TY - JOUR A1 - Adaku Chilaka, Cynthia A1 - Mally, Angela T1 - Mycotoxin Occurrence, Exposure and Health Implications in Infants and Young Children in Sub-Saharan Africa: A Review JF - Foods N2 - Infants and young children (IYC) remain the most vulnerable population group to environmental hazards worldwide, especially in economically developing regions such as sub-Saharan Africa (SSA). As a result, several governmental and non-governmental institutions including health, environmental and food safety networks and researchers have been proactive toward protecting this group. Mycotoxins, toxic secondary fungal metabolites, contribute largely to the health risks of this young population. In SSA, the scenario is worsened by socioeconomic status, poor agricultural and storage practices, and low level of awareness, as well as the non-establishment and lack of enforcement of regulatory limits in the region. Studies have revealed mycotoxin occurrence in breast milk and other weaning foods. Of concern is the early exposure of infants to mycotoxins through transplacental transfer and breast milk as a consequence of maternal exposure, which may result in adverse health effects. The current paper presents an overview of mycotoxin occurrence in foods intended for IYC in SSA. It discusses the imperative evidence of mycotoxin exposure of this population group in SSA, taking into account consumption data and the occurrence of mycotoxins in food, as well as biomonitoring approaches. Additionally, it discusses the health implications associated with IYC exposure to mycotoxins in SSA. KW - mycotoxin KW - occurrence KW - exposure KW - child health KW - sub-Saharan Africa Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-219250 SN - 2304-8158 VL - 9 IS - 11 ER - TY - JOUR A1 - Adam, W. A1 - Ahrweiler, M. A1 - Saha-Möller, C. R. A1 - Sauter, M. A1 - Schönberger, A. A1 - Epe, B. A1 - Müller, E. A1 - Schiffmann, D. A1 - Stopper, Helga A1 - Wild, D. T1 - Genotoxicity studies of benzofuran dioxetanes and epoxides with isolated DNA, bacteria and mammalian cells N2 - 1.2-Dioxetanes, very reactive and high energy molecules. are involved as labile intermediates in dioxygenase- activated aerobic metabolism and in physiological processes. Various toxico1ogica1 tests reveal that dioxetanes are indeed genotoxic. In supercoiled DNA of bacteriophage PM2 they induce endonucleasesensitive sites, most of them are FPG protein-sensitive base modifications (8-hydroxyguanine, fonnamidopyrimidines). Pyrimidinedimersand sites ofbase loss (AP sites) which were probed by UV endonuclease and exonuclease 111 are minor lesions in this system. While the alky1-substituted dioxetanes do not show any significant mutagenic activity in different Salmonella typhimurium strains, heteroarene dioxetanes such as benzofuran and furocoumarin dioxetanes are strongly mutagenic in S. typhimurium strain TA I 00. DNA adducts formed with an intermediary alkyJating agent appear to be responsible for the mutagenic activity of benzofuran dioxetane. We assume that the benzofuran epoxides, generated in situ from benzofuran dioxetanes by deoxygenation are the ultimate mutagens of the latter. since benzofuran epoxides are highly mutagenic in the S. typhimurium strain TAIOO and they form DNA adducts. as detected by the 212Ppostlabelling technique. Our results imply that the type of D NA darnage promoted by dioxetanes is dependent on the structural feature of dioxetanes. Furthermore, the direct photochemical DNA darnage by energy transfer. i.e., pyrimidine dimers, plays a minor role in the genotoxicity of dioxetanes. Instead, photooxidation dominates in isolated DNA. while radical darnage and alkylation prevail in the cellular system. KW - Toxikologie KW - 1 KW - 2-Dioxetane KW - Benzefuran dioxetane KW - Benzefuran epoxide KW - DNA damage KW - Mutagenicity KW - DNA adduct . Repair endonuclease KW - FPG protein Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-63420 ER - TY - JOUR A1 - Adami, Hans-Olov A1 - Dragsted, Lars A1 - Enig, Bent A1 - Hansen, Jens A1 - Haraldsdóttir, Jóhanna A1 - Hill, Michael J. A1 - Holm, Lars Erik A1 - Knudsen, Ib A1 - Larsen, Jens-Jorgen A1 - Lutz, Werner K. A1 - Osler, Merete A1 - Overvad, Kim A1 - Sabroe, Svend A1 - Sanner, Tore A1 - Strube, Michael A1 - Sorensen, Thorkild I. A. A1 - Thorling, Eivind B. T1 - Report from the working group on diet and cancer. N2 - No abstract available. KW - Krebs KW - Ernährung Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-71601 ER - TY - JOUR A1 - Agarwal, Shailesh R. A1 - Yang, Pei-Chi A1 - Rice, Monica A1 - Singer, Cherie A. A1 - Nikolaev, Viacheslav O. A1 - Lohse, Martin J. A1 - Clancy, Colleen E. A1 - Harvey, Robert D. T1 - Role of Membrane Microdomains in Compartmentation of cAMP Signaling JF - PLOS ONE N2 - Spatially restricting cAMP production to discrete subcellular locations permits selective regulation of specific functional responses. But exactly where and how cAMP signaling is confined is not fully understood. Different receptors and adenylyl cyclase isoforms responsible for cAMP production are not uniformly distributed between lipid raft and non-lipid raft domains of the plasma membrane. We sought to determine the role that these membrane domains play in organizing cAMP responses in HEK293 cells. The freely diffusible FRET-based biosensor Epac2-camps was used to measure global cAMP responses, while versions of the probe targeted to lipid raft (Epac2-MyrPalm) and non-raft (Epac2-CAAX) domains were used to monitor local cAMP production near the plasma membrane. Disruption of lipid rafts by cholesterol depletion selectively altered cAMP responses produced by raft-associated receptors. The results indicate that receptors associated with lipid raft as well as non-lipid raft domains can contribute to global cAMP responses. In addition, basal cAMP activity was found to be significantly higher in non-raft domains. This was supported by the fact that pharmacologic inhibition of adenylyl cyclase activity reduced basal cAMP activity detected by Epac2-CAAX but not Epac2-MyrPalm or Epac2-camps. Responses detected by Epac2-CAAX were also more sensitive to direct stimulation of adenylyl cyclase activity, but less sensitive to inhibition of phosphodiesterase activity. Quantitative modeling was used to demonstrate that differences in adenylyl cyclase and phosphodiesterase activities are necessary but not sufficient to explain compartmentation of cAMP associated with different microdomains of the plasma membrane. KW - protein-coupled-receptors KW - adenylyl-cyclase isoforms KW - adult cardiac myocytes KW - plasma membrane KW - lipid rafts KW - cholesterol depletion KW - BETA(2)-adrenergic receptor KW - living vells KW - cyclic-AMP KW - domains Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116673 SN - 1932-6203 VL - 9 IS - 4 ER - TY - JOUR A1 - Alldrick, A. J. A1 - Lutz, Werner K. T1 - Covalent binding of [2-\(^{14}\)C]2-amino-3,8-dimethylimidazo[4,5-f]-quinoxaline (MeIQx) to mouse DNA in vivo N2 - Fernale BALB/c mice were administered intragastrically with equimolar amounts of either [2-\(^{14}\)C]2-amino-3,8-dimethyi[ 4,5-J]qulnoxaline (MeiQx) or 2-acetylamino[9-\(^{14}\)C]fluorene (2AAF). DNA was isolated from tissues of mice killed either 6 or 24 h after administration. Analysis of liver DNA nucleotide digests by HPLC analysis revealed that all of the radioactivity was attributable to adduct formation. Tbe specific activities of DNA samples were converted to covalent bindlog indices (CBI, J.LIDOI adduct per mol DNA nucleotides/mmol chemical app6ed per kg animal body weight). CBI values of 25 and 9 were detennined for 2AAF and MeiQx in tbe llvers of mice killed 6 h after dosing. The values were in general agreement with the moderate carcinogenic potency of these compounds. The specific activities of DNA preparations obtained from the lddneys, spleens, stomachs, small intestines and large intestlnes of mice treated witb MeiQx and killed 6 h after doslng were S- to 35-times less tban those obtained witb the llver. DNA isolated from tbe lungs (a target organ for MeiQx tumorigenicity) of MeiQx-treated mice was not radiolabeUed at tbe limit of detection (CBI <0.3). With tbe exception of tbe gastrolntestinal tract, the specific activities of DNA samples isolated from mice killed 6 h after administration were higher than those from mice killed after 24 h. KW - Toxikologie Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60832 ER - TY - THES A1 - Anton, Selma T1 - Characterization of cAMP nanodomains surrounding the human Glucagon-like peptide 1 receptor using FRET-based reporters T1 - Charakterisierung der Rezeptor-assoziierten cAMP Nanodomänen des humanen Glucagon-like peptide 1 Rezeptors mittels FRET-basierter Sensoren N2 - Cyclic adenosine monophosphate (cAMP), the ubiquitous second messenger produced upon stimulation of GPCRs which couple to the stimulatory GS protein, orchestrates an array of physiological processes including cardiac function, neuronal plasticity, immune responses, cellular proliferation and apoptosis. By interacting with various effector proteins, among others protein kinase A (PKA) and exchange proteins directly activated by cAMP (Epac), it triggers signaling cascades for the cellular response. Although the functional outcomes of GSPCR-activation are very diverse depending on the extracellular stimulus, they are all mediated exclusively by this single second messenger. Thus, the question arises how specificity in such responses may be attained. A hypothesis to explain signaling specificity is that cellular signaling architecture, and thus precise operation of cAMP in space and time would appear to be essential to achieve signaling specificity. Compartments with elevated cAMP levels would allow specific signal relay from receptors to effectors within a micro- or nanometer range, setting the molecular basis for signaling specificity. Although the paradigm of signaling compartmentation gains continuous recognition and is thoroughly being investigated, the molecular composition of such compartments and how they are maintained remains to be elucidated. In addition, such compartments would require very restricted diffusion of cAMP, but all direct measurements have indicated that it can diffuse in cells almost freely. In this work, we present the identification and characterize of a cAMP signaling compartment at a GSPCR. We created a Förster resonance energy transfer (FRET)-based receptor-sensor conjugate, allowing us to study cAMP dynamics in direct vicinity of the human glucagone-like peptide 1 receptor (hGLP1R). Additional targeting of analogous sensors to the plasma membrane and the cytosol enables assessment of cAMP dynamics in different subcellular regions. We compare both basal and stimulated cAMP levels and study cAMP crosstalk of different receptors. With the design of novel receptor nanorulers up to 60nm in length, which allow mapping cAMP levels in nanometer distance from the hGLP1R, we identify a cAMP nanodomain surrounding it. Further, we show that phosphodiesterases (PDEs), the only enzymes known to degrade cAMP, are decisive in constraining cAMP diffusion into the cytosol thereby maintaining a cAMP gradient. Following the discovery of this nanodomain, we sought to investigate whether downstream effectors such as PKA are present and active within the domain, additionally studying the role of A-kinase anchoring proteins (AKAPs) in targeting PKA to the receptor compartment. We demonstrate that GLP1-produced cAMP signals translate into local nanodomain-restricted PKA phosphorylation and determine that AKAP-tethering is essential for nanodomain PKA. Taken together, our results provide evidence for the existence of a dynamic, receptor associated cAMP nanodomain and give prospect for which key proteins are likely to be involved in its formation. These conditions would allow cAMP to exert its function in a spatially and temporally restricted manner, setting the basis for a cell to achieve signaling specificity. Understanding the molecular mechanism of cAMP signaling would allow modulation and thus regulation of GPCR signaling, taking advantage of it for pharmacological treatment. N2 - G Protein gekoppelte Rezeptoren (GPCRs) stellen eine große und sehr vielfältige Familie an Membranproteinen dar, deren primäre Funktion die Signalübertragung von extrazellulären Stimuli in intrazelluläre Signale ist. Dank ihrer breiten Expression im gesamten menschlichen Körper regulieren sie unterschiedliche zelluläre Prozesse und damit deren physiologische Funktion, unter anderem die Sinnesempfindung, zelluläre Kommunikation und Neurotransmission. GPCRs stehen im Zusammenhang mit unterschiedlichen Erkrankungen wie Herzinsuffizienz, Krebs, neurologischen Funktionsstörungen und diverser metabolischer Krankheiten, weswegen sie als Ziele („Targets“) zur Behandlung verschiedener Erkrankungen erforscht und genutzt werden. Aufgrund ihrer Expression auf der Zelloberfläche sind sie leicht zugänglich, und die Diversität ihrer Liganden begünstigt zusätzlich ihre Nutzung als pharmakologische Targets. Heutzutage vermitteln bereits 30% aller weltweit zugelassenen Arzneistoffe ihre Wirkung an GPCRs. GPCRs üben ihre Funktion aus, indem sie hauptsächlich an G Proteine binden, welche wiederum die Produktion sogenannter second messenger in Gang setzen. cAMP ist das Hauptsignalmolekül der Rezeptoren, welche an das stimulatorische GS Protein koppeln. cAMP überträgt hunderte ankommende Signale in einer hochspezifischen Weise, indem es an unterschiedliche Effektorproteine bindet, welche sich in bestimmten zellulären Regionen befinden. Dadurch koordiniert dieses Signalmolekül eine Vielzahl zellulärer Prozesse, angefangen bei der Regulierung von Ionenkanalaktivität über die Kontraktilität glatter- und quergestreifter Muskulatur bis hin zur Genexpression, Zellproliferation und Apoptose. Durch die pleiotropen Effekte, welche durch cAMP reguliert werden, stellt sich die Frage, wie GS-gekoppelte Rezeptoren Signalspezifität erreichen, obwohl sie ihre Funktion durch dieses eine Signalmolekül ausführen. Ursprünglich ging man von einer uneingeschränkten Diffusion und dadurch homogenen Verteilung von cAMP in der Zelle aus. Diese Vorstellung ist jedoch nicht mit der Signalisierungsspezifität von GPCRs vereinbar, da unter diesen Umständen cAMP unselektiv all seine Effektorproteine in der gesamten Zelle aktivieren könnte. Daher entstand die Hypothese der cAMP-Kompartimentierung, wobei die Zelle lokal begrenzte Bereiche mit hohen oder niedrigen cAMP Konzentrationen umfassen würde. Jedoch gab es bisher keinerlei Beweise für die Existenz und die molekulare Zusammensetzung mutmaßlicher Domänen. Folglich setzten wir uns als Ziel, hochkonzentrierte cAMP-Kompartimente in der Zelle zu lokalisieren, ihre räumliche Dimension aufzuklären und ihre Rolle zur Realisierung zellulärer Signalisierungsspezifität zu ermitteln. Im Rahmen der vorliegenden Studie setzten wir einen Förster resonance energy transfer (FRET)-basierten cAMP Sensor ein, fusionierten ihn mit dem humanen glucagone-like peptide 1 Rezeptor (hGLP1R) als Prototyp eines GS-koppelnden Rezeptors, um cAMP am Ursprung des Signals zu messen. Mittels dieser Sensoren weisen wir eine Rezeptor-umgebende begrenzte cAMP Domäne nach, welche eine erhöhte cAMP Konzenztration aufweist (Figure ‎3.10). Bei Stimulation des Rezeptors mit GLP1 Konzenztrationen beginnend bei 10 fM entsteht eine Rezeptordomäne mit lokal erhöhten cAMP Konzentrationen, welche getrennt von Plasmamembran und Cytosol ist. Wir zeigen, dass das hGLP1R-Kompartiment geschützt ist vor cAMP Signalen, welche an weiteren, unabhängigen GS-gekoppelten Rezeptoren ihren Ursprung haben (Figure ‎3.11). Um die räumliche Dimension dieser Domäne zu untersuchen, verwendeten wir Nanolinker der Länge 30- und 60 nm als Abstandhalter zwischen Rezeptor und Sensor (Figure ‎3.12) und zeigen dabei, dass sich die Domäne über eine Länge von 60 Nanometern erstreckt, wobei ein abnehmender cAMP-Gradient erkennbar ist. Weiterhin beweisen wir, dass Phosphodiesterasen (PDEs) Schlüsselfaktoren für die Bildung des cAMP-Gradienten um den Rezeptor herum sind, indem sie die Diffusion ins Cytosol beschränken (Figure ‎3.13). Darüber hinaus zeigen wir (Figure ‎3.15), dass Rezeptor-spezifische cAMP Signale PKA-Phosphorylierung in der Rezeptordomäne auslösen und, dass AKAPs elementar für nanodomänen PKA-Aktivität sind, wohingegen die cytosolische PKA-Phosphorylierung unabhängig von AKAP-Targeting der PKA ist (Figure ‎3.16). Zusammenfassend beweisen unsere Ergebnisse die Existenz einer Rezeptor-umgebenden Nanodomäne mit erhöhten cAMP Spiegeln eines GS-gekoppelten Rezeptors. Zeitgleiche Studien in unserer Gruppe zeigen, dass cAMP in der Zelle weitgehend gebunden vorliegt und diffusionslimitiert ist. Dies stellt den Nachweis für eine eingeschränkte Diffusion als molekulare Voraussetzung für die Bildung von Signalkompartimenten dar. Wir gehen davon aus, dass unsere Ergebnisse ein Ausgangspunkt für die Aufklärung von Rezeptoren als Quelle für Signalkompartimente darstellen, jedoch bedarf es weiterer Studien, um die präzise molekulare Zusammensetzung und die beteiligten Proteine dieser Signaldomäne zu untersuchen. Das Grundverständnis der Signalisierungskaskaden auf molekularer Ebene könnte es uns ermöglichen, die zellulären Reaktionen zu manipulieren, um eine Fehlfunktion der Signalisierung in erkrankten Zellen wiederherzustellen. Da der hGLP1R entscheidend für Aufrechterhaltung ausgeglichener Blutglucosespiegel ist, würde die Erfassung der molekularen Details der kompartimentalisierten Signalübertragung die Feinabstimmung der Rezeptorsignale ermöglichen, um ihn als spezifisches Target zur Behandlung von Diabetes Mellitus einzusetzen. KW - FRET KW - cAMP KW - compartments KW - GPCR Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190695 ER - TY - JOUR A1 - Arimany-Nardi, Cristina A1 - Minuesa, Gerard A1 - Pastor-Anglada, Marçal A1 - Keller, Thorsten A1 - Erkizia, Itziar A1 - Koepsell, Hermann A1 - Martinez-Picado, Javier T1 - Role of Human Organic Cation Transporter 1 (hOCT1) Polymorphisms in Lamivudine (3TC) Uptake and Drug-Drug Interactions JF - Frontiers in Pharmacology N2 - Lamivudine (3TC), a drug used in the treatment of HIV infection, needs to cross the plasma membrane to exert its therapeutic action. Human Organic cation transporter 1 (hOCT1), encoded by the SLC22A1 gene, is the transporter responsible for its uptake into target cells. As SLC22A1 is a highly polymorphic gene, the aim of this study was to determine how SNPs in the OCT1-encoding gene affected 3TC internalization and its interaction with other co-administered drugs. HEK293 cells stably transfected with either the wild type form or the polymorphic variants of hOCT1 were used to perform kinetic and drug-drug interaction studies. Protein co-immunoprecipitation was used to assess the impact of selected polymorphic cysteines on the oligomerization of the transporter. Results showed that 3TC transport efficiency was reduced in all polymorphic variants tested (R61C, C88R, S189L, M420del, and G465R). This was not caused by lack of oligomerization in case of variants located at the transporter extracellular loop (R61C and C88R). Drug-drug interaction measurements showed that co-administered drugs [abacavir (ABC), zidovudine (AZT), emtricitabine (FTC), tenofovir diproxil fumarate (TDF), efavirenz (EFV) and raltegravir (RAL)], differently inhibited 3TC uptake depending upon the polymorphic variant analyzed. These data highlight the need for accurate analysis of drug transporter polymorphic variants of clinical relevance, because polymorphisms can impact on substrate (3TC) translocation but even more importantly they can differentially affect drug-drug interactions at the transporter level. KW - hOCT1 KW - pharmacogenetics KW - lamivudine KW - HIV infection KW - therapy Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-165236 VL - 7 IS - 175 ER - TY - JOUR A1 - Awad, Eman A1 - Othman, Eman M. A1 - Stopper, Helga T1 - Effects of resveratrol, lovastatin and the mTOR-inhibitor RAD-001 on insulin-induced genomic damage in vitro JF - Molecules N2 - Diabetes mellitus (DM) is one of the major current health problems due to lifestyle changes. Before diagnosis and in the early years of disease, insulin blood levels are elevated. However, insulin generates low levels of reactive oxygen species (ROS) which are integral to the regulation of a variety of intracellular signaling pathways, but excess levels of insulin may also lead to DNA oxidation and DNA damage. Three pharmaceutical compounds, resveratrol, lovastatin and the mTOR-inhibitor RAD-001, were investigated due to their known beneficial effects. They showed protective properties against genotoxic damage and significantly reduced ROS after in vitro treatment of cultured cells with insulin. Therefore, the selected pharmaceuticals may be attractive candidates to be considered for support of DM therapy. KW - genomic damage KW - insulin KW - resveratrol KW - lovastatin KW - mTOR-inhibitor RAD-001 Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-159260 VL - 22 IS - 12 ER - TY - JOUR A1 - Baertsch, A. A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Effect of inhalation exposure regimen on DNA binding potency of 1,2-dichloroethane in the rat N2 - 1 ,2-Dichloroethane (DCE) was reported to be carcinogenic in rats in a long-tenn bioassay using gavage in com oil (24 and 48 mg/kg/day), but not by inhalation (up to 150-250 ppm, 7 h/day, 5 days/week). The daily dose metabolized was similar in the two experiments. In order to address this discrepancy, the genotoxicity of DCE was investigated in vivo under different exposure conditions. Fernale F-344 rats (183-188 g) were exposed to [1,2-14C]DCE in a closed inhalation chamber to either a low, constant concentration (0.3 mg/l = 80 ppm for 4 h) or to a peak concentration (up to 18 mg/1 = 4400 ppm) for a few minutes. After 12 h in the chamber, the dose metabolized under the two conditions was 34 mg/kg and 140 mg/k:g. DNA was isolated from liver and lung and was purified to constant specific radioactivity. DNA was enzymaticaBy hydrolyzed to the 3' -nucleotides which were separated by reverse phase HPLC. Most radioactivity eluted without detectable or with little optical density' indicating that the major part of the DNA radioactivity was due to covalent binding of the test compound. The Ievel of DNA adducts was expressed in the dose-nonnalized units ofthe Covalent Binding Index, CBI = f.Lmol adduct per mol DNA nucleotide/ mmol DCE per kg body wt. In liver DNA, the different exposure regimens resulted in markedly different CBI values of 1.8 and 69, for "constant-low" and ''peak" DCE exposure Ievels. In the Jung, the respective values were 0.9 and 31. It is concluded that the DNA darnage by DCE depends upon the concentration-time profile and that the carcinogenic potency determined in the gavage study should not be used for low-Ievel inhalation exposure. KW - Toxikologie KW - 1 KW - 2-Dichloroethane KW - Carcinogens KW - DNA KW - binding KW - Rat KW - Inhalation KW - Dose response Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60743 ER - TY - JOUR A1 - Balasubramanian, Srikkanth A1 - Othman, Eman M. A1 - Kampik, Daniel A1 - Stopper, Helga A1 - Hentschel, Ute A1 - Ziebuhr, Wilma A1 - Oelschlaeger, Tobias A. A1 - Abdelmohsen, Usama R. T1 - Marine sponge-derived Streptomyces sp SBT343 extract inhibits staphylococcal biofilm formation JF - Frontiers in Microbiology N2 - Staphylococcus epidermidis and Staphylococcus aureus are opportunistic pathogens that cause nosocomial and chronic biofilm-associated infections. Indwelling medical devices and contact lenses are ideal ecological niches for formation of staphylococcal biofilms. Bacteria within biofilms are known to display reduced susceptibilities to antimicrobials and are protected from the host immune system. High rates of acquired antibiotic resistances in staphylococci and other biofilm-forming bacteria further hamper treatment options and highlight the need for new anti-biofilm strategies. Here, we aimed to evaluate the potential of marine sponge-derived actinomycetes in inhibiting biofilm formation of several strains of S. epidermidis, S. aureus, and Pseudomonas aeruginosa. Results from in vitro biofilm-formation assays, as well as scanning electron and confocal microscopy, revealed that an organic extract derived from the marine sponge-associated bacterium Streptomyces sp. SBT343 significantly inhibited staphylococcal biofilm formation on polystyrene, glass and contact lens surfaces, without affecting bacterial growth. The extract also displayed similar antagonistic effects towards the biofilm formation of other S. epidermidis and S. aureus strains tested but had no inhibitory effects towards Pseudomonas biofilms. Interestingly the extract, at lower effective concentrations, did not exhibit cytotoxic effects on mouse fibroblast, macrophage and human corneal epithelial cell lines. Chemical analysis by High Resolution Fourier Transform Mass Spectrometry (HRMS) of the Streptomyces sp. SBT343 extract proportion revealed its chemical richness and complexity. Preliminary physico-chemical characterization of the extract highlighted the heat-stable and non-proteinaceous nature of the active component(s). The combined data suggest that the Streptomyces sp. SBT343 extract selectively inhibits staphylococcal biofilm formation without interfering with bacterial cell viability. Due to absence of cell toxicity, the extract might represent a good starting material to develop a future remedy to block staphylococcal biofilm formation on contact lenses and thereby to prevent intractable contact lens-mediated ocular infections. KW - medicine KW - marine sponges KW - actinomycetes KW - Streptomyces KW - staphilococci KW - biofilms KW - contact lens Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171844 VL - 8 ER - TY - JOUR A1 - Banach, Katrin A1 - Bünemann, Moritz A1 - Hüser, Jörg A1 - Pott, Lutz T1 - Serum contains a potent factor that decreases \(\beta\)-adrenergic receptor-stimulated L-type Ca\(^{2+}\) current in cardiac myocytes N2 - No abstract available KW - Cardiac myocyte ; Beta-Receptor ; Muscarinic receptor ; cAMP ; G-protein ; Serum Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-32027 ER - TY - JOUR A1 - Bankoglu, Ezgi Eyluel A1 - Arnold, Charlotte A1 - Hering, Ilona A1 - Hankir, Mohammed A1 - Seyfried, Florian A1 - Stopper, Helga T1 - Decreased chromosomal damage in lymphocytes of obese patients after bariatric surgery JF - Scientific Reports N2 - The number of bariatric surgeries being performed worldwide has markedly risen. While the improvement in obesity-associated comorbidities after bariatric surgery is well-established, very little is known about its impact on cancer risk. The peripheral lymphocyte micronucleus test is a widely used method for the monitoring of chromosomal damage levels in vivo, and micronucleus frequency positively correlates with cancer risk. Therefore, the aim of this study was to compare the micronucleus frequency before and after bariatric surgery in obese subjects. Peripheral blood mononuclear cells were collected from 45 obese subjects before and at two time-points after bariatric surgery (6 and 12 months) to assess spontaneous micronucleus frequency. Consistent with the increased cancer risk previously shown, bariatric surgery-induced weight loss led to a significant reduction in lymphocyte micronucleus frequency after 12 months. Interestingly, comorbidities such as type 2 diabetes mellitus and metabolic syndrome further seemed to have an impact on the lymphocyte micronucleus frequency. Our findings may indicate a successful reduction of cancer risk in patients following weight loss caused by bariatric surgery. KW - obesity KW - bariatric surgery KW - cancer risk Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-177090 VL - 8 IS - 11195 ER - TY - JOUR A1 - Bankoglu, Ezgi Eyluel A1 - Schuele, Carolin A1 - Stopper, Helga T1 - Cell survival after DNA damage in the comet assay JF - Archives of Toxicology N2 - The comet assay is widely used in basic research, genotoxicity testing, and human biomonitoring. However, interpretation of the comet assay data might benefit from a better understanding of the future fate of a cell with DNA damage. DNA damage is in principle repairable, or if extensive, can lead to cell death. Here, we have correlated the maximally induced DNA damage with three test substances in TK6 cells with the survival of the cells. For this, we selected hydrogen peroxide (H\(_{2}\)O\(_{2}\)) as an oxidizing agent, methyl methanesulfonate (MMS) as an alkylating agent and etoposide as a topoisomerase II inhibitor. We measured cell viability, cell proliferation, apoptosis, and micronucleus frequency on the following day, in the same cell culture, which had been analyzed in the comet assay. After treatment, a concentration dependent increase in DNA damage and in the percentage of non-vital and apoptotic cells was found for each substance. Values greater than 20-30% DNA in tail caused the death of more than 50% of the cells, with etoposide causing slightly more cell death than H\(_{2}\)O\(_{2}\) or MMS. Despite that, cells seemed to repair of at least some DNA damage within few hours after substance removal. Overall, the reduction of DNA damage over time is due to both DNA repair and death of heavily damaged cells. We recommend that in experiments with induction of DNA damage of more than 20% DNA in tail, survival data for the cells are provided. KW - Cell death and comet assay KW - DNA damage KW - DNA repair Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-265339 VL - 95 IS - 12 ER - TY - JOUR A1 - Bankoglu, Ezgi Eyluel A1 - Stipp, Franzisca A1 - Gerber, Johanna A1 - Seyfried, Florian A1 - Heidland, August A1 - Bahner, Udo A1 - Stopper, Helga T1 - Effect of cryopreservation on DNA damage and DNA repair activity in human blood samples in the comet assay JF - Archives of Toxicology N2 - The comet assay is a commonly used method to determine DNA damage and repair activity in many types of samples. In recent years, the use of the comet assay in human biomonitoring became highly attractive due to its various modified versions, which may be useful to determine individual susceptibility in blood samples. However, in human biomonitoring studies, working with large sample numbers that are acquired over an extended time period requires some additional considerations. One of the most important issues is the storage of samples and its effect on the outcome of the comet assay. Another important question is the suitability of different blood preparations. In this study, we analysed the effect of cryopreservation on DNA damage and repair activity in human blood samples. In addition, we investigated the suitability of different blood preparations. The alkaline and FPG as well as two different types of repair comet assay and an in vitro hydrogen peroxide challenge were applied. Our results confirmed that cryopreserved blood preparations are suitable for investigating DNA damage in the alkaline and FPG comet assay in whole blood, buffy coat and PBMCs. Ex vivo hydrogen peroxide challenge yielded its optimal effect in isolated PBMCs. The utilised repair comet assay with either UVC or hydrogen peroxide-induced lesions and an aphidicolin block worked well in fresh PBMCs. Cryopreserved PBMCs could not be used immediately after thawing. However, a 16-h recovery with or without mitotic stimulation enabled the application of the repair comet assay, albeit only in a surviving cell fraction. KW - human biomonitoring KW - DNA damage KW - DNA repair KW - comet assay KW - blood samples Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-265326 VL - 95 IS - 5 ER - TY - JOUR A1 - Bankoglu, Ezgi Eyluel A1 - Tschopp, Oliver A1 - Schmitt, Johannes A1 - Burkard, Philipp A1 - Jahn, Daniel A1 - Geier, Andreas A1 - Stopper, Helga T1 - Role of PTEN in Oxidative Stress and DNA Damage in the Liver of Whole-Body Pten Haplodeficient Mice JF - PLoS One N2 - Type 2 diabetes (T2DM) and obesity are frequently associated with non-alcoholic fatty liver disease (NAFLD) and with an elevated cancer incidence. The molecular mechanisms of carcinogenesis in this context are only partially understood. High blood insulin levels are typical in early T2DM and excessive insulin can cause elevated reactive oxygen species (ROS) production and genomic instability. ROS are important for various cellular functions in signaling and host defense. However, elevated ROS formation is thought to be involved in cancer induction. In the molecular events from insulin receptor binding to genomic damage, some signaling steps have been identified, pointing at the PI3K/AKT pathway. For further elucidation Phosphatase and Tensin homolog (Pten), a tumour suppressor phosphatase that plays a role in insulin signaling by negative regulation of PI3K/AKT and its downstream targets, was investigated here. Dihydroethidium (DHE) staining was used to detect ROS formation in immortalized human hepatocytes. Comet assay and micronucleus test were performed to investigate genomic damage in vitro. In liver samples, DHE staining and western blot detection of HSP70 and HO-1 were performed to evaluate oxidative stress response. DNA double strand breaks (DSBs) were detected by immunohistostaining. Inhibition of PTEN with the pharmacologic inhibitor VO-OHpic resulted in increased ROS production and genomic damage in a liver cell line. Knockdown of Pten in a mouse model yielded increased oxidative stress levels, detected by ROS levels and expression of the two stress-proteins HSP70 and HO-1 and elevated genomic damage in the liver, which was significant in mice fed with a high fat diet. We conclude that PTEN is involved in oxidative stress and genomic damage induction in vitro and that this may also explain the in vivo observations. This further supports the hypothesis that the PI3K/AKT pathway is responsible for damaging effects of high levels of insulin. KW - insulin KW - mouse models DNA damage KW - oxidative stress KW - mammalian genomics KW - fatty liver KW - micronuclei KW - insulin signaling Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146970 VL - 11 IS - 11 ER - TY - JOUR A1 - Barile, Frank A. A1 - Berry, Colin A1 - Blaauboer, Bas A1 - Boobis, Alan A1 - Bolt, Herrmann M. A1 - Borgert, Christopher A1 - Dekant, Wolfgang A1 - Dietrich, Daniel A1 - Domingo, Jose L. A1 - Galli, Corrado L. A1 - Gori, Gio Batta A1 - Greim, Helmut A1 - Hengstler, Jan G. A1 - Heslop-Harrison, Pat A1 - Kacew, Sam A1 - Marquardt, Hans A1 - Mally, Angela A1 - Pelkonen, Olavi A1 - Savolainen, Kai A1 - Testai, Emanuela A1 - Tsatsakis, Aristides A1 - Vermeulen, Nico P. T1 - The EU chemicals strategy for sustainability: in support of the BfR position JF - Archives of Toxicology N2 - The EU chemicals strategy for sustainability (CSS) asserts that both human health and the environment are presently threatened and that further regulation is necessary. In a recent Guest Editorial, members of the German competent authority for risk assessment, the BfR, raised concerns about the scientific justification for this strategy. The complexity and interdependence of the networks of regulation of chemical substances have ensured that public health and wellbeing in the EU have continuously improved. A continuous process of improvement in consumer protection is clearly desirable but any initiative directed towards this objective must be based on scientific knowledge. It must not confound risk with other factors in determining policy. This conclusion is fully supported in the present Commentary including the request to improve both, data collection and the time-consuming and bureaucratic procedures that delay the publication of regulations. KW - pharmacology/toxicology KW - occupational medicine/industrial medicine KW - environmental health KW - biomedicine, general Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-307154 SN - 0340-5761 SN - 1432-0738 VL - 95 IS - 9 ER - TY - THES A1 - Bathe-Peters, Marc T1 - Spectroscopic approaches for the localization and dynamics of β\(_1\)- and β\(_2\)-adrenergic receptors in cardiomyocytes T1 - Spektroskopieansätze zur Bestimmung der Lokalisation und Dynamiken von β\(_1\)- und β\(_2\)-Adrenozeptoren in Kardiomyozyten N2 - In the heart the β\(_1\)-adrenergic receptor (AR) and the β\(_2\)-AR, two prototypical G protein-coupled receptors (GPCRs), are both activated by the same hormones, namely adrenaline and noradrenaline. Both receptors couple to stimulatory G\(_s\) proteins, mediate an increase in cyclic adenosine monophosphate (cAMP) and influence the contractility and frequency of the heart upon stimulation. However, activation of the β\(_1\)-AR, not the β\(_2\)-AR, lead to other additional effects, such as changes in gene transcription resulting in cardiac hypertrophy, leading to speculations on how distinct effects can arise from receptors coupled to the same downstream signaling pathway. In this thesis the question of whether this distinct behavior may originate from a differential localization of these two receptors in adult cardiomyocytes is addressed. Therefore, fluorescence spectroscopy tools are developed and implemented in order to elucidate the presence and dynamics of these endogenous receptors at the outer plasma membrane as well as on the T-tubular network of intact adult cardiomyocytes. This allows the visualization of confined localization and diffusion of the β\(_2\)-AR to the T-tubular network at endogenous expression. In contrast, the β\(_1\)-AR is found diffusing at both the outer plasma membrane and the T-tubules. Upon overexpression of the β\(_2\)-AR in adult transgenic cardiomyocytes, the receptors experience a loss of this compartmentalization and are also found at the cell surface. These data suggest that distinct signaling and functional effects can be controlled by specific cell surface targeting of the receptor subtypes. The tools at the basis of this thesis work are a fluorescent adrenergic antagonist in combination of fluorescence fluctuation spectroscopy to monitor the localization and dynamics of the lowly expressed adrenergic receptors. Along the way to optimizing these approaches, I worked on combining widefield and confocal imaging in one setup, as well as implementing a stable autofocus mechanism using electrically tunable lenses. N2 - Im Herzen werden der β\(_1\)-adrenerge Rezeptor (AR) und der β\(_2\)-AR, zwei prototypische GPCR, durch die Hormone Adrenalin und Noradrenalin aktiviert. Dabei interagieren beide Rezeptoren mit dem stimulatorischen G\(_s\) Protein, bewirken eine Erhöhung des cyclischen Adenosinmonophosphates (cAMP) und beeinflussen die Kontraktionskraft und Frequenz des Herzens nach einem Stimulus. Jedoch hat die Aktivierung des β\(_1\)-ARs, nicht des β\(_2\)-ARs, auch weitere Effekte, wie z.B. Veränderungen in der Transkription von Genen. Dies wiederum führt zu Spekulationen, wie solch unterschiedliche Effekte von Rezeptoren hervorgerufen werden können, die gleiche Signalwege bedienen. In dieser Arbeit wird untersucht, ob dieses unterschiedliche Verhalten durch eine ungleiche Verteilung dieser beiden Rezeptoren in adulten Kardiomyozyten hervorgerufen werden könnte. Dazu wird die Lokalisation und die Dynamik dieser endogenen Rezeptoren in der Plasmamembran sowie im T-tubulären Netzwerk von intakten adulten Kardiomyozyten, unter Entwicklung und Verwendung hochsensitiver Fluoreszenzspektroskopiemethoden, bestimmt. Dies ermöglicht die örtliche und dynamische Eingrenzung des β\(_2\)-adrenergen Rezeptors unter endogener Expression ausschließlich auf das T-tubuläre Netzwerk. Dementgegen stellt sich heraus, dass sich der β\(_1\)-adrenerge Rezeptor ubiquitär auf der äußeren Membran und den T-Tubuli befindet und diffundiert. In β\(_2\)-AR überexprimierenden transgenen Kardiomyozyten hingegen werden diese Kompartments nicht beibehalten und es findet eine Umverteilung der Rezeptoren, auch unter Einbezug der Zelloberfläche, statt. Diese Daten können stärker darauf hindeuten, dass einige Rezeptorsubtypen sich gezielt und spezifisch bestimmte Zelloberflächen aussuchen, um somit ihre verschiedenen Signale und funktionären Effekte erzeugen zu können. Zu den Techniken, die in dieser Arbeit die Bestimmung der Lokalisation und der Dynamiken der niedrig exprimierten adrenergen Rezeptoren zulassen, gehört die Anwendung von Fluoreszenzspektroskopiemethoden in Kombination mit einem fluoreszierenden β-adrenergen Antagonisten. Weitere Techniken, die im Rahmen dieser Arbeit entwickelt wurden und in weiterführenden Studien aufschlussreiche Erkenntnisse liefern könnten, umfassen die Entwicklung eines Setups aus einer Kombination aus Weitfeld- und Konfokalmikroskopie und die Implementierung eines stabilen Autofokus mit Hilfe einer elektrisch veränderbaren Linse. KW - G-Protein gekoppelte Rezeptoren KW - Beta-Adrenozeptor KW - Kardiomyozyt KW - Fluoreszenzmikroskopie KW - Fluoreszenzkorrelationsspektroskopie KW - Fluorescence KW - Fluorescence Microscopy KW - G Protein-Coupled Receptor KW - Autofocus KW - Microscopy KW - Beta-Adrenergic Receptor KW - Cardiomyocyte KW - Fluorescence Correlation Spectroscopy KW - FCS KW - GPCR Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-258126 ER - TY - JOUR A1 - Bauer, Benedikt A1 - Mally, Angela A1 - Liedtke, Daniel T1 - Zebrafish embryos and larvae as alternative animal models for toxicity testing JF - International Journal of Molecular Sciences N2 - Prerequisite to any biological laboratory assay employing living animals is consideration about its necessity, feasibility, ethics and the potential harm caused during an experiment. The imperative of these thoughts has led to the formulation of the 3R-principle, which today is a pivotal scientific standard of animal experimentation worldwide. The rising amount of laboratory investigations utilizing living animals throughout the last decades, either for regulatory concerns or for basic science, demands the development of alternative methods in accordance with 3R to help reduce experiments in mammals. This demand has resulted in investigation of additional vertebrate species displaying favourable biological properties. One prominent species among these is the zebrafish (Danio rerio), as these small laboratory ray-finned fish are well established in science today and feature outstanding biological characteristics. In this review, we highlight the advantages and general prerequisites of zebrafish embryos and larvae before free-feeding stages for toxicological testing, with a particular focus on cardio-, neuro, hepato- and nephrotoxicity. Furthermore, we discuss toxicokinetics, current advances in utilizing zebrafish for organ toxicity testing and highlight how advanced laboratory methods (such as automation, advanced imaging and genetic techniques) can refine future toxicological studies in this species. KW - danio rerio KW - alternative methods KW - organ toxicity KW - 3R KW - transgenic animals Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284225 SN - 1422-0067 VL - 22 IS - 24 ER - TY - THES A1 - Bayer, Tanja T1 - Toxicity and biotransformation of 1,1,1,3,3-Pentafluoropropane, 3,3,3-Trifluoropropionic acid and 1,1,1,3-Tetrachloropropane T1 - Toxizität und Biotransformation von 1,1,1,3,3-Pentafluorpropan, 3,3,3-Trifluorpropionsäure und 1,1,1,3-Tetrachlorpropan N2 - The biotransformation of 1,1,1,3,3-pentafluoropropane was investigated in rats and in in vitro systems. First, the metabolites were identified in vivo using GC/MS and 19F NMR analysis. The main metabolite was identified as trifluoroacetic acid, the minor metabolite as 3,3,3-trifluoropropionic acid and as a cleavage product, inorganic fluoride was found. As the in vitro system, liver microsomes from rat and human samples and rat liver homogenates were used. Trifluoroacetic acid and 3,3,3 trifluoropropionic acid were confirmed in vitro as metabolic intermediates, following biotransformation of 1,1,1,3,3-pentafluoropropane by the cytochrome P-450-system. Studies, designed for clarifying the cardiotoxicity of 1,1,1,3,3-pentafluoropropane were driven by the hypothesis that 3,3,3-trifluoropropionic acid is the toxic agent. This was based on the lethal toxicity, which was observed in previous in vivo experiments. In addition, the point of its structural similarity to toxic agents as for example monofluoroacetic acid or of possible metabolic intermediates like difluoroacrylic acid with known toxicity were considered to support this assumption. However, trifluoroacetic acid was neglected as the sought-after toxic agent because of its different toxic effects, known from literature. Investigations on the biotransformation of 3,3,3-trifluoropropionic acid were performed and resulted in no metabolic activity and in poor elimination of 3,3,3-trifluoropropionic acid in vivo. The histopathological effects on the heart, which were observed in the 90-day oral toxicity study of 1,1,1,3,3-pentafluoropropane in rats, namely mononuclear inflammatory cell infiltrations and degenerated myocardial fibers, were not observed after a 28 day repeated exposure of up to 10 mg/kg b.w. of 3,3,3-trifluoropropionic acid. However, a single high dose of 3,3,3-trifluoropropionic acid lead to severe toxicological effects. The difference in the observed toxic effects after a single and repeated administration may be due to adaptive mechanisms in rats. The toxicological effects included clinical signs like ataxia, coma and cramps. The conditions of the rats suggested possible inhibition of the energy supply to the organism. Furthermore, the interference of 3,3,3-trifluoropropionic acid in the functionality of the organism was investigated. Experiments were performed in vitro in rat liver and heart mitochondria to investigate effects on the mitochondrial ß-oxidation. However, the transformation of the substrate [U14C] palmitic acid in the ß oxidation pathway was not inhibited by 3,3,3-trifluoropropionic acid. In addition, no cytotoxicity of 3,3,3 trifluoropropionic acid was observed in the cell culture systems. The main effect after a single dose of 3,3,3-trifluoropropionic acid was seen in clinical pathology and metabonomic analysis. The decrease in blood glucose is considered to have the most far-reaching consequences for the toxicity of 3,3,3-trifluoropropionic acid. If considering this change as the primary effect after a single dose, secondary effects, for example, the above-mentioned clinical signs could be explained. In addition, the observed high level of ketone bodies might have been responsible for life-threatening possible ketoacidosis. In general, ketoacidosis occurs after an imbalance between glycolysis, lipolysis, TCA cycle activity and respiratory function. Based on the results, ß-oxidation of fatty acids was not affected, and due to the decrease in glucose levels and the high levels of acetyl CoA, glycolysis was considered not to be impaired. Increased amounts of acetyl CoA might be a result of insufficient activity of the TCA cycle. However, the inhibition of the TCA cycle can be based on the impairment of specific enzymes and/or on the involvement of messenger substrates like insulin. Supporting the first mentioned aspect are decreased levels of TCA cycle intermediates, like α-ketoglutarate or citrate, as seen in 1H-NMR spectra of urine. However, the second aspect would explain the drop in blood glucose with the impairment of glucose transporters or the impairment of the insulin balance. If a single dose of 3,3,3-trifluoropropionic acid had stimulated the insulin release, glycolysis would be activated, and high amounts of acetyl CoA would be produced. In case of impaired use by the TCA cycle, levels of ketone bodies would be increased. Experiments were designed to characterize the direct effect of 3,3,3-trifluoropropionic acid on rat insulinoma-derived INS-1 cells as possible increase in insulin release. Further investigations are necessary to answer in which step of the metabolic pathway 3,3,3-trifluoropropionic acid interferes or finally which specific enzyme is inhibited or activated by 3,3,3-trifluoropropionic acid, leading to the drop in blood glucose and finally in lethal toxicity. N2 - Die Biotransformation von 1,1,1,3,3-Pentafluorpropan wurde in Ratten und in in vitro Systemen untersucht. Die in der Ratte mit dem Urin ausgeschiedenen Metabolite wurden per GC/MS und 19F-NMR identifiziert. Als Hauptmetabolit entstand Trifluoressigsäure, als Nebenmetabolit 3,3,3-Trifluorpropionsäure und als Abspaltungsprodukt Fluorid. Als in in vitro Systeme wurden Ratten- und Humanleber-mikrosomen, sowie Rattenleberhomogenate verwendet. Auch hier wurden Trifluoressigsäure und 3,3,3-Trifluorpropionsäure als metabolische Zwischenprodukte identifiziert. Weitere in vivo Studien wurden durchgeführt um die beobachtete subchronische Kardiotoxizität von 1,1,1,3,3-Pentafluorpropan zu erklären. Da vorangegangene Experimente eine hohe letale Toxizität des Metaboliten 3,3,3-Trifluorpropionsäure zeigten, wurde dieser als das toxische Agens hypothetisiert. Diese Annahme unterstützend, ist dessen strukturelle Ähnlichkeit zu Substanzen mit bekannten toxischen Profilen wie Monofluoressigsäure oder Difluoracrylsäure, ein mögliches entstehendes Intermediat. Der Hauptmetabolit Trifluoressigsäure jedoch, wurde auf Grund seiner bekannten Toxizität als initiierendes Agens der Kardiotoxizität ausgeschlossen. In vivo Untersuchungen mit 3,3,3-Trifluorpropionsäure zeigten jedoch keine weitere metabolische Aktivität und eine geringe renale Ausscheidung an 3,3,3-Trifluorpropionsäure. Nach einer einmalig hohen Dosis von 3,3,3-Trifluorpropionsäure traten markante Symptome wie Ataxie, komatöse Zustände und Krämpfe auf. Dies deutete auf eine Beeinträchtigung des Energiezustandes des Organismus hin. Die histo-pathologischen Veränderungen des Herzens, mononukleäre Infiltrate von Entzündungszellen und degenerierte Myokard-Fasern, die für 1,1,1,3,3-Pentafluorpropan in einer 90-Tages Studie in Nagern beobachtet wurden, konnten jedoch nicht nach 28-tägiger Exposition mit 10 mg/kg Körpergewicht 3,3,3-Trifluorpropionsäure beobachtet werden. Die unterschiedlichen Effekte die nach einmaliger und wiederholter Gabe beobachtet wurden, lassen sich durch mögliche Adaptionsprozesse erklären, die initiale Schädigungen kompensieren. Die folgenden Experimente waren auf die funktionelle Beeinflussung des Organismus durch 3,3,3-Trifluorpropionsäure ausgerichtet. In vitro Untersuchungen in Mitochondrien von Rattenleber und –herz mit dem Umsatz des Modellsubstrates [U14C] Palmitinsäure zeigten jedoch keine Inhibierung der ß-Oxidation durch 3,3,3-Trifluorpropionsäure. Zytotoxizitätsassays wurden im Weiteren in der human-hepatonom Zell-Linie HepG2, und in der kardialen Muskelzell-Linie H9C2 mit folgenden Endpunkten durchgeführt: die Freisetzung von LDH, ein Parameter für die Membranintegrität, die MTT Reduktase Aktivität, ein Parameter für die metabolische Aktivität, und die Messung von Kristallviolett, ein Parameter für die Viabilität von Zellen. Für 3,3,3-Trifluorpropionsäure konnte jedoch keine Zytotoxizität beobachtet werden. Deutliche Effekte wurden hingegen in der klinischen Pathologie und anhand Metabonomics beobachtet. Diese bestanden vor allem in der Abnahme der Glukosekonzentration im Blut, das weitreichende Konsequenzen mit sich führt, und als primärer Effekt die sekundären Effekte wie die beobachtenden klinischen Symptome erklären könnte. Ein weiterer Schlüsselparameter war die Erhöhung von Ketonkörpern in Urin und Serum, welche für eine lebensbedrohliche mögliche Ketoazidosis verantwortlich sein kann und durch ein Ungleichgewicht im Energiehaushalt ausgelöst werden kann. Da eine Beeinträchtigung der ß Oxidation und der Glykolyse ausgeschlossen wurde, könnte das erhöhte Vorkommen von Acetyl-CoA auf eine limitierte Aktivität des Zitronensäurezyklus hindeuten. Grund hierfür kann die Inhibierung von beteiligten Enzymen sein oder auch der Einfluß von Messenger-Substraten wie Insulin. Ersteres wurde untermauert mit der Beobachtung in 1H NMR Spektren von Urin mit erhöhten Mengen an Intermediaten des Zitronensäurezyklus, wie α Ketoglutarate oder Zitrat. Letzteres würde den Abfall der Blutglukose, basierend auf Beeinflussung von Glukosetransportern oder des Insulinhaushaltes, erklären. Wenn 3,3,3-Trifluorpropionsäure die Freisetzung von Insulin stimulieren würde, würde der Abbau von Glukose aktiviert werden und erhöhte Mengen an Acetyl-CoA resultieren. Wenn gleichzeitig eine Beeinträchtigung des Zitronensäurezyklus vorliegt, kann dies zu einer Erhöhung an Ketonkörpern führen. Experimente zur Messung des Insulin- und Glukosespiegels wurden in vivo und in vitro mit der Ratteninsulinoma Zell-Linie INS-1 durchgeführt, um den Effekt von 3,3,3-Trifluorpropionsäure auf die Freisetzung von Insulin zu charakterisieren. Basierend auf diesen Ergebnissen sind weitere Untersuchungen erforderlich um den Metabolismus von 3,3,3-Trifluorpropionsäure, sowie dessen mögliche Interaktion mit Enzymen oder Rezeptoren aufzuklären, und um den raschen Glukoseabfall im Blut zu erklären, der zu einer letalen Toxizität führen kann KW - Fluorkohlenwasserstoffe KW - Biotransformation KW - Biotransformation KW - Fluorkohlenwasserstoffe KW - Metabonomix KW - HFC245fa KW - Trifluorpropionsäure KW - biotransformation KW - hydrofluorocarbons KW - metabonomics KW - HFC245fa KW - trifluoropropionic acid Y1 - 2005 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-15731 ER - TY - THES A1 - Bellwon, Patricia T1 - Kinetic assessment by in vitro approaches - A contribution to reduce animals in toxicity testing T1 - Evaluierung der Kinetik anhand von in vitro Systemen - Ein Beitrag um die Anzahl von Tierversuchen zur Toxizitätsprüfung zu reduzieren N2 - The adoption of directives and regulations by the EU requires the development of alternative testing strategies as opposed to animal testing for risk assessment of xenobiotics. Additionally, high attrition rates of drugs late in the discovery phase demand improvement of current test batteries applied in the preclinical phase within the pharmaceutical area. These issues were taken up by the EU founded 7th Framework Program “Predict-IV”; with the overall goal to improve the predictability of safety of an investigational product, after repeated exposure, by integration of “omics” technologies applied on well established in vitro approaches. Three major target organs for drug-induced toxicity were in focus: liver, kidney and central nervous system. To relate obtained dynamic data with the in vivo situation, kinetics of the test compounds have to be evaluated and extrapolated by physiologically based pharmacokinetic modeling. This thesis assessed in vitro kinetics of the selected test compounds (cyclosporine A, adefovir dipivoxil and cisplatinum) regarding their reliability and relevance to respective in vivo pharmacokinetics. Cells were exposed daily or every other day to the test compounds at two concentration levels (toxic and non-toxic) for up to 14 days. Concentrations of the test compounds or their major biotransformation products were determined by LC-MS/MS or ICP-MS in vehicle, media, cells and plastic adsorption samples generated at five different time-points on the first and the last treatment day. Cyclosporine A bioaccumulation was evident in primary rat hepatocytes (PRH) at the high concentration, while efficient biotransformation mediated by CYP3A4 and CYP3A5 was determined in primary human hepatocytes (PHH) and HepaRG cells. The lower biotransformation in PRH is in accordance with observation made in vivo with the rat being a poor model for CYP3A biotransformation. Further, inter-assay variability was noticed in PHH caused by biological variability in CYP3A4 and CYP3A5 activity in human donors. The inter-assay variability observed for PRH and HepaRG cells was a result of differences between vehicles regarding their cyclosporine A content. Cyclosporine A biotransformation was more prominent in HepaRG cells due to stable and high CYP3A4 and CYP3A5 activity. In addition, in vitro clearances were calculated and scaled to in vivo. All scaled in vitro clearances were overestimated (PRH: 10-fold, PHH: 2-fold, HepaRG cells: 2-fold). These results should be proven by physiologically-based pharmacokinetic modeling and additional experiments, in order to verify that these overestimations are constant for each system and subsequently can be diminished by implementation of further scaling factors. Brain cell cultures, primary neuronal culture of mouse cortex cells and primary aggregating rat brain cells, revealed fast achieved steady state levels of cyclosporine A. This indicates a chemical distribution of cyclosporine A between the aqueous and organic phases and only minor involvement of biological processes such as active transport and biotransformation. Hence, cyclosporine A uptake into cells is presumably transport mediated, supported by findings of transporter experiments performed on a parallel artificial membrane and Caco-2 cells. Plastic adsorption of cyclosporine A was significant, but different for each model, and should be considered by physiologically based pharmacokinetic modeling. Kinetics of adefovir dipivoxil highlights the limits of in vitro approaches. Active transporters are required for adefovir uptake, but were not functional in RPTECT/TERT1. Therefore, adefovir uptake was limited to passive diffusion of adefovir dipivoxil, which itself degrades time-dependently under culture conditions. Cisplatinum kinetics, studied in RPTEC/TERT1 cells, indicated intracellular enrichment of platinum, while significant bioaccumulation was not noted. This could be due to cisplatinum not reaching steady state levels within 14 days repeated exposure. As shown in vivo, active transport occurred from the basolateral to apical side, but with lower velocity. Hence, obtained data need to be modeled to estimate cellular processes, which can be scaled and compared to in vivo. Repeated daily exposure to two different drug concentrations makes it possible to account for bioaccumulation at toxic concentrations or biotransformation/extrusion at non-toxic concentrations. Potential errors leading to misinterpretation of data were reduced by analyses of the vehicles as the applied drug concentrations do not necessarily correspond to the nominal concentrations. Finally, analyses of separate compartments (medium, cells, plastic) give insights into a compound’s distribution, reduce misprediction of cellular processes, e.g. biotransformation, and help to interpret kinetic data. On the other hand, the limits of in vitro approaches have also been pointed out. For correct extrapolation to in vivo, it is essential that the studied in vitro system exhibits the functionality of proteins, which play a key role in the specific drug induced toxicity. Considering the benefits and limitations, it is worth to validate this long-term treatment experimental set-up and expand it on co-culture systems and on organs-on-chips with regard to alternative toxicity testing strategies for repeated dose toxicity studies. N2 - Die Erlassung von Richtlinien und Verordnungen durch die EU führte zu der Entwicklung von alternativen Testmethoden als Ersatz von Tierversuchen zur Risikobewertung von Xenobiotika. Des Weiteren weisen hohe Ausfallraten von Arzneimitteln in der späten Entwicklungsphase auf die Notwendigkeit hin, die bisher verwendeten Testmethoden der präklinischen Phase zu verbessern. Diese Punkte wurden in dem im siebten Rahmenprogramm der EU finanzierten Projekt „Predict-IV“ aufgegriffen. Ziel des Projektes war es, die Vorhersage der Arzneimittelsicherheit durch integrierte „omics“-Technologien, angewendet an etablierten in vitro Ansätzen, zu verbessern. Dabei standen drei Zielorgane bzgl. Arzneimittel-induzierter Organtoxizität im Mittelpunkt: Leber, Niere und zentrales Nervensystem, die jeweils durch Zelllinien oder primäre Zellen vertreten waren. Um die in vitro generierten Dynamik-Daten mit der in vivo Situation in Korrelation zu bringen, muss die Kinetik der Testsubstanz berücksichtigt und die Ergebnisse mit Hilfe von physiologisch-basierter pharmakokinetischer Modellierung extrapoliert werden. Ziel der vorliegenden Arbeit war es, Kinetik-Daten der gewählten Testsubstanzen (Cyclosporin A, Adefovir dipivoxil und Cisplatin) in vitro zu erheben und bzgl. ihrer Zuverlässigkeit sowie ihrer Relevanz verglichen mit in vivo Daten zu beurteilen. Hierfür wurden kultivierte Zellen täglich bzw. jeden zweiten Tag für zwei Wochen mit zwei verschiedenen Konzentrationen (toxisch und nicht toxisch) des Arzneimittels behandelt. Der Gehalt des applizierten Arzneimittels oder die Hauptmetaboliten wurden mittels LC MS/MS oder ICP-MS in Vehikel, Medium und Zellen sowie die vom Plastik adsorbierte Menge in Proben bestimmt, die am ersten und letzten Behandlungstag zu fünf unterschiedlichen Zeitpunkten gewonnen wurden. Eine eindeutige Bioakkumulation von Cyclosporin A wurde in primären Rattenhepatozyten nach Behandlung mit der hohen Konzentration festgestellt. Eine effiziente CYP3A4- und CYP3A5-vermittelte Biotransformation von Cyclosporin A wurde für primäre humane Hepatozyten sowie HepaRG Zellen beobachtet. Diese Ergebnisse stimmten mit der in vivo Situation überein. Ratten sind aufgrund ihrer geringen CYP3A Aktivität schlechte Tiermodelle für CYP3A-Biotransformationsstudien. Des Weiteren wurden Interassay-Schwankungen bei primären human Hepatozyten bemerkt, die auf die biologische Variabilität der CYP3A4- sowie CYP3A5-Aktivität zwischen den menschlichen Spendern zurückzuführen sind. Rattenhepatozyten und HepaRG Zellen hingegen wiesen Interassay-Schwankungen auf, die durch unterschiedliche Cyclosporin A Behandlungskonzentrationen zwischen den Replikaten verursacht wurden. Die Cyclosporin A Biotransformation war in HepaRG Zellen am stärksten ausgeprägt, was durch stabile und wesentlich höhere CYP3A4- und CYP3A5-Aktivität in HepaRG Zellen zu erklären ist. Zusätzlich wurden die in vitro Clearance-Werte bestimmt und auf in vivo Clearance-Werte extrapoliert. Alle extrapolierten Werte waren zu hoch geschätzt (primäre Rattenhepatozyten: 10fach, primäre human Hepatpzyten: 2fach, HepaRG Zellen: 2fach). Diese Ergebnisse sollten mittels physiologisch-basierter pharmakokinetischer Modellierung sowie durch weitere Experimente überprüft werden, um zu ermitteln, ob diese hohen Schätzungen für jedes System konstant sind und somit durch die Einführung von weiteren Skalierungsfaktoren verringert werden können. Kultivierte Gehirnzellen, primäre Nervenzellkulturen der Kortex von Mäusen und primäre Hirnzellaggregate der Ratte, zeigten schnell erreichte Cyclosporin A Gleichgewichtskonzentrationen. Diese Ergebnisse deuteten auf eine Verteilung von Cyclosporin A zwischen der wässrigen und organischen Phase hin, wobei biologische Prozesse nur eine untergeordnete Rolle spielen. Daher scheint die intrazelluläre Cyclosporin A Aufnahme Transporter-vermittelt zu sein. Ergebnisse der Transporter Experimente, die an einer künstlichen Membran und Caco-2 Zellen durchgeführt wurden, unterstützten diese Hypothese. Messungen der Plastikbindung von Cyclosporin A zeigten signifikante, aber für jedes Zellsystem unterschiedliche, Adsorptionsraten, die mittels physiologisch-basierter pharmakokinetischer Modellierung berücksichtigt werden sollten. Die Kinetik von Adefovir dipivoxil machte auf die Nachteile von in vitro Versuchen aufmerksam. Für die intrazelluläre Aufnahme von Adefovir sind aktive Transportproteine nötig, die jedoch in der Nierenzelllinie RPTEC/TERT1 nicht funktionell vorhanden sind. Daher war die Aufnahme von Adefovir auf die passive Diffusion von Adefovir dipivoxil beschränkt, das aber auch zeitabhängig unter den experimentellen Konditionen zerfiel. Die an RPTEC/TERT1 Zellen untersuchte Kinetik von Cisplatin deutete auf eine intrazelluläre Platin-Anreicherung hin, die jedoch nicht in einer signifikanten Bioakkumulation resultierte. Möglicherweise sind innerhalb von 14 Tagen die Gleichgewichtskonzentrationen von Cisplatin noch nicht erreicht. Die Kinetikprofile von Cisplatin in Medium ließen einen aktiven, von der basolateralen zur apikalen Seite gerichteten Cisplatin Transport erkennen, wie schon in vivo beschrieben, wobei die Geschwindigkeit dieser Transportprozesse in vitro langsamer zu sein scheint als in der intakte Niere. Daher müssen die generierten Daten zur Schätzung von zellulären Prozessen modelliert werden, um durch anschließende Extrapolation mit in vivo Daten verglichen werden zu können. Abschließend bleibt zu sagen, dass das experimentelle Design vorteilhaft war. Wiederholte tägliche Administration von zwei unterschiedlichen Konzentrationen eines Medikaments ermöglichte die Erfassung von Bioakkumulation bei toxischen Konzentrationen sowie Biotransformation/Export bei nicht-toxischen Konzentrationen. Potenzielle Fehler, die zu einer Fehlinterpretation führen könnten, wurden durch die exakte Bestimmung der tatsächlich applizierten Arzneimittelmenge reduziert, da nicht immer die applizierte Konzentration mit der Nominalkonzentration übereinstimmt. Darüber hinaus erwies es sich als Vorteil, die Arzneimittelkonzentrationen in den einzelnen Kompartimenten (Medium, Zellen und Plastik) zu bestimmen. Somit konnten zum einen Erkenntnisse über die Verteilung der Substanz gewonnen werden und zum anderen Fehleinschätzungen von zellulären Prozessen, z.B. Biotransformation, verhindert werden, was letzten Endes bei die Interpretation von Kinetik-Daten behilflich ist. Jedoch, wurden auch die Grenzen von in vitro Ansätzen deutlich. Für eine korrekte Extrapolation ist es unverzichtbar, dass die untersuchten in vitro Systeme funktionierende Proteine aufweisen, die bei der untersuchten Arzneimittel-induzierten Toxizität eine Schlüsselrolle übernehmen. Abschließend kann festgehalten werden, dass es, unter Berücksichtigung der Vor- und Nachteile, von Nutzen sein kann diesen Versuchsansatz der Langzeitbehandlung zu validieren und darüber hinaus auf Co Kultursysteme sowie Organ-Chips anzuwenden hinsichtlich der Entwicklung von Alternativmethoden für Toxizitätsstudien bei wiederholter Gabe. KW - cell culture KW - pharmacokinetics KW - repeated dose KW - in vitro KW - toxicity testing KW - Zellkultur KW - In vitro KW - Pharmakokinetik KW - Toxizitätstest Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122693 ER - TY - THES A1 - Bertelsmann, Dietmar T1 - Analysis of the Frequency of Kidney Toxicity in Preclinical Safety Studies using the eTOX Database T1 - Analyse der Häufigkeit von Nierentoxizität in präklinischen Sicherheitsstudien unter Verwendung der eTOX-Datenbank N2 - This research aimed to obtain reliable data on the frequency of different types of renal toxicity findings in 28-day oral gavage studies in Wistar rats, their consistency across species and study duration, as well as the correlation between histopathological endpoints and routinely used clinical chemistry parameters indicative of kidney injury. Analysis of renal histopathological findings was carried out through extraction of information from the IMI eTOX database. Spontaneous renal histopathological findings in 28-day oral gavage studies in control Wistar rats and beagle dogs confirmed tubular basophilia and renal dilation as the most frequent incidental findings in controls, whereas necrosis and glomerulosclerosis were not identified at all or only rarely as a background lesion. Histopathological evidence of necrosis and glomerulosclerosis was associated with changes in clinical chemistry parameters in 28-day oral gavage Wistar rat studies. Necrosis was frequently accompanied by a statistically significant rise in serum creatinine and serum urea, whereas serum albumin was frequently found to decrease statistically significantly in treatment groups in which necrosis was recorded. In contrast to necrosis, glomerulosclerosis was not associated with statistically significant changes in serum creatinine and urea in any of the 28-day oral gavage Wistar rat treatment groups, but appears to be best reflected by a pattern of statistically significantly lowered serum albumin and serum protein together with a statistically significant increase in serum cholesterol. As might have been expected based on the high background incidences of tubular basophilia and dilation, no consistent changes in any of the clinical chemistry parameters were evident in animals in which renal lesions were con� fined to renal tubular basophilia or dilation. In summary, the routinely provided clinical chemistry parameters are rather insensitive - novel kidney biomarkers such as Cystatin C, β-trace protein and Kidney injury molecule 1 should further be evaluated and integrated into routine preclinical and clinical practice. However, evaluation of clinical chemistry data was limited by the lack of individual animal data. Even though an extensive amount of preclinical studies is accessible through the eTOX database, comparison of consistency across time was limited by the limited number of shorter- and longer term studies conducted with the compounds identified as causing renal histopathological changes within a 28- day study in rats. A high consistency across time for both treatment-related tubular basophilia and treatment-related dilation cannot be confirmed for either of the two effects as these two findings were both induced only rarely in studies over a different treatment-duration other than 28 days after administration of the compounds which provoked the respective effect in a 28-day study. For the finding of necrosis consistency across time was low with the exception of “AZ_GGA_200002321”, in which renal papillary necrosis was identified consist� ently throughout different treatment durations (2, 4, 26, 104 weeks). No shorter and longer-term studies were available for the compounds identified as causing glomerulosclerosis within a 28-day study in rats. No consistent findings of the selected histopathological endpoints were identified in any of the corresponding 28-day oral gavage beagle dog studies after treatment with the identical compounds, which caused the respective ef� fect after 28-day treatment in rats. However, in the overwhelming majority of cases, beagle dogs were administered lower doses in these studies in compar� ison to the corresponding 28-day Wistar rat studies. Searching the eTOX database yielded no 28-day oral gavage studies in Wistar and Wistar Han rats in which accumulation of hyaline droplets, tubular atrophy or hyperplasia was recorded. Only one 28-day oral gavage Wistar rat study was identified with the histopathological result of neutrophilic inflammation. Consequently, evaluation of these four renal findings in relation to clinical chemistry parameters and consistency across time and species cannot be made. In summary, this work contributes knowledge through mining and evaluating the eTOX database on a variety of specific renal endpoints that frequently occur after administration of trial substances in 28-day oral gavage studies in Wistar rats in the field of preclinical toxicity with specific focus on their frequency relation to background findings, as well as consistency across time and species. Targeted statistical evaluation of in vivo data within joint research ventures such as the eTOX project, presents an enormous opportunity for an innovative future way of aiding preclinical research towards a more efficient research in the preclinical stage of drug development. This could be achieved through the aug� mentation of methodological strategies and possibly novel software tools in order to predict in vivo toxicology of new molecular entities by means of information that is already available before early stages of the drug development pipeline begin. N2 - Diese Arbeit zielte darauf ab, verlässliche Daten über die Häufigkeit verschiedener Arten von Nierentoxizitätsbefunden in 28-tägigen oralen Sondenstudien an Wistar-Ratten zu erhalten. Untersucht wurde weiterhin die Konsistenz der Toxizitätsbefunde unterschiedlicher Spezies und Studiendauer sowie die Korrelation zwischen histopathologischen Endpunkten und routinemäßig verwendeten klinisch-chemischen Parametern, die auf eine Nierenschädigung hinweisen. Die Analyse der histopathologischen Nierenbefunde wurde durch Extraktion von Informationen aus der IMI eTOX-Datenbank durchgeführt. Spontane renale histopathologische Befunde in 28-tägigen oralen Sondenstudien an Wistar-Ratten und Beagles bestätigten tubuläre Basophilie und renale Dilatation als häufigste Nebenbefunde bei den Kontrolltieren, während Nekrose und Glomerulosklerose gar nicht oder nur selten als Hintergrundläsion identifiziert wurden. Der histopathologische Nachweis von Nekrose und Glomerulosklerose war mit Änderungen der klinisch-chemischen Parameter in 28-tägigen Wistar-Rattenstudien mit oraler Sonde verbunden. Nekrose ging häufig mit einem statistisch signifikanten Anstieg von Serumkreatinin und Serumharnstoff einher, während Serumalbumin in Behandlungsgruppen, in denen Nekrose aufgezeichnet wurde, häufig statistisch signifikant abnahm. Im Gegensatz zur Nekrose war Glomerulosklerose in keiner der 28-tägigen Wistar-Ratten-Behandlungsgruppen mit oraler Sonde mit statistisch signifikanten Veränderungen von Serumkreatinin und Harnstoff assoziiert, sondern scheint sich am besten in einem Muster von statistisch signifikant erniedrigtem Serumalbumin und Serumprotein zusammen mit einem statistisch signifikanten Anstieg des Serumcholesterins widerzuspiegeln. Wie aufgrund der hohen Hintergrundinzidenzen von tubulärer Basophilie und Dilatation zu erwarten war, waren bei Tieren, bei denen Nierenläsionen auf renale tubuläre Basophilie oder Dilatation beschränkt waren, keine konsistenten Änderungen der klinisch-chemischen Parameter erkennbar. Zusammenfassend sind die routinemäßig bereitgestellten klinisch-chemischen Parameter eher unempfindlich - neuartige Nieren-Biomarker wie „Cystatin C“, „β-trace protein“ und „Kidney injury molecule 1“ sollten weiter evaluiert und in die routinemäßige präklinische und klinische Praxis integriert werden. Die Auswertung der Daten zur klinischen Chemie war jedoch durch das Fehlen individueller Tierdaten begrenzt. Trotz der umfangreichen Anzahl an präklinischen Studien in der eTOX-Datenbank wurde der zeitliche Vergleich der Konsistenz durch die begrenzte Anzahl von Kurz- und Langzeitstudien eingeschränkt, welche mit denselben Substanzen durchgeführt wurden, die innerhalb einer 28-Tage-Studie an Ratten als Verursacher von renalen histopathologischen Veränderungen identifiziert wurden. Eine hohe zeitliche Konsistenz sowohl für die behandlungsbedingte tubuläre Basophilie und Dilatation kann für keinen der beiden Effekte bestätigt werden, da diese beiden Befunde nur selten in Studien über eine andere Behandlungsdauer als 28 Tage nach Verabreichung derselben Substanzen, die den jeweiligen Effekt in einer 28-Tage-Studie hervorriefen, induziert wurden. Für den Befund der Nekrose war die zeitliche Konsistenz gering. Eine Ausnahme stellte Substanz "AZ_GGA_200002321" dar, bei der über verschiedene Behandlungsdauern (2, 4, 26, 104 Wochen) hinweg konstant renale papilläre Nekrose festgestellt wurde. Für die Substanzen, die in einer 28-Tage-Studie an Ratten als glomeruloskleroseauslösend identifiziert wurden, waren keine Kurz- und Langzeitstudien verfügbar. In keiner der korrespondierenden 28-Tage-Studien an Beagles mit oraler Sonde wurden konsistente Befunde der ausgewählten histopathologischen Endpunkte nach Behandlung mit den identischen Verbindungen, die den jeweiligen Effekt nach 28-tägiger Behandlung in Ratten verursachten, festgestellt. In der überwiegenden Mehrheit der Fälle wurden den Beagles in diesen Studien im Vergleich zu den entsprechenden 28-Tage-Wistar-Rattenstudien niedrigere Dosen verabreicht. In der eTOX-Datenbank konnten keine 28-tägigen oralen Sondenstudien an Wistar- und Wistar-Han-Ratten gefunden werden, in denen eine Akkumulation von hyalinen Tröpfchen, tubuläre Atrophie oder Hyperplasie aufgezeichet wurde. Nur eine 28-tägige Wistar-Rattenstudie wurde mit dem histopathologischen Ergebnis einer neutrophilen Entzündung identifiziert. Folglich kann eine Bewertung dieser vier Nierenbefunde in Bezug auf klinische Chemie und Konsistenz über Zeit und Spezies nicht vorgenommen werden. Insgesamt zeigt dieser Arbeit, dass eine gezielte statistische Auswertung von in vivo-Daten im Rahmen von Forschungsverbünden wie dem eTOX-Projekt eine enorme Chance bietet, die präklinische Forschung in Zukunft auf dem Weg zu einer effizienteren Forschung in der präklinischen Phase der Arzneimittelentwicklung zu unterstützen. Dies könnte außerdem durch die Erweiterung methodischer Strategien und möglicherweise neuartiger Software-Tools erreicht werden, um die In-vivo-Toxikologie neuer molekularer Entitäten mit Hilfe von Informationen vorherzusagen, die bereits vor Beginn der Arzneimittelentwicklungspipeline verfügbar sind. KW - renal toxicity KW - etox database KW - rats KW - toxicity Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-257104 ER - TY - JOUR A1 - Bittner, Nataly A1 - Boon, Andy A1 - Delbanco, Evert H. A1 - Walter, Christof A1 - Mally, Angela T1 - Assessment of aromatic amides in printed food contact materials: analysis of potential cleavage to primary aromatic amines during simulated passage through the gastrointestinal tract JF - Archives of Toxicology N2 - Recent analyses conducted by German official food control reported detection of the aromatic amides N-(2,4-dimethylphenyl)acetamide (NDPA), N-acetoacetyl-m-xylidine (NAAX) and 3-hydroxy-2-naphthanilide (Naphthol AS) in cold water extracts from certain food contact materials made from paper or cardboard, including paper straws, paper napkins, and cupcake liners. Because aromatic amides may be cleaved to potentially genotoxic primary amines upon oral intake, these findings raise concern that transfer of NDPA, NAAX and Naphthol AS from food contact materials into food may present a risk to human health. The aim of the present work was to assess the stability of NDPA, NAAX and Naphthol AS and potential cleavage to 2,4-dimethylaniline (2,4-DMA) and aniline during simulated passage through the gastrointestinal tract using static in vitro digestion models. Using the digestion model established by the National Institute for Public Health and the Environment (RIVM, Bilthoven, NL) and a protocol recommended by the European Food Safety Authority, potential hydrolysis of the aromatic amides to the respective aromatic amines was assessed by LC–MS/MS following incubation of the aromatic amides with digestive fluid simulants. Time-dependent hydrolysis of NDPA and NAAX resulting in formation of the primary aromatic amine 2,4-DMA was consistently observed in both models. The highest rate of cleavage of NDPA and NAAX was recorded following 4 h incubation with 0.07 M HCl as gastric-juice simulant, and amounted to 0.21% and 0.053%, respectively. Incubation of Naphthol AS with digestive fluid simulants did not give rise to an increase in the concentration of aniline above the background that resulted from the presence of aniline as an impurity of the test compound. Considering the lack of evidence for aniline formation from Naphthol AS and the extremely low rate of hydrolysis of the amide bonds of NDPA and NAAX during simulated passage through the gastrointestinal tract that gives rise to only very minor amounts of the potentially mutagenic and/or carcinogenic aromatic amine 2,4-DMA, risk assessment based on assumption of 100% cleavage to the primary aromatic amines would appear to overestimate health risks related to the presence of aromatic amides in food contact materials. KW - aromatic amides KW - primary aromatic amine KW - food contact materials KW - simulated digestion Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-324697 VL - 96 IS - 5 ER - TY - JOUR A1 - Boivin, Valérie A1 - Beyersdorf, Niklas A1 - Palm, Dieter A1 - Nikolaev, Viacheslav O. A1 - Schlipp, Angela A1 - Müller, Justus A1 - Schmidt, Doris A1 - Kocoski, Vladimir A1 - Kerkau, Thomas A1 - Hünig, Thomas A1 - Ertl, Georg A1 - Lohse, Martin J. A1 - Jahns, Roland T1 - Novel Receptor-Derived Cyclopeptides to Treat Heart Failure Caused by \(Anti-β_1-Adrenoceptor\) Antibodies in a Human-Analogous Rat Model JF - PLoS One N2 - Despite recent therapeutic advances the prognosis of heart failure remains poor. Recent research suggests that heart failure is a heterogeneous syndrome and that many patients have stimulating auto-antibodies directed against the second extracellular loop of the \(β_1\) adrenergic receptor \((β_1EC2)\). In a human-analogous rat model such antibodies cause myocyte damage and heart failure. Here we used this model to test a novel antibody-directed strategy aiming to prevent and/or treat antibody-induced cardiomyopathy. To generate heart failure, we immunised n = 76/114 rats with a fusion protein containing the human β1EC2 (amino-acids 195–225) every 4 weeks; n = 38/114 rats were control-injected with 0.9% NaCl. Intravenous application of a novel cyclic peptide mimicking \(β_1EC2\) (\(β_1EC2-CP\), 1.0 mg/kg every 4 weeks) or administration of the \(β_1-blocker\) bisoprolol (15 mg/kg/day orally) was initiated either 6 weeks (cardiac function still normal, prevention-study, n = 24 (16 treated vs. 8 untreated)) or 8.5 months after the 1st immunisation (onset of cardiomyopathy, therapy-study, n = 52 (40 treated vs. 12 untreated)); n = 8/52 rats from the therapy-study received \(β_1EC2-CP/bisoprolol\) co-treatment. We found that \(β_1EC2-CP\) prevented and (alone or as add-on drug) treated antibody-induced cardiac damage in the rat, and that its efficacy was superior to mono-treatment with bisoprolol, a standard drug in heart failure. While bisoprolol mono-therapy was able to stop disease-progression, \(β_1EC2-CP\) mono-therapy -or as an add-on to bisoprolol- almost fully reversed antibody-induced cardiac damage. The cyclo¬peptide acted both by scavenging free \(anti-β_1EC2-antibodies\) and by targeting \(β_1EC2\)-specific memory B-cells involved in antibody-production. Our model provides the basis for the clinical translation of a novel double-acting therapeutic strategy that scavenges harmful \(anti-β_1EC2-antibodies\) and also selectively depletes memory B-cells involved in the production of such antibodies. Treatment with immuno-modulating cyclopeptides alone or as an add-on to \(β_1\)-blockade represents a promising new therapeutic option in immune-mediated heart failure. KW - memory B cells KW - antibodies KW - T cells KW - B cells KW - heart KW - heart failure KW - kidneys KW - enzyme-linked immunoassays Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126028 VL - 10 IS - 2 ER - TY - JOUR A1 - Bommakanti, R. A1 - Bokoch, G. M. A1 - Tolley, J. O. A1 - Schreiber, R. E. A1 - Siemsen, D. W. A1 - Klotz, Karl-Norbert A1 - Jesaitis, A. J. T1 - Reconstitution of a physical complex between the N-formyl chemotactic peptide receptor and G protein: Inhibition by pertussis toxin-catalyzed ADP ribosylation N2 - Photoaffinity-labeled N-formyl chemotactic peptide receptors from human neutrophils solubilized in octyl glucoside exhibit two forms upon sucrose density gradient sedimentation, with apparent Sedimentation coefficients of approximately 4 and 7 S. Tbe 7 S form can be converted to the 4 S form by guanosine 5' -0- (3-thiotriphosphate) (GTP-yS) with an EC&o of -20 nM, suggesting that the 7 S form may represent a physical complex of the receptor with endogenous G protein (Jesaitis, A. J., Tolley, J. 0., Bokoch, G. M., and Allen, R. A. (1989) J. Cell Biol. 109, 2783-2790). To probe the nature of the 7 S form, we reconstituted the 7 S form from the 4 S form by adding purified G protein. The 4 S form, obtained by solubilizing GTP-yS-treated neutrophil plasma membranes, was incubated with purified (>95%) G. protein from bovine brain (containing both G\(_{ia1}\) and G\(_{ia2}\)) or with neutrophil G protein (G\(_a\)), and formation of the 7 S complex was analyzed on sucrose density gradients. The EC\(_{50}\) of 7 S complex formation induced by the two G proteins was 70 \(\pm\) 25 and 170 \(\pm\) 40 DM for G\(_a\) and G\(_1\), respectively. No complexation was measurable when bovine transducin (G\(_t\)) was used up to 30 times the EC\(_{50\) for G\(_a\). The EC\(_{50}\) for G\(_t\) was the same for receptors, obtained from formyl peptide-stimulated or unstimulated cells. The addition of 10 \(\mu\)M GTP-yS to the reconstituted 7 S complex caused a complete reversion of the receptor to the 4 S form, and anti-G\(_1\) peptide antisera immunosedimented the 7 S form. ADP-ribosylation of Gt prevented formation of the 7 S form even at 20 times the concentration of unribosylated G. normally used to attain 50% conversion to the 7 S form. These observations suggest that the 7 S species is a pbysical complex containing N-formyl chemotactic peptide receptor and G protein. KW - Toxikologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60406 ER - TY - JOUR A1 - Bommakanti, R. K. A1 - Klotz, Karl-Norbert A1 - Dratz, E. A. A1 - Jesaitis, A. J. T1 - A carboxyl-terminal tail peptide of neutrophil chemotactic receptor disrupts its physical complex with G protein N2 - No abstract available KW - Toxikologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60456 ER - TY - JOUR A1 - Brand, Susanne A1 - Amann, Kerstin A1 - Mandel, Philipp A1 - Zimnol, Anna A1 - Schupp, Nicole T1 - Oxidative DNA Damage in Kidneys and Heart of Hypertensive Mice Is Prevented by Blocking Angiotensin II and Aldosterone Receptors JF - PLOS ONE N2 - INTRODUCTION: Recently, we could show that angiotensin II, the reactive peptide of the blood pressure-regulating renin-angiotensin-aldosterone-system, causes the formation of reactive oxygen species and DNA damage in kidneys and hearts of hypertensive mice. To further investigate on the one hand the mechanism of DNA damage caused by angiotensin II, and on the other hand possible intervention strategies against end-organ damage, the effects of substances interfering with the renin-angiotensin-aldosterone-system on angiotensin II-induced genomic damage were studied. METHODS: In C57BL/6-mice, hypertension was induced by infusion of 600 ng/kg • min angiotensin II. The animals were additionally treated with the angiotensin II type 1 receptor blocker candesartan, the mineralocorticoid receptor blocker eplerenone and the antioxidant tempol. DNA damage and the activation of transcription factors were studied by immunohistochemistry and protein expression analysis. RESULTS: Administration of angiotensin II led to a significant increase of blood pressure, decreased only by candesartan. In kidneys and hearts of angiotensin II-treated animals, significant oxidative stress could be detected (1.5-fold over control). The redox-sensitive transcription factors Nrf2 and NF-κB were activated in the kidney by angiotensin II-treatment (4- and 3-fold over control, respectively) and reduced by all interventions. In kidneys and hearts an increase of DNA damage (3- and 2-fold over control, respectively) and of DNA repair (3-fold over control) was found. These effects were ameliorated by all interventions in both organs. Consistently, candesartan and tempol were more effective than eplerenone. CONCLUSION: Angiotensin II-induced DNA damage is caused by angiotensin II type 1 receptor-mediated formation of oxidative stress in vivo. The angiotensin II-mediated physiological increase of aldosterone adds to the DNA-damaging effects. Blocking angiotensin II and mineralocorticoid receptors therefore has beneficial effects on end-organ damage independent of blood pressure normalization. KW - aldosterone KW - oxidative stress KW - transcription factors KW - kidneys KW - heart KW - hypertension KW - DNA damage KW - blood pressure Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-118011 SN - 1932-6203 VL - 9 IS - 12 ER - TY - JOUR A1 - Breitenbach, Tim A1 - Lorenz, Kristina A1 - Dandekar, Thomas T1 - How to steer and control ERK and the ERK signaling cascade exemplified by looking at cardiac insufficiency JF - International Journal of Molecular Sciences N2 - Mathematical optimization framework allows the identification of certain nodes within a signaling network. In this work, we analyzed the complex extracellular-signal-regulated kinase 1 and 2 (ERK1/2) cascade in cardiomyocytes using the framework to find efficient adjustment screws for this cascade that is important for cardiomyocyte survival and maladaptive heart muscle growth. We modeled optimal pharmacological intervention points that are beneficial for the heart, but avoid the occurrence of a maladaptive ERK1/2 modification, the autophosphorylation of ERK at threonine 188 (ERK\(^{Thr188}\) phosphorylation), which causes cardiac hypertrophy. For this purpose, a network of a cardiomyocyte that was fitted to experimental data was equipped with external stimuli that model the pharmacological intervention points. Specifically, two situations were considered. In the first one, the cardiomyocyte was driven to a desired expression level with different treatment strategies. These strategies were quantified with respect to beneficial effects and maleficent side effects and then which one is the best treatment strategy was evaluated. In the second situation, it was shown how to model constitutively activated pathways and how to identify drug targets to obtain a desired activity level that is associated with a healthy state and in contrast to the maleficent expression pattern caused by the constitutively activated pathway. An implementation of the algorithms used for the calculations is also presented in this paper, which simplifies the application of the presented framework for drug targeting, optimal drug combinations and the systematic and automatic search for pharmacological intervention points. The codes were designed such that they can be combined with any mathematical model given by ordinary differential equations. KW - optimal pharmacological modulation KW - efficient intervention points KW - ERK signaling KW - optimal treatment strategies KW - optimal drug targeting KW - optimal drug combination Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285164 SN - 1422-0067 VL - 20 IS - 9 ER - TY - INPR A1 - Brenner, Marian A1 - Zink, Christoph A1 - Witzinger, Linda A1 - Keller, Angelika A1 - Hadamek, Kerstin A1 - Bothe, Sebastian A1 - Neuenschwander, Martin A1 - Villmann, Carmen A1 - von Kries, Jens Peter A1 - Schindelin, Hermann A1 - Jeanclos, Elisabeth A1 - Gohla, Antje T1 - 7,8-Dihydroxyflavone is a direct inhibitor of pyridoxal phosphatase T2 - eLife N2 - Vitamin B6 deficiency has been linked to cognitive impairment in human brain disorders for decades. Still, the molecular mechanisms linking vitamin B6 to these pathologies remain poorly understood, and whether vitamin B6 supplementation improves cognition is unclear as well. Pyridoxal phosphatase (PDXP), an enzyme that controls levels of pyridoxal 5’-phosphate (PLP), the co-enzymatically active form of vitamin B6, may represent an alternative therapeutic entry point into vitamin B6-associated pathologies. However, pharmacological PDXP inhibitors to test this concept are lacking. We now identify a PDXP and age-dependent decline of PLP levels in the murine hippocampus that provides a rationale for the development of PDXP inhibitors. Using a combination of small molecule screening, protein crystallography and biolayer interferometry, we discover and analyze 7,8-dihydroxyflavone (7,8-DHF) as a direct and potent PDXP inhibitor. 7,8-DHF binds and reversibly inhibits PDXP with low micromolar affinity and sub-micromolar potency. In mouse hippocampal neurons, 7,8-DHF increases PLP in a PDXP-dependent manner. These findings validate PDXP as a druggable target. Of note, 7,8-DHF is a well-studied molecule in brain disorder models, although its mechanism of action is actively debated. Our discovery of 7,8-DHF as a PDXP inhibitor offers novel mechanistic insights into the controversy surrounding 7,8-DHF-mediated effects in the brain. KW - 7,8-dihydroxyflavone (7,8-DHF) KW - pyridoxal phosphatase (PDXP) KW - vitamin B6 KW - PDXP inhibitors Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350446 ER - TY - THES A1 - Brink, Andreas T1 - The biological significance of chemically-induced DNA adducts in relation to background DNA damage T1 - Die biologische Bedeutung von chemisch induzierten DNA-Addukten in Relation zum Hintergrund-DNA-Schaden N2 - No abstract available KW - DNS-Schädigung KW - DNS-Strangbruch KW - HPLC-MS KW - API-Massenspektrometrie KW - LC-MS KW - Gentoxikologie KW - Mutagenitätstest KW - Dosis-Wirkungs-Beziehung KW - DNA-Addukte KW - Dosis-Wirkungs-Beziehung KW - Hintergrund-DNA-Schaden KW - Comet assay KW - DNA adducts KW - Dose response relationships KW - Background DNA damage Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-23850 ER - TY - JOUR A1 - Buss, P. A1 - Caviezel, M. A1 - Lutz, Werner K. T1 - Linear dose-response relationship for DNA adducts in rat liver from chronic exposure to aflatoxin B1 N2 - Male F-344 rats were given eH]aßatoxin B1 (AFB1) in the drinking water at three exposure Ievels (0.02, 0.6, 20 J,Lgll, resulting in average dose Ievels of 2.2, 73, 2110 nglkg per day). After 4, 6 and 8 weeks, DNA was ~ted frorn the livers and analyzed for aßatoxin-DNA adducts. Tbe Ievel of DNA adducts did not increase significantly after 4 weeks, indicating that a steady-state for adduct formation and removal had nearly been reached. At 8 weeks, the adduct Ievels were 0.91, 32 and 850 nucleotide-aßatoxin adducts per to' nucleotides, i.e. clearly proportional to the dose. At the high dose Ievel, a near SO% tumor incidence would be expected in a 2-year bioassay with F -344 rats while the low dose used is within the range of estlmated human dietary exposures to aßatoxin in W estem countries. The proportionality seen between exposure and steady-state DNA adduct Ievel is discussed with respect to a linear extrapolation of the tumor risk to low dose. KW - Toxikologie Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60779 ER - TY - JOUR A1 - Bösch, R. A1 - Friederich, U. A1 - Lutz, Werner K. A1 - Brocker, E. A1 - Bachmann, M. A1 - Schlatter, C. T1 - Investigations on DNA binding in rat liver and in Salmonella and on mutagenicity in the Ames test by emodin, a natural anthraquinone N2 - Emodin (1,6,8-trihydroxy-3-methylanthraquinone), an important aglycone found in natural anthraquinone glycosides frequently used in Iaxative drugs, was mutagenic in the Salmonellajmammalian microsome assay (Ames test) with a specificity for strain TA1537. The mutagenic activity was activationdependent with an optimal amount of S9 from Aroclor 1254-treated male Sprague-Dawley rats of 20% in the S9 mix (v jv) for 10 p.g emodin per plate. Heat inactivation of the S9 for 30 min at 60 ° C prevented mutagenicity. The addition of the cytochrome P-448 inhibitor 7,8-benzoflavone (18.5 nmoles per plate) reduced the mutagenic activity of 5.0 p.g emodin per plate to about one third, whereas the P-450 inhibitor metyrapone (up to 1850 nmoles per plate) was without effect. To test whether a metabolite" binds covalently to Salmonella DNA, [10-\(^{14}\)C]emodin was radiosynthesized, large batches of bacteria were incubated with [10-\(^{14}\)C]emodin and DNA was isolated. [G- \(^{3}\)H]Aflatoxin B1 (AFB1) was used as a positive control mutagen known to act via DNA binding. DNA obtained after aflatoxin treatment could be purified to constant specific activity. With emodin, the specific activity of DNA did not remain constant after repeated precipitations so that it is unlikely that the mutagenicity of emodin is due to covalent interaction of a metabolite with DNA. The antioxidants vitamin C and E or glutathione did not reduce the mutagenicity. Emodin was also negative with strain TA102. Thus, oxygen radicals are probably not involved. When emodin was incubated with S9 alone for up to 50 h before heat-inactivation of the enzymes and addition of bacteria, the mutagenic activity did not decrease. It is concluded that the mutagenicity of emodin is due to a chemically stable, oxidized metabolite forming physico-chemical associations with DNA, possibly of the intercalative type. In order to check whether an intact mammalian organism might be able to activate emodin to a DNA-binding metabolite, radiolabelled emodin was administered by oral gavage to male SD rats and liver DNA was isolated after 72 h. Very little radioactivity was associated with the DNA. Considering that DNA radioactivity could also be due to sources other than covalent interactions, an upper limit for the · covalent binding index, CBI = (p.moles chemical bound per moles DNA nucleotides)/(mmoles chemical administered per kg body weight) of 0.5 is deduced. This is 104 times below the CBI of AFB1. The demonstration of a lack of covalent interaction with DNA bothin Salmonellaandin rat liver is discussed in terms of a reduced hazard posed by emodin as a mutagenic drug in use in humans. KW - Toxikologie KW - DNA binding KW - (Rat liver) KW - (Salmonella) KW - Ames test KW - Emodin KW - Anthraquinone glycosides KW - natural Y1 - 1987 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60913 ER - TY - JOUR A1 - Bünemann, Moritz A1 - Pott, Lutz T1 - Membrane-delimited activation of muscarinic K current by an albumin-associated factor in guinea-pig atrial myocytes N2 - No abstract available KW - cardiac myocyte ; muscarinic K current ; G-protein ; Albumin ; serum Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-31300 ER - TY - JOUR A1 - Büsser, M. T. A1 - Lutz, Werner K. T1 - Stimulation of DNA synthesis in rat and mouse liver by various tumor promoters N2 - In order to investigate whether the Stimulation of liver DNA synthesis might be used to detect one class of hepatic tumor promoters, the incorporation of orally administered radiolabelled thymidine into liver DNA was detennined in rats and mice 24 h after a single oral gavage of test compounds at various dose Ievels. Three DNA-binding hepatocarcinogens, aflatoxin B1; benzidine and carbon tetrachloride, did not stimulate but rather inhibited DNA synthesis (not for CCla). Four hepatic tumor promoters, clofibrate, DDT, phenobarbital and thioacetamide, gave rise to a Stimulation in a dosedependent manner. Single oral doses between 0.02 and 0.3 mmol/kg were required to double the level of thymidine incorporation into liver DNA (= doubling dose, DD). Differentes between species or sex as obsprved in long-term carcinogenicity studies were reflected by a different stimulation of liver DNA synthesis. In agreement with the bioassay data, aldrin was positive only in male mice (DD = 0.007 mmol/kg) but not in male rats or female mice. 2,3, 7,8-TCDD was positive in male mice (DD = 10\(^{-6}\) mmol/kg) andin female rats (DD = 2 x 10\(^{-6}\) mmol/kg) but not in male rats. The assay was also able to distinguish between structural isomers with different carcinogenicities. [alpha]Hexachlorocyclohexane stimulated Iiver DNA synthesis with a doubling dose of about 0.2 mmol/kg in male rats whereas the [gamma]isomer was ineffective even at l mmol/kg. So far, only one result was inconsistent with carcinogenicity bioassay data. The different carcinogenicity of di(2-ethylhexyl)adipate (negative in rats) and di(2-ethylhe.xyl)phthalate (positive) was not detectable. 8oth plasticizers were positive in.this short-term system with DD's of 0. 7 mmol/kg for DEHA and 0.5 mmol/kg for DEHP. The proposed assay is discussed as an attempt to devise short-term assays for carcinogens not detected by the routine genotoxicity test systems. KW - Toxikologie Y1 - 1987 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60908 ER - TY - JOUR A1 - Calebiro, Davide A1 - Maiellaro, Isabella T1 - cAMP signaling microdomains and their observation by optical methods JF - Frontiers in Cellular Neuroscience N2 - The second messenger cyclic AMP (cAMP) is a major intracellular mediator of many hormones and neurotransmitters and regulates a myriad of cell functions, including synaptic plasticity in neurons. Whereas cAMP can freely diffuse in the cytosol, a growing body of evidence suggests the formation of cAMP gradients and microdomains near the sites of cAMP production, where cAMP signals remain apparently confined. The mechanisms responsible for the formation of such microdomains are subject of intensive investigation. The development of optical methods based on fluorescence resonance energy transfer (FRET), which allow a direct observation of cAMP signaling with high temporal and spatial resolution, is playing a fundamental role in elucidating the nature of such microdomains. Here, we will review the optical methods used for monitoring cAMP and protein kinase A (PKA) signaling in living cells, providing some examples of their application in neurons, and will discuss the major hypotheses on the formation of cAMP/PKA microdomains. KW - G protein-coupled receptor KW - cyclic AMP KW - signaling microdomain KW - fluorescence resonance energy transfer KW - neurons Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-118252 SN - 1662-5102 VL - 8 ER - TY - JOUR A1 - Cantoreggi, S. A1 - Dietrich, D. R. A1 - Lutz, Werner K. T1 - Induction of cell proliferation in the forestomach of F344 rats following subchronic administration of styrene 7,8-oxide and butylated hydroxyanisole N2 - The question addressed was whether Stimulation of cell proliferation could be responsible for tumor induction in the torestornach by styrene 7,8-oxide (SO). Male F344 rats were treated for 4 weeks with 0, 137,275, and 550 mglkg SO by p.o. gavage 3 times/week. Positive controls received 0, 0.5, I, and 2% butylated hydroxyanisole (BHA) in the diet for 4 weeks. Twenty-four h before termination of the experlment, the rats were implanted s.c. with an osmotic minipump deliverlog S-bromo-2'-deoxyuri· dine (BrdU). Cell proliferation in the forestomach was assessed by immunohistochemistry for BrdU incorporated into DNA. Cell number/mm section length and fraction of replicating cells (labeling Index) were determined in 3 domains of the forestomach, the saccus caecus, the midregion, and the prefundic region. With the exception of the prefundic reglon of the low-dose SO group, a significant increase of the labeling index was found in all regions both with SO and BHA. Rats treated with BHA showed, in addition, a dose-dependent increase in number and size of hyperplastic lesions. This was most pronounced in the prefundic region where carcinomas were reported to be localized. In this region, the number of dividing cells/mm section length was increased up to 17-fold. With SO, only marginal morphological changes were occasionally observed, despite the fact that the respective long-term treatment bad been reported to result in a higher carcinoma incidence than treatment with BHA. It ls concluded that the rate of replicating cells alone, numerically expressed by the labeling Index, is an lnsufficient tool for interpretlog the role of cell division in carcinogenesis. It is postulated that SO and BHA induce forestomach tumors via different mechanisms. While hyperplasia in the prefundic region most likely dominates the carcinogenicity of BHA, a mechanism combining marginal genotoxicity with strong promotion by increased cell proliferation appears to be involved in the tumorigenic action of SO. KW - Toxikologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60669 ER - TY - CHAP A1 - Cantoreggi, S. A1 - Gupta, R. C. A1 - Lutz, Werner K. T1 - An improved 32P-postlabelling assay for detection and quantitation of styrene 7,8-oxide-DNA adducts N2 - Using DNA modified with [7-3H]styrene 7,8-oxide (SO) in vitro we have standardized the 32P-postlabelling assay for detecting SO-DNA adducts. Nuclease P 1-enriched adducts were 32P-labelled and purified by high-salt ( 4.0 M ammonium formate, pH 6.1} C1s reverse-phase TLC. After elution from the layer with 2-butoxyethanol:H20 (4:6), adducts were separated by two-dimensional PEI cellulose TLC in non-urea solvents (2.0 M ammonium formate, pH 3.5, and 2.7 M sodium phosphate, pH 5.6). One major, three minor and several trace adducts were detected. The efficiency of the kinase reaction depended on the ATP concentration. Use of standard labelling conditions (['Y· 32P]ATP, <3000 Ci/mmol; <2 Mikromol) resulted in poor ( 4-7%) adduct recovery. An ATP concentration of 40 Mikromol, however, increased the labeJling efficiency by a factor of 5-8 (35-55% based on 3H-SO labelied DNA). The results indicate that the new separation technique is suitable for the relatively polar SO-DNA adducts and that high labelling efficiency can be achieved. KW - Medizin Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86305 ER - TY - JOUR A1 - Cantoreggi, S. A1 - Lutz, Werner K. T1 - Covalent binding of styrene to DNA in rat and mouse N2 - No abstract available KW - Toxikologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60693 ER - TY - JOUR A1 - Cantoreggi, S. A1 - Lutz, Werner K. T1 - Investigation of the covalent binding of styrene-7,8-oxide to DNA in rat and mouse N2 - Styrene-7,8-oxide (SO), the main intennediate metabolite of styrene, induces hyperkeratosis and tumors in the forestomach of rats and mice upon chronic administration by gavage. The aim of this study was to investigate wbether DNA binding could be responsible for the carcinogenic effect observed. [7-\(^3\)H]SO was administered by oral gavage in com oll to male CD rats at two dose levels (1.65 or 240 mg/kg). After 4 or 24 h, forestomach, glandular stomach and Uver were exclsed, DNA was isolated and its radioactivity detennined. At the 4 h time polnt, the DNA radioactivity was below the Iimit of detection in the torestornach and the liver. Expressed in the units of the covalent bindlng Index, CBI = (pmol adduct/mol DNA nucleotide)/(mmol cbemical administeredlkg body wt), the DNA-binding potency was below 2.6 and 2.0 respectively. In the glandular stomach at 4 b, and in most 24 b samples, DNA was slightly radiolabeled. Enzymatic degradation of the DNA and separation by HPLC ofthe normal nucleotides sbowed that the DNA rad.ioactivity represented biosynthetic incorporation of radlolabel into newly synthesized DNA. The Iimit of detection of DNA adducts in the glandular stomach was 1.0. In a second experlment, [7-\(^3\)H]SO was administered by i.p. injection to male 86C3Fl rnice. Liver DNA was analyzed after 2 h. No radloactivity was detectable at a Iimit of detection of CBI < 0.6. In agreement with the relatively long half-life of SO in animals, the cbemical reactivity of SO appears to be too low to result in a detectable production of DNA adducts in an in vivo situation. Upon comparison with the DNA-binding of other carcinogens, a purely genotoxic mechanism of tumorigenJc action of SO is unlikely. The observed tumorigenic potency in the forestomach could be the result of strong tumor promotion by high-dose cytotoxicity foUowed by regenerative hyperplasia. KW - Toxikologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60721 ER - TY - JOUR A1 - Capra, Valérie A1 - Busnelli, Marta A1 - Perenna, Alessandro A1 - Ambrosio, Manuela A1 - Accomazzo, Maria Rosa A1 - Galés, Celine A1 - Chini, Bice A1 - Rovati, G. Enrico T1 - Full and Partial Agonists of Thromboxane Prostanoid Receptor Unveil Fine Tuning of Receptor Superactive Conformation and G Protein Activation JF - PLoS ONE N2 - The intrahelical salt bridge between \(E/D^{3.49}\) and \(R^{3.50}\) within the E/DRY motif on helix 3 (H3) and the interhelical hydrogen bonding between the E/DRY and residues on H6 are thought to be critical in stabilizing the class A G protein-coupled receptors in their inactive state. Removal of these interactions is expected to generate constitutively active receptors. This study examines how neutralization of \(E^{3.49/6.30}\) in the thromboxane prostanoid (TP) receptor alters ligand binding, basal, and agonist-induced activity and investigates the molecular mechanisms of G protein activation. We demonstrate here that a panel of full and partial agonists showed an increase in affinity and potency for E129V and E240V mutants. Yet, even augmenting the sensitivity to detect constitutive activity (CA) with overexpression of the receptor or the G protein revealed resistance to an increase in basal activity, while retaining fully the ability to cause agonist-induced signaling. However, direct G protein activation measured through bioluminescence resonance energy transfer (BRET) indicates that these mutants more efficiently communicate and/or activate their cognate G proteins. These results suggest the existence of additional constrains governing the shift of TP receptor to its active state, together with an increase propensity of these mutants to agonist-induced signaling, corroborating their definition as superactive mutants. The particular nature of the TP receptor as somehow "resistant" to CA should be examined in the context of its pathophysiological role in the cardiovascular system. Evolutionary forces may have favored regulation mechanisms leading to low basal activity and selected against more highly active phenotypes. KW - coupled receptor KW - ligand binding KW - intracellular loop KW - molecular dynamics KW - Beta(1)-adrenergic receptor KW - ionic look KW - Beta(2)-adrenergic receptor KW - crystal structure KW - constitutive activity Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131013 VL - 8 IS - 3 ER - TY - JOUR A1 - Caviezel, M. A1 - Aeschbach, A. P. A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Reduction of covalent binding of aflatoxin B1 to rabbit liver DNA after immunization against this carcinogen N2 - The covalent binding of [3H]aflatoxin B1 (AF) to liver DNA was determined, 6 h after oral administration to male rabbits. A Covalent Binding Index, CBI (flmol AF/mol DNA-P)/(mmol AF/kg b. w.) = 8,500 was found. Pretreatment of rabbits with AF coupled to bovine serum albumin in Freund's adjuvant led to the production of AF-directed antibodies. Administration of [3H]AF to such immunized rabbits resulted in a CJH of only 2,500, i.e., the iiDJ{.lUnization provided a protection by a factor of more than 3. Although this is encouraging evidence for the potential of active immunization against genotoxic carcinogens, a nurober of pointswill have to be clarified, such as the time course for the DNA binding and the question of a possible shift to other target cells. KW - Krebs KW - DNA KW - Aflatoxin KW - Cancer prevention KW - Carcinogen KW - Covalent binding KW - DNA KW - Immunization Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-80116 ER - TY - JOUR A1 - Caviezel, M. A1 - Lutz, Werner K. A1 - Minini, U. A1 - Schlatter, C. T1 - Interaction of estrone and estradiol with DNA and protein of liver and kidney in rat and hamster in vivo and in vitro N2 - (6,7-\(^3\)H] Estrone (E) and [6,7-\(^3\)H]estradiol-17ß (E\(_2\)) have been synthesized by reduction of 6-dehydroestrone and 6-dehydroestradiol with tritium gas. Tritiated E and E\(_2\) were administered by oral gavage to female rats and to male and female hamsters on a dose level of about 300 \(\mu\)g/kg (54 mCi/kg). After 8 h, the liver was excised from the rats; liver and kidneys were taken from the hamsters. DNA was purified either directly from an organ homogenate or via chromatin. The radioactivity in the DNA was expressed in the units of the Covalent Binding Index, CBI = (\(\mu\)mol chemical bound per mol Similar considerations can be made for the liver where any true covalent DNA binding must be below a Ievel of 0.01. It is concluded that an observable tumor induction by estrone or estradiol is unlikely to be due to DNA binding. DNA-P)/(mmol chemical administered per kg b.w.). Rat liver DNA isolated via chromatin exhibited the very low values of 0.08 and 0.09 for E and E\(_2\) respectively. The respective figures in hamster liver were 0.08 and 0.11 in females and 0.21 and 0.18 in the males. DNA isolated from the kidney revealed a detectable radioactivity only in the female, with values of 0.03 and 0.05 for E and E\(_2\) respectively. The values for male hamster kidney were < 0.01 for both hormones. The minute radioactivity detectable in the DNA samples does not represent covalent binding to DNA, however, as indicated by' two sets of control experiments. (A) Analysis by HPLC of the nucleosides prepared by enzyme digest of liver DNA isolated directly or via chromatin did not reveal any consistent peak which could have been attributed to a nucleoside-steroid adduct. (B) All DNA radioactivity could be due to protein contaminations, because the specific activity of chromatin protein was determined to be more than 3 ,000 tim es high er than of DNA. The high affinity of the hormone to protein was also demonstrated by in vitro incubations, where it could be shown that the specific activity of DNA and protein was essentially proportional to the concentration of radiolabelled hormone in the organ homogenate, regardless of whether the animal was treated or whether the hormone was added in vitro to the homogenate. Carcinogens acting by covalent DNA binding can be classified according to potency on the basis of the Covalent Binding Index. Values of 10\(^3\)-10\(^4\) have been found for potent, 10\(^2\) for moderate, and 1-10 for weak carcinogens. Since estrone is moderately carcinogenic for the kidney of the male hamster, a CBI of about 100 would be expected. The actually measured Iimit of detection of 0.01 places covalent DNA binding among the highly unlikely mechanisms of action. KW - Toxikologie KW - Estrogen KW - Hormone KW - Carcinogenesis KW - DNA binding KW - Protein binding KW - Estrone Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60995 ER - TY - JOUR A1 - Chen, Wen A1 - Gaßner, Birgit A1 - Börner, Sebastian A1 - Nikolaev, Viacheslav O. A1 - Schlegel, Nicolas A1 - Waschke, Jens A1 - Steinbronn, Nadine A1 - Strasser, Ruth A1 - Kuhn, Michaela T1 - Atrial natriuretic peptide enhances microvascular albumin permeability by the caveolae-mediated transcellular pathway JF - Cardiovascular Research N2 - Aims Cardiac atrial natriuretic peptide (ANP) participates in the maintenance of arterial blood pressure and intravascular volume homeostasis. The hypovolaemic effects of ANP result from coordinated actions in the kidney and systemic microcirculation. Hence, ANP, via its guanylyl cyclase-A (GC-A) receptor and intracellular cyclic GMP as second messenger, stimulates endothelial albumin permeability. Ultimately, this leads to a shift of plasma fluid into interstitial pools. Here we studied the role of caveolae-mediated transendothelial albumin transport in the hyperpermeability effects of ANP. Methods and results Intravital microscopy studies of the mouse cremaster microcirculation showed that ANP stimulates the extravasation of fluorescent albumin from post-capillary venules and causes arteriolar vasodilatation. The hyperpermeability effect was prevented in mice with conditional, endothelial deletion of GC-A (EC GC-A KO) or with deleted caveolin-1 (cav-1), the caveolae scaffold protein. In contrast, the vasodilating effect was preserved. Concomitantly, the acute hypovolaemic action of ANP was abolished in EC GC-A KO and Cav-1−/− mice. In cultured microvascular rat fat pad and mouse lung endothelial cells, ANP stimulated uptake and transendothelial transport of fluorescent albumin without altering endothelial electrical resistance. The stimulatory effect on albumin uptake was prevented in GC-A- or cav-1-deficient pulmonary endothelia. Finally, preparation of caveolin-enriched lipid rafts from mouse lung and western blotting showed that GC-A and cGMP-dependent protein kinase I partly co-localize with Cav-1 in caveolae microdomains. Conclusion ANP enhances transendothelial caveolae-mediated albumin transport via its GC-A receptor. This ANP-mediated cross-talk between the heart and the microcirculation is critically involved in the regulation of intravascular volume. KW - caveolin-1 KW - microvessel permeability KW - atrial natriuretic peptide Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126562 N1 - Lizenzhinweis: The online version of this article has been published under an open access model. Users are entitled to use, reproduce, disseminate, or display the open access version of this article for noncommercial purposes provided that the original authorship is properly and fully attributed; the Journal, Learned Society and Oxford University Press are attributed as the original place of publication with correct citation details given; if an article is subsequently reproduced or disseminated not in its entirety but only in part or as a derivative work this must be clearly indicated. VL - 93 IS - 1 ER - TY - JOUR A1 - Cheng, Cheng A1 - Othman, Eman M. A1 - Stopper, Helga A1 - Edrada-Ebel, RuAngelie A1 - Hentschel, Ute A1 - Abdelmohsen, Usama Ramadan T1 - Isolation of petrocidin A, a new cytotoxic cyclic dipeptide from the marine sponge-derived bacterium \(Streptomyces\) sp. SBT348 JF - Marine Drugs N2 - A new cyclic dipeptide, petrocidin A (\(\textbf{1}\)), along with three known compounds—2,3-dihydroxybenzoic acid (\(\textbf{2}\)), 2,3-dihydroxybenzamide (\(\textbf{3}\)), and maltol (\(\textbf{4}\))—were isolated from the solid culture of \(Streptomyces\) sp. SBT348. The strain \(Streptomyces\) sp. SBT348 had been prioritized in a strain collection of 64 sponge-associated actinomycetes based on its distinct metabolomic profile using liquid chromatography/high-resolution mass spectrometry (LC-HRMS) and nuclear magnetic resonance (NMR). The absolute configuration of all α-amino acids was determined by HPLC analysis after derivatization with Marfey’s reagent and comparison with commercially available reference amino acids. Structure elucidation was pursued in the presented study by mass spectrometry and NMR spectral data. Petrocidin A (\(\textbf{1}\)) and 2,3-dihydroxybenzamide (\(\textbf{3}\)) exhibited significant cytotoxicity towards the human promyelocytic HL-60 and the human colon adenocarcinoma HT-29 cell lines. These results demonstrated the potential of sponge-associated actinomycetes for the discovery of novel and pharmacologically active natural products. KW - biology KW - sponges KW - actinomycetes KW - streptomyces KW - cyclic dipeptide KW - cytotoxic Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-172644 VL - 15 IS - 12 ER - TY - JOUR A1 - Chilaka, Cynthia Adaku A1 - Obidiegwu, Jude Ejikeme A1 - Chilaka, Augusta Chinenye A1 - Atanda, Olusegun Oladimeji A1 - Mally, Angela T1 - Mycotoxin regulatory status in Africa: a decade of weak institutional efforts JF - Toxins N2 - Food safety problems are a major hindrance to achieving food security, trade, and healthy living in Africa. Fungi and their secondary metabolites, known as mycotoxins, represent an important concern in this regard. Attempts such as agricultural, storage, and processing practices, and creation of awareness to tackle the menace of fungi and mycotoxins have yielded measurable outcomes especially in developed countries, where there are comprehensive mycotoxin legislations and enforcement schemes. Conversely, most African countries do not have mycotoxin regulatory limits and even when available, are only applied for international trade. Factors such as food insecurity, public ignorance, climate change, poor infrastructure, poor research funding, incorrect prioritization of resources, and nonchalant attitudes that exist among governmental organisations and other stakeholders further complicate the situation. In the present review, we discuss the status of mycotoxin regulation in Africa, with emphasis on the impact of weak mycotoxin legislations and enforcement on African trade, agriculture, and health. Furthermore, we discuss the factors limiting the establishment and control of mycotoxins in the region. KW - fungi KW - mycotoxin KW - legislation KW - food safety KW - food security Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-278941 SN - 2072-6651 VL - 14 IS - 7 ER - TY - JOUR A1 - Christian, Gentzsch A1 - Seier, Kerstin A1 - Drakopoulos, Antonios A1 - Jobin, Marie-Lise A1 - Lanoiselée, Yann A1 - Koszegi, Zsombor A1 - Maurel, Damien A1 - Sounier, Rémy A1 - Hübner, Harald A1 - Gmeiner, Peter A1 - Granier, Sébastien A1 - Calebiro, Davide A1 - Decker, Michael T1 - Selective and Wash‐Resistant Fluorescent Dihydrocodeinone Derivatives Allow Single‐Molecule Imaging of μ‐Opioid Receptor Dimerization JF - Angewandte Chemie International Edition N2 - μ‐Opioid receptors (μ‐ORs) play a critical role in the modulation of pain and mediate the effects of the most powerful analgesic drugs. Despite extensive efforts, it remains insufficiently understood how μ‐ORs produce specific effects in living cells. We developed new fluorescent ligands based on the μ‐OR antagonist E‐p‐nitrocinnamoylamino‐dihydrocodeinone (CACO), that display high affinity, long residence time and pronounced selectivity. Using these ligands, we achieved single‐molecule imaging of μ‐ORs on the surface of living cells at physiological expression levels. Our results reveal a high heterogeneity in the diffusion of μ‐ORs, with a relevant immobile fraction. Using a pair of fluorescent ligands of different color, we provide evidence that μ‐ORs interact with each other to form short‐lived homodimers on the plasma membrane. This approach provides a new strategy to investigate μ‐OR pharmacology at single‐molecule level. KW - single-molecule microscopy KW - fluorescent probes KW - G-protein coupled receptor KW - homodimerization KW - opioid ligands Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-212398 VL - 59 IS - 15 ER - TY - THES A1 - Claßen, Alexandra T1 - The ERK-cascade in the pathophysiology of cardiac hypertrophy T1 - Die ERK-Kaskade in der Pathophysiologie der Herzhypertrophie N2 - ERK1/2 are known key players in the pathophysiology of heart failure, but the members of the ERK cascade, in particular Raf1, can also protect the heart from cell death and ischemic injury. An additional autophosphorylation (ERK1 at Thr208, ERK2 at Thr188) empowers ERK1/2 translocation to the nucleus and phosphorylation of nuclear targets which take part in the development of cardiac hypertrophy. Thereby, targeting this additional phosphorylation is a promising pharmacological approach. In this thesis, an in silico model of ERK cascade in the cardiomyocyte is introduced. The model is a semi-quantitive model and its behavior was tested with different softwares (SQUAD and CellNetAnalyzer). Different phosphorylation states of ERK1/2 as well as different stimuli can be reproduced. The different types of stimuli include hypertrophic as well as non-hypertrophic stimuli. With the introduced in-silico model time courses and synergistic as well as antagonistic receptor stimuli combinations can be predicted. The simulated time courses were experimentally validated. SQUAD was mainly used to make predictions about time courses and thresholds, whereas CNA was used to analyze steady states and feedback loops. Furthermore, new targets of ERK1/2 which partially contribute, also in the formation of cardiac hypertrophy, were identified and the most promising of them were illuminated. Important further targets are Caspase 8, GAB2, Mxi-2, SMAD2, FHL2 and SPIN90. Cardiomyocyte gene expression data sets were analyzed to verify involved components and to find further significantly altered genes after induced hypertrophy with TAC (transverse aortic constriction). Changes in the ultrastructure of the cardiomyocyte are the final result of induced hypertrophy. N2 - ERK1/2 sind bekannte Schlüsselfiguren bei der Entstehung der Herzinsuffizienz. Weitere Komponenten der ERK-Kaskade, insbesondere Raf1, können das Herz jedoch vor Zelltod und ischämischem Schaden schützen. Eine zusätzliche Autophosphorylierung von ERK1 an Thr208 bzw. von ERK2 an Thr188 ermöglicht ERK1/2 die Translokation zum Zellkern und befähigt ERK dort zur Phosphorylierung von nukleosolischen Zielproteinen, welche eine Herzmuskelhypertrophie auslösen. Daher erscheint diese zusätzliche Autophosphorylierung als eine vielversprechende pharmakologische Zielstruktur. In dieser Arbeit wird ein in-silico Modell der ERK-Kaskade im Kardiomyozyten präsentiert. Das Modell ist ein semi-quantitatives Modell und wurde mit den Programmen SQUAD und CellNetAnalyzer getestet. Verschiedene Phosphorylierungs-Zustände von ERK1/2 als auch verschiedene Stimuli (hypertrophe als auch nicht-hypertrophe) können mit dem Modell reproduziert werden. Mit dem präsentierten in-silico Modell können sowohl zeitliche Abläufe als auch synergistische und antagonistische Effekte vorhergesagt werden. Die simulierten zeitlichen Abläufe wurden durch in-vitro Experimente validiert. SQUAD wurde hauptsächlich für die Modellierung von zeitlichen Abläufen und Schwellenwerte genutzt, wohingegen CellNetAnalyzer vor allen Dingen zur Analyse von Fließgleichgewichten und Rückkopplungs-Mechanismen genutzt wurde. Darüberhinaus wurden Zielstrukturen von ERK1/2, welche zusätzlich an der Entstehung der Herzhypertrophie mitwirken, identifiziert. Diese umfassen unter anderem Caspase 8, GAB2, Mxi-2, SMAD2, FHL2 und SPIN90. Gen-Expressions-Datensätze von Kardiomyozyten nach TAC (transverse aortic constriction) wurden analysiert. Diese wurden mit den im Model vorhandenen Strukturen verglichen und signifikant veränderte Expressionslevel wurden identifiziert. Veränderungen der Ultrastruktur des Kardiomyozyten sind das Ergebnis der induzierten Hypertrophie. KW - Herzhypertrophie KW - Systembiologie KW - ERK-cascade KW - ERK-Kaskade KW - cardiac hypertrophy KW - in-silico model KW - In-silico Modell Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229664 ER - TY - JOUR A1 - Cristalli, G. A1 - Eleuteri, A. A1 - Vittori, S. A1 - Volpini, R. A1 - Lohse, M. J. A1 - Klotz, Karl-Norbert T1 - 2-Alkynyl derivatives of adenosine and adenosine-5'-N-ethyluronamides as selective agonists at A\(_2\) adenosine receptors N2 - In the search for more selective A2-receptor agonists and on the basis that appropriate substitution at C2 is known to impart selectivity for A\(_2\) receptors, 2-alkynyladenosines 2a-d were resynthesized and evaluated in radioligand binding, adenylate cycla.se, and platelet aggregation studies. Binding of [\(^3\)H]NECA to A\(_2\) receptors of rat striatal membranes was inhibited by compounds 2a-d with K\(_i\) values ranging from 2.8 to 16.4 nM. 2-Alkynyladenosines also exhibited high-affmity binding at solubilized A\(_2\) receptors from human platelet membranes. Competition of 2-alkynyladenosines 2a-d for the antagonist radioligand [\(^3\)H]DPCPX and for the agonist [\(^3\)H]CCPA gave K\(_i\) values in the nanomolar range, and the compounds showed moderate A\(_2\) selectivity. In order to improve this selectivity, the correaponding 2-alkynyl derivatives of adenosine-5'-N-ethyluronamide 8a-d were synthesized and tested. A\(_1\) expected, the 5'-N-ethyluronamide derivatives retained the A\(_2\) affinity whereas the A\(_1\) affinity was attenuated, resulting in an up to 10-fold increase in A\(_2\) selectivity. A similar patternwas observed in adenylate cyclase assays andin platelet aggregation studies. A 30- to 45-fold selectivity for platelet A\(_2\) receptors compared to A\(_1\) receptors was found for compounds 8a-c in adenylate cyclase studies. KW - Toxikologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60412 ER - TY - JOUR A1 - Cristalli, G. A1 - Franchetti, P. A1 - Grifantini, M. A1 - Vittori, S. A1 - Klotz, Karl-Norbert A1 - Lohse, M. J. T1 - Adenosine receptor agonists: Synthesis and biological evaluation of 1-deaza analogues of adenosine N2 - In a search for more selective A\(_1\) adenosine receptor agonists, N\(^6\)-[(R)-(-)-1-methyl-2-phenethyl]-1-deazaadenosine (1-deaza-R-PIA, 3a), N\(^6\)-cyclopentyl-1-deazaadenosine (1-deazaCPA, 3b), N\(^6\)-cyclohexyl-l-deazaadenosine (1-deazaCHA, Sc), and the corresponding 2-chloro derivatives 2a-c were synthesized from 5,7-dichloro-3-ß-D-ribofuranosyl-3Himidazo[ 4,5-b]pyridine (1). On the other band, N-ethyl-1'-deoxy-1'-(1-deaza-6-amino-9H-purin-9-yl)-ß-D-ribofuranuronamide (1-deazaNECA, 10) was prepared from 7-nitro-3-ß-D-ribofuranosyl-3H-imidazo[4,5-b]pyridine (4), in an attempt to find a more selective A\(_2\) agonist. The activity of all deaza analogues at adenosine receptors has been determined in adenylate cyclase andin radioligand binding studies. 1-DeazaNECA (10) proved tobe a nonselective agonist at both subtypes of the adenosine receptor. It is about 10-fold less active than NECA but clearly more active than the parent compound 1-deazaadenosine as an inhibitor of platelet aggregation and as a stimulator of cyclic AMP accumulation. The N\(^6\)-substituted 1-deazaadenosines largely retain the A\(_1\) agonist activity of their parent compounds, but lose some of their A\(_2\) agonist activity. This results in A\(_1\)-selective compounds, of which N\(^6\)cyclopentyl- 2-chloro-1-deazaadenosine (1-deaza-2-Cl-CPA, 2b) was identified as the most selective agonist at A\(_1\) adenosine receptors so far known. The activity of all 1-deaza analogues confirms that the presence of the nitrogen atom at position 1 of the purine ring is not critical for A\(_1\) receptor mediated adenosine actions. KW - Toxikologie Y1 - 1988 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60262 ER - TY - JOUR A1 - Dekant, Raphael A1 - Langer, Michael A1 - Lupp, Maria A1 - Adaku Chilaka, Cynthia A1 - Mally, Angela T1 - In vitro and in vivo analysis of ochratoxin A-derived glucuronides and mercapturic acids as biomarkers of exposure JF - Toxins N2 - Ochratoxin A (OTA) is a widespread food contaminant, with exposure estimated to range from 0.64 to 17.79 ng/kg body weight (bw) for average consumers and from 2.40 to 51.69 ng/kg bw per day for high consumers. Current exposure estimates are, however, associated with considerable uncertainty. While biomarker-based approaches may contribute to improved exposure assessment, there is yet insufficient data on urinary metabolites of OTA and their relation to external dose to allow reliable estimates of daily intake. This study was designed to assess potential species differences in phase II biotransformation in vitro and to establish a correlation between urinary OTA-derived glucuronides and mercapturic acids and external exposure in rats in vivo. In vitro analyses of OTA metabolism using the liver S9 of rats, humans, rabbits and minipigs confirmed formation of an OTA glucuronide but provided no evidence for the formation of OTA-derived mercapturic acids to support their use as biomarkers. Similarly, OTA-derived mercapturic acids were not detected in urine of rats repeatedly dosed with OTA, while indirect analysis using enzymatic hydrolysis of the urine samples prior to LC–MS/MS established a linear relationship between urinary glucuronide excretion and OTA exposure. These results support OTA-derived glucuronides but not mercapturic acids as metabolites suitable for biomonitoring. KW - ochratoxin A KW - biomarker of exposure KW - glucuronide KW - mercapturic acid KW - mycotoxin Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-245146 SN - 2072-6651 VL - 13 IS - 8 ER - TY - JOUR A1 - Dekant, Wolfgang A1 - Bridges, James T1 - Assessment of reproductive and developmental effects of DINP, DnHP and DCHP using quantitative weight of evidence JF - Regulatory Toxicology and Pharmacology N2 - Quantitative weight of evidence (QWoE) methodology utilizes detailed scoring sheets to assess the quality/reliability of each publication on toxicity of a chemical and gives numerical scores for quality and observed toxicity. This QWoE-methodology was applied to the reproductive toxicity data on diisononylphthalate (DINP), di-n-hexylphthalate (DnHP), and dicyclohexylphthalate (DCHP) to determine if the scientific evidence for adverse effects meets the requirements for classification as reproductive toxicants. The scores for DINP were compared to those when applying the methodology DCHP and DnHP that have harmonized classifications. Based on the quality/reliability scores, application of the QWoE shows that the three databases are of similar quality; but effect scores differ widely. Application of QWoE to DINP studies resulted in an overall score well below the benchmark required to trigger classification. For DCHP, the QWoE also results in low scores. The high scores from the application of the QWoE methodology to the toxicological data for DnHP represent clear evidence for adverse effects and justify a classification of DnHP as category 1B for both development and fertility. The conclusions on classification based on the QWoE are well supported using a narrative assessment of consistency and biological plausibility. KW - n-hexyl phthalate KW - male rats KW - dicyclohexyl phthalate KW - Diisononyl phthalate KW - in-vivo KW - 2-Generation reproduction KW - testosterone production KW - sexual development KW - risk-assesment KW - fetal testis KW - weight of evidence KW - classification and labeling KW - reproductive and developmental toxicity KW - quantitative assessments Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-186750 VL - 81 ER - TY - JOUR A1 - Dekant, Wolfgang A1 - Klaunig, James E. T1 - Toxicology of decamethylcyclopentasiloxane (D5) JF - Regulatory Toxicology and Pharmacology N2 - Decamethylcyclopentasiloxane (D5) is a cyclic siloxane used in the formulation of consumer products as well as an industrial intermediate. A summary of the previous studies on the toxicology of D5 is provided. Toxicokinetic studies with D5 after dermal administration demonstrate a very low uptake of due to rapid evaporation. Following inhalation exposure, exhalation of unchanged D5 and excretion of metabolites with urine are major pathways for clearance in mammals. Due to this rapid clearance by exhalation, the potential for bioaccumulation of D5 is considered unlikely. The available toxicity data on D5 adequately cover the relevant endpoints regarding potential human health hazards. D5 was not DNA reactive or mutagenic in standard in vitro and in vivo test systems. D5 also did not induce developmental and reproductive toxicity in appropriately performed studies. In repeated studies in rats with subacute, subchronic and chronic inhalation exposure, mild effects on the respiratory tract typically seen after inhalation of irritating materials, increases in liver weight (28- and 90-day inhalation studies), and a small increase in the incidence of uterine adenocarcinoma (uterine tumor) in female rats (two-year inhalation chronic bioassay) were observed. The liver effects induced by D5 were consistent with D5 as a weak "phenobarbital-like" inducer of xenobiotic metabolizing enzymes and these effects are considered to be an adaptive response. Mechanistic studies to elucidate the mode-of-action for uterine tumor induction suggest an interaction of D5 with dopamine signal transduction pathways altering the pituitary control of the estrus cycle. The resulting estrogen imbalance may cause the small increase in uterine tumor incidence at the highest D5-exposure concentration over that seen in control rats. A genotoxic mechanism or a direct endocrine activity of D5 is not supported as a mode-of-action to account for the induction of uterine tumors by the available data. KW - Prolactin KW - Fischer 344 rats KW - MMQ cells KW - Reproductive toxicity KW - Carcinogenicity KW - Silicones KW - Enzyme induction Y1 - 2016 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190914 VL - 74 IS - Supplement ER - TY - JOUR A1 - Djelić, Ninoslav A1 - Borozan, Sunčica A1 - Dimitrijević-Srećković, Vesna A1 - Pajović, Nevena A1 - Mirilović, Milorad A1 - Stopper, Helga A1 - Stanimirović, Zoran T1 - Oxidative stress and DNA damage in peripheral blood mononuclear cells from normal, obese, prediabetic and diabetic persons exposed to thyroid hormone in vitro JF - International Journal of Molecular Sciences N2 - Diabetes, a chronic group of medical disorders characterized byhyperglycemia, has become a global pandemic. Some hormones may influence the course and outcome of diabetes, especially if they potentiate the formation of reactive oxygen species (ROS). There is a close relationship between thyroid disorders and diabetes. The main objective of this investigation was to find out whether peripheral blood mononuclear cells (PBMCs) are more prone to DNA damage by triiodothyronine (T\(_3\)) (0.1, 1 and 10 μM) at various stages of progression through diabetes (obese, prediabetics, and type 2 diabetes mellitus—T2DM persons). In addition, some biochemical parameters of oxidative stress (catalase-CAT, thiobarbituric acid reactive substances—TBARS) and lactate dehydrogenase (LDH) were evaluated. PBMCs from prediabetic and diabetic patients exhibited increased sensitivity for T\(_3\) regarding elevated level of DNA damage, inhibition of catalase, and increase of TBARS and LDH. PBMCs from obese patients reacted in the same manner, except for DNA damage. The results of this study should contribute to a better understanding of the role of thyroid hormones in the progression of T2DM. KW - diabetes KW - oxidative stress KW - DNA damage KW - lymphocytes KW - thyroid hormone Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285988 SN - 1422-0067 VL - 23 IS - 16 ER - TY - THES A1 - Duraphe, Prashant T1 - Identification and characterization of AUM, a novel human tyrosine phosphatase T1 - Identifizierung und Charakterisierung von AUM, einer neuen humanen Tyrosin-Phosphatase N2 - Protein Phosphatasen werden aufgrund der Aminosäuresequenzen ihrer aktiven Zentren in drei große Familien unterteilt. In einer neu entdeckten Familie von Phosphatasen ist das aktive Zentrum durch die Sequenz DXDX(T/V) charakterisiert. Diese Aspartat-abhängigen Phosphatasen gehören zu der Superfamilie der Hydrolasen vom Haloazid Dehalogenase(HAD)-Typ, einer evolutionär konservierten und ubiquitär verbreiteten Enzymfamilie. Bislang konnten 58 menschliche HAD Enzyme durch Datenbankanalysen identifiziert werden. Ihre Funktionen sind jedoch nach wie vor nur rudimentär verstanden. Im Rahmen dieser Arbeit wurde zunächst das Komplement aller menschlichen HAD Phosphatasen durch Datenbank-Recherchen erfasst. Zusammen mit phylogenetischen Analysen gelang es, eine zum damaligen Zeitpunkt unbekannte, putative Phosphatase zu identifizieren, die eine vergleichsweise hohe Sequenz-Homologie zu der Zytoskelettregulierenden HAD Phosphatase Chronophin aufweist. Dieses neuartige Enzym wurde kloniert und mit biochemischen und zellbiologischen Methoden charakterisiert. Auf der Basis dieser Befunde bezeichnen wir dieses neuartige Protein als AUM (actin remodeling, ubiquitously expressed, magnesium-dependent HAD phosphatase).Mittels Northern blot, real-time PCR und Western blot Analysen konnte gezeigt werden, dass AUM in allen untersuchten menschlichen und murinen Geweben exprimiert wird. Die höchste Expression konnte in Hodengewebe nachgewiesen werden. Durch immunohistochemische Untersuchungen konnte gezeigt werden, dass AUM spezifisch in reifenden Keimzellen mit einem Expressionsmaximum zum Zeitpunkt der Spermiogenese exprimiert wird. Um die Substratpräferenz von AUM zu charakterisieren, wurde zunächst ein peptidbasierter in vitro Phosphatase-Substrat-Screen durchgeführt. Hierbei wurden 720 aus menschlichen Phosphoproteinen abgeleitete Phosphopeptide untersucht. Interessanterweise dephosphorylierte AUM ausschließlich Phosphotyrosin (pTyr)-enthaltende Peptide. Nur 17 pTyr-Peptide (~2% aller untersuchten Peptide) fungierten als AUM-Substrate. Diese Daten legen eine hohe Substratspezifität von AUM nahe. Zu den putativen AUM Substraten gehören Proteine, die in die Dynamik der Zytoskelett-Reorganisation sowie in Tyrosin Kinasevermittelte Signalwege eingebunden sind. In Übereinstimmung mit den Ergebnissen dieses Phosphopeptid-Screens konnte mittels Phosphatase overlay assays sowie in Zellextrakten aus Pervanadat-behandelten HeLa Zellen demonstriert werden, dass AUM eine begrenzte Anzahl Tyrosin-phosphorylierter Proteinen dephosphorylieren kann.In zellulären Untersuchungen wurde die mögliche Rolle von AUM im Rahmen der durch den epidermalen Wachstumsfaktor (EGF) ausgelösten Tyrosin-Phosphorylierung in einer Spermatogonien Zelllinie (GC-1 spg-Zellen) analysiert. So konnte nachgewiesen werden, dass die Überexpression von AUM zu einer moderaten Abnahme Tyrosin phosphorylierter Proteine nach EGF-Stimulation führte. Im Gegensatz dazu löste jedoch die durch RNAInterferenz vermittelte Depletion von endogenem AUM einen robusten Anstieg Tyrosinphosphorylierter Proteine aus, zu denen auch der EGF-Rezeptor selbst zählt. Zusätzlich zu dem EGF-Rezeptor wurde die Src-Kinase im Zuge des Phosphopeptid- Screens als mögliches AUM Substrat identifiziert. Daher wurden in vitro Kinase/Phosphatase-Assays mit gereinigtem Src und AUM durchgeführt. Mit diesem Ansatz konnte erstmals gezeigt werden, dass AUM in der Lage ist, die Src-Kinase zu aktivieren, während Src AUM phosphoryliert und die AUM Phosphatase-Aktivität blockiert. Diese Ergebnisse deuten auf eine gekoppelte, wechselseitige Regulation von AUM und Src hin. Obwohl die Details dieser Regulation derzeit noch unklar sind, zeigen unsere initialen Ergebnisse, dass AUM die Src-Aktivität unabhängig von seiner Phosphatase Aktivität steigert, während Src die AUM Phosphatase-Aktivität Kinase-abhängig vermindert. Auf zellulärer Ebene sind AUM-depletierte Zellen durch Veränderungen der Aktin- Zytoskelett-Dynamik und der Zelladhäsion charakterisiert. So weisen AUM-defiziente Zellen stabilisierte Aktin Streßfasern und vergrößerte fokale Adhäsionen auf. Weiterhin sind AUMdepletierte Zellen durch ein beschleunigtes spreading auf Fibronektin gekennzeichnet. Wir haben mit AUM ein bisher nicht beschriebenes Mitglied der Familie Aspartat-abhängiger Phosphatasen entdeckt. In dieser Arbeit ist es gelungen, AUM phylogenetisch, biochemisch und zellbiologisch zu charakterisieren. Unsere Ergebnisse legen nahe, dass AUM einen wichtigen, neuartigen Regulator der Src-vermittelten Zytoskelett-Dynamik im Rahmen der Zelladhäsion und Migration darstellt. N2 - Protein phosphatases can be classified into at least three major families based on amino acid sequences at their active sites. A newly emerging phosphatase family contains the active site sequence DXDX(T/V), and belongs to the haloacid dehalogenase (HAD) superfamily of hydrolases, a ubiquitous and evolutionarily conserved enzyme family. Although the existence of 58 human HAD enzymes has been predicted by database analysis, our understanding of their biological functions remains rudimentary.By database mining amd phylogenetic analysis of human HAD phosphatases, we have found a marked increase in cell area of spreading cells, as well as accelerated cell spreading onfibronectin. Taken together, we have identified and characterized AUM as a novel member of the emerging family of aspartate-dependent protein tyrosine phosphatases. Our findings implicate AUM as an important regulator of Src-dependent cytoskeletal dynamics during cell adhesion and migration. a previously unidentified enzyme with homology to Chronophin, a cytoskeletal regulatory HAD phosphatase. We have cloned and characterized this novel enzyme and named it AUM,for actin remodeling, ubiquitously expressed, magnesium-dependent HAD phosphatase. By Northern blot, real-time PCR and Western blot analysis, we show that AUM is broadly expressed in all major human and mouse tissues with highest levels found in testis. Using immunohistochemistry, we can show that AUM is specifically expressed in maturing germ cells and that its expression peaks during spermiogenesis. To characterize the substrate preference of AUM, we have conducted an in vitro phosphatase substrate screen with 720 phosphopeptides derived from human phosphorylation sites. AUM exclusively dephosphorylates phosphotyrosine (pTyr)-containing peptides. Furthermore, only 17 pTyr peptides (~2% of all pTyr peptides investigated) acted as AUM substrates, indicating a high degree of substrate specificity. Putative AUM substrates include proteins involved in cytoskeletal dynamics and tyrosine kinase signaling.In accordance with the phosphopeptide screen, phosphatase overlay assays employing whole-cell extracts of pervanadate-treated HeLa cells show that AUM dephosphorylates only a limited number of tyrosyl-phosphorylated proteins.The role of AUM for cellular signaling was investigated in response to epidermal growth factor (EGF) stimulation in a spermatogonial cell line (GC-1 spg). The overexpression of AUM reduces, whereas the RNAi-mediated depletion of endogenous AUM increases EGF inducedtyrosine phosphorylation, including changes in the phosphorylation of the EGF receptor itself. Interestingly, in vitro kinase/phosphatase assays with purified Src and AUM indicate that AUM can activate Src, which in turn phosphorylates and inactivates AUM. Although it is at present unclear how Src and AUM regulate each other, our initial findings suggests that AUM enhances Src kinase activity independently of its phosphatase activity, whereas Src diminishes AUM phosphatase activity in a kinase dependent manner. On a cellular level, AUM-depleted cells are characterized by altered actin cytoskeletal dynamics and adhesion, as indicated by stabilized actin filaments, enlarged focal adhesions,a marked increase in cell area of spreading cells, as well as accelerated cell spreading on fibronectin. Taken together, we have identified and characterized AUM as a novel member of the emerging family of aspartate-dependent protein tyrosine phosphatases. Our findings implicate AUM as an important regulator of Src-dependent cytoskeletal dynamics during cell adhesion and migration. KW - Tyrosin KW - Phosphatase KW - Signal transduction KW - Cell adhesion KW - Actin cytoskeleton KW - Src KW - Spermatogenesis Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-44256 ER - TY - JOUR A1 - Däniken, A. von A1 - Friederich, U. A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Tests for mutagenicity in Salmonella and covalent binding to DNA and protein in the rat of the riot control agent o-chlorobenzylidene malononitrile (CS) N2 - The aim of this study was to determine whether o-chlorobenzylidene malononitrile ( CS) exhibits any genotoxic activity towards Salmonella or mammalian DNA in vivo. CS was synthesized with a [\(^{14}\)C]-label at the benzylic carbon atom. It was administered i. p. at a dose level of 13 mg/kg (1 mCi/kg) to young adult male rats. Liverand kidney DNA was isolated after 8, 25, and 75 h. The radioactivity was at (liver, 8 and 75 h) or below (all other samples) the limit of detection of 3 dpm. Therefore, a possible binding of CS to DNA is at least 10\(^5\) times lower than that of the strong hepatocarcinogen aflatoxin B1, and 4,000 times lower than that of vinyl chloride. In contrast to this lack of DNA binding, but in agreement with the chemical reactivity of CS, a binding to nuclear proteins could be detected with specific activities ranging between 50 and 121 dpm/mg for liver and between 3 and 41 dpm/mg for kidney. Protein binding could well be responsible for its pronounced cytotoxic effects. Cs was also tested in the Ames Salmonella/microsome assay. Strains TA 1535, TA 1537, TA 1538, TA 98, and TA 100 were used with or without pre-incubation. Only with strain TA 100 and only without pre-incubation, a doubling of the number of revertants was detectable at the highest dose Ievels used, 1,000 and 2,000 !lg CS per plate. With pre-incubation of TA 100 with CS, a slight increase of the number of revertants was seen at 100 and 500 !lg per plate, and a subsequent fall below control values at 1,000 J.tg. A check for the number of surviving bacteria revealed a strong bacteriotoxicity of the higher doses of es so that the calculated mutation frequencies, i.e., the oumber of revertants per number of surviving bacteria, increased with doses up to 500 !J.g. This toxicity could be counteracted in part by the addition of increasing amounts of rat liver microsomes. In the view of these results, and taking into account the rare and low exposure of man, it is concluded that CS will not create a risk for the induction of point mutations or of carcinogenic processes mediated by DNA binding. KW - Toxikologie KW - o-Chlorobenzylidene malononitrile KW - Riot control agents KW - DNA Binding KW - Salmonella/microsome assay KW - Carcinogens KW - Mutagens Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61073 ER - TY - JOUR A1 - Däniken, A. von A1 - Lutz, Werner K. A1 - Jäckh, R. A1 - Schlatter, C. T1 - Investigation of the potential for binding of Di(2-ethylhexyl) phthalate (DEHP) and Di(2-ethylhexyl) adipate (DEHA) to liver DNA in vivo N2 - Investigation of the Potential for Binding of Di(2-ethylhexyl) Phthalate (DEHP) and Di(2- ethylhexyl) Adipate (DEHA) to Liver DNA in Vivo. VON DÄNIKEN, A., LUTZ, W. K., JÄCKH, R., AND ScHLATTER, C. (1984). Toxico/. App/. Pharmaco/. 73, 373-387. It was the aim oftbis investigation to determine whether covalent binding of di(2-ethylhexyl) phthalate (DEHP) to rat liver DNA and of di(2-ethylhexyl) adipate (DEHA) to mouse liver DNA could be a mechanism of action contributing to the observed induction of liver tumors after lifetime feeding of the respective rodent species with high doses of DEHP and DEHA. For this purpose, DEHP and DEHA radiolabeled in different parts of the molecule were administered orally to female rats and mice, respectively, with or witbout pretreatment for 4 weeks with 1% unlabeled compound in the diet. Liver DNA was isolated after 16 hr and analyzed for radioactivity. The data were converted to a covalent binding index, CBI = (micromoles of substance bound per mole of DNA nucleotides)/(millimoles of substance applied per kilogram body weight), in order to allow a quantitative comparison also with other carcinogens and noncarcinogens. Administration of [\(^{14}\)H]carboxylate-labeled DEHP to rats resulted in no measurable DNA radioactivity. The Iimit of detection, CBI < 0.02 was about 100 times below the CBI of compounds where an observable tumor-inducing potential could be due to genotoxicity. With [\(^{14}\)C]- and [\(^{3}\)H]DEHP labeled in the alcohol moiety, radioactivity was clearly measurable in rat liver DNA. HPLC analysis of enzyme-degraded or acid-hydrolyzed DNA revealed that the natural nucleosides or purine bases were radiolabeled whereas no radioactivity was detectable in those fractions where tbe carcinogenmodified nucleoside or base adducts are expected. The respective Iimits of detection were at 0.07 and 0.04 CBI units for the \(^{14}\)C and \(^{3}\)H Iabels, respectively. The experiments with [\(^{14}\)C]- and [\(^{3}\)H]DEHA, labeled in the alcobol moiety and administered to mice, revealed aminute radioactivity of <50 dpm/mg liver DNA, too little to allow a nucleoside analysis to determine that fraction of the radioactivity which bad been incorporated via biosynthesis. Expressed in the CBI units, values of 0.05 to 0.15 for \(^{14}\)C and 0.01 to 0.12 for \(^{3}\)H resulted. Determination of the level· of \(^{14}\)C02 expiration revealed a linear correlation with the speciftc activity of DNA. Experiments with 2-ethyl[ 1-\(^{14}\)C]hexanol perfonned with both rats and mice allowed the conclusion tbat most if not all DEHA radioactivity in mouse liver DNA was due to biosynthetic incorporation. A maximum possible true DNA binding by DEHA must be below CBI 0.01. Pretreatment of the animals witb unlabeled compound bad no effect on the DNA radioactivities in either species. The present negative data, in conjunction witb other negative short-term tests for mutagenicity, strongly indicate that covalent interaction with DNA is highly unlikely to be the mode of tumorigenic action of DEHP and DEHA in rodents. KW - Toxikologie Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61004 ER - TY - JOUR A1 - Däniken, A. von A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Lack of covalent binding to rat liver DNA of the hypolipidemic drugs clofibrate and fenofibrate N2 - \(^{14}\)C-Labelled clofibric acid and fenofibric acid were administered p.o. to 200 g male and female rats. After 10 h, liver nuclear DNA and protein were isolated and the radioactivity was determined. Binding to protein was clearly measurable whereas no binding to DNA could be detected from any drug. A comparison of the Iimit of detection of such DNA binding with well-known chemical carcinogens revealed that the known hepatocarcinogenicity of clofibrate cannot be based upon an initiating, DNA damaging, mode of action but must be due to other, nongenotoxic, mechanisms such as peroxisome proliferation, hepatomegaly, or cytotoxicity due to protein binding. The risk assessment in man and the interpretation of the carcinogenicity data for rodents are discussed. KW - Toxikologie Y1 - 1981 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61087 ER - TY - JOUR A1 - Eberl, Hanna A1 - Rebs, Sabine A1 - Hoppe, Stefanie A1 - Sedaghat-Hamedani, Farbod A1 - Kayvanpour, Elham A1 - Meder, Benjamin A1 - Streckfuss-Bömeke, Katrin T1 - Generation of an RBM20-mutation-associated left-ventricular non-compaction cardiomyopathy iPSC line (UMGi255-A) into a DCM genetic background to investigate monogenetic cardiomyopathies JF - Stem Cell Research N2 - RBM20 mutations account for 3 % of genetic cardiomypathies and manifest with high penetrance and arrhythmogenic effects. Numerous mutations in the conserved RS domain have been described as causing dilated cardiomyopathy (DCM), whereas a particular mutation (p.R634L) drives development of a different cardiac phenotype: left-ventricular non-compaction cardiomyopathy. We generated a mutation-induced pluripotent stem cell (iPSC) line in which the RBM20-LVNC mutation p.R634L was introduced into a DCM patient line with rescued RBM20-p.R634W mutation. These DCM-634L-iPSC can be differentiated into functional cardiomyocytes to test whether this RBM20 mutation induces development of the LVNC phenotype within the genetic context of a DCM patient. KW - cell biology KW - developmental biology KW - general medicine KW - RBM20 mutations KW - DCM genetic background KW - monogenetic cardiomyopathies Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350565 SN - 1873-5061 VL - 74 ER - TY - THES A1 - Emami-Nemini, Alexander Darius T1 - Differential parathyroid hormone receptor signaling directed by adaptor proteins T1 - Steuerung differenzieller Signalgebung des Parathormon Rezeptors durch Adapterproteine N2 - The superfamily of G protein-coupled receptors (GPCR) regulates numerous physiological and pathophysiological processes. Hence GPCRs are of significant interest for pharmacological therapy. Embedded into cytoplasmic membranes, GPCRs represent the core of large signaling complexes, which are critical for transduction of exogenous stimuli towards activation of downstream signaling pathways. As a member of the GPCR family B, the parathyroid hormone receptor (PTHR) activates adenylyl cyclases, phospholipases C β as well as mitogen-activated protein kinase-dependent signaling pathways, thereby mediating endocrine and paracrine effects of parathyroid hormone (PTH) and parathyroid hormone-related peptide (PTHrP), respectively. This regulates, calcium homeostasis, bone metabolism and bone development. Paradoxically, PTH is able to induce both catabolic and anabolic bone metabolism. The anabolic effect of PTH is successfully applied in the therapy of severe osteoporosis. Domination of anabolic or catabolic bone-metabolism is entailed by temporal and cell-type specific determinants. The molecular bases are presumably differential arrangements of adaptor proteins within large signaling complexes that may lead to differential activation of signaling pathways, thereby regulating physiological effects. The molecular mechanisms are largely unclear; thus, there is significant interest in revealing a better understanding of PTHR-related adaptor proteins. To identify novel adaptor proteins which direct PTHR signaling pathways, a proteomic screening approach was developed. In this screening, vav2, a guanine-nucleotide exchange factor (GEF) for small GTPases which regulates cytoskeleton reorganization, was found to interact with intracellular domains of PTHR. Evidence is provided that vav2 impairs PTH-mediated phospholipase C β (PLCβ) signaling pathways by competitive interactions with G protein αq subunits. Vice versa, PTH was shown to regulate phosphorylation and subsequent GEF activity of vav2. These findings may thus shed new light on the molecular mechanisms underlying the effects of PTH on bone metabolism by PLC-signaling, cell migration and cytoskeleton organization. In addition to the understanding of intracellular molecular signaling processes, screening for ligands is a fundamental and demanding prerequisite for modern drug development. To this end, ligand binding assays represent a fundamental technique. As a substitution for expensive and potentially harmful radioligand binding, fluorescence-based ligand-binding assays for PTHR were developed in this work. Based on time-resolved fluorescence, several assay variants were established to facilitate drug development for the PTHR. N2 - Die Superfamilie der G-Protein-gekoppelten Rezeptoren (GPCRs) reguliert eine Vielzahl von physiologischen und pathophysiologischen Prozessen, was sie bedeutend für die Pharmakotherapie macht. Eingebettet in die Zytoplasmamembran sind GPCRs das Zentrum von Signalkomplexen, die eine Transduktion äußerer Stimuli zur Aktivierung von nachgeschalteten Signalwegen ermöglichen. Der zur Familie B der GPCRs gehörige Parathormon-Rezeptor (PTHR) aktiviert Adenylyl-Zyklasen-, Phospholipasen Cβ- und Mitogen-aktivierte Proteinkinase (MAPK)-abhängige Signalwege, wodurch endokrine und parakrine Wirkungen des Parathormons (PTH) und des Parathormon-ähnlichen Peptides (PTHrP) vermittelt werden. Dies ermöglicht die Regulation der Calcium-Homöostase, des Knochenmetabolismus und der Knochenentwicklung. Paradoxerweise kann PTH sowohl katabole als auch anabole Effekte auf den Knochenstoffwechsel induzieren. Den anabolen Effekt von PTH nutzt man erfolgreich in der Therapie der schweren Osteoporose. Ob ein anaboler oder kataboler Knochenmetabolismus überwiegt, wird durch zeitliche und Zelltyp-spezifische Faktoren bestimmt. Dem zugrunde liegt vermutlich unter anderem eine differenzielle Anordnung verschiedener Adapterproteine innerhalb der Signalkomplexe, die zur differenziellen Aktivierung von Signalwegen führen und so eine Steuerung bestimmter physiologischer Effekte ermöglichen. Die molekularen Mechanismen sind jedoch noch weitgehend unklar, weshalb großes Interesse besteht, ein besseres Verständnis über die PTHR-assoziierten Adapterproteine zu entwickeln. Zur Identifizierung neuer Adapterproteine, die PTHR-Signalwege beeinflussen, wurde in dieser Arbeit ein auf dem Proteom-basierender Screening-Ansatz entwickelt. Dieser führte zur Entdeckung einer Interaktion von intrazellulären Domänen des PTHR mit vav2, einem Guanin-Nukleotid Austauschfaktor (GEF) für kleine GTPasen, der die Zytoskelett-Reorganisation steuert. Des Weiteren wurde nachgewiesen, dass vav2 über kompetitive Interaktionen mit G Protein αq Untereinheiten PTH-vermittelte Phospholipase Cβ (PLCβ)-abhängige Signalwege beeinflusst. Umgekehrt wurde gezeigt, dass PTH die Phosphorylierung und damit die GEF Aktivität von vav2 reguliert. Diese Befunde können Aufschluss über molekulare Mechanismen geben, die den Wirkungen von PTH auf den Knochenstoffwechsel durch PLC-Signalwege, Zellmigration und Zytoskelett-Reorganisation zugrunde liegen. Neben dem Verständnis über molekulare Prozesse der intrazellulären Signalgebung ist die Suche nach Liganden eine herausfordernde Grundvoraussetzung für die aktuelle Arzneistoffentwicklung. Liganden-Bindungs-Experimente stellen dafür elementare Techniken dar. Zur Substitution kostenintensiver und potentiell gesundheitsschädlicher Radioliganden-Bindungen, wurden in dieser Arbeit Fluoreszenz-basierte Liganden-Bindungs-Experimente für den PTHR entwickelt. Basierend auf Zeit-aufgelöster Fluoreszenz wurden mehrere Varianten dieser Experimente etabliert, um die Arzneistoffentwicklung am PTHR zu unterstützen. KW - G-Protein gekoppelte Rezeptoren KW - Parathormon KW - G-Protein gekoppelte Rezeptoren KW - Parathormon KW - vav2 KW - Guanin Nukleotid Austauschfaktor KW - G protein coupled receptor KW - parathyroid hormone KW - vav2 KW - guanine nucleotide exchange factor KW - Guaninnucleotid-Austauschfaktoren Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-72369 ER - TY - THES A1 - Eman, Maher Othman Sholkamy T1 - In Vitro and In Vivo Analysis of Insulin-Induced Oxidative Stress and DNA Damage T1 - In vitro und in vivo Untersuchungen von Insulin-induzierten oxidativen Stress und DNA-Schäden N2 - Hyperinsulinemia, a condition with excessively high insulin blood levels, is related to an increased cancer incidence. Diabetes mellitus, metabolic syndrome, obesity and polycystic ovarian syndrome are the most common of several diseases accompanied by hyperinsulinemia. Since an elevated cancer risk especially for colon and kidney cancers, was reported for those patients, we investigated for the first time the induction of genomic damage by insulin mainly in HT29 (human colon cells), LLC-PK1 (pig kidney cells), HK2 (human kidney cells) and peripheral lymphocytes, and to confirm the genotoxicity of insulin in other cells from different tissues. To ascertain that the insulin effects were not only limited to permanent cell lines, rat primary colon, kidney, liver and fatty tissue cells were also studied. To connect the study and the findings to in vivo conditions, two in vivo models for hyperinsulinemia were used; Zucker diabetic fatty rats in a lean and diabetic state infused with different insulin concentrations and peripheral lymphocytes from type 2 diabetes mellitus patients. First, the human colon adenocarcinoma cells (HT29) showed significant elevation of DNA damage using comet assay and micronucleus frequency analysis upon treatment with 5 nM insulin in standard protocols. Extension of the treatment to 6 days lowered the concentration needed to reach significance to 0.5-1 nM. Insulin enhanced the cellular ROS production as examined by the oxidation of the dyes 2´,7´-dichlorodihydrofluorescein diacetate (H2DCF-DA) and dihydroethidium (DHE). The FPG modified comet assay and the reduction of damage by the radical scavenger tempol connected the insulin-mediatedDNA damage to ROS production. To investigate the sources of ROS upon insulin stimulation, apocynin and VAS2870 as NADPH oxidase inhibitors and rotenone as mitochondrial inhibitor were applied in combination with insulin and all of them led to a reduction of the genomic damage. Investigation of the signaling pathway started by evaluation of the binding of insulin to its receptor and to the IGF-1 receptor. The results showed the involvement of both receptors in the signaling mechanism. Following the activation of both receptors, PI3K activation occurs leading to phosphorylation of AKT which in turn activates two pathways for ROS production, the first related to mitochondria and the second through activation of Rac1 , resulting in the activation of Nox1. Both pathways could be activated through AKT or through the mitochondrial ROS which in turn could activates Nox1. Studying another human colon cancer cell line, Caco-2 and rat primary colon cells in vitro confirmed the effect of insulin on cellular chromatin. We conclude that pathophysiological levels of insulin can cause DNA damage in colon cells, which may contribute to the induction or progression of colon cancer. Second, in kidney cells, insulin at a concentration of 5 nM caused a significant increase in DNA damage in vitro. This was associated with the formation of reactive oxygen species (ROS). In the presence of antioxidants, blockers of the insulin and IGF-1 receptors, and a phosphatidylinositol 3-kinases (PI3K) inhibitor, the insulin mediated DNA damage was reduced. Phosphorylation of AKT was increased and p53 accumulated. Inhibition of the mitochondrial and NADPH oxidase related ROS production reduced the insulin mediated damage. In primary rat cells insulin also induced genomic damage. HK2 cells were used to investigate the mechanistic pathway in the kidney The signaling is identical to the one in the colon cells untill the activation of the mitochondrial ROS production, because after the activation of PI3K activation of Nox4 occurs at the same time across talk between mitochondria and Nox4 activation has been suggested and might play a role in the observed effects. In the in vivo model, kidneys from healthy, lean ZDF rats, which were infused with insulin to yield normal or high blood insulin levels, while keeping blood glucose levels constant, the amounts of ROS and p53 were elevated in the high insulin group compared to the control level group. ROS and p53 were also elevated in diabetic obese ZDF rats. The treatment of the diabetic rats with metformin reduced the DNA oxidation measured as 8-oxodG as well as the ROS production in that group. HL60 the human premyelocytic cells and cultured lymphocytes as models for the hemopoietic system cells showed a significant induction for DNA damage upon treatment with insulin. The diabetic patients also exhibited an increase in the micronucleus formation over the healthy individuals. In the present study, we showed for the first time that insulin induced oxidative stress resulting in genomic damage in different tissues, and that the source of the produced ROS differs between the tissues. If the same mechanisms are active in patients, hyperinsulinemia might cause genomic damage through the induction of ROS contributing to the increased cancer risk, against which the use of antioxidants as well as mitochondrial and NADPH oxidase inhibitors might exert protective effects with cancer preventive potential under certain conditions. Normal healthy human plasma insulin concentrations are in the order of 0.04 nM after overnight fasting and increase to less than about 0.2 nM after a meal. Pathophysiological levels can reach 1 nM and can stay above 0.2 nM for the majority of the daytime yielding condictions close to the insulin concentrations determined in the present study. Whether the observed effects also occur in vivo and whether they actually initiate or promote tumor formation remains to be determined. However, if proof of that can be obtained, our experiments with inhibitors indicate chances for pharmacological intervention applying antioxidants or enzyme inhibitors. It will not be the aim to reduce ROS in any case or as much as possible because ROS have now been recognized as important signaling molecules and participatants in immune defense, but a reduction to physiological levels instead of pathophysiological levels in the context of a disease associated with ROS overproduction might be beneficial. N2 - Hyperinsulinämie, ein Zustand mit sehr hohen Blutspiegeln an Insulin, ist mit einer erhöhten Krebsinzidenz verbunden. Diabetes mellitus, das metabolische Syndrom, Adipositas und das polyzystische Ovarialsyndrom sind die häufigsten Krankheiten, die mit Hyperinsulinämie einhergehen. Da ein erhöhtes Krebsrisiko insbesondere für Krebserkrankungen des Dickdarms und der Niere beobachtet wurde, untersuchten wir erstmals die Induktion von Genomschäden durch Insulin in HT29-Zellen (humane Dickdarmzellen), LLC-PK1-Zellen (Nierenzellen vom Schwein), HK2-Zellen (humane Nierenzellen) und peripheren humanen Lymphozyten. Um die Gentoxizität von Insulin zu bestätigen, wurden auch andere Zellen aus unterschiedlichen Geweben untersucht. Um sicherzustellen, dass die Effekte durch Insulin nicht auf permanente Zelllinien beschränkt sind, wurden außerdem primäre Rattenzellen aus Dickdarm, Niere, Leber und Fettgewebe untersucht. Um die Befunde auf die in-vivo-Situation übertragen zu können, kamen zwei Hyperinsulinämie-Modelle zum Einsatz: mit Insulin infundierte ZDF-Ratten (Zucker Diabetic Fatty Rats) und periphere Lymphozyten von Patienten mit Diabetes Typ 2. Zuerst konnte in humanen Adenokarzinomzellen des Dickdarms (HT29) eine signifikante Erhöhung des DNA-Schadens in Standard-Protokollen des Comet Assays und des Mikrokerntests nach Behandlung mit 5 nM Insulin gezeigt werden. Bei Verlängerung der Behandlungszeit auf 6 Tage wurden signifikante Effekte bereits ab 0,5 nM beobachtet. Insulin erhöhte die zelluläre ROS-Produktion, die als Oxidation der Farbstoffe 2‘,7‘-Dichlorodihydrofluoresceindiacetat (H2DCF-DA) und Dihydroethidium (DHE) nachgewiesen wurde. Befunde aus dem FPG-modifizierten Comet Assay und das Ergebnis, dass der Radikalfänger Tempol die Zellen schützte stellen die Verbindung zwischen Insulin-verursachtem DNA-Schaden und ROS produktion her. Um die ROS-Quelle nach Stimulation mit Insulin zu untersuchen, wurden Apocynin und VAS2870 als NADPH-Oxidase-Inhibitoren und Rotenon als Inhibitor der Mitochondrien mit Insulin kombiniert. Alle diese Stoffe reduzierten den Genomschaden. Zur Charakterisierung der Signalwege wurde zunächst die Bindung von Insulin an seinen Rezeptor und an den IGF1-Rezeptor untersucht. Beide Rezeptoren sind an der Signaltransduktion beteiligt. Nach Aktivierung der Rezeptoren wird die PI3K aktiviert, dies führt zur Phosphorylierung von AKT. Dadurch werden zwei Wege zur ROS-Produktion aktiviert, der erste involviert die mitochondriale Atmungskette , der zweite agiert durch Rac1-Aktivierung. Letzteres resultiert in der Aktivierung der NADPH-Oxidase Isoform Nox1. Der Effekt von Insulin auf zelluläres Chromatin konnte in einer weiteren humanen Dickdarmkrebs-Zelllinie und in primären Dickdarmzellen der Ratte in vitro bestätigt werden. Wir schlussfolgern aus diesen Ergebnissen, dass pathophysiologische Insulin-Blutspiegel DNA-Schäden im Dickdarm verursachen können. Dies könnte zur Induktion oder Progression von Dickdarmkrebs beitragen. Weiterhin verursachte Insulin bei einer Konzentration von 5 nM einen signifikanten Anstieg von DNA-Schäden in vitro. Dies war verbunden mit der Bildung von reaktiven Sauerstoffspezies (ROS). Bei Anwesenheit von Antioxidantien, von Inhibitoren des Insulin-Rezeptors bzw. des IGF-1-Rezeptors und eines Phosphatidylinositol-3-Kinase(PI3K)-Inhibitors war der Insulin-vermittelte DNA-Schaden reduziert. Phosphorylierung von AKT war erhöht und das Protein P53 akkumulierte. Inhibierung der ROS-Produktion der Mitochondrien bzw. der NADPH-Oxidase reduzierte den Insulin-vermittelten Schaden. In primären Rattenzellen induzierte Insulin ebenfalls Genomschaden. HK2-Zellen wurden zur Untersuchung der mechanistischen Signalwege in der Niere eingesetzt. Die Signalwege entsprechen denen der Dickdarmzellen bis zur Aktivierung der ROS-Produktion in den Mitochondrien. Als Folge der Aktivierung von PI3K wird Nox4 aktiviert. Eine Verbindung zwischen Mitochondrien und Nox4-Aktivierung wird vorgeschlagen. Als in-vivo-Modell wurden gesunde ZDF-Ratten mit Insulin infundiert, um normale bzw. erhöhte Insulin-Blutspiegel bei konstanten Glukose-Blutspiegeln zu erreichen. In den Nieren war der Gehalt an ROS und an P53 in der Gruppe mit erhöhten Insulin-Blutspiegeln im Vergleich zur Kontrolle erhöht. ROS und P53 waren ebenfalls in den diabetischen und adipösen ZDF-Ratten erhöht. Die Behandlung der diabetischen Ratten mit Metformin reduzierte die DNA-Oxidation, die in Form von 8-oxodG bestimmt wurde, und die ROS-Produktion in dieser Gruppe. HL60-Zellen und kultivierte Lymphozyten als Modelle für das hämatopoetische System zeigten eine signifikante Induktion von DNA-Schäden nach Behandlung mit Insulin. Diabetes-Patienten zeigten eine erhöhte Mikrokern-Bildung im Vergleich zu gesunden Probanden. In der vorliegenden Studie konnten wir erstmals zeigen, dass Insulin-induzierter oxidativer Stress zu Genomschaden führt, und dass in unterschiedlichen Geweben ROS aus verschiedenen Quellen stammten. Falls diese Mechanismen auch in Patienten auftreten, könnte Hyperinsulinämie durch ROS-Induktion zu Genomschaden führen und damit zu einem erhöhten Krebsrisiko beitragen. Unter bestimmten Bedingungen könnten Antioxidantien bzw. Inhibitoren der Mitochondrien oder der NADPH-Oxidase protektive Effekte ausüben. KW - Insulin KW - Oxidativer Stress KW - DNS-Schädigung KW - oxidativer Stress KW - DNA Schaden KW - Insulin KW - Insulin KW - Oxidative Stress KW - DNA Damage Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-69274 ER - TY - JOUR A1 - Epe, B. A1 - Harttig, U. A1 - Stopper, Helga A1 - Metzler, M. T1 - Covalent binding of reactive estrogen metabolites to microtubular protein as a possible mechanism of aneuploidy induction and neoplastic cell transformation N2 - Neoplastic cell transfonnation induced by estrogens and some other carcinogen& such as benzene appears to involve the induction of mitotic aneuploidy rather than DNA damage and point mutations. As metabolic activation may also play an important roJe in the mechanism of carcinogenesis of these nongenotoxic compounds, we have studied the Interaction of reactive quinone metabolites of various estrogens and of benzene with the major microtubular protein, tubulin, in a cell-free system. Covalent binding of the radioactively labeled metabolites to the a- and 13-subunit of tubulin was found to depend on the structure of the metabolite. When the adducted tubulins were tested in vitro for their ability to polymerize to microtubules, Inhibition of microtubule assembly was obsened in every case, although to varying extents. It is proposed that the fonnation of covalent tubulin adducts may impair the formation of mitotic spindies and thus contribute to chromosomal nondisjunction and aneuploidy induction. KW - Toxikologie Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-63478 ER - TY - JOUR A1 - Epe, Bernd A1 - Häring, Martin A1 - Ramaiah, Danaboyina A1 - Stopper, Helga A1 - Abou-Elzahab, Mohamed M. A1 - Adam, Waldemar A1 - Saha-Möller, Chantu R. T1 - DNA damage induced by furocoumarin hydroperoxides plus UV (360 nm) N2 - Wben irradiated at 360 nm, furocoumarins with a hydroperoxide group in a side chain effciently give rise to a type of DNA damage that can best be explained by a photoinduced generation of hydroxyl radicals from the excited pbotosensitizers. The observed DNA damage profiles, i.e. the ratios of single-strand breaks, sites of base loss (AP sites) and base modifications sensitive to fonnamidopyrimidine-DNA glycosylase (FPG protein) and endonuclease m, are similar to the DNA damage profile produced by hydroxyl radicals generated by lonizing radiation or by xanthine and xanthine oxidase in the presence of Fe(III)-EDTA. No such damage is observed with the corresponding furocoumarin alcohols or in the absence of near-UV radiation. The damage caused by the photo-excited hydroperoxides is not influenced by superoxide dismutase (SOD) or catalase or by D2O as solvent. The presence of t-butanol, however, reduces both the formation of single-strand breaks and of base odifications sensitive to FPG protein. The cytotoxicity caused by one of the hydroperoxides in L5178Y mome lymphoma cells is found to be dependent on the near-UV irradiation and to be much higher than that of the corresponding alcohol. Therefore the new type of photoinduced damage occurs inside cells. Intercalating photosensitizers with an attached hydroperoxide group might represent a novel and versatile class of DNA damaging agents, e.g. for phototherapy. KW - DNS-Schädigung Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86870 ER - TY - JOUR A1 - Fathy, Moustafa A1 - Fawzy, Michael Atef A1 - Hintzsche, Henning A1 - Nikaido, Toshio A1 - Dandekar, Thomas A1 - Othman, Eman M. T1 - Eugenol exerts apoptotic effect and modulates the sensitivity of HeLa cells to cisplatin and radiation JF - Molecules N2 - Eugenol is a phytochemical present in different plant products, e.g., clove oil. Traditionally, it is used against a number of different disorders and it was suggested to have anticancer activity. In this study, the activity of eugenol was evaluated in a human cervical cancer (HeLa) cell line and cell proliferation was examined after treatment with various concentrations of eugenol and different treatment durations. Cytotoxicity was tested using lactate dehydrogenase (LDH) enzyme leakage. In order to assess eugenol’s potential to act synergistically with chemotherapy and radiotherapy, cell survival was calculated after eugenol treatment in combination with cisplatin and X-rays. To elucidate its mechanism of action, caspase-3 activity was analyzed and the expression of various genes and proteins was checked by RT-PCR and western blot analyses. Eugenol clearly decreased the proliferation rate and increased LDH release in a concentration- and time-dependent manner. It showed synergistic effects with cisplatin and X-rays. Eugenol increased caspase-3 activity and the expression of Bax, cytochrome c (Cyt-c), caspase-3, and caspase-9 and decreased the expression of B-cell lymphoma (Bcl)-2, cyclooxygenase-2 (Cox-2), and interleukin-1 beta (IL-1β) indicating that eugenol mainly induced cell death by apoptosis. In conclusion, eugenol showed antiproliferative and cytotoxic effects via apoptosis and also synergism with cisplatin and ionizing radiation in the human cervical cancer cell line. KW - eugenol KW - HeLa cells KW - cisplatin KW - radiation KW - apoptosis Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193227 SN - 1420-3049 VL - 24 IS - 21 ER - TY - THES A1 - Fazeli, Gholamreza T1 - Signaling in the induction of genomic damage by endogenous compounds T1 - Signalwege bei der Induktion von Genomschäden durch endogene Substanzen N2 - Reactive oxygen species (ROS) are continuously generated in cells and are involved in physiological processes including signal transduction but also their damaging effects on biological molecules have been well described. A number of reports in the literature implicate excessive oxidative stress and/or inadequate antioxidant defense in the pathogenesis of cancer, atherosclerosis, chronic and age related disorders. Several studies have indicated that activation of the renin-angiotensin-aldosterone-system can lead to the formation of ROS. Epidemiological studies have revealed higher renal cell cancer incidences and also higher cancer mortalities in hypertensive individuals. Recently, our group has shown that perfusion of the isolated mouse kidney with Ang II or treatment of several cell lines with Ang II leads to formation of DNA damage and oxidative base modifications. Here, we tried to scrutinize the pathway involved in genotoxicity of Ang II. We confirmed the genotoxicity of Ang II in two kidney cell lines of human origin. Ang II treatment led to the production of superoxide anions which we could hinder when we used the membrane permeable superoxide dismutase (SOD) mimetic TEMPOL. One of the enzymes which is activated in the cells after Ang II treatment and is able to produce ROS is NADPH oxidase. We demonstrated the activation of NADPH oxidase in response to Ang II by upregulation of its p47 subunit using RT-PCR. Also, pPhosphorylation of p47 subunit of NADPH oxidase after Ang II treatment was enhanced. Using two inhibitors we showed that NADPH oxidase inhibition completely prevents DNA damage by Ang II treatment. To differentiate between Nox2 and Nox4 isoforms of NADPH oxidase subunits in the genotoxicity of Ang II, we performed siRNA inhibition and found a role only for Nox4, while Nox2 was not involved. Next, we investigated PKC as a potential activator of NADPH oxidase. We showed that PKC becomes phosphorylated after Ang II treatment and also that inhibition of PKC hinders Ang II from damaging the cells. Our results from using several inhibitors of different parts of the pathway revealed that PKC activation in this pathway is dependent on the action of PLC on membrane phospholipids and production of IP3. IP3 binds to its receptor at endoplasmic reticulum (ER), opening a channel which allows calcium efflux into the cytoplasm. In this manner, both ER calcium stores and extracellular calcium cooperate so that Ang II can exert its genotoxic effect. PLC is activated by AT1R stimulation. We could also show that the genotoxicity of Ang II is mediated via AT1R signaling using the AT1R antagonist candesartan. In conclusion, here we have shown that Ang II is able to damage genomic damage in cell lines of kidney origin. The observed damage is associated with production of ROS. A decrease in Ang II-induced DNA damage was observed after inhibition of G-proteins, PLC, PKC and NADPH oxidase and interfering with intra- as well as extracellular calcium signaling. This leads to the following preliminary model of signaling in Ang II-induced DNA damage: binding of Ang II to the AT1 receptor activates PLC via stimulation of G-proteins, resulting in the activation of PKC in a calcium dependent manner which in turn, activates NADPH oxidase. NADPH oxidase with involvement of its Nox4 subunit then produces reactive oxygen species which cause DNA damage. Dopamine content and metabolism in the peripheral lymphocytes of PD patients are influenced by L-Dopa administration. The PD patients receiving a high dose of L-Dopa show a significantly higher content of dopamine in their lymphocytes compared to PD patients who received a low dose of L-Dopa or the healthy control. Central to many of the processes involved in oxidative stress and oxidative damage in PD are the actions of monoamine oxidase (MAO), the enzyme which is responsible for the enzymatic oxidation of dopamine which leadsing to production of H2O2 as a by-product. We investigated whether dopamine oxidation can cause genotoxicity in lymphocytes of PD patents who were under high dose L-Dopa therapy and afterward questioned the occurrence of DNA damage after dopamine treatment in vitro and tried to reveal the mechanism by which dopamine exerts its genotoxic effect. The frequency of micronuclei in peripheral blood lymphocytes of the PD patients was not elevated compared to healthy age-matched individuals, although the formation of micronuclei revealed a positive correlation with the daily dose of L-Dopa administration in patients who received L-Dopa therapy together with dopamine receptor agonists. In vitro, we describe an induction of genomic damage detected as micronucleus formation by low micromolar concentrations in cell lines with of different tissue origins. The genotoxic effect of dopamine was reduced by addition of the antioxidants TEMPOL and dimethylthiourea which proved the involvement of ROS production in dopamine-induced DNA damage. To determine whether oxidation of dopamine by MAO is relevant in its genotoxicity, we inhibited MAO with two inhibitors, trans-2-phenylcyclopropylamine hydrochloride (PCPA) and Ro 16-6491 which both reduced the formation of micronuclei in PC-12 cells. We also studied the role of the dopamine transporter (DAT) and dopamine type 2 receptor (D2R) signaling in the genotoxicity of dopamine. Inhibitors of the DAT, GBR-12909 and nomifensine, hindered dopamine-induced genotoxicity. These results were confirmed by treatment of MDCK and MDCK-DAT cells, the latter containing the human DAT gene, with dopamine. Only MDCK-DAT cells showed elevated chromosomal damage and dopamine uptake. Although stimulation of D2R with quinpirole in the absence of dopamine did not induce genotoxicity in PC-12 cells, interference with D2R signaling using D2R antagonist and inhibition of G-proteins, phosphoinositide 3 kinase and extracellular signal-regulated kinases reduced dopamine-induced genotoxicity and affected the ability of DAT to take up dopamine. Furthermore, the D2R antagonist sulpiride inhibited the dopamine-induced migration of DAT from cytosol to cell membrane. Overall, the neurotransmitter dopamine causes DNA damage and oxidative stress in vitro. There are also indications that high dose L-Dopa therapy might lead to oxidative stress. Dopamine exerts its genotoxicity in vitro upon transport into the cells and oxidization oxidation by MAO. Transport of dopamine by DAT has the central role in this process. D2R signaling is involved in the genotoxicity of dopamine by affecting activation and cell surface expression of DAT and hence modulating dopamine uptake. We provided evidences for receptor-mediated genotoxicity of two compounds with different mechanism of actions. The involvement of these receptors in many human complications urges more investigations to reveal whether abnormalities in the endogenous compounds-mediated signaling can play a role in the initiation of new conditions like carcinogenesis. N2 - Reaktive Sauerstoffspezies (ROS) werden kontinuierlich in Zellen generiert und sind an physiologischen Prozessen wie der Signaltransduktion beteiligt. Aber auch ihre schädigenden Auswirkungen auf biologische Moleküle sind seit langem bekannt. Eine Reihe von Literaturberichten sieht einen Zusammenhang zwischen übermäßigem oxidativen Stress oder einer unzureichenden antioxidativen Verteidigung und Krebs, Atherosklerose und chronischen bzw. altersbedingten Erkrankungen. Mehrere Studien haben belegt, dass die Aktivierung des Renin-Angiotensin-Aldosteron-Systems zur Bildung von ROS führen kann. Epidemiologische Studien haben gezeigt, dass Nierenkarzinom-Inzidenzen und -Mortalitäten bei Hypertonikern erhöht sind. Vor kurzem konnte unsere Gruppe zeigen, dass die Perfusion von isolierten Maäusen-Nieren und dieoder Behandlung mehrerer Zelllinien mit Angiotensin II (Ang II) zur Bildung von DNA-Schäden und oxidativen Basenmodifikationen führt. Ziel der vorliegenden Arbeit war es, die Signalwege der Genotoxizität von Ang II zu bestimmen. Wir bestätigten dDie Genotoxiziät von Ang II in zwei Nieren-Zelllinien humaner Herkunft konnte bestätigt werden. Wir zeigten, dass Ang II-Behandlung zur Produktion von Superoxid-Anionen führt, die durch das membrangängige Superoxid-Dismutase-Mimetikum TEMPOL verhindert werden kann. Eines der Enzyme, das in den Zellen nach Ang II-Behandlung aktiviert wird und ROS produzieren kann, ist die NADPH-Oxidase. Die mittels RT-PCR gemessene Hochregulierung von p47 beweist die Aktivierung der NADPH-Oxidase nach Ang II-Behandlung. Auch die Phosphorylierung von p47 nach Ang II-Behandlung wurde gesteigert. Mittels zweier Inhibitoren zeigten wir, dass NADPH-Oxidase-Hemmung DNA-Schäden durch Ang II-Behandlung vollständig verhindert. Wir versuchten, die Rolle der Nox2- und Nox4-Isoformen der NADPH-Oxidase-Untereinheiten bei der Genotoxizität von Ang II zu differenzieren. Hemmung mittels siRNA bestätigte nur eine Beteiligung der Nox4. Anschließend überprüften wir die Rolle der PKC als potentiellem Aktivator der NADPH-Oxidase. Wir zeigten, dass die PKC nach Ang II-Behandlung PKC phosphoryliert wird und durch die Hemmung der PKC Ang II-induzierten Schäden verhindert werdenird. Die Verwendung mehrerer Inhibitoren der verschiedenen Teile des Signalweges zeigte, dass die PKC-Aktivierung von der Reaktion der PLC mit Membranphospholipiden und der Produktion von IP3 und DAG abhängig ist. IP3 bindet an seinen Rezeptor am Endoplasmatischen Retikulum (ER)., dDie in der Folge auftretende Öffnung eines Kanals ermöglicht einen Calcium-Ausstrom in das Cytoplasma. Auf diese Weise sind sowohl ER-Calcium als auch extrazelluläres Calcium an der Ang II-induzierten genotoxische Wirkung beteiligt. PLC wird durch AT1R-Stimulation aktiviert. Wir konnten mit Hilfe des AT1R-Antagonisten Candesartan auch zeigen, dass die Genotoxizität von Ang II über AT1R-Signaltransduktion vermittelt wird. Zusammenfassend haben wir gezeigt, dass Ang II genomische Schäden in humanen Nieren-Zelllinien verursacht. Die Schäden sind mit der Produktion von ROS verbunden. Eine Reduktion der Ang II-induzierten DNA-Schäden wurde nach Hemmung vonder G-Proteinen, der PLC, PKC und NADPH-Oxidase und Beeinflussung intra- sowie extrazellulärer Calium-Signalgebung gezeigt. Dies führt zu folgendem vorläufigen Modell der Signaltransduktion der von Ang II-induzierten DNA-Schäden: Die Bindung von Ang II an den AT1-Rezeptor aktiviert die PLC durch Stimulationerung der G-Proteine und die PKC in Calcium-abhängiger Weise, dies wiederum aktiviert die NADPH-Oxidase. Die NADPH Oxidase unter Beteiligung ihrerseiner Nox4-Untereinheit erzeugt dann reaktive Sauerstoffspezies, die DNA-Schäden verursachen. Dopamingehalt und -stoffwechsel in peripheren Lymphozyten von Parkinson-Patienten werden durch L-Dopa-Gabe beeinflusst. Die Patienten, die eine hohe Dosis L-Dopa erhalten, zeigen einen signifikant höheren Gehalt an Dopamin in den Lymphozyten im Vergleich zu Patienten, die eine niedrige Dosis L-Dopa erhalten oder der gesunden Kontrollgruppe. Im Mittelpunkt vieler Prozesse bei der Entstehung von oxidativem Stress und oxidativer Schäden bei Parkinson-Patienten steht die Monoaminoxidase (MAO), die für die enzymatische Oxidation von Dopamin und in der Folge für die Entstehung von H2O2 verantwortlich ist. Wir untersuchten, ob die Oxidation von Dopamin genotoxische Wirkung in Lymphozyten von Parkinson-Patienten mit hochdosierter L-Dopa-Therapie induzieren kann. Danach überprüftenfragten wir, ob die Behandlung mit Dopamin in vitro DNA-Schäden induzieren kann und versuchten aufzuzeigen, durch welchen Mechanismus Dopamin seine genotoxische Wirkung entfaltet. Die Häufigkeit von Mikrokernen in peripheren Lymphozyten der Parkinson-Patienten war nicht erhöht im Vergleich zur gesunden Kontrollgruppe, allerdings zeigte die Mikrokernfrequenz eine positive Korrelation mit der täglichen L-Dopa-Dosis bei Patienten, die eine L-Dopa-Therapie zusammen mit einem Dopamin-Rezeptor-Agonisten erhielten. In vitro beobachteten wir bei niedrigen mikromolaren Konzentrationen eine Induktion des genomischen Schadens in Zelllinien, die aus verschiedenen Geweben stammten. Die genotoxische Wirkung von Dopamin wurde durch Zugabe der Antioxidantien TEMPOL und DMTU reduziert, wodurch die Beteiligung von ROS gezeigt werden konnte. Um festzustellen, ob die Oxidation von Dopamin durch MAO für die Genotoxizität relevant ist, hemmten wir MAO mit zwei Inhibitoren, trans-2-Phenylcyclopropylamin-Hydrochlorid (PCPA) und Ro 16-6491, die beide die Bildung von Mikrokernen in PC-12-Zellen reduzieren konnten. Wir untersuchten auch die Rolle des Dopamin-Transporters (DAT) und Dopamin-Typ-2-Rezeptor (D2R)-assoziierter Signalwege in der Genotoxizität von Dopamin. Die Inhibitoren des DAT, GBR-12909 und Nomifensin verhinderten die Dopamin-induzierte Genotoxizität. Diese Ergebnisse wurden durch Behandlung von MDCK- und MDCK-DAT- Zellen (die das humane DAT-Gen besitzen) mit Dopamin bestätigt. Nur MDCK-DAT-Zellen zeigten erhöhte chromosomale Schäden und Dopaminaufnahme. Obwohl die Stimulation mit dem D2R-Rezeptor-Agonisten Quinpirol in Abwesenheit von Dopamin keine Genotoxizität in PC-12-Zellen induzierte, reduzierten sowohl ein D2R-Antagonist, wie auch Inhibitoren des in der Signalkaskade involvierten G-Proteins, der Phosphoinositol-3-Kinase und der extrazellulären signalregulierten Kinasen die Aufnahme von Dopamin mittels DAT und die Dopamin-vermittelte Genotoxizität. Der D2R-Antagonist Sulpirid hemmte die Dopamin-induzierte Migration von DAT aus dem Cytosol zur Zellmembran. Insgesamt verursacht der Neurotransmitter Dopamin DNA-Schäden und oxidativen Stress in vitro. Es gibt Hinweise, dass eine hochdosierte L-Dopa-Therapie zu oxidativem Stress führt. In vitro führt Dopamin zu Genotoxizität durch den Transport in die Zellen und Oxidation durch MAO. Der Transport von Dopamin durch DAT spielt eine zentrale Rolle in diesem Prozess. Die D2R-Signalwege sind an der Genotoxizität von Dopamin durch Auswirkung auf die Aktivierung und Membranexpression von DAT und damit der Dopaminaufnahme beteiligt. KW - Angiotensin II KW - Mutagenität KW - DNS-Schädigung KW - DNA-Schaden KW - Genotoxizität KW - genotoxicity KW - DNA damage Y1 - 2010 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-55634 ER - TY - JOUR A1 - Federico, Stephanie A1 - Redenti, Sara A1 - Sturlese, Mattia A1 - Ciancetta, Antonella A1 - Kachler, Sonja A1 - Klotz, Karl-Norbert A1 - Cacciari, Barbara A1 - Moro, Stefano A1 - Spalluto, Giampiero T1 - The Influence of the 1-(3-Trifluoromethyl-Benzyl)-1H-Pyrazole-4-yl Moiety on the Adenosine Receptors Affinity Profile of Pyrazolo[4,3-e][1,2,4]Triazolo[1,5-c]Pyrimidine Derivatives JF - PLoS One N2 - A new series of pyrazolo[4,3-e][1,2,4]triazolo[1,5-c]pyrimidine (PTP) derivatives has been developed in order to explore their affinity and selectivity profile at the four adenosine receptor subtypes. In particular, the PTP scaffold was conjugated at the C2 position with the 1-(3-trifluoromethyl-benzyl)-1H-pyrazole, a group believed to confer potency and selectivity toward the human (h) A\(_{2B}\) adenosine receptor (AR) to the xanthine ligand 8-(1-(3-(trifluoromethyl) benzyl)-1H-pyrazol-4-yl)-1,3-dimethyl-1H-purine-2,6(3H, 7H)-dione (CVT 6975). Interestingly, the synthesized compounds turned out to be inactive at the hA\(_{2B}\) AR but they displayed affinity at the hA\(_3\) AR in the nanomolar range. The best compound of the series (6) shows both high affinity (hA\(_3\) AR K\(_i\) = 11 nM) and selectivity (A\(_1\)/A\(_3\) and A\(_{2A}\)/A\(_3\) > 9090; A\(_{2B}\)/A\(_3\) > 909) at the hA\(_3\) AR. To better rationalize these results, a molecular docking study on the four AR subtypes was performed for all the synthesized compounds. In addition, CTV 6975 and two close analogues have been subjected to the same molecular docking protocol to investigate the role of the 1-(3-trifluoromethyl-benzyl)-1H-pyrazole on the binding at the four ARs. KW - drug KW - human A(3) KW - protein-coupled receptors KW - classification KW - subtypes KW - potent KW - antagonists KW - mast cells KW - targets KW - A(2B) receptors KW - international union Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-137133 VL - 10 IS - 12 ER - TY - THES A1 - Fink, Kristin T1 - Toxins in Renal Disease and Dialysis Therapy : Genotoxic Potential and Mechanisms T1 - Toxine in Nierenerkrankung und Dialyse Therapie : Genotoxisches Potential und Mechanismus N2 - In patients suffering from end-stage renal disease who are treated by hemodialysis genomic damage as well as cancer incidence is elevated. One possible cause for the increased genomic damage could be the accumulation of genotoxic substances in the blood of patients. Two possible sources for those toxins have to be considered. The first possibility is that substances from dialysers, the blood tubing system or even contaminated dialysis solutions may leach into the blood of the patients during dialysis. Secondly, the loss of renal filtration leads to an accumulation of substances which are normally excreted by the kidney. If those substances possess toxic potential, they are called uremic toxins. Several of these uremic toxins are potentially genotoxic. Within this thesis several exemplary uremic toxins have been tested for genotoxic effects (homocysteine, homocysteine-thiolactone,leptine, advanced glycated end-products). Additionally, it was analysed whether substances are leaching from dialysers or blood tubing and whether they cause effects in in vitrotoxicity testing. The focus of chemical analytisis was on bisphenol A (BPA), the main component of plastics used in dialysers and dialyser membranes. N2 - Patienten, die an terminaler Niereninsuffizienz leiden und mittels Hämodialyse behandelt werden, weisen einen erhöhten Genomschaden auf. Dieser könnte ursächlich für die erhöhte Krebsinzidenz dieser Patientengruppe sein. Eine der möglichen Ursachen für den erhöhten Genomschaden stellt die Akkumulation genotoxischer Substanzen im Blut der Patienten dar. Diese Substanzen können prinzipiell aus zwei unterschiedlichen Quellen stammen. Erstens besteht die Möglichkeit, dass während der Dialyse Substanzen aus den Dialysatoren, dem Blutschlauchsystem oder gar aus verunreinigtem Dialysat in das Blut der Patienten übertreten. Zweitens führt der Verlust der Nierenfunktion zu einer stark verminderten Exkretion harnpflichtiger Substanzen. Diese Substanzen akkumulieren im Blut und bilden, sofern sie ein toxisches Potential besitzen, die Gruppe der so genannten urämischen Toxine. Einige dieser urämischen Toxine sind potentiell auch genotoxisch. Im Rahmen der vorliegenden Dissertation wurden exemplarische Vertreter der urämischen Toxine auf ihre genotoxische Wirkung hin untersucht (Homocstein, Homocystein-Thiolacton, Leptin, Advanced Glycation End-Products). Außerdem wurde analysiert, ob Substanzen aus Dialysatormembranen oder dem Blutschlauchsystem austreten und in in vitro-Toxizitätstests Effekte zeigen. Der Fokus der Analytik lag hierbei auf dem Nachweis von Bisphenol A, dem Hauptbestandteil verschiedener Kunststoffe die für Dialysatoren und Dialysatormembranen verwendet werden. KW - Bisphenol A KW - Homocystein KW - Extrakorporale Dialyse KW - Genomschaden KW - Urämische Toxine KW - bisphenol a KW - homocysteine KW - dialysis KW - genomic damage KW - uremic toxins Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-31082 ER - TY - JOUR A1 - Fischer, W. H. A1 - Beland, P. E. A1 - Lutz, Werner K. T1 - DNA adducts, cell proliferation and papilloma latency time in mouse skin after repeated dermal application of DMBA and TPA N2 - 'lbe mouse skin tumor model was used to investigate whether the Ievel of DNA 8dducts and/or the rate of cell division in the epidermis are indicators of the risk of cancer formation for an individual in an outbred animal popul8tion. A high risk was considered to be reftected by 8 short latency period for the 8ppearance of 8 papilloma. Fernale NMRI mice were treated twice weekly with 2.5 nmol 7 ,12-dimethylbenz[a]antbracene (DMBA) and 3 nmoi12-0-tetradecanoylphorbol-13- 8cetate (TPA) and the appearance of papillomas was registered. The first papilloma 8ppeared after 7.5 weeks. After 17 weeks, when 12 of 14 mice bad 8t least one papilloma, an osmotic minipump deliverlog 5-bromo-2'deoxyuridine (BrdU) was implanted into eacb mouse for 24 h. The mice were killed after 24 h ~d the epidermis was analyzed for D:MBA-nucleotide 8dducts by 32p.postlabeling, for the cell number per unit skin length, and for the labeling index for DNA synthesls. Unexpectedly, D:MBA-nucleotide 8dduct Ievels were highest in those anima1s wbich showed the Iongest latency periods. Adduct Ievels were negatively correlated with the 18beling index, indicating that dilution of adducts by cell division was a predominant factor in determining average adduct concentrations. Individual tumor-latency time was not corTelated with either cell ntunber or labeling index. This could be due to the fact that the measurements only provided 8veraged data and gave no infonnation on the specific situation in clones of premalignant cells. Under the conditions of tbis assay, therefore, neither DNA adduct Ievels nor information on the average kinetics of cell division bad a predidive value for the individual amcer risk withln a group of outbred animals receiving the same treatment KW - Toxikologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60673 ER - TY - JOUR A1 - Fischer, W. H. A1 - Lutz, Werner K. T1 - Short communication : Mouse skin papilloma formation by chronic dermal application of 7,12-dimethylbenz[a]anthracene is not reduced by diet restriction N2 - No abstract available KW - Toxikologie Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60644 ER - TY - JOUR A1 - Frey, Anna A1 - Gassenmaier, Tobias A1 - Hofmann, Ulrich A1 - Schmitt, Dominik A1 - Fette, Georg A1 - Marx, Almuth A1 - Heterich, Sabine A1 - Boivin-Jahns, Valérie A1 - Ertl, Georg A1 - Bley, Thorsten A1 - Frantz, Stefan A1 - Jahns, Roland A1 - Störk, Stefan T1 - Coagulation factor XIII activity predicts left ventricular remodelling after acute myocardial infarction JF - ESC Heart Failure N2 - Aims Acute myocardial infarction (MI) is the major cause of chronic heart failure. The activity of blood coagulation factor XIII (FXIIIa) plays an important role in rodents as a healing factor after MI, whereas its role in healing and remodelling processes in humans remains unclear. We prospectively evaluated the relevance of FXIIIa after acute MI as a potential early prognostic marker for adequate healing. Methods and results This monocentric prospective cohort study investigated cardiac remodelling in patients with ST-elevation MI and followed them up for 1 year. Serum FXIIIa was serially assessed during the first 9 days after MI and after 2, 6, and 12 months. Cardiac magnetic resonance imaging was performed within 4 days after MI (Scan 1), after 7 to 9 days (Scan 2), and after 12 months (Scan 3). The FXIII valine-to-leucine (V34L) single-nucleotide polymorphism rs5985 was genotyped. One hundred forty-six patients were investigated (mean age 58 ± 11 years, 13% women). Median FXIIIa was 118 % (quartiles, 102–132%) and dropped to a trough on the second day after MI: 109%(98–109%; P < 0.001). FXIIIa recovered slowly over time, reaching the baseline level after 2 to 6 months and surpassed baseline levels only after 12 months: 124 % (110–142%). The development of FXIIIa after MI was independent of the genotype. FXIIIa on Day 2 was strongly and inversely associated with the relative size of MI in Scan 1 (Spearman’s ρ = –0.31; P = 0.01) and Scan 3 (ρ = –0.39; P < 0.01) and positively associated with left ventricular ejection fraction: ρ = 0.32 (P < 0.01) and ρ = 0.24 (P = 0.04), respectively. Conclusions FXIII activity after MI is highly dynamic, exhibiting a significant decline in the early healing period, with reconstitution 6 months later. Depressed FXIIIa early after MI predicted a greater size of MI and lower left ventricular ejection fraction after 1 year. The clinical relevance of these findings awaits to be tested in a randomized trial. KW - blood coagulation factor XIII KW - ST-elevation myocardial infarction KW - healing and remodelling processes KW - cardiac magnetic resonance imaging Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-236013 VL - 7 IS - 5 ER - TY - THES A1 - Förtsch, Christina T1 - Pneumolysin: the state of pore-formation in context to cell trafficking and inflammatory responses of astrocytes T1 - Pneumolysin: Einfluss der Porenbildung auf zelluläre Transportprozesse und inflammatorische Antworten in Astrozyten N2 - Pneumolysin, a protein toxin, represents one of the major virulence factors of Streptococcus pneumoniae. This pathogen causes bacterial meningitis with especially high disease rates in young children, elderly people and immunosuppressed patients. The protein toxin belongs to the family of cholesterol-dependent cytolysins, which require membrane cholesterol in order to bind and to be activated. Upon activation, monomers assemble in a circle and undergo conformational change. This conformational change leads to the formation of a pore, which eventually leads to cell lysis. This knowledge was obtained by studies that used a higher concentration compared to the concentration of pneumolysin found in the cerebrospinal fluid of meningitis patients. Thus, a much lower concentration of pneumolysin was used in this work in order to investigate effects of this toxin on primary mouse astrocytes. Previously, a small GTPase activation, possibly leading to cytoskeletal changes, was found in a human neuroblastoma cell line. This led to the hypothesis that pneumolysin can lead to similar cytoskeletal changes in primary cells. The aim of this work was to investigate and characterise the effects of pneumolysin on primary mouse astrocytes in terms of a possible pore formation, cellular trafficking and immunological responses. Firstly, the importance of pore-formation on cytoskeletal changes was to be investigated. In order to tackle this question, wild-type pneumolysin and two mutant variants were used. One variant was generated by exchanging one amino acid in the cholesterol recognising region, the second variant was generated by deleting two amino acids in a protein domain that is essential for oligomerisation. These variants should be incapable of forming a pore and were compared to the wild-type in terms of lytic capacities, membrane binding, membrane depolarisation, pore-formation in artificial membranes (planar lipid bilayer) and effects on the cytoskeleton. These investigations resulted in the finding that the pore-formation is required for inducing cell lysis, membrane depolarisation and cytoskeletal changes in astrocytes. The variants were not able to form a pore in planar lipid bilayer and did not cause cell lysis and membrane depolarisation. However, they bound to the cell membrane to the same extent as the wild-type toxin. Thus, the pore-formation, but not the membrane binding was the cause for these changes. Secondly, the effect of pneumolysin on cellular trafficking was investigated. Here, the variants showed no effect, but the wild-type led to an increase in overall endocytotic events and was itself internalised into the cell. In order to characterise a possible mechanism for internalisation, a GFP-tagged version of pneumolysin was used. Several fluorescence-labelled markers for different endocytotic pathways were used in a co-staining approach with pneumolysin. Furthermore, inhibitors for two key-players in classical endocytotic pathways, dynamin and myosin II, were used in order to investigate classical endocytotic pathways and their possible involvement in toxin internalisation. The second finding of this work is that pneumolysin is taken up into the cell via dynamin- and caveolin-independent pinocytosis, which could transfer the toxin to caveosomes. From there, the fate of the toxin remains unknown. Additionally, pneumolysin leads to an overall increase in endocytotic events. This observation led to the third aim of this work. If the toxin increases the overall rate of endocytosis, the question arises whether toxin internalisation favours bacterial tissue penetration of the host or whether it serves as a defence mechanism of the cell in order to degrade the protein. Thus, several proinflammatory cytokines were investigated, as previous studies describe an effect of pneumolysin on cytokine production. Surprisingly, only interleukin 6-production was increased after toxin-treatment and no effect of endocytotic inhibitors on the interleukin 6-production was observed. The conclusion from this finding is that pneumolysin leads to an increase of interleukin 6, which would not depend on the endocytotic uptake of pneumolysin. The production of interleukin 6 would enhance the production of acute phase proteins, T-cell activation, growth and differentiation. On the one hand, this activation could serve pathogen clearance from infected tissue. On the other hand, the production of interleukin 6 could promote a further penetration of pathogen into host tissue. This question should be further investigated. N2 - Das Protein-Toxin Pneumolysin ist einer der entscheidenden Virulenzfaktoren von Streptococcus pneumoniae. Dieses Protein-Toxin gehört zur Familie der cholesterinabhängigen Zytolysine, die Membrancholesterol für ihre Aktivierung und Bindung benötigen. Nach der Membranbindung ordnen sich die Toxinmonomere kreisförmig an und ändern ihre Konformation, wodurch eine Pore entsteht, die dann zu einer Lyse der Zelle führt. Vor kurzem wurde nach Pneumolysinbehandlung in einer humanen Neuroblastomzelllinie eine Aktivierung kleiner GTPasen gefunden, die für zytoskelettale Veränderungen entscheidend sind (z.B. Zellbewegungen). Deshalb wurde die Hypothese aufgestellt, dass Pneumolysin diese zytoskelettalen Veränderungen auch in primären neuronalen Zellen auslösen könnte. Das Ziel dieser Arbeit war, die Effekte von Pneumolysin auf primäre Mausastrozyten im Hinblick auf Porenbildung, zelluläre Transportprozesse und immunologische Antworten zu untersuchen. Im ersten Teil wird die Bedeutung der Porenbildung auf zytoskelettale Veränderungen untersucht. Hierbei wurden lytische Fähigkeiten, Membranbindung, Membrandepolarisation, Porenbildung im künstlichen Bilayer und Effekte auf das Zytoskelett untersucht. Sowohl der Wildtyp als auch die Varianten zeigten die gleiche Stärke an Membranbindung. Diese Untersuchungen weisen darauf hin, dass die Porenbildung für die Zell-Lyse, Membrandepolarisation und zytoskelettale Veränderungen in Mausastrozyten wichtig ist und führt zu der Schlussfolgerung, dass nicht die Membranbindung, sondern die Porenbildung entscheidend für die beobachteten zytoskelettalen Veränderungen ist. Im zweiten Teil dieser Arbeit wurde der Effekt des Pneumolysin auf zelluläre Transportprozesse untersucht. Erneut zeigten die Pneumolysinvarianten keine Wirkung, während der Wildtyp die Gesamtrate der Endozytose erhöhte. Weiterhin wurde nur der Wildtyp internalisiert. Um einen möglichen Mechanismus für die Internalisierung des Toxins vorschlagen zu können, wurde Pneumolysin als GFP-markiertes Toxin genutzt. Weiterhin wurden einige Marker für unterschiedliche endozytotische Transportprozesse genutzt um eine Ko-lokalisation mit Pneumolysin-GFP zu ermöglichen. Des Weiteren wurden Inhibitoren für zwei Schlüsselproteine endozytotischer Vorgänge, Dynamin und Myosin II, genutzt. Die Ergebnisse dieser Untersuchungen zeigten, dass Pneumolysin wahrscheinlich durch dynamin- und caveolin-unabhängige Pinozytose in die Zelle aufgenommen wird. Dieser Mechanismus führt zu der Bildung von Caveosomen, deren weiterer Transport, und somit das Schicksal des internalisierten Toxins, bis heute noch nicht aufgeklärt ist. Die Beobachtung, dass Pneumolysin die Gesamtrate an Endozytose erhöht, führte zum dritten Teil dieser Arbeit. Wenn das Toxin die Gesamtrate an Endozytose erhöht, stellt sich die Frage, ob dieser Vorgang der Zerstörung des Toxins – also einer Abwehr der Zelle – dient, oder ob diese Internalisierung eine Strategie des Pathogens ist, um tiefer in das Wirtsgewebe einzudringen. Aktuelle Studien belegen, dass Pneumolysin einen Einfluss auf inflammatorische Antworten des Immunsystems hat. Aus diesem Grund wurden unterschiedliche proinflammatorische Zytokine untersucht. Überraschenderweise zeigte sich nur eine Erhöhung des Interleukin 6 nach der Toxinbehandlung. Weiterhin hatten die Endozytoseinhibitoren keinen Effekt auf die Produktion dieses proinflammatorischen Zytokins. Pneumolysin führt also zu einem Anstieg der Interleukin 6 Produktion, diese Produktion ist jedoch unabhängig von der Internalisierung dieses Toxins. Die Produktion dieses Interleukins würde zur Produktion der Akute-Phase Proteine, der Aktivierung der T-Zell Antwort, zu Wachstum und Zelldifferenzierung führen. Einerseits könnte diese Aktivierung die Infektion durch das Pathogen bekämpfen. Andererseits könnte S. pneumoniae die erhöhte Produktion durch PLY an Interleukin 6 nutzen um weiter in das Wirtsgewebe vordringen zu können. Diese Frage sollte noch durch weitere Experimente untersucht werden. KW - Streptococcus pneumoniae KW - Toxin KW - Hirnhautentzündung KW - Entzündung KW - Astrozyt KW - Pore KW - Pneumolysin KW - Meningitis KW - Inflammation KW - Zelltransport KW - Porenbildung KW - Pneumolysin KW - Meningitis KW - Inflammation KW - cellular-trafficking KW - Pore-formation Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-70892 ER - TY - JOUR A1 - Förtsch, Christina A1 - Hupp, Sabrina A1 - Ma, Jiangtao A1 - Mitchell, Timothy J. A1 - Maier, Elke A1 - Benz, Roland A1 - Iliev, Asparouh I. T1 - Changes in Astrocyte Shape Induced by Sublytic Concentrations of the Cholesterol-Dependent Cytolysin Pneumolysin Still Require Pore-Forming Capacity N2 - Streptococcus pneumoniae is a common pathogen that causes various infections, such as sepsis and meningitis. A major pathogenic factor of S. pneumoniae is the cholesterol-dependent cytolysin, pneumolysin. It produces cell lysis at high concentrations and apoptosis at lower concentrations. We have shown that sublytic amounts of pneumolysin induce small GTPase-dependent actin cytoskeleton reorganization and microtubule stabilization in human neuroblastoma cells that are manifested by cell retraction and changes in cell shape. In this study, we utilized a live imaging approach to analyze the role of pneumolysin’s pore-forming capacity in the actin-dependent cell shape changes in primary astrocytes. After the initial challenge with the wild-type toxin, a permeabilized cell population was rapidly established within 20–40 minutes. After the initial rapid permeabilization, the size of the permeabilized population remained unchanged and reached a plateau. Thus, we analyzed the non-permeabilized (non-lytic) population, which demonstrated retraction and shape changes that were inhibited by actin depolymerization. Despite the non-lytic nature of pneumolysin treatment, the toxin’s lytic capacity remained critical for the initiation of cell shape changes. The non-lytic pneumolysin mutants W433F-pneumolysin and delta6-pneumolysin, which bind the cell membrane with affinities similar to that of the wild-type toxin, were not able to induce shape changes. The initiation of cell shape changes and cell retraction by the wild-type toxin were independent of calcium and sodium influx and membrane depolarization, which are known to occur following cellular challenge and suggested to result from the ion channel-like properties of the pneumolysin pores. Excluding the major pore-related phenomena as the initiation mechanism of cell shape changes, the existence of a more complex relationship between the pore-forming capacity of pneumolysin and the actin cytoskeleton reorganization is suggested. KW - Toxikologie KW - pneumolysin KW - pore formation KW - cytoskeleton Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-69084 ER - TY - JOUR A1 - Gimpl, G. A1 - Gerstberger, R. A1 - Mauss, U. A1 - Klotz, Karl-Norbert A1 - Lang, R. E. T1 - Solubilization and characterization of active neuropeptide-Y receptors from rabbit kidney N2 - Active neuropeptide Y receptors were solubilized from rabbit kidney membranes using the zwitterionic detergent 3-[ (3-cholamidopropy l)dimethylammonio ]- 1-propanesulfonic acid (CHAPS). In membrane fragmentsandsoluble extracts neuropeptide Y bindingwas time dependent, saturable, reversible, and of high affinity. Scatchard analysis of equilibrium binding data indicated a single class of binding sites with respective Kn and Bmax values of 0.09 nM and 530 fmol/mg of protein for the membrane-bound receptors and 0.10 nM and 1585 fmol/mg of protein for the soluble receptors. Neuropeptide Y bindingwas specifically inhibited by the nonhydrolyzable GTP analog guanosine 5' -0- (3-thiotripbosphate) in a concentration-dependent manner, with IC\(_{50}\) values of 28 and 0.14 \(\mu\)M for membrane- bound and soluble receptors, respectively, suggesting that neuropeptide Y receptors are functionally coupled to GTP-binding regulatory proteins. CrossHoking studies were performed with the heterobifunctional N-hydroxysuccinimidyl-4-azidobenzoate and the monofunctional neuropeptide Y derivative, azidobenzoyl and led to the identification of a 100 kDa peptide that should represent the covalently labeled neuropeptide Y receptor. KW - Toxikologie Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60375 ER - TY - THES A1 - Glaser, Nina T1 - Influence of natural food compounds on DNA stability T1 - Einfluss natürlicher Nahrungsbestandteile auf die DNA Stabilität N2 - Cancer is one of the leading causes of death all over the world. Malnutrition and toxic contaminations of food with substances such as mycotoxins have been thought to account for a high percentage of cancers. However, human diet can deliver both mutagens and components that decrease the cancer risk. Genomic damage could be reduced by food components through different mechanisms such as scavenging of reactive oxygen species. In the first part of this study we tried to investigate the effects of patulin and resveratrol on DNA stability in V79 cells. Patulin is a mycotoxin, which is frequently found in spoiled apples and other fruits. The WHO has established a safety level of 50 µg/L, which is indeed not observed by all manufacturers. The acute toxicity of patulin in high concentrations is well known, however its potential carcinogenicity is still a matter of debate. Therefore we wanted to investigate further steps in the mechanism of patulin-induced genotoxicity. Patulin caused the formation of micronuclei and nucleoplasmic bridges in a dose-dependent manner. Further analysis revealed that patulin induced both kinetochore-negative and positive micronuclei. Time course of incubation indicate a new mechanism for patulin-induced nucleoplasmic bridge formation. We hypothized a mechanism via cross-linking of DNA, which was confirmed by a modified version of comet assay. Incubations of cells with patulin led to an increased number of multinucleated cells and multipolar mitoses. Cell cytometry revealed a G2 arrest by patulin, which might explain the amplification of centrosomes and patulin-induced aneuploidy. Patulin cause a dose-dependent DNA damage in comet assay which was influenced by the cellular GSH content. However, an induction of oxidative stress was just seen with higher concentrations of patulin. Levels of cellular glutathione were increased after 24 h incubation indicating an adaptive response to patulin-induced stress. There is growing interest in polyphenols such as resveratrol which have shown many positive effects on human health. The beneficial properties are partially attributed to their ability to scavenge reactive oxygen species. Co-incubation of V79 cells with patulin and 10 µM of the antioxidant resveratrol led to a slight reduction of micronucleus frequency compared to cells which were just treated with patulin. However, in higher concentrations resveratrol themselves caused the formation of micronuclei in V79 cells. Kinetochore analysis indicated only clastogenic properties for resveratrol but no disturbance of mitosis. The antioxidant properties of resveratrol were shown in ferric reducing antioxidant power (FRAP) assay. However, in cellular system resveratrol in higher concentrations revealed also prooxidative properties, as shown in 2,7-dichlordihydrofluorescein (DCF) assay. The increased level of glutathione after resveratrol treatment might reflect an adaptive response to resveratrol-induced oxidative stress. For the second part of this thesis we investigated the effects of an anthocyanin-rich grape extract on hypertensive Ren-2 rats. Ren-2 rats are an accepted genetically modified rat model for the investigation of hypertension and increased oxidative stress. We divided 23 female Ren-2 rats into three groups. One group was fed with an anthocyanin-rich Dacapo grape extract, one group was treated with the angiotensin converting enzyme (ACE) inhibitor ramipril and the third group was kept without medication during the experiment. After one week untreated group showed a clear increase in systolic and diastolic blood pressure compared to the ramipril treated rats. This was in part attenuated in the animals fed with anthocyanin-rich Dacapo grape extract. Effects on blood pressure were also reflected in an increased thirst of untreated and extract fed animals. Comet assay with cells of kidney and liver revealed a slight protective impact of Dacapo extract on DNA damage compared to the other groups. Similar results were obtained after evaluation of ɣ-H2AX-staining of kidney and heart sections. However, in the small intestine oppositional effects were seen, indicating an increased number of double strand breaks probably due to the high local concentration of polyphenols after oral ingestion. Antioxidative properties of the extract were shown in FRAP assay. However, this effect was not reflected in an increased antioxidative capacity in serum or a protective impact in the dihydroethidium (DHE) assay. The extract showed protective effects on DNA damage in comet assay and ɣ-H2AX-staining, but was not able to reduce hypertension back to the control level of ramipril treated animals. High local concentrations could also result in an increased damage of the affected tissue. Therefore, the administration of such concentrated compounds should be handled with care. N2 - Krebs ist eine der häufigsten weltweiten Todesursachen. Fehlernährung und Kontaminationen der Nahrungsmittel mit Toxinen wie Schimmelpilzgift tragen zu einem hohen Prozentsatz zu Krebserkrankungen bei. Allerdings enthält die Nahrung neben Mutagenen auch Bestandteile, die dazu beitragen das Krebsrisiko zu senken. Schäden am Genom können durch Nahrungsbestandteile über verschiedene Mechanismen, wie zum Beispiel das Abfangen von freien Radikalen reduziert werden. Im ersten Teil dieser Studie haben wir versucht die Effekte von Patulin und Resveratrol auf die DNA Stabilität von V79 Zellen zu untersuchen. Patulin ist ein Schimmelpilztoxin, welches häufig in verfaulten Äpfeln und anderen Früchten gefunden wird. Die WHO hat einen Grenzwert von 50 µg/L festgelegt, der jedoch nicht von allen Herstellern eingehalten wird. Die akute Giftwirkung von Patulin in hohen Dosen ist gut bekannt, wohingegen seine potentielle Kanzerogenität immer noch umstritten ist. Daher wollten wir weitere Schritte der Patulin induzierten Genotoxizität aufdecken. Patulin führte zu einer dosisabhängigen Bildung von Mikrokernen und Nucleoplasmic Bridges. Weitere Untersuchungen zeigten, dass Patulin sowohl kinetochor-positive wie auch kinetochor-negative Mikrokerne verursacht. Bei der Analyse des Zeitverlaufs einer Patulininkubation deutete sich ein neuer Mechanismus für die Patulin induzierte Bildung von Nucleoplasmic Bridges an. Wir haben die Hypothese einer Quervernetzung von DNA-Strängen aufgestellt, die durch eine modifizierte Version des Comet Assays bestätigt wurde. Die Inkubation mit Patulin führte zudem zu einer erhöhten Anzahl von vielkernigen Zellen und multipolaren Mitosen. Mittels Durchflusszytometrie konnten wir einen durch Patulin verursachten G2 Arrest nachweisen, der die Amplifikation von Centrosomen und die Patulin induzierte Aneuploidie erklären könnte. Patulin verursachte einen dosisabhängigen Schaden im Comet Assay, der durch den zellulären Glutathiongehalt beeinflusst ist. Eine Auslösung von oxidativem Stress wurde dagegen erst bei höheren Konzentrationen an Patulin beobachtet. Der zelluläre Gluathiongehalt war nach 24 h Inkubationszeit erhöht, was auf eine adaptive Antwort auf den durch Patulin verursachten zellulären Stress hindeutet. Polyphenole wie Resveratrol gewinnen zunehmend an Bedeutung, da zahlreiche positive Effekte auf die menschliche Gesundheit bewiesen wurden. Diese vorteilhaften Eigenschaften werden zum Teil ihrer Eigenschaft als Radikalfänger zugeschrieben. Die Co-Inkubation von V79 Zellen mit Patulin und Resveratrol führte zu einer leichten Reduktion der Mikrokernfrequenz im Vergleich zu Zellen, die nur mit Patulin inkubiert wurden. Allerdings löste Resveratrol in höheren Konzentrationen selbst die Bildung von Mikrokernen aus. Die Kinetochor-Analyse zeigte für Resveratrol clastogene Eigenschaften aber keine störende Effekte auf den Ablauf der Mitose. Die antioxidativen Eigenschaften von Resveratrol wurden im FRAP (ferric reducing antioxidant power) -Assay nachgewiesen. Im Gegensatz dazu wurden im zellulären System mittels DCF (2,7-Dichlordihydro-fluorescein) -Assay in höheren Konzentrationen auch prooxidative Eigenschaften festgestellt. Der erhöhte zelluläre Glutathionspiegel nach Resveratrol-Behandlung könnte dabei auf eine adaptive Anwort auf den durch Resveratrol ausgelösten oxidativen Stress hindeuten Im zweiten Teil dieser Doktorabeit haben wir die Effekte eines anthocyanreichen Traubenextrakts auf hypertensive Ren-2 Ratten untersucht. Ren-2 Ratten sind ein anerkanntes genetisch modifiziertes Rattenmodell zur Untersuchung von Bluthochdruck und erhöhtem oxidativem Stress. Wir haben 23 weibliche Ren-2 Ratten in 3 Gruppen geteilt. Eine Gruppe wurde mit einem anthocyan-reichen Dacapo Traubenextrakt gefüttert, eine Gruppe wurde mit dem ACE (angiotensin converting enzyme) Inhibitor Ramipril behandelt und eine dritte Gruppe wurde während dem Experiment nicht medikamentös behandelt. Nach einer Woche zeigte die nicht therapierte Gruppe einen deutlichen Anstieg des systolischen und diastolischen Blutdrucks. Dieser Anstieg war bei der mit anthocyanreichem Dacapo Traubenextrakt gefütterten Gruppe abgeschwächt. Die Effekte auf den Blutdruck spiegelten sich auch in einer erhöhten Trinkmenge der unbehandelten und mit Extrakt behandelten Tiere wider. Ein Comet Assay mit Nieren- und Leberzellen zeigte einen schwachen schützenden Einfluß des Dacapoextrakts auf den DNA Schaden im Vergleich zu den anderen Behandlungsgruppen. Ähnliche Ergebnisse wurden auch bei der Auswertung der ɣ-H2AX Färbung in Nieren- und Herzschnitten erzielt. Im Dünndarm wurden dagegen gegensätzliche Effekte beobachtet, die auf eine erhöhte Doppelstrangfrequenz durch die hohe lokale Konzentration an Polyphenolen nach oraler Aufnahme hindeuten. Die antioxidative Eigenschaften des Extrakts wurden im FRAP_Assay nachgewiesen. Diese Effekte spiegelten sich jedoch nicht in einer erhöhten antioxidativen Kapazität des Serums oder einem schützenden Effekt im DHE-Assay wider. Der Extrakt zeigte schützende Eigenschaften im Comet Assay und in der ɣ-H2AX-Färbung, war aber nicht in der Lage den Bluthochdruck auf das Kontrollniveau der Ramipril-behandelten Tiere herabzusenken. Hohe lokale Konzentrationen können auch zu einem erhöhten Schaden des betroffenen Gewebes führen. Daher sollte die Anwendung solcher hochkonzentrierter Präparate mit Vorsicht bedacht werden. KW - Patulin KW - Anthocyane KW - Resveratrol KW - Oxidativer Stress KW - Mutagenität KW - Genotoxizität KW - Patulin KW - anthocyanins KW - resveratrol KW - genotoxicity KW - oxidative stress Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-72872 ER - TY - JOUR A1 - Gmach, Philipp A1 - Bathe-Peters, Marc A1 - Telugu, Narasimha A1 - Miller, Duncan C. A1 - Annibale, Paolo T1 - Fluorescence spectroscopy of low-level endogenous β-adrenergic receptor expression at the plasma membrane of differentiating human iPSC-derived cardiomyocytes JF - International Journal of Molecular Sciences N2 - The potential of human-induced pluripotent stem cells (hiPSCs) to be differentiated into cardiomyocytes (CMs) mimicking adult CMs functional morphology, marker genes and signaling characteristics has been investigated since over a decade. The evolution of the membrane localization of CM-specific G protein-coupled receptors throughout differentiation has received, however, only limited attention to date. We employ here advanced fluorescent spectroscopy, namely linescan Fluorescence Correlation Spectroscopy (FCS), to observe how the plasma membrane abundance of the β\(_1\)- and β\(_2\)-adrenergic receptors (β\(_{1/2}\)-ARs), labelled using a bright and photostable fluorescent antagonist, evolves during the long-term monolayer culture of hiPSC-derived CMs. We compare it to the kinetics of observed mRNA levels in wildtype (WT) hiPSCs and in two CRISPR/Cas9 knock-in clones. We conduct these observations against the backdrop of our recent report of cell-to-cell expression variability, as well as of the subcellular localization heterogeneity of β-ARs in adult CMs. KW - GPCR KW - β-adrenergic receptors KW - hiPSC-CM KW - cardiomyocyte KW - fluorescence correlation spectroscopy KW - FCS KW - fluorescence KW - CRISPR/Cas9 KW - differentiation Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-288277 SN - 1422-0067 VL - 23 IS - 18 ER - TY - JOUR A1 - Godbole, Amod A1 - Lyga, Sandra A1 - Lohse, Martin J. A1 - Calebiro, Davide T1 - Internalized TSH receptors en route to the TGN induce local G\(_{S}\)-protein signaling and gene transcription JF - Nature Communications N2 - A new paradigm of G-protein-coupled receptor (GPCR) signaling at intracellular sites has recently emerged, but the underlying mechanisms and functional consequences are insufficiently understood. Here, we show that upon internalization in thyroid cells, endogenous TSH receptors traffic retrogradely to the trans-Golgi network (TGN) and activate endogenous Gs-proteins in the retromer-coated compartment that brings them to the TGN. Receptor internalization is associated with a late cAMP/protein kinase A (PKA) response at the Golgi/TGN. Blocking receptor internalization, inhibiting PKA II/interfering with its Golgi/TGN localization, silencing retromer or disrupting Golgi/TGN organization all impair efficient TSH-dependent cAMP response element binding protein (CREB) phosphorylation. These results suggest that retrograde trafficking to the TGN induces local G\(_{S}\)-protein activation and cAMP/PKA signaling at a critical position near the nucleus, which appears required for efficient CREB phosphorylation and gene transcription. This provides a new mechanism to explain the functional consequences of GPCR signaling at intracellular sites and reveals a critical role for the TGN in GPCR signaling. KW - G protein-coupled receptors KW - fluorescence imaging KW - hormone receptors KW - trans-Golgi network Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170375 VL - 8 IS - 443 ER - TY - JOUR A1 - Gonzales-Calero, G. A1 - Cubero, A. A1 - Klotz, Karl-Norbert T1 - G protein coupled A\(_1\) adenosine receptors in coated vesicles of mammalian brain. Characterization by radioligand binding and photoaffinity labeling N2 - A\(_1\) adenosine receptors in coated vesicles have been characterized by radioligand binding and photoaflinity labelling. Saturation experiments with the antagonist 8-cyclopentyl-1 ,3-[\(^3\)H]dipropyl-xanthine ([\(^3\)H]DPCPX) gave a Kdvalue of 0.7 nM and a Bmax value of 82± 13 fmol/mg protein. For the highly A\(_1\)-selective agonist 2-chloro-N\(^6\)-[\(^3\)H]cyclopentyladenosine ([\(^3\)H]CCPA) a Kd value of 1.7 nM and a Bmax value of 72 ± 29 fmol/mg protein was estimated. Competition of agonists for [\(^3\)H]DPCPX binding gave a pharmacological profile with R-N\(^6\)-phenylisopropyladenosine (R-PIA) > CCPA > S-PIA > 5'-N-ethylcarboxamidoadenosine (NECA), which is identical to brain membranes. The competition curves were best fitted according to a two-site model, suggesting the existence of two affinity states. GTP shifted the competition curve for CCP A to the right and only one affinity state similar to the low affinity state in the absence of GTP was detected. The photoreactive agonist 2-azido-N\(^6\)- \(^{125}\)I-p-hydroxyphenylisopropyladenosine ([\(^{125}\)I]AHPIA) specifically labelled a single protein with an apparent molecular weight of 35,000 in coated vesicles, which is identical to A\(_1\) receptors labelled in brain membranes. Therefore, coated vesicles contain A\(_1\) adenosine receptors with similar binding characteristics as membrane-bound receptors, including GTP-sensitive high-affinity agonist binding. Photoaffinity labelling data suggest that A\(_1\) receptors in these vesicles are not a processed receptor fonn. These results confirm that A\(_1\) receptors in coated vesicles are coupled to a G-protein, and it appears that the A\(_1\) receptor systems in coated vesicles andin plasma membranes are identical. KW - Toxikologie KW - Adenosine receptors KW - coated vesicles KW - G-protein KW - radioligand KW - photoaffinity labelling KW - brain membranes Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60435 ER - TY - JOUR A1 - Gonzalez-Calero, G. A1 - Cubero, A. A1 - Klotz, Karl-Norbert T1 - Characterization and photoaffinity labeling of A1 adenosine receptors in coated visicles form bovine brain N2 - The antagonist (3 II ) DPCPX exhi bitcd a Kd of 0. 4 nM at coalcd vcsicles from bovine brain. Agonist compelition for ( 3 11) DPCPX bind in~ revcaled two affini ty slales for gonists. The pholoaffinity probe I25 I -AHPIA specifically labelled a band with a molecular weight of 35 Kd. KW - Pharmakologie Y1 - 1991 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86004 ER - TY - JOUR A1 - Grilli, S. A1 - Lutz, Werner K. A1 - Parodi, S. T1 - Possible implications from results of animal studies in human risk estimations for benzene: nonlinear dose-response relationship due to saturation of metabolism N2 - To date, all risk assessment studies on benzene have been based almost exclusively on epiderniological data. Wehave attempted a more integrated and quantitative evaluation of carcinogenic risk for hurnans, trying to utilize, in addition to the epidemiological data, all data available, specifically data on metabolism, genotoxicity, and carcinogenicity in small rodents. An integrated evaluation of the globality of the available data seems to suggest a progressive saturation of metabolic capacity both for man and rodents between 10 and 100 ppm. The most susceptible target cells seem tobe different in humans (predominant induction of myelogenous leukemia) and small rodents (induction of a wide variety of tumors). Nevertheless, both epidemiological and experimental carcinogenicity data tend to indicate a flattening ofthe response for the highest dosages, again suggesting a general Saturation of mechanisms of metabolic activation, extended to different target tissues. From a quantitative point of view, the data suggest a carcinogenic potency at 10 ppm two to three times higher than that computable by a linear extrapolation from data in the 100 ppm range. These observations are in accord with the recent proposal of the European Economic Community of reducing benzene time-weighted average occupationallevels from 10 to 5 ppm. KW - Toxikologie KW - Benzene KW - Risk estimation KW - Carcinogenicity KW - Genotoxicity KW - Metabolism saturation KW - Dose-response relationship Y1 - 1987 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60936 ER - TY - JOUR A1 - Gross, E. A1 - Ruzicka, T. A1 - Restorff, B. von A1 - Stolz, W. A1 - Klotz, Karl-Norbert T1 - High-affinity binding and lack of growth-promoting activity of 12(S)-hydroxyeicosatetraenoic acid (12(S)-HETE) in a human epidermal cell line N2 - No abstract available KW - Toxikologie Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60358 ER - TY - JOUR A1 - Grunicke, H. A1 - Pyerin, W. A1 - Eisenbrand, G. A1 - Havemann, K. A1 - Rabes, H. M. A1 - Molling, K. A1 - Schwab, M. A1 - Lutz, Werner K. A1 - Wahrendorf, J. A1 - Schirrmacher, V. T1 - 7th International Symposium of the Division of Experimental Cancer Research (AEK) of the German Cancer Society : [Meeting report] N2 - No abstract available KW - Toxikologie Y1 - 1994 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60651 ER - TY - JOUR A1 - Gunz, D. A1 - Shephard, S. E. A1 - Lutz, Werner K. T1 - Can nongenotoxic carcinogens be detected with the lacI transgenic mouse mutation assay? N2 - No abstract available KW - Toxikologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60707 ER - TY - JOUR A1 - Guth, Sabine A1 - Hüser, Stephanie A1 - Roth, Angelika A1 - Degen, Gisela A1 - Diel, Patrick A1 - Edlund, Karolina A1 - Eisenbrand, Gerhard A1 - Engel, Karl-Heinz A1 - Epe, Bernd A1 - Grune, Tilman A1 - Heinz, Volker A1 - Henle, Thomas A1 - Humpf, Hans-Ulrich A1 - Jäger, Henry A1 - Joost, Hans-Georg A1 - Kulling, Sabine E. A1 - Lampen, Alfonso A1 - Mally, Angela A1 - Marchan, Rosemarie A1 - Marko, Doris A1 - Mühle, Eva A1 - Nitsche, Michael A. A1 - Röhrdanz, Elke A1 - Stadler, Richard A1 - van Thriel, Christoph A1 - Vieths, Stefan A1 - Vogel, Rudi F. A1 - Wascher, Edmund A1 - Watzl, Carsten A1 - Nöthlings, Ute A1 - Hengstler, Jan G. T1 - Contribution to the ongoing discussion on fluoride toxicity JF - Archives of Toxicology N2 - Since the addition of fluoride to drinking water in the 1940s, there have been frequent and sometimes heated discussions regarding its benefits and risks. In a recently published review, we addressed the question if current exposure levels in Europe represent a risk to human health. This review was discussed in an editorial asking why we did not calculate benchmark doses (BMD) of fluoride neurotoxicity for humans. Here, we address the question, why it is problematic to calculate BMDs based on the currently available data. Briefly, the conclusions of the available studies are not homogeneous, reporting negative as well as positive results; moreover, the positive studies lack control of confounding factors such as the influence of well-known neurotoxicants. We also discuss the limitations of several further epidemiological studies that did not meet the inclusion criteria of our review. Finally, it is important to not only focus on epidemiological studies. Rather, risk analysis should consider all available data, including epidemiological, animal, as well as in vitro studies. Despite remaining uncertainties, the totality of evidence does not support the notion that fluoride should be considered a human developmental neurotoxicant at current exposure levels in European countries. KW - pharmacology/toxicology KW - occupational medicine/industrial medicine KW - environmental health KW - biomedicine, general Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-307161 SN - 0340-5761 SN - 1432-0738 VL - 95 IS - 7 ER - TY - JOUR A1 - Hadi, Naji Said Aboud A1 - Bankoglu, Ezgi Eyluel A1 - Stopper, Helga T1 - Genotoxicity of pyrrolizidine alkaloids in metabolically inactive human cervical cancer HeLa cells co-cultured with human hepatoma HepG2 cells JF - Archives of Toxicology N2 - Pyrrolizidine alkaloids (PAs) are secondary plant metabolites, which can be found as contaminant in various foods and herbal products. Several PAs can cause hepatotoxicity and liver cancer via damaging hepatic sinusoidal endothelial cells (HSECs) after hepatic metabolization. HSECs themselves do not express the required metabolic enzymes for activation of PAs. Here we applied a co-culture model to mimic the in vivo hepatic environment and to study PA-induced effects on not metabolically active neighbour cells. In this co-culture model, bioactivation of PA was enabled by metabolically capable human hepatoma cells HepG2, which excrete the toxic and mutagenic pyrrole metabolites. The human cervical epithelial HeLa cells tagged with H2B-GFP were utilized as non-metabolically active neighbours because they can be identified easily based on their green fluorescence in the co-culture. The PAs europine, riddelliine and lasiocarpine induced micronuclei in HepG2 cells, and in HeLa H2B-GFP cells co-cultured with HepG2 cells, but not in HeLa H2B-GFP cells cultured alone. Metabolic inhibition of cytochrome P450 enzymes with ketoconazole abrogated micronucleus formation. The efflux transporter inhibitors verapamil and benzbromarone reduced micronucleus formation in the co-culture model. Furthermore, mitotic disturbances as an additional genotoxic mechanism of action were observed in HepG2 cells and in HeLa H2B-GFP cells co-cultured with HepG2 cells, but not in HeLa H2B-GFP cells cultured alone. Overall, we were able to show that PAs were activated by HepG2 cells and the metabolites induced genomic damage in co-cultured HeLa cells. KW - co-culture KW - micronuclei KW - mitotic disturbance KW - cytochrome P450s KW - membrane transporters KW - pyrrolizidine alkaloids Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-324708 VL - 97 IS - 1 ER - TY - JOUR A1 - Hegi, M. E. A1 - Ulrich, D. A1 - Sagelsdorff, P. A1 - Richter, C. A1 - Lutz, Werner K. T1 - No measurable increase in thymidine glycol or 8-hydroxydeoxyguanosine in liver DNA of rats treated with nafenopin or choline-devoid low-methionine diet N2 - Male rats were treated for 2 months with 1000 ppm nafenopin in the diet or for 4 or 7 days with a choline-devoid low-methionine diet. DNA was isolated from the livers and analyzed for the presence of cis-thymidine glycol-3'-phosphate (cis-dTGp) by 32P-postlabeling and for the Ievel of 8-hydroxy-deoxyguanosine (8-0H-dG) by electrochemical detection (ECD). In no DNA sample was the Ievel of cis-dTGp above the Iimit of detection of 1 modified thymidine per 106 nucleotides. With 8-0H-dG, a background Ievel of this modification of 20 8-0H-dG per 106 nucleosides was found in liver DNA of control rats, which was not affected by either treatment. It is postulated for thymidine glycol that a potential increase was below the Iimit of detection or was rapidly repaired in vivo and that the steady-state Ievel of endogenous 8-hydroxydeoxyguanosine appears not tobe influenced by the treatments chosen. KW - Toxikologie KW - Oxygen radical KW - DNA KW - Genotoxicity KW - Rat liver peroxisome KW - Choline deficiency KW - Thymidine glycol KW - 8-Hydroxy-deoxyguanosine Y1 - 1990 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60790 ER - TY - JOUR A1 - Hegi, M.E. A1 - Sagelsdorff, P. A1 - Lutz, Werner K. T1 - Detection by \(^{32}\)P-postlabeling of thymidine glycol in gamma-irradiated DNA N2 - No abstract available KW - Toxikologie Y1 - 1989 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60863 ER - TY - JOUR A1 - Hintzsche, Henning A1 - Jastrow, Christian A1 - Kleine-Ostmann, Thomas A1 - Kärst, Uwe A1 - Schrader, Thorsten A1 - Stopper, Helga T1 - Terahertz electromagnetic fields (0.106 THz) do not induce manifest genomic damage in vitro N2 - Terahertz electromagnetic fields are non-ionizing electromagnetic fields in the frequency range from 0.1 to 10 THz. Potential applications of these electromagnetic fields include the whole body scanners, which currently apply millimeter waves just below the terahertz range, but future scanners will use higher frequencies in the terahertz range. These and other applications will bring along human exposure to these fields. Up to now, only a limited number of investigations on biological effects of terahertz electromagnetic fields have been performed. Therefore, research is strongly needed to enable reliable risk assessment. Cells were exposed for 2 h, 8 h, and 24 h with different power intensities ranging from 0.04 mW/cm2 to 2 mW/cm2, representing levels below, at, and above current safety limits. Genomic damage on the chromosomal level was measured as micronucleus formation. DNA strand breaks and alkali-labile sites were quantified with the comet assay. No DNA strand breaks or alkali-labile sites were observed as a consequence of exposure to terahertz electromagnetic fields in the comet assay. The fields did not cause chromosomal damage in the form of micronucleus induction. KW - Toxikologie Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-76268 ER - TY - JOUR A1 - Hintzsche, Henning A1 - Montag, Gracia A1 - Stopper, Helga T1 - Induction of micronuclei by four cytostatic compounds in human hematopoietic stem cells and human lymphoblastoid TK6 cells JF - Scientific Reports N2 - For mutagenicity testing, primary lymphocytes or mammalian cell lines are employed. However, the true target for carcinogenic action of mutagenic chemicals may be stem cells. Since hematopoietic cancers induced by chemical agents originate at the hematopoietic stem cell (HSC) stage and since one of the side effects of chemotherapeutic cancer treatment is the induction of secondary tumors, often leukemias, HSC may be a suitable cell system. We compared the sensitivity of HSC with the genotoxicity testing cell line TK6 for chromosomal mutations. HSC were less sensitive than TK6 cells for the genotoxic effects of the model genotoxins and chemotherapeutic agents doxorubicin, vinblastine, methyl methanesulfonate (MMS) and equally sensitive for mitomycin C (MMC). However, loss of viability after mitomycin C treatment was higher in HSC than in TK6 cells. Among the factors that may influence sensitivity for genomic damage, the generation or response to reactive oxygen species (ROS) and the effectiveness of DNA damage response can be discussed. Here we show that HSC can be used in a standard micronucleus test protocol for chromosomal mutations and that their sensitivity was not higher than that of a classical testing cell line. KW - apoptosis KW - haematopoietic stem cells KW - TK6 cells KW - micronuclei Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176210 VL - 8 IS - 3371 ER - TY - JOUR A1 - Hoffmann, Linda S A1 - Schmidt, Peter M A1 - Keim, Yvonne A1 - Hoffmann, Carsten A1 - Schmidt, Harald H H W A1 - Stasch, Johannes-Peter T1 - Fluorescence Dequenching Makes Haem-Free Soluble Guanylate Cyclase Detectable in Living Cells JF - PLOS ONE N2 - In cardiovascular disease, the protective NO/sGC/cGMP signalling-pathway is impaired due to a decreased pool of NO-sensitive haem-containing sGC accompanied by a reciprocal increase in NO-insensitive haem-free sGC. However, no direct method to detect cellular haem-free sGC other than its activation by the new therapeutic class of haem mimetics, such as BAY 58-2667, is available. Here we show that fluorescence dequenching, based on the interaction of the optical active prosthetic haem group and the attached biarsenical fluorophor FlAsH can be used to detect changes in cellular sGC haem status. The partly overlap of the emission spectrum of haem and FlAsH allows energy transfer from the fluorophore to the haem which reduces the intensity of FlAsH fluorescence. Loss of the prosthetic group, e. g. by oxidative stress or by replacement with the haem mimetic BAY 58-2667, prevented the energy transfer resulting in increased fluorescence. Haem loss was corroborated by an observed decrease in NO-induced sGC activity, reduced sGC protein levels, and an increased effect of BAY 58-2667. The use of a haem-free sGC mutant and a biarsenical dye that was not quenched by haem as controls further validated that the increase in fluorescence was due to the loss of the prosthetic haem group. The present approach is based on the cellular expression of an engineered sGC variant limiting is applicability to recombinant expression systems. Nevertheless, it allows to monitor sGC's redox regulation in living cells and future enhancements might be able to extend this approach to in vivo conditions. KW - spontaneously hypersensitive-rats KW - nitric-oxide KW - down-regulation KW - energy-transfer KW - cyclic-gmp KW - protein KW - activation KW - identification KW - in-vivo KW - no Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-139631 VL - 6 IS - 8 ER - TY - JOUR A1 - Holler, E. A1 - Fischer, H. A1 - Weber, C. A1 - Stopper, Helga A1 - Steger, H. A1 - Simek, H. T1 - A DNA polymerase with unusual properties from the slime mold Physarum polycephalum N2 - Two forms of a DNA polymerase have been purified from microplasmodia of Physarum polycephalum by poly(ethyleneimine) precipitation and chromatography on DEAE-Sephacel, phosphocellulose, heparin Sepharose, hydroxyapatite, DNA-agarose, blue-Sepharose. They were separated from DNA polymerase cx on phosphocellulose and from each other on heparin-Sepharose. Form HS1 enzymewas 30-40% pure and form HS2 enzyme 60% with regard toprotein contents of the preparations. Form HS2 enzymewas generated from form HS1 enzyme on prolonged standing of enzyme preparations. The DNA polymerases were obtained as complexes of a 60-kDa protein associated with either a 135-kDa (HS1) or a 110-kDa (HS2) DNA-polymerizing polypeptidein a 1:1 molar stoichiometry. The biochemical function of the 60-kDa protein remained unknown. The complexes tended to dissociate during gradient centrifugation and during partition chromatography as weil as during polyacrylamide gradient gel electrophoresis under nondenaturing conditions at high dilutions of samples. Both forms existed in plasmodia extracts, their proportions depending on several factors including those which promoted proteolysis. The DNA polymerases resembled eucaryotic DNA polymerase ß by several criteria and were functionally indistinguishable from each other. It is suggested that lower eucaryotes contain repair DNA polymerases, which are similar to those of eubacteria on a molecular mass basis. KW - Toxikologie Y1 - 1987 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-63501 ER - TY - JOUR A1 - Huber, K. W. A1 - Lutz, Werner K. T1 - Methylation of DNA in stomach and small intestine of rats after oral administration of methylamine and nitrite N2 - Young adult male Sprague-Dawley rats were given 30 \(\mu\)mol/kg body weight [\(^{14}\)C]methylamine hydrochloride and 700 \(\mu\)mol/ kg body weight sodium nilrite by oral gavage. DNA isolated from the stomach and from the first 15 cm of the smaß intestine was methylated, containing 7-methylguanine (7mG) at a level of one 7mG molecule per 5x10\8^6\) and lx10\(^7\) nucleotides, respectively. No 7mG was found fn the liver at a limit of detection of one 7mG molecule per 2xl0\(^8\) nucleotides. ln a second experiment, the excised stomachs were incubated with deoxyribonuclease before the isolation of the DNA in order to degrade DNA in the Iumen and in the uppermost lining cells. This treatment resulted in a 30% decrease in the yield of DNA and a 90% reduction in the level of 7mG formation. The results show that nitrosation of a primary alkylamine yields a precursor of an alkylating agent which has a long enough lifetime to diffuse towards and react with intracellular DNA. A correlation of DNA methylation in the stomach with the corresponding tumor formation by the methylating carcinogen N-methyi-N'-nitro-N-nitroso-guanidine was used to estimate the roJe of DNA damage resulting from endogenous nitrosation of dietary methylamine in man. It was concluded that the risk resulting from this single amine must be negligible bot that a similar evaluation of other primary amines is required before the over-aU role of primary amine nitrosation in the etiology of human gastric cancer can be assessed. KW - Toxikologie Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-60984 ER - TY - JOUR A1 - Huber, K. W. A1 - Lutz, Werner K. T1 - Methylation of DNA by incubation with methylamine and nitrite N2 - DNA was incubated in septum-closed reaction vials with [\(^{14}\)C]methylamine and nitrite. The DNA was purified, hydrolysed with hydrochloric acid, and the purines were analysed by h.p.l.c. 7-Methylguanine was detectable as a result of DN A methylation in experiments perfonned in 100 mM acetate at pH 4. Using different concentrations of amine and nitrite a first order reaction for total amine and a second order for total nilrite could be shown. A study on the pH dependence using 100 mM malonate buffer, pH 2.0-6.0, revealed a maximum rate at pH 3.5, with steep slopes above and below this pH value, in agreement with a mathematical analysis of the reaction equations. The data show that the alkylating agent fonned spontaneously by nitrosation and deamination of a primary amine has a long enough lifetime to react with DNA in vitro. Using the reactioil orders established here, an extrapolation to lower concentrations found in the stomach can now be perfonned. Future in vivo experiments on the methylation of gastro-intestinal DNA then would show to what extent DNA in a cell is protected from alkylation. KW - Toxikologie Y1 - 1984 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61011 ER - TY - THES A1 - Hupp, Sabrina T1 - Modulation of Actin Dynamics by the Cholesterol-Dependent Cytolysin Pneumolysin - a novel mechanism beyond pore formation T1 - Einfluß des CDCs Pneumolysin auf die Aktin-Dynamik - neue Eigenschaften eines Poren-bildenden Toxins N2 - Streptococcus pneumoniae is one of the major causes of bacterial meningitis, which mainly affects young infants in the developing countries of Africa, Asia (esp. India) and South America, and which has case fatality rates up to 50% in those regions. Bacterial meningitis comprises an infection of the meninges and the sub-meningeal cortex tissue of the brain, whereat the presence of pneumolysin (PLY), a major virulence factor of the pneumococcus, is prerequisite for the development of a severe outcome of the infection and associated tissue damage (e. g. apoptosis, brain edema, and ischemia). Pneumolysin belongs to the family of pore forming, cholesterol-dependent cytolysins (CDCs), bacterial protein toxins, which basically use membrane-cholesterol as receptor and oligomerize to big aggregates, which induce cell lysis and cell death by disturbance of membrane integrity. Multiple recent studies, including this work, have revealed a new picture of pneumolysin, whose cell-related properties go far beyond membrane binding, pore formation and the induction of cell death and inflammatory responses. For a long time, it has been known that bacteria harm the tissues of their hosts in order to promote their own survival and proliferation. Many bacterial toxins aim to rather hijack cells than to kill them, by interacting with cellular components, such as the cytoskeleton or other endogenous proteins. This study was able to uncover a novel capacity of pneumolysin to interact with components of the actin machinery and to promote rapid, actin-dependent cell shape changes in primary astrocytes. The toxin was applied in disease-relevant concentrations, which were verified to be sub-lytic. These amounts of toxin induced a rapid actin cortex collapse in horizontal direction towards the cell core, whereat membrane integrity was preserved, indicating an actin severing function of pneumolysin, and being consistent with cell shrinkage, displacement, and blebbing observed in live cell imaging experiments. In contrast to neuroblastoma cells, in which pneumolysin led to cytoskeleton remodeling and simultaneously to activation of Rac1 and RhoA, in primary astrocytes the cell shape changes were seen to be primarily independent of small GTPases. The level of activated Rac1 and RhoA did not increase at the early time points after toxin application, when the initial shape changes have been observed, but at later time points when the actin-dependent displacement of cells was slower and less severe, probably presenting the cell’s attempt to re-establish proper cytoskeleton function. A GUV (giant unilamellar vesicle) approach provided insight into the effects of pneumolysin in a biomimetic system, an environment, which is strictly biochemical, but still comprises cellular components, limited to the factors of interest (actin, Arp2/3, ATP, and Mg2+ on one side, and PLY on the other side). This approach was able to show that the wildtype-toxin, but not the Δ6 mutant (mutated in the unfolding domain, and thus non-porous), had the capacity to exhibit its functions through a membrane bilayer, meaning it was able to aggregate actin, which was located on the other side of the membrane, either via direct interaction with actin or in an Arp2/3 activating manner. Taking a closer look at these two factors with the help of several different imaging and biochemical approaches, this work unveiled the capacity of pneumolysin to bind and interact both with actin and Arp2 of the Arp2/3 complex. Pneumolysin was capable to slightly stabilize actin in an actin-pyrene polymerization assay. The same experimental setup was applied to show that the toxin had the capacity to lead to actin polymerization through activation of the Arp2/3 complex. This effect was additionally confirmed with the help of fluorescent microscopy of rhodamine (TRITC)-tagged actin. Strongest Arp2/3 activation, and actin nucleation/polymerization is achieved by the VCA domain of the WASP family proteins. However, addition of PLY to the Arp2/3–VCA system led to an enhanced actin nucleation, suggesting a synergistic activation function of pneumolysin. Hence, two different effects of pneumolysin on the actin cytoskeleton were observed. On the one hand an actin severing property, and on the other hand an actin stabilization property, both of which do not necessarily exclude each other. Actin remodeling is a common feature of bacterial virulence strategies. This is the first time, however, that these properties were assigned to a toxin of the CDC family. Cytoskeletal dysfunction in astrocytes leads to dysfunction and unregulated movement of these cells, which, in context of bacterial meningitis, can favor bacterial penetration and spreading in the brain tissue, and thus comprises an additional role of pneumolysin as a virulence factor of Streptococcus pneumonia in the context of brain infection. N2 - S. pneumoniae gehört zur Gruppe der Pathogene, die bakterielle Meningitis verursachen, eine Infektion, die hauptsächlich bei Neugeborenen und Kleinkindern in den Entwicklungsländern von Afrika, Asien und Südamerika auftritt, und in diesen Regionen Sterblichkeitsraten von bis zu 50% aufweist. Meningitis ist eine Infektion der Hirnhäute und dem sich direkt darunter befindlichen Cortex-Gewebe. Pneumolysin (PLY), ein Haupt-Pathogenitätsfaktor des sog. Pneumococcus, ist hauptsächlich verantwortlich für einen schweren Verlauf der Infektion und für Gewebeschädigungen, wie Apoptose, Hirnödemen und Ischämie. Pneumolysin gehört zur Familie der Cholesterol-abhängigen Cytolysine (CDCs), bakteriellen Protein-Toxinen, die an Membran-Cholesterol binden, sich zu großen Aggregaten zusammenschließen und durch die Beeinträchtigung der Membranintegrität (Porenbildung) Zell-Lyse und Zelltod verursachen. Zahlreiche neuere Studien, darunter auch diese Arbeit, haben ein neues Bild von Pneumolysin aufgezeigt, dessen Eigenschaften weit über die Membranbindung, die Poren-Bildung und die Induktion von Zelltod und inflammatorischen Prozessen hinausgehen. Es ist weithin bekannt, dass Bakterien das Gewebe ihres Wirts schädigen, um ihre eigene Vermehrung und ihre Ausbreitung zu begünstigen. In diesem Zusammenhang fungieren bakterielle Toxine als Pathogenitätsfaktoren, die mit zellulären Komponenten, wie dem Zytoskelett und anderen Zytosol-Proteinen interagieren, was allerdings bevorzugt zu Zellveränderungen, und seltener zum Zelltod führt. Die vorliegende Arbeit konnte zeigen, dass Pneumolysin schnelle, und zum Teil gravierende, Aktin-abhängige Zellstruktur-Veränderungen in primären Astrozyten hervorruft. Hierbei wurde das Toxin in Konzentrationen appliziert, die im Liquor von Meningitis-Patienten detektiert werden können, und die zusätzlich als sub-lytisch für Astrozyten in Zellkultur verifiziert wurden. Diese Toxin-Mengen führten zu einem schnellen, horizontalen Aktinkortex-Kollaps, wobei die Membranintegrität erhalten blieb. Dies deutete auf eine „Severing“-Funktion (das Abtrennen oder Zerschneiden von Aktinfilamenten) von Pneumolysin hin, was mit den Beobachtungen übereinstimmt, die in Experimenten mit lebendigen Zellen gemacht wurden (Zellveränderungen, Zellbewegungen und „Blebbings“). Im Gegensatz zu Neuroblastoma Zellen, in denen Pneumolysin Zytoskelett-Veränderungen, und gleichzeitig die Aktivierung von Rac1 und RhoA verursachte, waren die Zell-Veränderungen bei Astrozyten primär unabhängig von der Aktivierung kleiner GTPasen. Obwohl gezeigt werden konnte, dass die Veränderungen vom Aktin-Zytosklett abhängig waren, war das Level an Rac1 und RhoA in den frühen Phasen nach der Toxin-Gabe nicht erhöht. Eine Aktivierung der GTPasen konnte dahingegen zu späteren Zeitpunkten detektiert werden, in denen die Zellbewegung abgeschwächt und verlangsamt war. Die späte Aktivierung kann als Reaktion der Zelle auf die vom Toxin ausgelösten Veränderungen gesehen werden, die zu einer Wiederherstellung der normalen Zytoskelett-Funktion führen soll. GUV-Experimente ermöglichten eine genauere Betrachtung der Pneumolysin-Effekte in einem biomimetischen, jedoch strikt biochemischen Ansatz, der alle zellulären Komponenten enthält, die untersucht werden sollen (Pneumolysin, Aktin, Arp2/3, ATP, und Mg2+). Im GUV-System befand sich das Toxin im Inneren der Vesikel, und Aktin in der extra-vesikulären Suspension, einem Verhältnis genau umgekehrt zum zellullären System. Zusätzlich wurden Arp2/3 und ATP/Mg2+, für die Aktin-Polymerisierung essentielle Faktoren, in der Aktin-Suspension zur Verfügung gestellt. Die GUV-Experimente konnten zeigen, dass Wildtyp-Pneumolysin, allerdings nicht seine Mutante Δ6-PLY (Mutation in der sog. unfolding domain, und deshalb nicht Poren-bildend), seine Effekte auf das Aktin-Zytoskelett durch die Membran-Barriere hindurch, in einer Membran-gebundenen Form ausüben kann. Aktin wurde an den Stellen höchster Toxinbindung aggregiert, was entweder über eine direkte Interaktion von PLY mit Aktin, oder über eine Aktivierung des Aktin-Effektors Arp2/3 durch Pneumolysin erklärt werden kann. Weitere biochemische Ansätze (wie enzyme-linked sorbent assays, ELSAs) und Mikroskopie-Techniken (Immunocyto-Chemie) konnten beweisen, dass Pneumolysin sowohl mit Aktin, als auch mit Arp2 (einer Komponente des heptameren Arp2/3 Proteinkomplexes) direkt interagieren kann. Aktin-Pyren Experimente und Fluoreszenzmikroskopie (von TRITC-markiertem Aktin) wiesen auf eine Kapazität von Pneumolysin hin, Aktin direkt zu stabilisieren, und über die Aktivierung von Arp2/3 eine Aktin-Polymerisierung hervorrufen zu können. KW - Hirnhautentzündung KW - Bakteriengift KW - Perforine KW - Actin KW - Meningitis KW - Meningitis KW - Bacterial Toxins KW - Pneumolysin KW - Actin KW - Pore formation Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-70889 ER - TY - JOUR A1 - Hupp, Sabrina A1 - Förtsch, Christina A1 - Wippel, Carolin A1 - Ma, Jiangtao A1 - Mitchell, Timothy J. A1 - Iliev, Asparouh I. T1 - Direct Transmembrane Interaction between Actin and the Pore-Competent, Cholesterol-Dependent Cytolysin Pneumolysin JF - Journal of Molecular Biology N2 - The eukaryotic actin cytoskeleton is an evolutionarily well-established pathogen target, as a large number of bacterial factors disturb its dynamics to alter the function of the host cells. These pathogenic factors modulate or mimic actin effector proteins or they modify actin directly, leading to an imbalance of the precisely regulated actin turnover. Here, we show that the pore-forming, cholesterol-dependent cytolysin pneumolysin (PLY), a major neurotoxin of Streptococcus pneumoniae, has the capacity to bind actin directly and to enhance actin polymerisation in vitro. In cells, the toxin co-localised with F-actin shortly after exposure, and this direct interaction was verified by Förster resonance energy transfer. PLY was capable of exerting its effect on actin through the lipid bilayer of giant unilamellar vesicles, but only when its pore competence was preserved. The dissociation constant of G-actin binding to PLY in a biochemical environment was 170–190 nM, which is indicative of a high-affinity interaction, comparable to the affinity of other intracellular actin-binding factors. Our results demonstrate the first example of a direct interaction of a pore-forming toxin with cytoskeletal components, suggesting that the cross talk between pore-forming cytolysins and cells is more complex than previously thought. KW - pore-forming toxin KW - cholesterol-dependent cytolysin KW - actin KW - membrane KW - pneumolysin Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132297 VL - 425 IS - 3 ER - TY - JOUR A1 - Ilin, Alexander A1 - Kulmanov, Murat A1 - Nersesyan, Armen A1 - Stopper, Helga T1 - Genotoxic activity of the new pharmaceutical FS-1 in Salmonella/microsome test and mouse lymphoma L5178Y cells JF - Journal of BUON N2 - Purpose: The purpose of this study was to determine possible genotoxic effects of a new very promising antibacterial/ antiviral drug FS-1. Methods: The drug was tested in TA98, TA100, TA102, TA 1535 and TA1537 strains of Salmonella (Ames test) with and without metabolic activation, and also in mouse lymphoma L5178Y cells by means of micronucleus and comet assays. In microbes the drug was tested at concentrations up to 500 \(\mu\)g/plate and in mouse lymphoma cells up to 2,000 \(\mu\)g/ml. Results: In both test-systems in all experiments completely negative results were obtained although FS-1 was tested at maximum tolerated doses. Conclusions: The drug is not genotoxic. This is advantageous because many antibacterial/antiviral drugs possess such activity. KW - mutagenicity KW - antibacterial/antiviral drug KW - comet assay KW - mouse lymphoma L5178Y KW - Salmonella/microsome assay KW - micronucleus test Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143769 VL - 20 IS - 2 ER - TY - THES A1 - İşbilir, Ali T1 - Localization and Trafficking of CXCR4 and CXCR7 T1 - Lokalisation und Verteilung von CXCR4 und CXCR7 N2 - G protein-coupled receptors (GPCRs) constitute the largest class of membrane proteins, and are the master components that translate extracellular stimulus into intracellular signaling, which in turn modulates key physiological and pathophysiological processes. Research within the last three decades suggests that many GPCRs can form complexes with each other via mechanisms that are yet unexplored. Despite a number of functional evidence in favor of GPCR dimers and oligomers, the existence of such complexes remains controversial, as different methods suggest diverse quaternary organizations for individual receptors. Among various methods, high resolution fluorescence microscopy and imagebased fluorescence spectroscopy are state-of-the-art tools to quantify membrane protein oligomerization with high precision. This thesis work describes the use of single molecule fluorescence microscopy and implementation of two confocal microscopy based fluorescence fluctuation spectroscopy based methods for characterizing the quaternary organization of two class A GPCRs that are important clinical targets: the C-X-C type chemokine receptor 4 (CXCR4) and 7 (CXCR7), or recently named as the atypical chemokine receptor 3 (ACKR3). The first part of the results describe that CXCR4 protomers are mainly organized as monomeric entities that can form transient dimers at very low expression levels allowing single molecule resolution. The second part describes the establishment and use of spatial and temporal brightness methods that are based on fluorescence fluctuation spectroscopy. Results from this part suggests that ACKR3 forms clusters and surface localized monomers, while CXCR4 forms increasing amount of dimers as a function of receptor density in cells. Moreover, CXCR4 dimerization can be modulated by its ligands as well as receptor conformations in distinct manners. Further results suggest that antagonists of CXCR4 display distinct binding modes, and the binding mode influences the oligomerization and the basal activity of the receptor: While the ligands that bind to a “minor” subpocket suppress both dimerization and constitutive activity, ligands that bind to a distinct, “major” subpocket only act as neutral antagonists on the receptor, and do not modulate neither the quaternary organization nor the basal signaling of CXCR4. Together, these results link CXCR4 dimerization to its density and to its activity, which may represent a new strategy to target CXCR4. N2 - G protein-gekoppelte Rezeptoren (GPCRs) bilden die größte Klasse der Membranproteine und sind entscheidend an der Übersetzung extrazellulärer Reize in intrazelluläre Signale beteiligt, welche wiederum unzählige physiologische und pathophysiologische Prozesse regulieren. Die Forschungsergebnisse der letzten drei Jahrzehnte deutet darauf hin, dass viele GPCRs mittels noch weitgehend unbekannter Mechanismen miteinander Komplexe bilden können. Trotz vielfältiger Beobachtungen, die für die funktionelle Relevanz von GPCR-Dimeren und -Oligomeren sprechen, ist deren Existenz dennoch weiterhin umstritten, vor allem da verschiedene Methoden auf unterschiedliche quaternäre Anordnungen derselben Rezeptoren hinweisen. Von den derzeit verfügbaren Methoden zur genauen Untersuchung der GPCR Dimerisierung/-Oligomerisierung, stellen die hochauflösende Fluoreszenzmikroskopie sowie die bildbasierte Fluoreszenzspektroskopie die Techniken der Wahl dar. Die hier vorliegende Arbeit beschreibt die Anwendung der Einzelmolekül Fluoreszenzmikroskopie sowie zweier konfokalmikroskopischer Methoden zur Messung der Fluoreszenzfluktuation, mit deren Hilfe die quaternäre Anordnung zweier klinisch hochattraktiver Klasse A GPCRs untersucht wurde: der C-X-C Typ Chemokinrezeptoren 4 (CXCR4) und 7 (CXCR7), letzterer auch bekannt als atypischer Chemokinrezeptor 3 (ACKR3). Der erste Teil der Ergebnisse legt anhand Untersuchungen an einzelnen Molekülen dar, dass CXCR4 überwiegend in Form monomerer Einheiten auftritt, die bei sehr geringen Expressionsleveln kurzlebige Dimere bilden können. Der zweite Teil beschreibt die Etablierung und Anwendung räumlicher und zeitlicher Brillanzmethoden, die auf der spektroskopischen Untersuchung der Fluoreszenzfluktuation beruhen. Die Ergebnisse dieses Abschnitts deuten darauf hin, dass ACKR3 sowohl in Form beständiger Rezeptor-Cluster, und monomere Einheit an der Oberfläche lebender Zellen auftritt. CXCR4 ist bei zunehmender Rezeptordichte hingegen vermehrt in Form von Dimeren zu finden. Zudem kann die Dimerisierung von CXCR4 von dessen Liganden, als auch von der drei dimensionalen Anordnung der Rezeptorteilstrukturen (Rezeptorkonformation)auf unterschiedliche Weise reguliert werden. Die weiteren Ergebnisse legen nahe, dass Antagonisten auf unterschiedliche Weise an CXCR4 binden können und dass der jeweilige Bindungsmodus entscheidend für den Einfluss des Liganden auf Oligomerisierung und basale Aktivität von CXCR4 ist: Während Liganden, die an eine kleinere Untertasche des Rezeptors binden, sowohl die Dimerisierung als auch die Basalaktivität unterdrücken, fungieren Verbindungen, die an eine andere, größere Untertasche binden, lediglich als neutrale Antagonisten und zeigen keinerlei Einfluss auf die quaternäre Anordnung und basale Aktivität von CXCR4. Zusammenfassend verknüpfen diese Ergebnisse CXCR4-Dimerisierung mit der Rezeptordichte in Zellen und seiner Aktivität, was die Grundlage für neue Strategien zur phamakologischen Modulation von CXCR4 darstellen könnte. KW - G-Protein gekoppelter Rezeptor KW - GPCR KW - Receptor KW - Chemokine KW - oligomerization KW - CXCR4 Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-249378 ER - TY - JOUR A1 - Jaggi, W. A1 - Lutz, Werner K. A1 - Lüthy, J. A1 - Zweifel, U. A1 - Schlatter, C. T1 - In vivo covalent binding of aflatoxin metabolites isolated from animal tissue to rat-liver DNA N2 - Ring-labelled [\(^{14}\)C)aflatoxin B\(_1\) (AFB\(_1\)), prepared by biosynthesis. or generally labelled [\(^3\)H]AFB\(_1\) was administered by oral gavage to young adult male rats. After 6 hr. the liver was removed and two fractions were isolated, namely macromolecules, which contamed about 3 % of the initial dose of AFB\(_1\) radioactivity. and water-soluble, low-molecular aftatoxin conjugates containing about0·2% of the administered radioactivity. These two fractions were administered orally to other rats in order to determine the potential of radioactive aftatoxin residues for covalent binding to DNA. Such binding can be used as an indicator for carcinogenic potency. Liver DNA was isolated 9-12 hr after admmistration of the aflatoxin derivatives and in no case was any radioactivity detected on the DNA. It can be deduced on the basis of the limit of detection of radioactivity on the DNA, that macromolecule bound AFB\(_1\) derivatives are at least 4000 times less active than AFB\(_1\) with respect to covalent binding to rat-liver DNA. and that the water-soluble conjugates are at least 100 times less potent than AFB, itself. It is concluded that the carcinogenic risk for humans who consume liver or meat. containing such aflatoxin residues is negligible when compared with the risk from intake of aftatoxins in other food items. KW - Toxikologie Y1 - 1980 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61101 ER - TY - JOUR A1 - Jaggi, W. A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Comparative studies on the covalent binding of the carcinogen benzo(a)pyrene to DNA in various model systems N2 - The covalent binding of tritiated benzo(a)pyrene (BP) to DNA has been determined in rat liver in vivo, in rat liver perfused in situ, after incubation of BP with liver single cells, with liver homogenate, with liver microsomes and DNA, with fibroblasts from a rat granulorna pouch, and with · 2 cell lines. Li ver single cells were found to be a valuable compromise between the rnost sensitive system (microsomal incubation of BP with DNA) and the biologically most relevant system (in vivo ). KW - Toxikologie Y1 - 1979 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61131 ER - TY - JOUR A1 - Jaggi, W. A1 - Lutz, Werner K. A1 - Schlatter, C. T1 - Covalent binding of ethinylestradiol and estrone to rat liver DNA in vivo N2 - Thecovalent bindingof [6,7-\(^3\)H]ethinylestradiol (EE)and [6,7-\(^3\)H]estrone (E) to liver DNA of 200 g female ratswas measured 8 h after the administration of 80 \(\mu\)g (9.2 mCi) estrogen by gavage. The binding is 1.5 for EE and 1.1 for E, expressedas binding to DNA/dose, in units of \(\mu\)mol hormonefmol DNA phosphate/mmole honnone/kg body wt. It is in the same order of magnitude as for benzene and about 10 000 tim es below the binding of typical liver carcinogens, such as aflatoxin B\(_1\) or N,N-dimethylnitrosamine. KW - Toxikologie Y1 - 1978 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-61162 ER - TY - JOUR A1 - Janevski, J. A1 - Choh, V. A1 - Stopper, Helga A1 - Schiffmann, D. A1 - De Boni, U. T1 - Diethylstilbestrol alters the morphology and calcium levels of growth cones of PC12 cells in vitro N2 - Diethylstilbestrol (DES) is a synthetic estrogen with carcinogenic properties. DES is known to alter cytoskeletal components, including the organization of actin stress fibres in C6 rat glioma cells. ln a test of the hypothesis that DES disrupts actin Filaments of growth cones in neuron-like cells, DES-induced changes in filopodial lengths were quantified in rat pheochromocytoma (PC12) cells in vitro. DES significantly altered growth cone morphology, with collapse of growth cone filopodia and neurite retraction invariably occurring at a concentration of 10 MikroM. At 5 MikroM DES, transient reductions in total filopodiallengths occurred. At DES concentrations of 0.1 nM and 1 nM, reductions in total filopodiallengths occurred in a fraction of growth cones. Evidence exists which shows that growth cone activity and morphology are intimately linked to Ieveis of intracellular, free calcium and that DES increases such levels. Measurements of free intracellular calcium levels by fluorescence microscopy, at times concurrent with the DES-induced reduction in total filopodial lengths, showed that calcium levels were indeed significantly increased by 10 MirkoM DES. Labelling of filamentaus actin (f-actin) with FITC-phalloidin showed that the f-actin distribution in growth cones exposed to DES could not be differentiated from the distribution found in spontaneously retracting growth cones. Tagether with evidence which showed that growth cone motility was not affected, the results are taken to indicate that DES, rather than acting directly on the cytoskeleton, exerts its effects indirectly, by a calcium-induced destabilization of actin filaments in the growth cone. KW - Calcium KW - Zellskelett KW - Wachstumskonus KW - Diethylstilbestrol KW - Diethylstilbestrol KW - rat pheochromocytoma cells KW - growth cone KW - cytoskeleton KW - calcium Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86858 ER - TY - JOUR A1 - Janz, Anna A1 - Walz, Katharina A1 - Cirnu, Alexandra A1 - Surjanto, Jessica A1 - Urlaub, Daniela A1 - Leskien, Miriam A1 - Kohlhaas, Michael A1 - Nickel, Alexander A1 - Brand, Theresa A1 - Nose, Naoko A1 - Wörsdörfer, Philipp A1 - Wagner, Nicole A1 - Higuchi, Takahiro A1 - Maack, Christoph A1 - Dudek, Jan A1 - Lorenz, Kristina A1 - Klopocki, Eva A1 - Ergün, Süleyman A1 - Duff, Henry J. A1 - Gerull, Brenda T1 - Mutations in DNAJC19 cause altered mitochondrial structure and increased mitochondrial respiration in human iPSC-derived cardiomyocytes JF - Molecular Metabolism N2 - Highlights • Loss of DNAJC19's DnaJ domain disrupts cardiac mitochondrial structure, leading to abnormal cristae formation in iPSC-CMs. • Impaired mitochondrial structures lead to an increased mitochondrial respiration, ROS and an elevated membrane potential. • Mutant iPSC-CMs show sarcomere dysfunction and a trend to more arrhythmias, resembling DCMA-associated cardiomyopathy. Background Dilated cardiomyopathy with ataxia (DCMA) is an autosomal recessive disorder arising from truncating mutations in DNAJC19, which encodes an inner mitochondrial membrane protein. Clinical features include an early onset, often life-threatening, cardiomyopathy associated with other metabolic features. Here, we aim to understand the metabolic and pathophysiological mechanisms of mutant DNAJC19 for the development of cardiomyopathy. Methods We generated induced pluripotent stem cell-derived cardiomyocytes (iPSC-CMs) of two affected siblings with DCMA and a gene-edited truncation variant (tv) of DNAJC19 which all lack the conserved DnaJ interaction domain. The mutant iPSC-CMs and their respective control cells were subjected to various analyses, including assessments of morphology, metabolic function, and physiological consequences such as Ca\(^{2+}\) kinetics, contractility, and arrhythmic potential. Validation of respiration analysis was done in a gene-edited HeLa cell line (DNAJC19tv\(_{HeLa}\)). Results Structural analyses revealed mitochondrial fragmentation and abnormal cristae formation associated with an overall reduced mitochondrial protein expression in mutant iPSC-CMs. Morphological alterations were associated with higher oxygen consumption rates (OCRs) in all three mutant iPSC-CMs, indicating higher electron transport chain activity to meet cellular ATP demands. Additionally, increased extracellular acidification rates suggested an increase in overall metabolic flux, while radioactive tracer uptake studies revealed decreased fatty acid uptake and utilization of glucose. Mutant iPSC-CMs also showed increased reactive oxygen species (ROS) and an elevated mitochondrial membrane potential. Increased mitochondrial respiration with pyruvate and malate as substrates was observed in mutant DNAJC19tv HeLa cells in addition to an upregulation of respiratory chain complexes, while cellular ATP-levels remain the same. Moreover, mitochondrial alterations were associated with increased beating frequencies, elevated diastolic Ca\(^{2+}\) concentrations, reduced sarcomere shortening and an increased beat-to-beat rate variability in mutant cell lines in response to β-adrenergic stimulation. Conclusions Loss of the DnaJ domain disturbs cardiac mitochondrial structure with abnormal cristae formation and leads to mitochondrial dysfunction, suggesting that DNAJC19 plays an essential role in mitochondrial morphogenesis and biogenesis. Moreover, increased mitochondrial respiration, altered substrate utilization, increased ROS production and abnormal Ca\(^{2+}\) kinetics provide insights into the pathogenesis of DCMA-related cardiomyopathy. KW - cell biology KW - molecular biology KW - dilated cardiomyopathy with ataxia KW - genetics KW - metabolism KW - mitochondria KW - OXPHOS KW - ROS KW - contractility Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350393 SN - 2212-8778 VL - 79 ER - TY - JOUR A1 - Jarzina, Sebastian A1 - Di Fiore, Stefano A1 - Ellinger, Bernhard A1 - Reiser, Pia A1 - Frank, Sabrina A1 - Glaser, Markus A1 - Wu, Jiaqing A1 - Taverne, Femke J. A1 - Kramer, Nynke I. A1 - Mally, Angela T1 - Application of the adverse outcome pathway concept to in vitro nephrotoxicity assessment: kidney injury due to receptor-mediated endocytosis and lysosomal overload as a case study JF - Frontiers in Toxicology N2 - Application of adverse outcome pathways (AOP) and integration of quantitative in vitro to in vivo extrapolation (QIVIVE) may support the paradigm shift in toxicity testing to move from apical endpoints in test animals to more mechanism-based in vitro assays. Here, we developed an AOP of proximal tubule injury linking a molecular initiating event (MIE) to a cascade of key events (KEs) leading to lysosomal overload and ultimately to cell death. This AOP was used as a case study to adopt the AOP concept for systemic toxicity testing and risk assessment based on in vitro data. In this AOP, nephrotoxicity is thought to result from receptor-mediated endocytosis (MIE) of the chemical stressor, disturbance of lysosomal function (KE1), and lysosomal disruption (KE2) associated with release of reactive oxygen species and cytotoxic lysosomal enzymes that induce cell death (KE3). Based on this mechanistic framework, in vitro readouts reflecting each KE were identified. Utilizing polymyxin antibiotics as chemical stressors for this AOP, the dose-response for each in vitro endpoint was recorded in proximal tubule cells from rat (NRK-52E) and human (RPTEC/TERT1) in order to (1) experimentally support the sequence of key events (KEs), to (2) establish quantitative relationships between KEs as a basis for prediction of downstream KEs based on in vitro data reflecting early KEs and to (3) derive suitable in vitro points of departure for human risk assessment. Time-resolved analysis was used to support the temporal sequence of events within this AOP. Quantitative response-response relationships between KEs established from in vitro data on polymyxin B were successfully used to predict in vitro toxicity of other polymyxin derivatives. Finally, a physiologically based kinetic (PBK) model was utilized to transform in vitro effect concentrations to a human equivalent dose for polymyxin B. The predicted in vivo effective doses were in the range of therapeutic doses known to be associated with a risk for nephrotoxicity. Taken together, these data provide proof-of-concept for the feasibility of in vitro based risk assessment through integration of mechanistic endpoints and reverse toxicokinetic modelling. KW - adverse outcome pathway (AOP) KW - nephrotoxicity KW - QIVIVE KW - risk assessment KW - key event relationship KW - In vitro toxicity testing Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-284796 SN - 2673-3080 VL - 4 ER -