Global ETD Search

31	Untersuchung des Effektes der Leukotrienbiosynthesehemmung nach experimentellem Schädel-Hirn-Trauma Voigt, Cornelia 26 June 2013 (has links) (PDF) Gegenstand der Dissertationsschrift ist die Untersuchung des Effektes einer Hemmung der Leukotrienbiosynthese auf die Entwicklung des Schädel-Hirn-Traumas (SHT) nach experimenteller fokaler Kontusionsverletzung im Rattenmodell. Die Ergebnisse der Arbeit wurden im Jahre 2011 in einer Publikation veröffentlicht. Das SHT ist eine schwerwiegende globale Erkrankung mit hoher Inzidenz und Mortalität. Diese führt zu hohen Kosten für das Gesundheitssystem, zum einen durch die akute Behandlung im Krankenhaus, zum anderen durch die sich daran anschließenden rehabilitativen Maßnahmen. Nach der primär biomechanischen Verletzung des Hirns, die nicht beeinflussbar ist, bietet die anschließende sekundäre Hirnschädigung aufgrund verschiedener Stoffwechselprozesse Angriffspunkte für eine (medikamentöse) Therapie des SHT. Die sekundären Hirnschäden werden maßgeblich durch die Entwicklung eines perikontusionellen Hirnödems und dem daraus resultierenden Anstieg des intrakraniellen Druckes beeinflusst. Wie in vorangegangenen Untersuchungen gezeigt werden konnte, kam es nach experimentellem SHT zu einem signifikanten Anstieg der Leukotrienwerte im Liquor von Ratten. Dies warf die Frage nach der Rolle der Leukotriene (LT) im posttraumatischen Hirnstoffwechsel bezüglich der Ödementwicklung auf. Ziel dieser Arbeit war der Nachweis einer direkten Beteiligung von Leukotrienen an der sekundären Hirnschädigung und das Aufzeigen eines möglichen therapeutischen Zuganges durch Substitution von Leukotrienbiosynthesehemmern. Dafür wurde bei adulten Ratten ein fokales SHT induziert. Anschließend wurden in zwei Therapiegruppen zwei unterschiedlich wirkende Leukotrieninhibitoren mehrmalig oral verabreicht und die Ausprägung des SHTs nach 24 bzw. 72 Stunden mittels Magnetresonanztomographie (MRT) und immunhistochemischen Aufarbeitung der Hirne mit einer nicht therapierten Kontrollgruppe verglichen. Bei einem dieser LT-Inhibitoren handelte es sich um ein Weihrauchpräparat, das als Nahrungsergänzungsmittel bereits zu erhalten ist und somit auch potentiell am Menschen zur Anwendung kommen kann. Die Ergebnisse waren vielversprechend und zeigten in beiden Therapiegruppen ein verringertes Kontusionsvolumen im MRT und immunhistochemisch einen geringeren Verlust von Neuronen im perikontusionellen Bereich. Somit scheinen Leukotriene einen Anteil an den sekundären Schädigungsprozessen nach SHT zu tragen. Weitere Untersuchungen, vor allem bezüglich eines eventuell verbesserten klinischen Outcome durch Leukotrienbiosynthesehemmung, erscheinen sinnvoll um den potentiellen Einsatz von LT-Synthesehemmstoffen in der Therapie des SHT in Erwägung ziehen zu können. Schädelhirntrauma SHT Leukotriene Ratte Boscari Boswelliasäuren brain trauma leucotrienes controlled cortical impact model ddc:610
32	Leukotrienes and leukotriene receptors : potential roles in cardiovascular diseases / Qiu, Hong, January 2007 (has links) Diss. (sammanfattning) Stockholm : Karol. inst., 2007. / Härtill 4 uppsatser.
33	The nuclear factor k[kappa]B signal transduction pathway : its role in atherogenesis and intimal hyperplasia / Bu, De-xiu, January 2006 (has links) Diss. (sammanfattning) Stockholm : Karol. inst., 2006. / Härtill 4 uppsatser.
34	Studies on molecular properties and functional regulation of terminal leukotriene C₄ synthases and cysteinyl-leukotriene receptor signalling in human endothelium / Schröder, Oliver, January 2007 (has links) Diss. (sammanfattning) Stockholm : Karolinska institutet, 2007. / Härtill 4 uppsatser.
35	Catalytic mechanisms and evolution of leukotriene A₄ hydrolyse / Tholander, Fredrik Otto, January 2006 (has links) Diss. (sammanfattning) Stockholm : Karolinska institutet, 2006. / Härtill 6 uppsatser.
36	Lipid mediators in the development and resolution of experimental lyme arthritis Blaho, Victoria Alison. January 2007 (has links) Thesis (Ph. D.)--University of Missouri-Columbia, 2007. / The entire dissertation/thesis text is included in the research.pdf file; the official abstract appears in the short.pdf file (which also appears in the research.pdf); a non-technical general description, or public abstract, appears in the public.pdf file. "May 2007" Includes bibliographical references.
37	Aminopeptidase básica e leucotrieno-A4-hidrolase em ratos sensíveis e insensíveis à indução de artrite por colágeno tipo II / Basic aminopeptidase and Leukotriene-A4-hydrolase of rats sensitive and insensitive to induction of arthritis by type-II collagen Mariana Trivilin Mendes 01 February 2013 (has links) Atualmente, ainda é incerto se a hidrólise de L-arginil-β-naftilamida (ArgNA) e do leucotrieno (LT) A4 pela LT-A4-hidrolase (LT-A4-H) (EC 3.3.2.6) e pela aminopeptidase básica (APB) (EC 3.4.11.6) tem influência no desenvolvimento da artrite induzida por colágeno (CIA). O objetivo deste estudo foi investigar a inter-relação entre LT-A4-H, APB e LT-B4 em ratos submetidos à CIA. Cromatografia líquida de alta eficiência (HPLC), ensaio imunoenzimático (EIA), espectrofluorimetria e reação quantitativa em tempo real em cadeia da polimerase (qPCR) foram usados como metodologias. A existência dos genes para as proteínas EC 3.3.2.6 e EC 3.4.11.6 foi confirmada no tecido sinovial (TS) de ratos controles sadios. A hidrólise de ArgNA aumentou na fração solúvel (FS) dos animais submetidos à CIA que desenvolveram a doença (artríticos-CIA) em comparação com aqueles que não desenvolveram a doença (resistentes-CIA) e com os controles sadios. No líquido sinovial (SY) e no plasma sanguíneo houve menor hidrólise de ArgNA em resistentes em comparação aos artríticos e controles. Nas células mononucleares do sangue periférico (PBMCs), os níveis de hidrólise de ArgNA aumentaram na FS de controles e na fração de membrana (FM) dos resistentes em comparação aos artríticos. Em comparação com controles sadios, a hidrólise de LT-A4 aumentou no SY e na FS de PBMCs de artríticos e resistentes. A hidrólise de LT-A4 também aumentou na FM do TS de resistentes e diminuiu na FM de PBMCs em artríticos e resistentes. Em todos estes compartimentos a hidrólise de ArgNA permaneceu inalterada ou relacionou-se inversamente com a hidrólise de LT-A4, comparativamente aos controles sadios. A hidrólise de ArgNA diferiu entre os artríticos e resistentes em FM-TS, FS-TS, FM-PBMCs, SY e no plasma sanguíneo. Uma relação no mesmo sentido foi encontrada entre alterações na hidrólise de LT-A4 e nos níveis de LT-B4 apenas em SY e FM-PBMCs dos artríticos e resistentes e em FM-TS dos resistentes, comparativamente aos controles sadios. Em conclusão, a atividade APB é um novo marcador que distingue ratos artríticos e resistentes no modelo CIA. Os níveis de LT-B4 em ratos não são controlados somente pela LT-A4-H. Alterações na atividade LT-A4-H e nos níveis de LT-B4 são indistinguíveis entre artríticos e resistentes, mas tais alterações marcadamente distinguem essas duas condições da condição saudável. LT-A4-H e APB estão relacionadas de uma forma compartimento-dependente, atuando como enzimas independentes, com modulação diferencial das suas especificidades, eficiências e/ou afinidades catalíticas sobre os substratos epóxi e peptídico, ou como enzimas bifuncionais, cujas atividades são inversamente relacionadas devido à inibição concorrente de uma destas atividades / Whether L-arginyl-β-naphthylamide (ArgNA) and leukotriene (LT)-A4 hydrolyses by LT-A4 hydrolase (LT-A4-H) (EC 3.3.2.6) and basic aminopeptidase (APB) (EC 3.4.11.6) influence the development of collagen-induced arthritis (CIA) is presently uncertain. The objective of this study was to investigate the interrelationship among LT-A4-H, APB and LT-B4 in CIA rats. High-performance liquid chromatography (HPLC), enzyme immunoassay (EIA), spectrofluorometry and quantitative real time polymerase chain reaction (qPCR) were used as methodologies. The existence of genes for EC 3.3.2.6 and EC 3.4.11.6 proteins were confirmed in the synovial tissue (TS) of healthy control rats. ArgNA hydrolysis was higher in soluble fraction (FS) in rats submitted to CIA that developed the disease (CIA-arthritic) than in those that did not develop the disease (CIA-resistant) or healthy control. Synovial fluid (SY) and blood plasma had lower ArgNA hydrolysis in CIA-resistant than in CIA-arthritic or control. In the peripheral blood mononuclear cells (PBMCs) the levels of ArgNA hydrolysis increased in FS of control and in membrane-bound fraction (FM) of CIA-resistant in comparison with CIA-arthritic. Compared with healthy control, LT-A4 hydrolysis increased in SY and in FS from PBMCs of CIA-arthritic and CIA-resistant. LT-A4 hydrolysis also increased in FM from TS of CIA-resistant and decreased in PBMCs-FM of CIA-arthritic and CIA-resistant. In all these locations hydrolysis of ArgNA remained unchanged or it was inversely related with LT-A4 hydrolysis, comparatively to healthy control. ArgNA hydrolysis differed between CIA-arthritic and CIA-resistant in TS-FM, TS-FS, PBMCs-FM, SY and blood plasma. A same-sense relationship was found between changes on LT-A4 hydrolysis and LT-B4 levels only in SY and PBMCs-FM of CIA-arthritic and CIA-resistant and in TS-FM of CIA-resistant, comparatively to healthy control. In conclusion, the APB activity is a novel distinctive marker of CIA-arthritic and CIA-resistant statuses. The levels of LT-B4 in rats are not controlled only by LT-A4-H. Changes on LT-A4-H activity and LT-B4 levels are indistinguishable between CIA-resistant and CIA-arthritic, but such variations markedly distinguish these two statuses from healthy status. LT-A4-H and APB are related in a compartment-dependent manner acting as independent enzymes with differential modulation of their specificity, efficiency and/or catalytic affinity on the aminoacyl and epoxy substrates, or as bifunctional enzymes which activities are inversely related due to the concurrent inhibition of one of these Aminopeptidase Artrite Autoimunidade Enzimas bifuncionais Leucotrieno Modelo animal Aminopeptidase Animal model Arthritis Autoimmunity Bifunctional enzymes Leukotriene
38	Avaliação da participação de mediadores lipídicos nas infecções experimentais induzidas por diferentes isolados de Mycobacterium tuberculosis de humanos / Evaluation of lipid mediators participation in the experimental infections induced by different isolates of Mycobacterium tuberculosis from human. Elyara Maria Soares 13 September 2013 (has links) Os mecanismos que conferem resistência do Mycobacterium tuberculosis (Mtb) à destruição pelo hospedeiro, além da sua capacidade em permanecer e/ou multiplicar-se no interior das células fagocitárias são ainda pouco compreendidos. Nosso grupo de pesquisa tem contribuído para o entendimento do papel dos mediadores lipídicos, que incluem prostaglandinas (PGs) e leucotrienos (LTs) na tuberculose. PGs inibem a resposta imune celular TH1, a produção de citocinas e a fagocitose, e assim facilita a infecção. LTs estão envolvidos no recrutamento de leucócitos, e na modulação da síntese de citocinas, no aumento da fagocitose e dos mecanismos microbicidas, e assim contribui para a eliminação da micobactéria. Neste projeto, avaliamos in vivo e in vitro a produção dos mediadores lipídicos induzidos por cepas de Mtb isolados de pacientes com tuberculose ativa. Demonstramos neste trabalho que macrófagos alveolares infectados com os bacilos da cepa SV009 levam a maior produção de TNF- e nitrito, do que aqueles infectados com a cepa SV068. Em contraste, macrófagos alveolares infectados com os bacilos da cepa SV068 induzem a produção de muito mais LTB4, quando comparado aos bacilos da cepa SV009. Obtivemos maior recuperação de unidades formadoras de colônia (UFC) de macrófagos alveolares tratados com MK886 e infectados com bacilos da cepa SV068; enquanto que mais UFCs foram recuperadas após o tratamento com ácido caféico e infecção com a cepa SV009. Com relação a formação de corpúsculos lipídicos (CLs), observamos um maior número destes quando macrófagos alveolares foram infectados com bacilos da cepa SV068. Ainda, observamos diminuição de CLs quando tratados com MK886 ou ácido caféico. Os bacilos da cepa SV068 foram mais fagocitados, mas os macrófagos não foram muito eficazes na atividade microbicida dos mesmos. Nos experimentos in vivo vimos que camundongos balb/c infectados com a cepa SV068 morrem mais e o tratamento com MK886 parcialmente os protege e a mortalidade não está relacionada com a maior carga bacilar no pulmão ou baço. Houve aumento no recrutamento de neutrófilos induzido pela infecção especialmente após infecção com os bacilos da cepa SV068, sendo que o tratamento com MK886 inibe significativamente o recrutamento quando comparado à infecção com os bacilos da cepa SV009. Células mononucleares também foram recrutadas e permaneceram aumentadas até o final do período observado, sem muitas diferenças significativas quando comparamos a infecção com os isolados SV009 e SV068. A produção de nitrito também encontrou-se elevada em animais infectados com bacilos da cepa SV068. A análise histopatológica dos pulmões dos animais infectados mostrou intensa reação inflamatória com maior comprometimento do parênquima pulmonar dos camundongos infectados bacilos da cepa SV068, com intensa deposição de colágeno e multiplicação bacilar. Encontramos diferenças significativas em relação à producão de citocinas IL-6, IL-10, IL-1, IFN-, TNF- and IL-12 após infecção de 30 e 60 dias com as cepas SV009 e SV068. Também mostramos que há diferenças na produção de LTB4 e PGE2 após 30 e 60 dias de infecção com as cepas SV009 e SV068 em células do camundongos balb/c. Experimentos com animais 129 e 5LO-/- infectados com as duas cepas também foram realizados, e vimos que os animais 5LO-/- são mais suscetíveis à infecção especialmente quando infectados com a cepa SV068. Sugerimos que as cepas são diferentes, mas dependentes de um conjunto de fatores, e nossos dados sugerem que dentre estes mecanismos a produção de TNF- e também de mediadores lipídicos (LTB4 e PGE2) estão envolvidos. / The mechanisms that confer resistance to Mycobacterium tuberculosis (Mtb) for destruction by the host, in addition to its ability to retain and/or multiply within phagocytic cells are still poorly understood. Our research group has contributed to the understanding of the role of lipid mediators, including prostaglandins (PGs) and leukotrienes (LTs) in tuberculosis. PGs inhibit Th1 cell immune response, cytokine production and phagocytosis, thus facilitating the infection. LTs are involved in the leukocytes recruitment, and modulation of cytokine synthesis, phagocytosis and microbicidal mechanisms enhancement, and contribute to the elimination of the mycobacteria. In this project, we evaluated in vivo and in vitro the lipid mediators production induced by Mtb strains isolated from patients with active tuberculosis. We demonstrated in this study that alveolar macrophages infected with bacilli from SV009 strain lead to an increase of TNF- production and nitrite, than those infected with the strain SV068. In contrast, alveolar macrophages infected with bacilli from SV068 strain induced more LTB4 production when compared to SV009 infection. We obtained higher recovery colony forming units (CFU) of alveolar macrophages treated with MK886 and infected with bacilli from SV068 strain; while more CFUs were recovered after treatment with caffeic acid and infection with bacilli from SV009 strain. Regarding the lipid bodies (LBs) formation, we observed a greater number of these structures, when alveolar macrophages were infected with bacilli from SV068 strain. Still, we observed a decrease of LBs when the macrophages were treated with MK886 and caffeic acid. Bacilli from SV068 strain were more phagocytosed, but macrophages were not very effective in the microbicidal activity. In the in vivo experiments we found that mice infected with SV068 strain die more than the other and MK886 treatment partially protects the mice, besides, the mortality is not related to the higher bacterial load in the lung or spleen. There was an increase in neutrophil recruitment induced after infection, especially after infection with SV068 strain, and treatment with MK886 significantly inhibits recruitment when compared to infection with SV009 strain. Mononuclear cells were also recruited and remained increased until the end of the observed period, without many significant differences when comparing infection with SV009 and SV068 strains. The nitrite production was also found greater in animals infected with bacilli from SV068 strain. Histopathological analysis of the infected mice lungs showed an intense inflammatory reaction with greater impairment of the mice lungs when infected with bacilli from SV068 strain with an intense collagen deposition and multiplication of bacilli. We suggest that the SV068 strain is more virulent and participates of the immune response by lipid mediators dependent mechanisms. Leucotrieno B4 Mycobacterium tuberculosis Prostaglandina E2 Leukotriene B4 Mycobacterium tuberculosis Prostaglandin E2
39	The Role of Cysteinyl Leukotriene Receptor 2 in Thrombocyte Aggregation Reyna, Julianna 12 1900 (has links) Cysteinyl leukotriene receptor 2, a G-protein coupled receptor known to be expressed and functional on human platelets. However, it seems that upon ligand activation the cysteinyl leukotriene receptor 2 activates a variety of signaling pathways in multiple cell types among different species. Previously, a former laboratory member Vrinda Kulkarni found cysteinyl leukotriene receptor 2 to be expressed on the surface of adult zebrafish thrombocytes. In this work I studied the characteristics of aggregation in adult zebrafish thrombocytes with the knockdown of cysteinyl leukotriene receptor 2. I used a newly developed knockdown method to study the function of cysteinyl leukotriene receptor 2. Knockdown of the cysteinyl leukotriene was confirmed using RT-PCR results showed p=.001, reduced sell surface level of expression of the cysteinyl leukotriene receptor 2 results showed that p=.002. I found that the knockdown of cysteinyl leukotriene receptor 2 results in prothrombotic thrombocytes by using flow cytometry p=.0001. Cysteinyl leukotriene receptor 2 thrombocyte aggregation adult zebrafish G proteins -- Receptors. Leukotrienes. Blood platelets -- Aggregation.
40	Investigation of the neutrophil-directed anti-inflammatory properties of the cysteinyl leukotriene receptor antagonist, montelukast Lodder, Cornelia Magdalena 26 April 2012 (has links) Montelukast (ML) is primarily an antagonist of type 1 cysteinyl leukotriene receptors (CysLT1R), an activity which underpins its therapeutic efficacy in bronchial asthma. However, ML has also been reported to be useful in the treatment of acute and chronic inflammatory disorders of both infective and non-infective origin in which CysLTs are unlikely to be the predominant mediators of harmful inflammatory responses. These include conditions such as chronic obstructive pulmonary disease and cystic fibrosis in which the neutrophil is believed to be the primary offender, suggesting that ML may possess neutrophil-targeted, CysLT1R-independent mechanisms of anti-inflammatory activity. Accordingly, the laboratory research presented in this thesis was designed with the primary objectives of characterizing possible CysLT1R-dependent and – independent neutrophil-targeted anti-inflammatory activities of ML in vitro, and consisted of 3 phases. These were investigation of: i) the effects of the CysLTs, LTC4 and LTD4 (in the absence and presence of ML) on mobilization of intracellular Ca2+ stores, generation of reactive oxygen species (ROS) and release of primary and secondary granule proteinases; ii) the effects of ML on a series of pro-inflammatory activities of neutrophils following activation of the cells with the chemoattractants FMLP and platelet-activating factor (PAF); and iii) the interactive, anti-inflammatory effects on neutrophils of ML in combination with the long-acting beta-2 agonist, formoterol. In addition to the aforementioned activities, measurement of the production and expression of CR3, as well as generation of inositol triphosphate (IP3), cyclic AMP, and activities of the enzymes cAMP- and cGMP-phosphodiesterases (PDEs) in isolated neutrophil cytosol and membrane fractions, were also included. The following assays were used: i) chemiluminescence procedures for the detection of ROS; ii) a colourimetric procedure for the detection of elastase; iii) ELISA procedures for the detection of the matrix metalloproteinases (MMPs) 8- and -9, LTB4, and cyclic AMP; iv) fura-2-based spectrofluorimetry and a radiometric procedure for monitoring cytosolic Ca2+ fluxes; v) flow cytometry for CR3; and vi) radioassays for IP3 and activity of cAMP- and cGMP-PDEs. Exposure of neutrophils to LTD4, but not LTC4, activated a very modest and transient increase in cytosolic Ca2+, but failed to initiate the generation of ROS or release of elastase or MMP-8. However, brief pre-treatment with either LTC4 or LTD4 sensitized the cells for increased production of ROS and release of granule proteinases following activation with FMLP, which was partially attenuated by inclusion of ML. In the second part of the study, pre-treatment of neutrophils with ML, at therapeutically relevant concentrations, resulted in dose-related inhibition of the FMLP- or PAF-activated generation of ROS and LTB4, as well as the release of elastase, with the former being unaffected by an inhibitor of 5-lipoxygenase (MK886), compatible with a CysLT1R-independent mechanism of anti-inflammatory activity. From a mechanistic perspective, these interactions of ML with neutrophils were associated with accelerated clearance of Ca2+ from the cytosol of the cells which could not be attributed to inhibition of production of IP3, but was, however, associated with increased levels of cAMP, apparently as a consequence of non- specific inhibition of cyclic nucleotide phosphodiesterases. In the third part of the study, combining ML with formoterol caused (in most cases) additive inhibitory effects on the generation of ROS and LTB4, release of granule proteinases, as well as expression of CR3, which again were associated with elevations in cAMP and interference with Ca2+ mobilization. In conclusion, ML appears to attenuate neutrophil activation by CysLT1R-dependent and –independent mechanisms. In the case of the former by interfering with the modest sensitizing (priming) interactions of LTC4 and LTD4 with neutrophils, and in the latter by inhibition of PDEs, leading a to sustained elevation in cAMP, resulting in rapid clearance of Ca2+ from the cytosol and decreased uptake of the cation from the extracellular milieu. / Thesis (PhD)--University of Pretoria, 2011. / Immunology / Unrestricted Bronchial asthma Montelukast UCTD

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