-O-demethylgrandisin: 617.72 mg/kg and 429.95 mg/kg, respectively. Both were classified under the GSH category 4. / A substituição ou redução do uso de animais em experimentos para a avaliação de toxicidade tem sido bastante encorajada e tem recebido grandes incentivos, inclusive financeiros, governamentais e institucionais. No entanto, a substituição completa da maioria dos testes mandatórios por agências reguladoras do setor ainda não é realidade, a exemplo, o teste de toxicidade oral aguda sistêmica. Neste contexto, se aplica a validação de testes in vitro para estimar dados in vivo. No presente trabalho, realizamos a validação in house do protocolo internacional e multilaboratorial recomendado pelo Interagency Coordinating Committee on the Validation of Alternative Methods (ICCVAM): Utilização da Citotoxicidade In Vitro na Estimativa de Doses Iniciais para Testes de Toxicidade Oral Aguda Sistêmica. Para tal, utilizamos o método de captação do corante vermelho neutro e a linhagem celular fibroblástica de camundongos BALB/c 3T3-A31. Dentre as substâncias recomendadas pelo ICCVAM para a validação do método foram investigadas 9 substâncias. A metabolização de produtos pelo organismo vivo é uma grande limitação dos testes in vitro. Utilizamos a grandisina, um tipo de ligana com grande potencial antitumoral e seu metabólito majoritário como substâncias modelos. Com utilização do metabólito conseguimos transpor esta barreira dos testes in vitro. Os resultados demonstraram que os dados obtidos estão em consonância com os dados da literatura sendo possível classificar ambas as substâncias na categoria GHS 4: grandisina e 4-Odemetilgrandisina: 617,72 mg/kg and 429,95 mg/kg, respectivamente. Correlação IC50 x DL50 Corante Vermelho Neutro Balb/c 3T3-A31 Grandisina Metabólito Correlation IC50 x LD50 NRU assay Balb/c 3T3-A31 cells Grandisin Metabolite CNPQ::CIENCIAS DA SAUDE
58	Toxocaríase murina experimental: diagnóstico por PCR e comparação com técnicas imunológicas / Experimental murine toxocariasis: PCR diagnosis and its comparison with immunological techniques Fonseca, Gabriela Rodrigues e 03 July 2018 (has links) A toxocaríase é considerada uma das cinco parasitoses negligenciadas pelo Centers for Disease Control and Prevention e recebe ainda pouca atenção. As metodologias diagnósticas conhecidas são bem estabelecidas, apresentando, porém, limitações caracterizadas, sobretudo, pela ocorrência de reações-cruzadas. A biologia molecular mostra grandes avanços para o diagnóstico eficaz de diversas parasitoses, mas ainda carece de estudos em amostras de fácil obtenção para o diagnóstico da toxocaríase. Para aprimorar o conhecimento sobre a importância da técnica da Reação em Cadeia da Polimerase Convencional (PCR) e sua relação com técnicas diagnósticas já conhecidas, foram utilizados 42 camundongos BALB/c, machos, entre 6 a 8 semanas de vida, divididos em três grupos, inoculados com 5, 50 ou 500 ovos larvados e sangrados pelo plexo orbital aos 15, 30, 60 e 90 dias pós infecção. Ainda, do total, 24 camundongos foram sangrados aos 120 dias pós infecção. Ao final do experimento, foi realizada a recuperação de larvas e a PCR de tecido hepático, cérebro e carcaça de camundongos dos grupos infectados. As amostras de soro foram processadas pelas técnicas de ELISA, Western-blotting e PCR. O ELISA e o Western-blotting mostraram resultados reagentes em todas as datas para a maioria dos inóculos de ovos, com relação diretamente proporcional entre a detecção de anticorpos e a carga parasitária. Durante o período da infecção, a detecção de IgG foi mais intensa próxima aos 60 dias pós-infecção para a maioria dos inóculos de ovos, por ambos os métodos imunológicos. Apesar de identificar DNA de larvas e vermes adultos, a PCR não foi capaz de detectar DNA do parasito em amostras de soro em todos os grupos e datas pós-infecção. Em contrapartida, foi detectado DNA do parasito em todos os órgãos com ao menos um dos primers utilizados. Foram recuperadas larvas na maioria dos órgãos com maior porcentagem de recuperação relatada nos animais inoculados com 50 ovos larvados. O diagnóstico molecular, utilizando sangue do paciente, ainda não pode ser considerado uma ferramenta para o diagnóstico dessa infecção / Toxocariasis is considered by the Centers for Disease Control and Prevention one of the five neglected diseases and still receives little attention. The diagnostic methods are well established, presenting, however, limitations characterized mainly by the occurrence of cross-reactions. Molecular biology shows great advance for the effective diagnosis of several parasitic infections, but still lacks studies using samples that are easily obtained for the diagnosis of toxocariasis. In order to refine the knowledge about the importance of Conventional Polymerase Chain Reaction (PCR) and its relation with known techniques, 42 BALB/c male mice, between 6-8 weeks of age were inoculated with 5, 50 and 500 embryonated eggs respectively and bled by the orbital plexus at 15, 30, 60 and 90 days post infection. Also, 24 of 42 animals were bled the same way at 120 days post-infection. At the end of the experiment, larval recovery and conventional PCR were performed in liver, brain and carcass of mice of the infected groups. Serum samples were processed by ELISA, Western-blotting and PCR. The ELISA and Western-blotting techniques showed positive results in all days post infection for most eggs inocula and showed a directly proportional dependence between the infective dose and the level of antibodies. During the course of the infection, IgG detection was most intense near 60 days post infection for most eggs inocula, for both diagnostic methods. Despite positive DNA identification in larvae and adult worms, PCR wasn\'t able to detect parasite DNA in serum samples in all infected groups and days post infection. In contrast, parasite DNA was detected in all organs with at least one of the primers. Larvae were recovered from most organs, and animals inoculated with 50 embryonated eggs showed the highest percentage of larval recovery. Molecular diagnosis using patient\'s blood is not the best tool for toxocariasis diagnosis so far Balb c Blotting western Camundongos Ensaio de imunoadsorção enzimática Enzyme-linked immunosorbent assay PCR Polymerase chain reaction Toxocara canis Toxocara canis Toxocaríase Toxocariasis Western blotting
59	Effect of ascorbic acid on 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine-induced toxicity in the brain of balb/c mouse. / CUHK electronic theses & dissertations collection January 2004 (has links) by Chan Tak Yee Bonita. / "July 2004." / Thesis (Ph.D.)--Chinese University of Hong Kong, 2004. / Includes bibliographical references (p. 121-137). / Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Mode of access: World Wide Web. / Abstracts in English and Chinese. Vitamin C--Therapeutic use Mice--Diseases Pyridine Ascorbic Acid--therapeutic use Mice, Inbred BALB C
60	Toxocaríase murina experimental: diagnóstico por PCR e comparação com técnicas imunológicas / Experimental murine toxocariasis: PCR diagnosis and its comparison with immunological techniques Gabriela Rodrigues e Fonseca 03 July 2018 (has links) A toxocaríase é considerada uma das cinco parasitoses negligenciadas pelo Centers for Disease Control and Prevention e recebe ainda pouca atenção. As metodologias diagnósticas conhecidas são bem estabelecidas, apresentando, porém, limitações caracterizadas, sobretudo, pela ocorrência de reações-cruzadas. A biologia molecular mostra grandes avanços para o diagnóstico eficaz de diversas parasitoses, mas ainda carece de estudos em amostras de fácil obtenção para o diagnóstico da toxocaríase. Para aprimorar o conhecimento sobre a importância da técnica da Reação em Cadeia da Polimerase Convencional (PCR) e sua relação com técnicas diagnósticas já conhecidas, foram utilizados 42 camundongos BALB/c, machos, entre 6 a 8 semanas de vida, divididos em três grupos, inoculados com 5, 50 ou 500 ovos larvados e sangrados pelo plexo orbital aos 15, 30, 60 e 90 dias pós infecção. Ainda, do total, 24 camundongos foram sangrados aos 120 dias pós infecção. Ao final do experimento, foi realizada a recuperação de larvas e a PCR de tecido hepático, cérebro e carcaça de camundongos dos grupos infectados. As amostras de soro foram processadas pelas técnicas de ELISA, Western-blotting e PCR. O ELISA e o Western-blotting mostraram resultados reagentes em todas as datas para a maioria dos inóculos de ovos, com relação diretamente proporcional entre a detecção de anticorpos e a carga parasitária. Durante o período da infecção, a detecção de IgG foi mais intensa próxima aos 60 dias pós-infecção para a maioria dos inóculos de ovos, por ambos os métodos imunológicos. Apesar de identificar DNA de larvas e vermes adultos, a PCR não foi capaz de detectar DNA do parasito em amostras de soro em todos os grupos e datas pós-infecção. Em contrapartida, foi detectado DNA do parasito em todos os órgãos com ao menos um dos primers utilizados. Foram recuperadas larvas na maioria dos órgãos com maior porcentagem de recuperação relatada nos animais inoculados com 50 ovos larvados. O diagnóstico molecular, utilizando sangue do paciente, ainda não pode ser considerado uma ferramenta para o diagnóstico dessa infecção / Toxocariasis is considered by the Centers for Disease Control and Prevention one of the five neglected diseases and still receives little attention. The diagnostic methods are well established, presenting, however, limitations characterized mainly by the occurrence of cross-reactions. Molecular biology shows great advance for the effective diagnosis of several parasitic infections, but still lacks studies using samples that are easily obtained for the diagnosis of toxocariasis. In order to refine the knowledge about the importance of Conventional Polymerase Chain Reaction (PCR) and its relation with known techniques, 42 BALB/c male mice, between 6-8 weeks of age were inoculated with 5, 50 and 500 embryonated eggs respectively and bled by the orbital plexus at 15, 30, 60 and 90 days post infection. Also, 24 of 42 animals were bled the same way at 120 days post-infection. At the end of the experiment, larval recovery and conventional PCR were performed in liver, brain and carcass of mice of the infected groups. Serum samples were processed by ELISA, Western-blotting and PCR. The ELISA and Western-blotting techniques showed positive results in all days post infection for most eggs inocula and showed a directly proportional dependence between the infective dose and the level of antibodies. During the course of the infection, IgG detection was most intense near 60 days post infection for most eggs inocula, for both diagnostic methods. Despite positive DNA identification in larvae and adult worms, PCR wasn\'t able to detect parasite DNA in serum samples in all infected groups and days post infection. In contrast, parasite DNA was detected in all organs with at least one of the primers. Larvae were recovered from most organs, and animals inoculated with 50 embryonated eggs showed the highest percentage of larval recovery. Molecular diagnosis using patient\'s blood is not the best tool for toxocariasis diagnosis so far Camundongos Ensaio de imunoadsorção enzimática PCR Toxocara canis Toxocaríase Western blotting Balb c Blotting western Enzyme-linked immunosorbent assay Polymerase chain reaction Toxocara canis Toxocariasis

Search results