Influência do sistema renina angiotensina na modulação do estado redox, no balanço autonômico e na hipertrofia cardíaca induzida pelo hipertireoidismo experimental

Baraldi, Dhãniel Dias

January 2012

O hipertireoidismo é uma patologia epidemiologicamente importante, que afeta o sistema cardiovascular de forma proeminente. O estado hipertireoideo pode afetar o metabolismo basal, consumo de O2 celular, sistema renina angiotensina, assim como, estimular a produção de espécies ativas de oxigênio. Estas alterações produzem consequências morfológicas, funcionais, bioquímicas e moleculares no tecido cardíaco. A hipertrofia cardíaca, decorrente do hipertireoidismo, instala-se devido a uma série de eventos que sinalizam à proliferação e sobrevivência celular, envolvendo as espécies ativas de oxigênio, a ativação do sistema renina angiotensina cardíaco e o sistema nervoso autonômico. Neste estudo, bloqueamos o receptor AT1 da angiotensina II para avaliarmos a influência do sistema renina angiotensina cardíaco sobre o desenvolvimento da hipertrofia cardíaca, a participação do balanço autonômico sobre o coração e o papel das espécies ativas de oxigênio neste processo, em modelo experimental de hipertireoidismo. Para isto, foram utilizados ratos Wistar machos, pesando cerca de 220g, divididos em 4 grupos experimentais: Controle (C), Losartan (L) (10 mg/Kg de peso corporal/dia, 28 dias, sonda intragástrica) , T4 (12mg/L água de beber, 28 dias), e T4+L. Foram avaliados a massa cardíaca, análise espectral do balanço simpato-vagal, a expressão protéica do receptor AT1 da Angiotensina II e da gp91phox, peróxido de hidrogênio (H2O2), Nrf-2 e Heme-oxigenase-1 (HO-1) no tecido cardíaco. A hipertrofia cardíaca e o desequilíbrio autonômico induzidos pelo hipertireoidismo foram atenuados no grupo T4+L. Os níveis de H2O2, Nrf-2, gp91phox e HO-1 foram elevados no grupo T4, e significativamente reduzidos no grupo T4+L, quando comparados ao grupo Controle. A expressão protéica do receptor AT1 esteve elevada nos dois grupos hipertireoideos. Os resultados obtidos sugerem que o bloqueio do receptor AT1 promove importante impacto sobre o balanço simpato-vagal e a hipertrofia cardíaca, no hipertireoidismo, sendo as espécies ativas de oxigênio e o sistema Nrf-2/HO-1 possíveis mediadores destas alterações. / Hyperthyroidism is an epidemiologic relevant pathology, which substantially affects the cardiovascular system. The hyperthyroid state may affect basal metabolism, O2 cell consumption, renin-angiotensin system, and increase reactive oxygen species production. Those alterations produce morphological, biochemical, functional and molecular consequences in cardiac tissue. Hyperthyroidism induced cardiac hypertrophy develops due to a set of events, which signals cell survival and proliferation, including reactive oxygen species, cardiac rennin-angiotensin system, and autonomic nervous system. In the present study, the role of cardiac renin-angiotensin system on development of hyperthyroidism induced cardiac hypertrophy, and the involvement of autonomic nervous system and reactive oxygen species, were assessed trough blockade of angiotensin II receptor AT1. For that, were used male Wistar rats, weighting about 220g, divided in 4 experimental groups,: Control (C), Losartan (L) (10mg/Kg body weight/day, 28 days, intragastric probe), T4 (12mg/L L-thyroxin in drinking water, 28 days), and T4+L. Cardiac mass, spectral analysis (autonomic balance), hydrogen peroxide (H2O2), and myocardial protein expression of angiotensin II receptor (AT1), NADPH oxidase, Nrf-2, and heme-oxygenase-1 (HO-1), were quantified. Cardiac hypertrophy and autonomic umbalance induced by thyroid hormones were attenuated in the T4+losartan group. The H2O2, as well as Nrf-2, gp91phox, AT1 and HO-1 immunocontent were elevated in T4 group. All these effects were attenuated by losartan, except AT1 levels. The overall results suggest that blockade of AT1 receptor lead to relevant impact on autonomic balance and cardiac hypertrophy, being ROS and Nrf-2/ HO-1 system possible mediators in this alterations in experimental hyperthyroidism.

Hipertireoidismo

Hipertrofia cardíaca

Hormônios tireóideos

Sistema renina-angiotensina

Losartan

Espécies reativas de oxigênio

Modelos animais de doenças

Losartan

Renin-angiotensin system

Heme-oxygenase

Thyroid hormones

Cardiac hypertrophy

Spectral analysis

Reactive oxygen species

Influência do sistema renina angiotensina na modulação do estado redox, no balanço autonômico e na hipertrofia cardíaca induzida pelo hipertireoidismo experimental

Baraldi, Dhãniel Dias

January 2012

O hipertireoidismo é uma patologia epidemiologicamente importante, que afeta o sistema cardiovascular de forma proeminente. O estado hipertireoideo pode afetar o metabolismo basal, consumo de O2 celular, sistema renina angiotensina, assim como, estimular a produção de espécies ativas de oxigênio. Estas alterações produzem consequências morfológicas, funcionais, bioquímicas e moleculares no tecido cardíaco. A hipertrofia cardíaca, decorrente do hipertireoidismo, instala-se devido a uma série de eventos que sinalizam à proliferação e sobrevivência celular, envolvendo as espécies ativas de oxigênio, a ativação do sistema renina angiotensina cardíaco e o sistema nervoso autonômico. Neste estudo, bloqueamos o receptor AT1 da angiotensina II para avaliarmos a influência do sistema renina angiotensina cardíaco sobre o desenvolvimento da hipertrofia cardíaca, a participação do balanço autonômico sobre o coração e o papel das espécies ativas de oxigênio neste processo, em modelo experimental de hipertireoidismo. Para isto, foram utilizados ratos Wistar machos, pesando cerca de 220g, divididos em 4 grupos experimentais: Controle (C), Losartan (L) (10 mg/Kg de peso corporal/dia, 28 dias, sonda intragástrica) , T4 (12mg/L água de beber, 28 dias), e T4+L. Foram avaliados a massa cardíaca, análise espectral do balanço simpato-vagal, a expressão protéica do receptor AT1 da Angiotensina II e da gp91phox, peróxido de hidrogênio (H2O2), Nrf-2 e Heme-oxigenase-1 (HO-1) no tecido cardíaco. A hipertrofia cardíaca e o desequilíbrio autonômico induzidos pelo hipertireoidismo foram atenuados no grupo T4+L. Os níveis de H2O2, Nrf-2, gp91phox e HO-1 foram elevados no grupo T4, e significativamente reduzidos no grupo T4+L, quando comparados ao grupo Controle. A expressão protéica do receptor AT1 esteve elevada nos dois grupos hipertireoideos. Os resultados obtidos sugerem que o bloqueio do receptor AT1 promove importante impacto sobre o balanço simpato-vagal e a hipertrofia cardíaca, no hipertireoidismo, sendo as espécies ativas de oxigênio e o sistema Nrf-2/HO-1 possíveis mediadores destas alterações. / Hyperthyroidism is an epidemiologic relevant pathology, which substantially affects the cardiovascular system. The hyperthyroid state may affect basal metabolism, O2 cell consumption, renin-angiotensin system, and increase reactive oxygen species production. Those alterations produce morphological, biochemical, functional and molecular consequences in cardiac tissue. Hyperthyroidism induced cardiac hypertrophy develops due to a set of events, which signals cell survival and proliferation, including reactive oxygen species, cardiac rennin-angiotensin system, and autonomic nervous system. In the present study, the role of cardiac renin-angiotensin system on development of hyperthyroidism induced cardiac hypertrophy, and the involvement of autonomic nervous system and reactive oxygen species, were assessed trough blockade of angiotensin II receptor AT1. For that, were used male Wistar rats, weighting about 220g, divided in 4 experimental groups,: Control (C), Losartan (L) (10mg/Kg body weight/day, 28 days, intragastric probe), T4 (12mg/L L-thyroxin in drinking water, 28 days), and T4+L. Cardiac mass, spectral analysis (autonomic balance), hydrogen peroxide (H2O2), and myocardial protein expression of angiotensin II receptor (AT1), NADPH oxidase, Nrf-2, and heme-oxygenase-1 (HO-1), were quantified. Cardiac hypertrophy and autonomic umbalance induced by thyroid hormones were attenuated in the T4+losartan group. The H2O2, as well as Nrf-2, gp91phox, AT1 and HO-1 immunocontent were elevated in T4 group. All these effects were attenuated by losartan, except AT1 levels. The overall results suggest that blockade of AT1 receptor lead to relevant impact on autonomic balance and cardiac hypertrophy, being ROS and Nrf-2/ HO-1 system possible mediators in this alterations in experimental hyperthyroidism.

Hipertireoidismo

Hipertrofia cardíaca

Hormônios tireóideos

Sistema renina-angiotensina

Losartan

Espécies reativas de oxigênio

Modelos animais de doenças

Losartan

Renin-angiotensin system

Heme-oxygenase

Thyroid hormones

Cardiac hypertrophy

Spectral analysis

Reactive oxygen species

Régulation de l’hème oxygénase-1 dans les macrophages au cours des pathologies pulmonaires liées à l’exposition de la fumée de cigarette / Regulation of heme oxygenase-1 in macrophages in smoking related pulmonary disease

Goven, Delphine

10 July 2009

L’intoxication tabagique, source d’oxydants, est un facteur de risque important de développement de l’emphysème pulmonaire et du pneumothorax spontané primitif. Les macrophages alvéolaires contribuent pour une large part à l’inflammation pulmonaire au cours de ces pathologies en produisant des métalloprotéases et des espèces réactives de l’oxygène à l’origine du déséquilibre des balances protéase/anti-protéase et oxydant/antioxydant. L'hème oxygénase-1 (HO-1), exprimée principalement par les macrophages, est une enzyme clé des défenses anti-oxydantes pulmonaires. Nous avons initialement étudié l’expression et la localisation cellulaire de l’HO-1 et de ses régulateurs potentiels (Nrf2, Keap1, Bach1 et HIF-1a) dans les macrophages alvéolaires au cours de l’emphysème pulmonaire post-tabagique et du pneumothorax spontané primitif. Les voies de régulation de l’expression de ces protéines ont été analysées in vitro sur des macrophages dérivés de la lignée THP-1 exposés ou non au condensat de fumée de cigarette et à l’hypoxieréoxygénation visant à mimer une partie des effets de l’atélectasie-réexpansion observée lors de la prise en charge thérapeutique des pneumothorax récidivants. Les travaux présentés dans cette thèse nous ont permis de mettre en évidence une altération de l’expression de la voie Nrf2/Keap1-Bach1 associée à une diminution de l’expression des enzymes anti-oxydantes, dont l’HO-1, dans les macrophages alvéolaires au cours de l’emphysème pulmonaire sévère post-tabagique, malgré un stress oxydant important. In vitro, ces altérations pourraient être liées à une activation spécifique des MAPKinases ERK1/2 et JNK par le condensat de fumée de cigarette. Nous avons également montré que la stimulation du système de l’HO-1 était probablement orchestrée par la voie du facteur HIF-1a, et non par celle de Nrf2, dans les macrophages alvéolaires au cours du pneumothorax spontané primitif récidivant du sujet fumeur. Ces résultats pourraient contribuer à une meilleure connaissance de la physiopathologie de l’emphysème pulmonaire et permettre d’envisager de nouvelles approches thérapeutiques basées sur la préservation et/ou la restauration de l’équilibre Nrf2/Keap1-Bach1. Nos travaux suggèrent également que la physiopathologie du pneumothorax spontané primitif est différente chez les patients fumeurs et non fumeurs. Le pneumothorax du sujet fumeur est associé à un stress oxydant pulmonaire et à une induction de l’HO-1 probablement orchestrée par HIF-1a. Ces résultats, confirmés in vitro, mettent en évidence une interaction potentielle entre le stress oxydant et l’hypoxie-réoxygénation / Chronic cigarette smoking, a source of oxidants, is an important risk factor for lung emphysema and primary spontaneous pneumothorax development. Alveolar macrophages are mainly involved in lung inflammation observed in these pathologies through the production of metalloproteases and reactive oxygen species resulting to protease/anti-protease and oxidant/anti-oxidant imbalances. Heme oxygenase-1 (HO-1), mainly expressed in macrophages, is a key enzyme in pulmonary anti-oxidant defences. Therefore, the first aim of our studies was to investigate the expression and cellular localisation of HO-1 and its potential regulators (Nrf2, Keap1, Bach1 and HIF-1a) in alveolar macrophages from smoking related lung emphysema and primary spontaneous pneumothorax. Regulation pathways involved in expression of these proteins were assessed in vitro in macrophage cell line THP-1 exposed or not to cigarette smoke condensate and with or without hypoxia-reoxygenation mimicking parts of events induced by atelectasia-reexpansion during recurrent pneumothorax constitution and treatment. In these studies, we showed an altered expression of Nrf2/Keap1- Bach1 pathway associated with a reduced expression of anti-oxidants enzymes, like HO-1, in alveolar macrophages from smoking related lung emphysema patients, despite an important oxidative stress. These alterations might be related to cigarette smoke condensate activated ERK1/2 and JNK MAPKinases as observed in THP-1 cells. Furthermore, we showed that HO- 1 system induction was mediated by HIF-1a instead of Nrf2 pathway in alveolar macrophages from smoking related recurrent primary spontaneous pneumothorax. These findings may contribute to a better knowledge of the pathophysiology of lung emphysema and could provide new therapeutic approaches based on preservation and/or restoration of Nrf2/Keap1-Bach1 equilibrium. Our results also suggest that the pathophysiology of primary spontaneous pneumothorax could be different in smokers and non smokers. Spontaneous pneumothorax in smokers is associated with lung oxidative stress and the orchestrated induction of HO-1 probably via HIF-1a. These results provide a new link between oxidative stress and hypoxia/reoxygenation

Emphysème pulmonaire

Stress oxydant

Hème oxygénase-1

Macrophages

Fumée de cigarette

Nrf2

HIF-1a

MAPK

Hypoxie-réoxygénation

Lung emphysema

Oxidative stress

Heme oxygenase-1

Macrophages

Cigarette smoke

Nrf2

HIF-1a

MAPK

Hypoxiareoxygenation

The role of chaperone proteins in neurodegenerative diseases

Zhang, Xuekai

January 2013

Many neurodegenerative diseases are characterized by the accumulation of misfolded proteins that often share common morphological and biochemical features, and can similarly co-localize with several other proteins, including various chaperone proteins. Chaperone proteins, like heat shock protein 27 (HSP27), heme oxygenase 1 (HO-1) and clusterin, have been implicated as potent modulators of misfolded proteins, thus may play important roles in the pathogenesis of neurodegenerative diseases. The present study aims to investigate their roles in the pathogenesis of Frontotemporal lobar degeneration (FTLD), Alzheimer's disease (AD), Parkinson's disease (PD), and Motor neuron disease (MND) by determining their distribution and amount via immunohistochemical staining and western blotting in diseased and control subjects.There were distinct patterns of HSP27 and clusterin immunostaining in different brain regions. For HSP27, patients with AD and FTLD were in general more severely affected than were patients with MND and control subjects. For clusterin, patients with AD and FTLD were more severely affected than control subjects where neurons and glial cells were concerned, while patients with AD and control subjects were more severely affected than those with FTLD where diffuse and cored plaques were concerned. However, there were no obvious differences in the pattern of HO-1 immunostaining in various brain regions in patients with AD or FTLD relative to control subjects. Moreover, there was no association between HSP27, HO-1 and clusterin with disease or histological type, and the ‘classic’ neuropathological changes in FTLD, AD and MND were not immunoreactive to any of these proteins. There were significant correlations between the degrees of HO-1 and clusterin immunostaining in many brain areas for both AD and FTLD cases, and for all cases overall, but none between HSP27 and clusterin or HSP27 and HO-1. Present results suggest an involvement with ongoing cellular stress, misfolded or unfolded protein accumulation or the deficits/failure of other relevant protein quality control systems, in the pathogenesis of these neurodegenerative diseases. Present work may therefore have implications for the further development of ideas concerning the cause or treatment of neurodegenerative diseases where there is aberrant accumulation of misfolded, aggregated protein, and perhaps for conformational diseases in general. However, there are still many issues remain to be elucidated. Further research aimed at understanding the function and mechanisms of the chaperone system, and other protein quality control mechanisms, in the pathogenesis of neurodegenerative diseases is still needed.

616.8

Pharmacotherapies and Aortic Heme Oxygenase-1 Expression in Patients with Abdominal Aortic Aneurysm

Hofmann, Anja, Hamann, Bianca, Klimova, Anna, Müglich, Margarete, Wolk, Steffen, Busch, Albert, Frank, Frieda, Sabarstinski, Pamela, Kapalla, Marvin, Nees, Josef Albin, Brunssen, Coy, Poitz, David M., Morawietz, Henning, Reeps, Christian

06 June 2024

Background: Treatment of cardiovascular risk factors slows the progression of small abdominal aortic aneurysms (AAA). Heme oxygenase-1 (HO-1) is a stress- and hemin-induced enzyme providing cytoprotection against oxidative stress when overexpressed. However, nothing is known about the effects of cardiometabolic standard therapies on HO-1 expression in aortic walls in patients with end-stage AAA. Methods: The effects of statins, angiotensin-converting enzyme (ACE) inhibitors, angiotensin II receptor blockers (ARBs), calcium channel blockers (CCBs), betablockers, diuretics, acetylsalicylic acid (ASA), and therapeutic anticoagulation on HO-1 mRNA and protein expressions were analyzed in AAA patients using multivariate logistic regression analysis and comparison of monotherapy. Results: Analysis of monotherapy revealed that HO-1 mRNA and protein expressions were higher in patients on diuretics and lower in patients on statin therapy. Tests on combinations of antihypertensive medications demonstrated that ACE inhibitors and diuretics, ARBs and diuretics, and beta-blockers and diuretics were associated with increase in HO-1 mRNA expression. ASA and therapeutic anticoagulation were not linked to HO-1 expression. Conclusion: Diuretics showed the strongest association with HO-1 expression, persisting even in combination with other antihypertensive medications. Hence, changes in aortic HO-1 expression in response to different medical therapies and their effects on vessel wall degeneration should be analyzed in future studies.

info:eu-repo/classification/ddc/540

ddc:540

info:eu-repo/classification/ddc/610

ddc:610

HO-1 induction by Co-PPIX suppresses experimental skin inflammation, T cell immunity and dendritic cell maturation and function

Listopad, Joanna Jadwiga

19 April 2007

Die Hämoxygenase 1 (HO-1) ist ein Stressprotein mit antientzündlichen, immunsupprimierenden und zytoprotektiven Eigenschaften, welche in vielen Tiermodellen nachgewiesen wurden. Die zugrunde liegenden Mechanismen sind wenig bekannt. Diese Arbeit demonstriert erstmalig, dass die physiologische Induktion von HO-1 wichtig für die Limitierung von T-Zell-abhängigen Hautentzündungen ist. So führt der HO-1-Inhibitor, Zinn-Protoporphyrin IX (Sn-PPIX), zu einer verstärkten Hautentzündung im Mausmodell. Die pharmakologische Induktion von HO-1 durch Kobalt-Protoporphyrin IX, Co-PPIX, hemmt dagegen die Entzündung in DNFB- bzw. TMA-induzierten murinen Kontaktallergiemodellen sowohl bei Verabreichung von Co-PPIX während der Sensibilisierung als auch vor der Auslösung. Bemerkenswerterweise hemmt eine Co-PPIX-Behandlung die Antigen-induzierte T-Zellproliferation ex vivo in Milzzellen von behandelten Mäusen und in vitro in humanen mononukleären Zellen des peripheren Blutes. Da eine HO-1-Induktion durch Co-PPIX nur in Monozyten und in aus Monozyten abgeleiteten myloischen Dendritischen Zellen (MDDC), nicht aber in T-Zellen, beobachtet wurde, fokussierten alle weiteren Untersuchungen auf Antigen-präsentierende Zellen. HO-1-Induktion durch Co-PPIX reduziert die Expression von MHC-Klasse II und akzessorischen Molekülen und steigert die Phagozytose und den oxidativen Burst von Monozyten. Die immunphänotypische Differenzierung und Maturierung von MDDC wird gehemmt. Funktionsteste zeigen eine Reduktion der Expression und Sekretion von proinflammatorischen und immunstimulatorischen Zytokinen, während die Sekretion des antientzündlichen Zytokins IL-10 gesteigert ist. Die Fähigkeit der MDDC zur Antigenpräsentation gegenüber T-Helferzellen ist für Allo- und Recallantigene stark herabgesetzt. Mittels adenoviraler HO-1-Transduktion von MDDC konnte die Spezifität der Effekte bestätigt werden. Diese Daten zeigen, dass eine verstärkte HO-1-Aktivität die Dendritischen Zellen zu einem unreifen und immunkompromittierten Phänotyp verändert und weisen darauf hin, dass die HO-1-Induktion einen wichtigen Ansatz für die Hemmung der zellulären Immunität und für die Behandlung von T-Zell-abhängigen Hautentzündungen darstellt. / Heme oxygenase 1 (HO-1) is an antiinflammatory stress protein. Its immunosuppressive and cytoprotective activities have been demonstrated in several animal models. The underlying mechanisms, however, are poorly understood. This study demonstrates for the first time that the physiological induction of HO-1 is important for the limitation and resolution of T cell-dependent skin inflammation. So, the HO-1 inhibitor, tin protoporphyrin IX (Sn-PPIX), augments cutaneous inflammation in mouse model. Moreover, pharmacologic HO-1 induction by the potent HO-1 inducer, cobaltic protoporphyrin IX (Co-PPIX), inhibits inflammation when applied around sensitization or before challenge in murine DNFB- and TMA-induced contact hypersensitivity models. Remarkably, Co-PPIX treatment inhibits antigen-driven T cell proliferation both ex vivo in murine splenocytes and in vitro in human peripheral blood mononuclear cells. Since induction of HO-1 mRNA and protein was found in monocytes and monocyte-derived myeloid dendritic cells (MDDC) but not T cells, further investigations focused on antigen-presenting cells. HO-1 induction by Co-PPIX depresses monocytic MHC class II and accessory molecule expression whereas phagocytosis and respiratory burst activities are augmented. Moreover, HO-1 induction inhibits the immunophenotypic differentiation and maturation of MDDC. Functional analysis revealed a decreased proinflammatory cytokine production whereas secretion of the antiinflammatory cytokine IL-10 is increased. Remarkably, the antigen-presenting capacity of MDDC for T-helper cells is diminished both for allo- and for recall-antigens. Adenoviral HO-1 transduction of MDDC confirmed that the effects are mediated by HO-1. These data indicate that an enhanced HO-1 activity switches myeloid DCs to an immature and functionally compromised phenotype and suggest that HO-1 induction represents an important approach for depressing T cell immunity and for the treatment of T cell-dependent skin inflammation.

Hämoxygenase 1

Dendritische Zellen

Kobalt-Protoporphyrin IX

Hautentzündung

Hemmung

Heme oxygenase 1

dendritic cells

Cobaltic protoporphyrin IX

cutaneous inflammation

suppression

570 Biologie

32 Biologie

YF 2600

WF 9895

ddc:570

Induktion und Regulation der Hämoxygenase-1 in humanen Hepatozyten

Müller, Eda

04 October 2002

Der nach Leberoperation und -transplantation auftretende Ischämie-/ Reperfusionsschaden (I/R) und die konsekutive Inflammation des Lebergewebes stellen ein bedeutendes klinisches Problem dar. In der vorliegenden Arbeit wurden Einflüsse der warmen und kalten Ischämie (100% N2 bei 37°C bzw. 4°C) sowie der Exposition inflammatorischer Zytokine und Endotoxin (IL-1beta, 10 U/ml; IFN-gamma, 100 U/ml; TNF-alpha, 500 U/ml; LPS, 5 µg/ml) auf die Expression der Hämoxygenase-1 (HO- 1) mRNA und seines Proteins, einem Vertreter der Hitze-Schock-Proteine mit potentiell antioxidativer Wirkung, in humanen Hepatozytenprimärkulturen untersucht. Warme und kalte Ischämie stimulierten die HO-1 mRNA Expression in humanen Hepatozyten nach 0,5 bis 1h. Das HO-1 Protein wurde über 0,5-6h maximal exprimiert. Der Zellschaden, gemessen an der AST und LDH Freisetzung unter ischämischen Bedingungen wurde insbesondere nach 24 h beobachtet. Nach Zytokinexposition wurde die höchste Expressionsrate der mRNA durch IFN-gamma hervorgerufen, gefolgt von TNF-alpha, LPS und IL-1beta. Jedes einzelne Zytokin stimulierte die HO-1 mRNA Expression nach 0,5 h, erreichte ein Maximum nach 3 h und fiel nach 6 h ab. Nach Stimulation mit einem Zytokinmix (CM; IFN-gamma, TNF-alpha, IL-1beta, LPS) trat ein Maximum der HO-1 mRNA Expression erst nach 6 h ein, wobei ein signifikanter Zellschaden nach 12 h beobachtet wurde. Die HO-1 mRNA und Proteinexpression war nach Exposition von 6 h des Sauerstoffperoxides (H2O2, 200- 1000 µM) erhöht. Die HO-1 mRNA und Proteinexpression war nach S- nitrosoacetylpenicillamin (0.5 mM) Exposition, einem NO Donator, für 3-12 h verstärkt. Nach Cobalt-protoporphyrin (CoPP, 1µM) Exposition, einem potenten HO-1 Induktor, wurde eine erhöhte mRNA- und Proteinexpression beobachtet. Dass CoPP die HO-1 mRNA- und Proteinneusynthese induziert, konnte durch die selektive Blockade mit Actinomycin D und Cycloheximide bewiesen werden. Die Neusynthese konnte ebenfalls unter warmer und kalter Ischämie gezeigt werden. Hemin (10 µM), ein weiterer Induktor der HO-1, induzierte die HO-1 mRNA nach 3 h und das Protein nach 6 h. Die HO-1 Enzymaktivität wurde mittels Bilirubinbildung und Messung des Fe2+ Gehalts der Zellen bestimmt. Bei der Bilirubinbildung wurde die höchste Aktivität nach warmer Ischämie gemessen, gefolgt von kalter Ischämie, CM und der Kontrollgruppe. Die intrazelluläre Fe2+ Messung ergab ebenfalls die höchste Enzymaktivität nach warmer Ischämie. Die Vorbehandlung humaner Hepatozyten mit CoPP (1-50 µM) für 8 h, schützte die Zellen teilweise vor einer warmen und kalten Ischämie. Zusammenfassend zeigt diese Arbeit, dass die pharmakologische Induktion der HO-1 somit bei großen allgemeinchirurgischen Eingriffen, wie der Leberteilresektion oder der Transplantation, einen protektiven Effekt entfalten könnte. / Hepatic injury induced by ischemia/ reperfusion (I/R) and inflammation following surgeries or transplantations creates important clinical problems. In this study, the effect of inflammatory conditions such as cytokine/ endotoxin exposure (IL-1beta, IFN-gamma, TNF-alpha, LPS), warm and cold ischemia on HO-1 mRNA and protein, a member of heat shock proteins, was investigated. It was observed that IFN-gamma caused the highest HO-1 mRNA expression, followed by TNF-alpha, LPS and IL- 1beta. Each stimuli increased HO-1 mRNA expression after 0.5 h, peaked at 3 h and decreased after 6 h. Highest HO-1 protein expression was observed after 0.5 to 1 h of stimulation with IFN-gamma, which was followed by LPS, TNF-alpha and IL-1beta. The peak of HO-1 expression using all four stimuli (CM) was after 6 h. CM caused a significant increase in LDH and AST after 12 h. Warm and cold ischemia stimulated HO-1 mRNA expression in human hepatocytes at 0.5-1 h. HO-1 protein expression had its maximum between 0.5-6 h. Cellular damage measured as the release of LDH and AST was significant after 24 h. Mimicking oxydative stress, hepatocytes were exposed to 200-1000 µM H2O2 for 6 h which also showed an increased HO-1 mRNA and protein expression. HO-1 mRNA and protein expression revealed an increase after SNAP exposure at 3-12 h. Results with CoPP (10 µM), a potent inducer of HO- 1, displayed an increase in HO-1 mRNA and protein expression. It was proved, that CoPP induced new synthesis of mRNA and protein by its blocking agents such as actinomycin D and cycloheximide, respectively. Hemin (10 µM), another inducer of HO-1, triggered HO-1 mRNA expression after 3 h and protein expression after 6 h. The HO-1 enzyme activity was measured by bilirubin production after exposure to CM, as well as warm and cold ischemia. The highest enzyme activity was found after warm ischemia, followed by cold ischemia, CM and then by the control group. Fe2+ content of the cells, used as another method to judge HO-1 activity, confirmed our findings. Pre-treatment of human hepatocytes with different concentrations of CoPP (1-50 µM) protect cells against warm or cold ischemia. Therefore, we conclude that pharmacological induction of HO-1 may have therapeutic potential under inflammatory conditions such as seen during liver resection or liver transplantation.

Lebertransplantation

Ischämie

Hämoxygenase 1

Inflammation

humane Hepatozyten

Leberresektion

liver transplantation

ischemia

Heme oxygenase 1

inflammation

human hepatocytes

liver resection

610 Medizin und Gesundheit

33 Medizin

XG 7650

ddc:610

Stress biomarkers in a rat model of decompression sickness /

Caviness, James A.

January 2005

Thesis (M.S.)--Uniformed Services University of the Health Sciences, 2005. / Typescript (photocopy).

Some aspects of molecular mechanisms of xenobiotics' hepatotoxicity and hepatoprotection : Modulatory roles of natural polyphenols

Lekic, Nataša

January 2013

Background & Aims: Oxidative stress and apoptosis are proposed mechanisms of cellular injury in studies of xenobiotic hepatotoxicity. The aim of this work is to find early signal markers of drug-induced injury of the liver by focusing on select antioxidant/oxidant and apoptotic genes. As well, to address the relationship between conventional liver dysfunction markers and the measured mRNA and protein expressions in the D-galactosamine/lipopolysaccharide and tert-butylhydroperoxide hepatotoxicity models. Furthermore, potential hepatoprotective capabilities of antioxidant polyphenols quercetin and curcumin were evaluated in relation to its modulation of the oxidative stress and apoptotic parameters in the given xenobiotic hepatotoxicity models. Methods: Biochemical markers testing the hepatic function included aminotransferases (ALT, AST) and bilirubin. Measurements of TBARS and conjugated dienes were used to assess lipoperoxidation. Plasma levels of catalase and reduced glutathione were used as indicators of the oxidative status of the cell. Real time PCR was used to analyse the mRNA expressions of the inducible nitric oxide synthase (NOS-2), heme oxygenase-1 (HO-1), superoxide dismutase (SOD-1), glutathione peroxidase (Gpx-1), caspase 3 (Casp3), BH3 interacting domain death agonist (Bid) and Bcl-2...