TY - JOUR A1 - Wagner, Michael A1 - Bertero, Edoardo A1 - Nickel, Alexander A1 - Kohlhaas, Michael A1 - Gibson, Gary E. A1 - Heggermont, Ward A1 - Heymans, Stephane A1 - Maack, Christoph T1 - Selective NADH communication from α-ketoglutarate dehydrogenase to mitochondrial transhydrogenase prevents reactive oxygen species formation under reducing conditions in the heart JF - Basic Research in Cardiology N2 - In heart failure, a functional block of complex I of the respiratory chain provokes superoxide generation, which is transformed to H\(_2\)O\(_2\) by dismutation. The Krebs cycle produces NADH, which delivers electrons to complex I, and NADPH for H\(_2\)O\(_2\) elimination via isocitrate dehydrogenase and nicotinamide nucleotide transhydrogenase (NNT). At high NADH levels, α-ketoglutarate dehydrogenase (α-KGDH) is a major source of superoxide in skeletal muscle mitochondria with low NNT activity. Here, we analyzed how α-KGDH and NNT control H\(_2\)O\(_2\) emission in cardiac mitochondria. In cardiac mitochondria from NNT-competent BL/6N mice, H\(_2\)O\(_2\) emission is equally low with pyruvate/malate (P/M) or α-ketoglutarate (α-KG) as substrates. Complex I inhibition with rotenone increases H2O2 emission from P/M, but not α-KG respiring mitochondria, which is potentiated by depleting H\(_2\)O\(_2\)-eliminating capacity. Conversely, in NNT-deficient BL/6J mitochondria, H2O2 emission is higher with α-KG than with P/M as substrate, and further potentiated by complex I blockade. Prior depletion of H\(_2\)O\(_2\)-eliminating capacity increases H\(_2\)O\(_2\) emission from P/M, but not α-KG respiring mitochondria. In cardiac myocytes, downregulation of α-KGDH activity impaired dynamic mitochondrial redox adaptation during workload transitions, without increasing H\(_2\)O\(_2\) emission. In conclusion, NADH from α-KGDH selectively shuttles to NNT for NADPH formation rather than to complex I of the respiratory chain for ATP production. Therefore, α-KGDH plays a key role for H\(_2\)O\(_2\) elimination, but is not a relevant source of superoxide in heart. In heart failure, α-KGDH/NNT-dependent NADPH formation ameliorates oxidative stress imposed by complex I blockade. Downregulation of α-KGDH may, therefore, predispose to oxidative stress in heart failure. KW - mitochondria KW - α-Ketoglutarate dehydrogenase KW - reactive oxygen species KW - nicotinamide nucleotide transhydrogenase Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-234907 SN - 0300-8428 VL - 115 ER - TY - THES A1 - Mohammadi, Milad T1 - Role of oxidized phospholipids in inflammatory pain T1 - Rolle von oxidierten Phospholipiden bei entzündlichen Schmerzen N2 - Introduction: During inflammation, reactive oxygen species (ROS) such as Hydrogen peroxide accumulate at the inflammation site and by oxidizing lipids, they produce metabolites such as 4-hydroxynonenal (4-HNE) and oxidized phospholipids (OxPLs). Transient receptor potential ankyrin 1 (TRPA1) and vanilloid 1 (TRPV1) are ligand gated ion channels that are expressed on nociceptors and their activation elicits pain. Hydrogen peroxide and 4-HNE are endogenous ligands for TRPA1 and their role in inflammatory pain conditions has been shown. OxPLs play a major pro-inflammatory role in many pathologies including atherosclerosis and multiple sclerosis. E06/T15 is a mouse IgM mAb that specifically binds oxidized phosphatidylcholine. D-4F is an apolipoprotein A-I mimetic peptide with a very high affinity for OxPLs and possess anti-inflammatory properties. E06 mAb and D-4F peptide protect against OxPLs-induced damage in atherosclerosis in vivo. Methods: To investigate the role of ROS and their metabolites in inflammatory pain, I utilized a combination of diverse and complex behavioral pain measurements and binding assays. I examined E06 mAb and D-4F as local treatment options for hypersensitivity evoked by endogenous and exogenous activators of TRPA1 and TRPV1 as well as in inflammatory and OxPL-induced pain models in vivo. 4-HNE, hydrogen peroxide as ROS source and mustard oil (AITC) were used to activate TRPA1, while capsaicin was used to activate TRPV1. Results: Intraplantar injection of oxidized 1-palmitoyl-2-arachidonoyl-sn-glycero-3-phosphocholine (OxPAPC) into rats’ hind paw elicited thermal and mechanical hypersensitivity. Genetic and pharmacological evidence in vivo confirmed the role of TRPA1 in OxPLs-induced hypersensitivity. OxPLs formation increased in complete Freund’s adjuvant (CFA)-induced inflamed rats’ paw. E06 mAb and D-4F prevented OxPAPC–induced mechanical and thermal hypersensitivity (hyperalgesia) as well as CFA-induced mechanical hypersensitivity. Also, all irritants induced thermal and mechanical hypersensitivity as well as affective-emotional responses and spontaneous nocifensive behaviors. E06 mAb blocked prolonged mechanical hypersensitivity by all but hydrogen peroxide. In parallel, D-4F prevented mechanical hypersensitivity induced by all irritants as well as thermal hypersensitivity induced by capsaicin and 4-HNE. In addition, competitive binding assays showed that all TRPA1/V1 agonists induced prolonged formation of OxPLs in the paw tissue explaining the anti-nociceptive properties of E06 mAb and D-4F. Finally, the potential of gait analysis as a readout for non-provoked pain behavioral measurements were examined. Conclusion and implications: OxPLs were characterized as novel targets in inflammatory pain. Treatment with the monoclonal antibody E06 or apolipoprotein A-I mimetic peptide D-4F are suggested as potential inflammatory pain medications. OxPLs’ role in neuropathic pain is yet to be investigated. N2 - Im entzündeten Gewebe akkumulieren reaktive Sauerstoffspezies (ROS) sowie oxidierte Phospholipide (OxPLs). ROS und in der Reaktionskette nachgeschaltete Verbindungen, wie 4- Hydroxynonenal (4-HNE) aktivieren Transiente Rezeptor Potential (TRP) Ionenkanäle: Ankyrin 1 (TRPA1) und Vanilloid 1 (TRPV1). Diese TRP-Kanäle werden auf Nozizeptoren exprimiert und rufen Schmerz z.B. bei Entzündung hervor. OxPLs sind an vielen entzündungsfördernden Prozessen maßgebend beteiligt und spielen eine Schlüsselrolle bei Pathologie von Atherosklerose und Multipler Sklerose. E06/T15 ist ein Maus IgM-mAb, welcher spezifisch an oxidierte Phosphatidylcholine bindet. D-4F ist ein Apolipoprotein A-I (ApoA-I) mimetisches Peptid, das eine sehr hohe Affinität für OxPLs aufweist und auch entzündungshemmende Eigenschaften besitzt. E06 mAb und D-4F schützen vor Atherosklerose in vivo. Um die mögliche Rolle von OxPLs beim Entzündungsschmerz zu untersuchen, verwendete ich eine Kombination von verschiedenen und komplexen Schmerzverhaltensmessungen, Bindungsassays und immunhistologische Färbungen. ... KW - Inflammatory pain KW - Oxidized phospholipids KW - reactive oxygen species KW - ROS KW - 4-HNE KW - HNE KW - OxPL Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-192402 ER - TY - THES A1 - Brandes, Nicolas T1 - Oxidative Thiol Modifications in Pro- and Eukaryotic Organisms T1 - Oxidative Thiol Modifikationen in Pro- und Eukaryotischen Organismen N2 - Cystein spielt eine wichtige Rolle in der Biochemie vieler Proteine. Aufgrund der Redox-Eigenschaften und der hohen Reaktivität der freien Thiol-Gruppe sowie dessen Fähigkeit Metallionen zu koordinieren, ist Cystein oft Bestandteil von katalytischen Zentren vieler Enzyme. Zudem lassen sich Cysteine durch reaktive Sauerstoff- und Stickstoffspezies leicht reversibel oxidativ modifizieren. In den letzten Jahren wurde gezeigt, dass Proteine redox-bedingte Thiol-Modifikationen nutzen, um Veränderungen ihrer Aktivität zu steuern. Diese redox-regulierten Proteine spielen eine zentrale Rolle in vielen physiologischen Prozessen. Das erste Ziel meiner Arbeit war die Identifizierung von Stickstoffmonoxid (NO)-sensitiven Proteinen in E. coli. Die redox-bedingten Funktionsänderungen solcher Proteine erklären möglicherweise die veränderte Physiologie von E. coli Zellen, die unter NO-Stress leiden. Um E. coli Proteine zu identifizieren, die unter Einwirkung von NO-Stress reversibel Thiol-modifiziert werden, wandte ich eine Kombination aus differentiellem Thiol-Trapping und 2D Gel-Elektrophorese an. Es wurden zehn Proteinen identifiziert, welche NO-sensitive Thiol-Gruppen enthalten. Genetische Studien ergaben, dass Modifikationen an AceF & IlvC mitverantwortlich sind für die NO-induzierte Wachstumshemmung. Bemerkenswert ist es, dass die Mehrheit der identifizierten Proteine speziell nur gegen reaktive Stickstoffspezies empfindlich ist, welches an einem der identifizierten Stickstoffmonoxid-sensitiven Proteinen, der kleinen Untereinheit von Glutamate synthase, getestet wurde. In vivo und in vitro Aktivitätsstudien zeigten, dass es zu einer schnellen Inaktivierung von Glutamate synthase nach NO-Behandlung kommt, das Protein aber resistent gegenüber anderen Oxidationsmittel ist. Diese Resultate implizieren, dass reaktive Sauerstoff- und Stickstoffspezies unterschiedliche physiologische Vorgänge in Bakterien beeinflussen. Das zweite Ziel meiner Arbeit war es, redox-sensitive Proteine in S. cerevisiae zu identifizieren und deren Redox-Zustand als in vivo Read-Out zu verwenden, um die Rolle von oxidativen Stress während des Alterungsprozess eukaryotischer Zellen zu analysieren. Zunächst bestimmte ich in Hefezellen mit Hilfe von OxICAT, einer hochsensiblen quantitativen Methode, die Thiol-Trapping mit Massenspektrometrie verbindet, den exakten in vivo Thiol-Status von fast 300 Proteinen. Diese Proteine lassen sich in vier Gruppen einteilen: 1) Proteine, deren Cysteinreste resistent gegen Oxidation sind; 2) Proteine, in denen Cysteinmodifikationen strukturelle Aufgaben übernehmen; 3) Proteine mit oxidationsempfindlichen Cysteinen, die bereits eine gewisse Oxidation in exponentiell wachsenden Hefezellen aufweisen; 4) Proteine, die reduziert sind, aber redox-sensitive Cysteinreste enthalten, die die Funktion der Proteine bei Vorhandensein von oxidativen Stress beeinflussen. Die Sensitivität dieser Proteine gegenüber oxidativen Stress wurde durch Exposition subletaler Konzentrationen von H2O2 oder Superoxid auf Hefezellen nachgewiesen. Es wurde gezeigt, dass die wichtigsten zellulären Angriffspunkte von H2O2- und Superoxid-bedingtem Stress Proteine sind, die an Vorgängen der Translation, Glykolyse, des Citratzyklus und der Aminosäure-Biosynthese beteiligt sind. Diese Zielproteine zeigen, dass Zellen für die Bekämpfung von oxidativen Stress Metabolite schnell in Richtung des Pentosephosphatweges umleiten, um die Produktion des Reduktionsmittels NADPH sicherzustellen. Die hier präsentierten Ergebnisse belegen, dass die quantitative Bestimmung des Oxidationsstatus von Proteinen eine wertvolle Methode ist, um redox-sensitive Cysteinreste zu identifizieren. Die OxICAT Technologie wurde dann verwendet, um das genaue Ausmaß und die Entstehung von oxidativen Stress in chronologisch alternden S. cerevisiae Zellen zu bestimmen. Für diese Bestimmung wurde der Oxidationsstatus von Proteinen in alternden Hefezellen als physiologischer Read-Out verwendet. Ich zeigte, dass die zelluläre Redox-Homöostase in chronologisch alternden Hefezellen global zusammenbricht, wobei es sich dabei um einen Prozess handelt, der dem Zelltod vorausgeht. Der Beginn dieses Zusammenbruchs scheint mit der Lebensdauer der Hefezellen zu korrelieren, da Kalorienrestriktion die Lebensdauer der Hefezellen erhöht und den Zusammenbruch des Redox-Gleichgewichts verzögert. Die Oxidation einer kleinen Anzahl an Proteinen (z.B. Thioredoxin reductase) geht dem Redox-Zusammenbruch deutlich voraus, was maßgeblich zum Verlust der Redox-Homöostase beitragen könnte. Diese Studien an alternden Hefezellen erweitern unser Verständnis, wie sich Veränderungen in der Redox-Homöostase auf die Lebensdauer von Hefezellen auswirken. Zudem bestätigen die hier präsentierten Ergebnisse die Bedeutung von oxidativen Thiol-Modifikationen als eine der wichtigsten posttranslationalen Proteinmodifikationen in pro-und eukaryotischen Organismen N2 - Cysteines play important roles in the biochemistry of many proteins. The high reactivity, redox properties, and ability of the free thiol group to coordinate metal ions designate cysteines as the amino acids of choice to form key catalytic components of many enzymes. Also, cysteines readily react with reactive oxygen and nitrogen species to form reversible oxidative thiol modifications. Over the last few years, an increasing number of proteins have been identified that use redox-mediated thiol modifications to modulate their function, activity, or localization. These redox-regulated proteins are central players in numerous important cellular processes. First aim of this study was to discover nitric oxide (NO) sensitive proteins in E. coli, whose redox-mediated functional changes might explain the physiological alterations observed in E. coli cells suffering from NO-stress. To identify E. coli proteins that undergo reversible thiol modifications upon NO-treatment in vivo, I applied a differential thiol trapping technique combined with two-dimensional gel analysis. 10 proteins were found to contain thiol groups sensitive to NO-treatment. Subsequent genetic studies revealed that the oxidative modifications of AceF & IlvC are, in part, responsible for the observed NO-induced growth inhibition. Noteworthy, the majority of identified protein targets turned out to be specifically sensitive towards reactive nitrogen species. This oxidant specificity was tested on one NO-sensitive protein, the small subunit of glutamate synthase. In vivo and in vitro activity studies demonstrated that glutamate synthase rapidly inactivates upon nitric oxide treatment but is resistant towards other oxidative stressors. These results imply that reactive oxygen and nitrogen species affect distinct physiological processes in bacteria. The second aim of my study was to identify redox-sensitive proteins in S. cerevisiae and to use their redox state as in vivo read-out to assess the role of oxidative stress during the eukaryotic aging process. I first determined the precise in vivo thiol status of almost 300 yeast proteins located in the cytosol and sub-cellular compartments of yeast cells using a highly quantitative mass spectrometry based thiol trapping technique, called OxICAT. The identified proteins can be clustered in four groups: 1) proteins, whose cysteine residues are oxidation resistant; 2) proteins with structurally or functionally important cysteine modifications 3) proteins with highly oxidation-sensitive active site cysteines, which are partially oxidized in exponentially growing yeast cells due to their exquisite sensitivity towards low amounts of ROS; 4) proteins that are reduced in exponentially growing cells but harbor redox-sensitive cysteine(s) that affect the catalytic function of the protein during oxidative stress. These oxidative stress sensitive proteins were identified by exposure of yeast cells to sublethal concentrations of H2O2 or superoxide. It was shown that the major targets of peroxide- and superoxide-mediated stress in the cell are proteins involved in translation, glycolysis, TCA cycle and amino acid biosynthesis. These targets indicate that cells rapidly redirect the metabolic flux and energy towards the pentose phosphate pathway in an attempt to ensure the production of the reducing equivalent NADPH to counterattack oxidative stress. These results reveal that the quantitative assessment of a protein’s oxidation state is a valuable tool to identify catalytically active and redox-sensitive cysteine residues. The OxICAT technology was then used to precisely determine extent and onset of oxidative stress in chronologically aging S. cerevisiae cells by utilizing the redox status of proteins as physiological read-out. I found that chronological aging yeast cells undergo a global collapse of the cellular redox homeostasis, which precedes cell death. The onset of this collapse appears to correlate with the yeast life span, as caloric restriction increases the life span and delays the redox collapse. These results suggest that maintenance of the redox balance might contribute to the life expanding benefits of regulating the caloric intake of yeast. Clustering analysis of all oxidatively modified proteins in chronological aging yeast revealed a subset of proteins whose oxidative thiol modifications significantly precede the general redox collapse. Oxidation of these early target proteins, which most likely results in a loss of their activity, might contribute to or even cause the observed loss of redox homeostasis (i.e., thioredoxin reductase) in chronologically aging yeast. These studies in aging yeast expand our understanding how changes in redox homeostasis affect the life span of yeast cells and confirm the importance of oxidative thiol modifications as key posttranslational modifications in pro- and eukaryotic organisms. KW - Oxidativer Stress KW - Cystein KW - Saccharomyces cerevisiae KW - Escherichia coli KW - Wasserstoffperoxid KW - Hyperoxide KW - Sauerstoffradikal KW - Thiolgruppe KW - Altern KW - Oxidation KW - Biologische Oxidation KW - Oxidative Thiol Modifikationen KW - Reaktive Sauerstoffspezies KW - Chronologisches Altern KW - Reversibel KW - Posttranslational KW - oxidative thiol modification KW - chronological aging KW - reactive oxygen species KW - Saccharomyces cerevisiae KW - thioredoxin reductase Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-46542 ER - TY - JOUR A1 - Schwemmlein, Julia A1 - Maack, Christoph A1 - Bertero, Edoardo T1 - Mitochondria as therapeutic targets in heart failure JF - Current Heart Failure Reports N2 - Purpose of Review We review therapeutic approaches aimed at restoring function of the failing heart by targeting mitochondrial reactive oxygen species (ROS), ion handling, and substrate utilization for adenosine triphosphate (ATP) production. Recent Findings Mitochondria-targeted therapies have been tested in animal models of and humans with heart failure (HF). Cardiac benefits of sodium/glucose cotransporter 2 inhibitors might be partly explained by their effects on ion handling and metabolism of cardiac myocytes. Summary The large energy requirements of the heart are met by oxidative phosphorylation in mitochondria, which is tightly regulated by the turnover of ATP that fuels cardiac contraction and relaxation. In heart failure (HF), this mechano-energetic coupling is disrupted, leading to bioenergetic mismatch and production of ROS that drive the progression of cardiac dysfunction. Furthermore, HF is accompanied by changes in substrate uptake and oxidation that are considered detrimental for mitochondrial oxidative metabolism and negatively affect cardiac efficiency. Mitochondria lie at the crossroads of metabolic and energetic dysfunction in HF and represent ideal therapeutic targets. KW - mitochondria KW - heart failure KW - reactive oxygen species KW - MitoQ KW - elamipretide KW - SGLT2 inhibitors KW - cardiac metabolism Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-324015 VL - 19 IS - 2 ER - TY - JOUR A1 - Dudek, Jan A1 - Maack, Christoph T1 - Mechano-energetic aspects of Barth syndrome JF - Journal of Inherited Metabolic Disease N2 - Energy-demanding organs like the heart are strongly dependent on oxidative phosphorylation in mitochondria. Oxidative phosphorylation is governed by the respiratory chain located in the inner mitochondrial membrane. The inner mitochondrial membrane is the only cellular membrane with significant amounts of the phospholipid cardiolipin, and cardiolipin was found to directly interact with a number of essential protein complexes, including respiratory chain complexes I to V. An inherited defect in the biogenesis of cardiolipin causes Barth syndrome, which is associated with cardiomyopathy, skeletal myopathy, neutropenia and growth retardation. Energy conversion is dependent on reducing equivalents, which are replenished by oxidative metabolism in the Krebs cycle. Cardiolipin deficiency in Barth syndrome also affects Krebs cycle activity, metabolite transport and mitochondrial morphology. During excitation-contraction coupling, calcium (Ca\(^{2+}\)) released from the sarcoplasmic reticulum drives sarcomeric contraction. At the same time, Ca\(^{2+}\) influx into mitochondria drives the activation of Krebs cycle dehydrogenases and the regeneration of reducing equivalents. Reducing equivalents are essential not only for energy conversion, but also for maintaining a redox buffer, which is required to detoxify reactive oxygen species (ROS). Defects in CL may also affect Ca\(^{2+}\) uptake into mitochondria and thereby hamper energy supply and demand matching, but also detoxification of ROS. Here, we review the impact of cardiolipin deficiency on mitochondrial function in Barth syndrome and discuss potential therapeutic strategies. KW - Barth syndrome KW - respiratory chain KW - reactive oxygen species KW - cardiolipin KW - mitochondria Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-257512 VL - 45 IS - 1 ER - TY - JOUR A1 - Meierjohann, Svenja T1 - Hypoxia independent drivers of melanoma angiogenesis JF - Frontiers in Oncology N2 - Tumor angiogenesis is a process which is traditionally regarded as the tumor’s response to low nutrient supply occurring under hypoxic conditions. However, hypoxia is not a pre-requisite for angiogenesis. The fact that even single tumor cells or small tumor cell aggregates are capable of attracting blood vessels reveals the early metastatic capability of tumor cells. This review sheds light on the hypoxia-independent mechanisms of tumor angiogenesis in melanoma. KW - melanoma KW - angiogenesis KW - hypoxia-independent KW - reactive oxygen species KW - NF-κB Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125586 VL - 5 IS - 120 ER - TY - JOUR A1 - Ockermann, Philipp A1 - Lizio, Rosario A1 - Hansmann, Jan T1 - Healthberry 865\(^®\) and a subset of its single anthocyanins attenuate oxidative stress in human endothelial in vitro models JF - Nutrients N2 - Oxidative stress and inflammation play a pivotal role in the development of cardiovascular diseases, an ever-growing worldwide problem. As a non-pharmacological approach, diet, especially a flavonoid-rich diet, showed promising results in the reduction of cardiovascular diseases and alleviation of their symptoms. In this study, in vitro systems based on human microvascular endothelial cells (hmvEC) and human umbilical cord endothelial cells (HUVEC) were established to determine the effect of Healthberry 865\(^®\) (HB) and ten of its relating single anthocyanins on oxidative stress. Furthermore, five metabolites were used in order to examine the effect of anthocyanin's most common breakdown molecules. The results showed an effect of HB in both models after 24 h, as well as most of its single anthocyanins. Cyanidin-rutinoside, peonidin-galactoside, and petunidin-glucoside had a model-specific effect. For the metabolites, phloroglucinaldeyhde (PGA) showed an effect in both models, while vanillic acid (VA) only had an effect in HUVEC. When combined, a combination of several anthocyanins did not have a cumulative effect, except for combining glucosides in hmvEC. The combination of PGA and VA even revealed an inhibitive behavior. Overall, the study demonstrates the antioxidative effect of HB and several of its single anthocyanins and metabolites, which are partially model specific, and coincides with animal studies. KW - anthocyanins KW - reactive oxygen species KW - HUVEC KW - microvascular endothelial cells Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-281887 SN - 2072-6643 VL - 14 IS - 14 ER - TY - THES A1 - Czisch, Michael T1 - Die Rolle von Bcl-2 bei der UV- und TRAIL-induzierten Keratinozytenapoptose T1 - The role of Bcl-2 in UV- and TRAIL-induced keratinocyte apoptosis N2 - In Keratinozyten wird sowohl durch UVB als auch durch PUVA-Bestrahlung Apoptose induziert. Wir untersuchten die in Keratinozyten durch UVB, PUVA, UVA und Todesliganden wie TRAIL ausgelösten Apoptosewege näher. UVB und PUVA, nicht aber UVA-Bestrahlung lösen in vitro Keratinozytenapoptose aus. 2-4 h nach UVB beobachteten wir die Aktivierung von Caspasen. Nach PUVA setzt die Aktivierung von Caspasen wesentlich später ein, nämlich erst 12 h nach Bestrahlung. Passend dazu, ist ein Verlust des mitochondrialen Transmembranpotentials 6-8 h nach UVB und 12-14 h nach PUVA detektierbar. Die Überexpression des Proteins Bcl-2 verhindert den Verlust des mitochondrialen Transmembranpotentials und die Caspase-Aktivierung nach UVB, und vermittelt auch einen klonogen Schutz, unabhängig von der Bildung reaktiver Sauerstoffradikale. Im Gegensatz dazu verzögert es den Verlust des Transmembranpotentials und die Caspase-Aktivierung nach PUVA nur und verhindert sie nicht. PUVA-bestrahlte Zellen können sich nicht weiter teilen, sind also durch Bcl-2 nicht klonogen geschützt. N2 - An important response of keratinocytes to UVB or PUVA irradiation is the induction of apoptosis. In order to understand the apoptotic responses of keratinocytes, we compared UVB, PUVA, UVA irradiated and TRAIL-treated keratinocytes for the activation of major apoptosis signalling pathways. UVB and PUVA, but not UVA irradiation induced keratinocyte apoptosis in vitro. Activation of caspases was detectable within 2 – 4 h after UVB irradiation. Interestingly, caspase activation following PUVA was delayed, beginning by 12 hours post irradiation. In line, mitochondrial transmembrane potential (MTP) decreased 6 – 8 hours after UVB, whereas PUVA mediated MTP loss started only 12 - 14h post irradiation. Interestingly, Bcl-2 overexpression protected against UVB induced early MTP loss and caspase activation. Moreover, Bcl-2 also protected clonogenic survival following UVB irradiation independent of the UV-induced generation of reactive oxygen species. In marked contrast, although Bcl-2 delayed PUVA induced MTP loss and caspase activation, Bcl-2 overexpressing keratinocytes failed to protect clonogenic survival following PUVA. Interestingly, similar levels of ROS were produced by UVA and PUVA irrespective of the expression of Bcl-2, suggesting that ROS generation does not have a major role in PUVA induced activation of apoptosis signalling. We conclude that distinct pathways independent of caspases are employed to exert the cell death program in PUVA and UVB induced apoptosis. While PUVA-induced cell death overcomes Bcl-2 protected mitochondrial pathways of apoptosis, UVB induced cell death is dose-dependently protected by Bcl-2. Our data suggest that PUVA-induced DNA damage rather than ROS generation plays the key role for PUVA induced apoptosis. KW - Bcl-2 KW - Apoptose KW - UV KW - UVB KW - UVA KW - PUVA KW - Keratinozyten KW - HaCaT KW - TRAIL KW - Zytochrom c KW - Caspasen KW - ROS KW - Mitochondrium KW - Bcl-2 KW - apoptosis KW - UV KW - UVB KW - UVA KW - PUVA KW - keratinocytes KW - HaCaT KW - TRAIL KW - cytochrome c KW - caspases KW - reactive oxygen species KW - mitochondria Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-10903 ER - TY - JOUR A1 - Oehler, Beatrice A1 - Kloka, Jan A1 - Mohammadi, Milad A1 - Ben-Kraiem, Adel A1 - Rittner, Heike L. T1 - D-4F, an ApoA-I mimetic peptide ameliorating TRPA1-mediated nocifensive behaviour in a model of neurogenic inflammation JF - Molecular Pain N2 - Background High doses of capsaicin are recommended for the treatment of neuropathic pain. However, low doses evoke mechanical hypersensitivity. Activation of the capsaicin chemosensor transient receptor potential vanilloid 1 (TRPV1) induces neurogenic inflammation. In addition to the release of pro-inflammatory mediators, reactive oxygen species are produced. These highly reactive molecules generate oxidised phospholipids and 4-hydroxynonenal (4-HNE) which then directly activate TRP ankyrin 1 (TRPA1). The apolipoprotein A-I mimetic peptide D-4F neutralises oxidised phospholipids. Here, we asked whether D-4F ameliorates neurogenic hypersensitivity in rodents by targeting reactive oxygen species and 4-HNE in the capsaicin-evoked pain model. Results Co-application of D-4F ameliorated capsaicin-induced mechanical hypersensitivity and allodynia as well as persistent heat hypersensitivity measured by Randell–Selitto, von Frey and Hargreaves test, respectively. In addition, mechanical hypersensitivity was blocked after co-injection of D-4F with the reactive oxygen species analogue H2O2 or 4-HNE. In vitro studies on dorsal root ganglion neurons and stably transfected cell lines revealed a TRPA1-dependent inhibition of the calcium influx when agonists were pre-incubated with D-4F. The capsaicin-induced calcium influx in TRPV1-expressing cell lines and dorsal root ganglion neurons sustained in the presence of D-4F. Conclusions D-4F is a promising compound to ameliorate TRPA1-dependent hypersensitivity during neurogenic inflammation. KW - TRPA1 KW - capsaicin KW - reactive oxygen species KW - oxidised lipids KW - pain KW - targeting Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-236061 VL - 16 ER - TY - JOUR A1 - Otto, Christoph A1 - Hahlbrock, Theresa A1 - Eich, Kilian A1 - Karaaslan, Ferdi A1 - Jürgens, Constantin A1 - Germer, Christoph-Thomas A1 - Wiegering, Armin A1 - Kämmerer, Ulrike T1 - Antiproliferative and antimetabolic effects behind the anticancer property of fermented wheat germ extract JF - BMC Complementary and Alternative Medicine N2 - Background Fermented wheat germ extract (FWGE) sold under the trade name Avemar exhibits anticancer activity in vitro and in vivo. Its mechanisms of action are divided into antiproliferative and antimetabolic effects. Its influcence on cancer cell metabolism needs further investigation. One objective of this study, therefore, was to further elucidate the antimetabolic action of FWGE. The anticancer compound 2,6-dimethoxy-1,4-benzoquinone (DMBQ) is the major bioactive compound in FWGE and is probably responsible for its anticancer activity. The second objective of this study was to compare the antiproliferative properties in vitro of FWGE and the DMBQ compound. Methods The IC\(_{50}\) values of FWGE were determined for nine human cancer cell lines after 24 h of culture. The DMBQ compound was used at a concentration of 24 μmol/l, which is equal to the molar concentration of DMBQ in FWGE. Cell viability, cell cycle, cellular redox state, glucose consumption, lactic acid production, cellular ATP levels, and the NADH/NAD\(^+\) ratio were measured. Results The mean IC\(_{50}\) value of FWGE for the nine human cancer cell lines tested was 10 mg/ml. Both FWGE (10 mg/ml) and the DMBQ compound (24 μmol/l) induced massive cell damage within 24 h after starting treatment, with changes in the cellular redox state secondary to formation of intracellular reactive oxygen species. Unlike the DMBQ compound, which was only cytotoxic, FWGE exhibited cytostatic and growth delay effects in addition to cytotoxicity. Both cytostatic and growth delay effects were linked to impaired glucose utilization which influenced the cell cycle, cellular ATP levels, and the NADH/NAD\(^+\) ratio. The growth delay effect in response to FWGE treatment led to induction of autophagy. Conclusions FWGE and the DMBQ compound both induced oxidative stress-promoted cytotoxicity. In addition, FWGE exhibited cytostatic and growth delay effects associated with impaired glucose utilization which led to autophagy, a possible previously unknown mechanism behind the influence of FWGE on cancer cell metabolism. KW - cytostatic KW - FWGE KW - benzoquinone KW - cancer cells KW - reactive oxygen species KW - autophagy KW - cytotoxicity Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146013 VL - 16 IS - 160 ER - TY - JOUR A1 - Kleefeldt, Florian A1 - Bömmel, Heike A1 - Broede, Britta A1 - Thomsen, Michael A1 - Pfeiffer, Verena A1 - Wörsdörfer, Philipp A1 - Karnati, Srikanth A1 - Wagner, Nicole A1 - Rueckschloss, Uwe A1 - Ergün, Süleyman T1 - Aging‐related carcinoembryonic antigen‐related cell adhesion molecule 1 signaling promotes vascular dysfunction JF - Aging Cell N2 - Aging is an independent risk factor for cardiovascular diseases and therefore of particular interest for the prevention of cardiovascular events. However, the mechanisms underlying vascular aging are not well understood. Since carcinoembryonic antigen‐related cell adhesion molecule 1 (CEACAM1) is crucially involved in vascular homeostasis, we sought to identify the role of CEACAM1 in vascular aging. Using human internal thoracic artery and murine aorta, we show that CEACAM1 is upregulated in the course of vascular aging. Further analyses demonstrated that TNF‐α is CEACAM1‐dependently upregulated in the aging vasculature. Vice versa, TNF‐α induces CEACAM1 expression. This results in a feed‐forward loop in the aging vasculature that maintains a chronic pro‐inflammatory milieu. Furthermore, we demonstrate that age‐associated vascular alterations, that is, increased oxidative stress and vascular fibrosis, due to increased medial collagen deposition crucially depend on the presence of CEACAM1. Additionally, age‐dependent upregulation of vascular CEACAM1 expression contributes to endothelial barrier impairment, putatively via increased VEGF/VEGFR‐2 signaling. Consequently, aging‐related upregulation of vascular CEACAM1 expression results in endothelial dysfunction that may promote atherosclerotic plaque formation in the presence of additional risk factors. Our data suggest that CEACAM1 might represent an attractive target in order to delay physiological aging and therefore the transition to vascular disorders such as atherosclerosis. KW - aging KW - anti‐aging KW - cytokines KW - inflammation KW - mouse KW - reactive oxygen species Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-201231 VL - 2019 IS - 18 ER -