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 - JOUR A1 - Jochmann, Svenja A1 - Elkenani, Manar A1 - Mohamed, Belal A. A1 - Buchholz, Eric A1 - Lbik, Dawid A1 - Binder, Lutz A1 - Lorenz, Kristina A1 - Shah, Ajay M. A1 - Hasenfuß, Gerd A1 - Toischer, Karl A1 - Schnelle, Moritz T1 - Assessing the role of extracellular signal‐regulated kinases 1 and 2 in volume overload‐induced cardiac remodelling JF - ESC Heart Failure N2 - Aims Volume overload (VO) and pressure overload (PO) induce differential cardiac remodelling responses including distinct signalling pathways. Extracellular signal‐regulated kinases 1 and 2 (ERK1/2), key signalling components in the mitogen‐activated protein kinase (MAPK) pathways, modulate cardiac remodelling during pressure overload (PO). This study aimed to assess their role in VO‐induced cardiac remodelling as this was unknown. Methods and results Aortocaval fistula (Shunt) surgery was performed in mice to induce cardiac VO. Two weeks of Shunt caused a significant reduction of cardiac ERK1/2 activation in wild type (WT) mice as indicated by decreased phosphorylation of the TEY (Thr‐Glu‐Tyr) motif (−28% as compared with Sham controls, P < 0.05). Phosphorylation of other MAPKs was unaffected. For further assessment, transgenic mice with cardiomyocyte‐specific ERK2 overexpression (ERK2tg) were studied. At baseline, cardiac ERK1/2 phosphorylation in ERK2tg mice remained unchanged compared with WT littermates, and no overt cardiac phenotype was observed; however, cardiac expression of the atrial natriuretic peptide was increased on messenger RNA (3.6‐fold, P < 0.05) and protein level (3.1‐fold, P < 0.05). Following Shunt, left ventricular dilation and hypertrophy were similar in ERK2tg mice and WT littermates. Left ventricular function was maintained, and changes in gene expression indicated reactivation of the foetal gene program in both genotypes. No differences in cardiac fibrosis and kinase activation was found amongst all experimental groups, whereas apoptosis was similarly increased through Shunt in ERK2tg and WT mice. Conclusions VO‐induced eccentric hypertrophy is associated with reduced cardiac ERK1/2 activation in vivo. Cardiomyocyte‐specific overexpression of ERK2, however, does not alter cardiac remodelling during VO. Future studies need to define the pathophysiological relevance of decreased ERK1/2 signalling during VO. KW - ERK1/2 KW - volume overload KW - aortocaval fistula model KW - cardiac remodelling KW - eccentric hypertrophy Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-212735 VL - 6 IS - 5 SP - 1015 EP - 1026 ER - TY - JOUR A1 - Tan, Aaron A1 - Babak, Maria V. A1 - Venkatesan, Gopalakrishnan A1 - Lim, Clarissa A1 - Klotz, Karl-Norbert A1 - Herr, Deron Raymond A1 - Cheong, Siew Lee A1 - Federico, Stephanie A1 - Spalluto, Giampiero A1 - Ong, Wei-Yi A1 - Chen, Yu Zong A1 - Loo, Jason Siau Ee A1 - Pastorin, Giorgia T1 - Design, Synthesis and Evaluation of New Indolylpyrimidylpiperazines for Gastrointestinal Cancer Therapy JF - Molecules N2 - Human A3 adenosine receptor hA3AR has been implicated in gastrointestinal cancer, where its cellular expression has been found increased, thus suggesting its potential as a molecular target for novel anticancer compounds. Observation made in our previous work indicated the importance of the carbonyl group of amide in the indolylpyrimidylpiperazine (IPP) for its human A2A adenosine receptor (hA2AAR) subtype binding selectivity over the other AR subtypes. Taking this observation into account, we structurally modified an indolylpyrimidylpiperazine (IPP) scaffold, 1 (a non-selective adenosine receptors’ ligand) into a modified IPP (mIPP) scaffold by switching the position of the carbonyl group, resulting in the formation of both ketone and tertiary amine groups in the new scaffold. Results showed that such modification diminished the A2A activity and instead conferred hA3AR agonistic activity. Among the new mIPP derivatives (3–6), compound 4 showed potential as a hA3AR partial agonist, with an Emax of 30% and EC50 of 2.89 ± 0.55 μM. In the cytotoxicity assays, compound 4 also exhibited higher cytotoxicity against both colorectal and liver cancer cells as compared to normal cells. Overall, this new series of compounds provide a promising starting point for further development of potent and selective hA3AR partial agonists for the treatment of gastrointestinal cancers. KW - gastrointestinal cancer KW - hA3AR KW - partial agonists KW - indolylpyrimidylpiperazines Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193271 SN - 1420-3049 VL - 24 IS - 20 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 - Segerer, Gabriela T1 - Characterization of cell biological and physiological functions of the phosphoglycolate phosphatase AUM T1 - Charakterisierung zellbiologischer und physiologischer Funktionen der Phosphoglykolat-Phosphatase AUM N2 - Mammalian haloacid dehalogenase (HAD)-type phosphatases are a large and ubiquitous family of at least 40 human members. Many of them have important physiological functions, such as the regulation of intermediary metabolism and the modulation of enzyme activities, yet they are also linked to diseases such as cardiovascular or metabolic disorders and cancer. Still, most of the mammalian HAD phosphatases remain functionally uncharacterized. This thesis reveals novel cell biological and physiological functions of the phosphoglycolate phosphatase PGP, also referred to as AUM. To this end, PGP was functionally characterized by performing analyses using purified recombinant proteins to investigate potential protein substrates of PGP, cell biological studies using the spermatogonial cell line GC1, primary mouse lung endothelial cells and lymphocytes, and a range of biochemical techniques to characterize Pgp-deficient mouse embryos. To characterize the cell biological functions of PGP, its role downstream of RTK- and integrin signaling in the regulation of cell migration was investigated. It was shown that PGP inactivation elevates integrin- and RTK-induced circular dorsal ruffle (CDR) formation, cell spreading and cell migration. Furthermore, PGP was identified as a negative regulator of directed lymphocyte migration upon integrin- and GPCR activation. The underlying mechanisms were analyzed further. It was demonstrated that PGP regulates CDR formation and cell migration in a PLC- and PKC-dependent manner, and that Src family kinase activities are required for the observed cellular effects. Upon integrin- and RTK activation, phosphorylation levels of tyrosine residues 1068 and 1173 of the EGF receptor were elevated and PLCγ1 was hyper-activated in PGP-deficient cells. Additionally, PGP-inactivated lymphocytes displayed elevated PKC activity, and PKC-mediated cytoskeletal remodeling was accelerated upon loss of PGP activity. Untargeted lipidomic analyses revealed that the membrane lipid phosphatidylserine (PS) was highly upregulated in PGP-depleted cells. These data are consistent with the hypothesis that the accumulation of PS in the plasma membrane leads to a pre-assembly of signaling molecules such as PLCγ1 or PKCs that couple the activation of integrins, EGF receptors and GPCRs to accelerated cytoskeletal remodeling. Thus, this thesis shows that PGP can affect cell spreading and cell migration by acting as a PG-directed phosphatase. To understand the physiological functions of PGP, conditionally PGP-inactivated mice were analyzed. Whole-body PGP inactivation led to an intrauterine growth defect with developmental delay after E8.5, resulting in a gradual deterioration and death of PgpDN/DN embryos between E9.5 and E11.5. However, embryonic lethality upon whole-body PGP inactivation was not caused by a primary defect of the (cardio-) vascular system. Rather, PGP inactivated embryos died during the intrauterine transition from hypoxic to normoxic conditions. Therefore, the potential impact of oxygen on PGP-dependent cell proliferation was investigated. Analyses of mouse embryonic fibroblasts (MEFs) generated from E8.5 embryos and GC1 cells cultured under normoxic and hypoxic conditions revealed that normoxia (~20% O2) causes a proliferation defect in PGP-inactivated cells, which can be rescued under hypoxic (~1% O2) conditions. Mechanistically, it was found that the activity of triosephosphate isomerase (TPI), an enzyme previously described to be inhibited by phosphoglycolate (PG) in vitro, was attenuated in PGP-inactivated cells and embryos. TPI constitutes a critical branch point between carbohydrate- and lipid metabolism because it catalyzes the isomerization of the glycolytic intermediates dihydroxyacetone phosphate (DHAP, a precursor of the glycerol backbone required for triglyceride biosynthesis) and glyceraldehyde 3’-phosphate (GADP). Attenuation of TPI activity, likely explains the observed elevation of glycerol 3-phosphate levels and the increased TG biosynthesis (lipogenesis). Analyses of ATP levels and oxygen consumption rates (OCR) showed that mitochondrial respiration rates and ATP production were elevated in PGP-deficient cells in a lipolysis-dependent manner. However under hypoxic conditions (which corrected the impaired proliferation of PGP-inactivated cells), OCR and ATP production was indistinguishable between PGP-deficient and PGP-proficient cells. We therefore propose that the inhibition of TPI activity by PG accumulation due to loss of PGP activity shifts cellular bioenergetics from a pro-proliferative, glycolytic metabolism to a lipogenetic/lipolytic metabolism. Taken together, PGP acts as a metabolic phosphatase involved in the regulation of cell migration, cell proliferation and cellular bioenergetics. This thesis constitutes the basis for further studies of the interfaces between these processes, and also suggests functions of PGP for glucose and lipid metabolism in the adult organism. N2 - Haloazid Dehalogenase (HAD)-Typ Phosphatasen in Säugetieren gehören zu einer großen ubiquitären Proteinfamilie, zu der auch mindestens 40 Phosphatasen, die im menschlichen Organismus vertreten sind, zählen. Eine Vielzahl dieser Phosphatasen hat wichtige physiologische Funktionen beispielsweise als regulatorische Enzyme im Metabolismus. Gleichzeitig werden sie in Verbindung mit Erkrankungen des kardiovaskulären Systems, Stoffwechselstörungen und Krebs gebracht. Dennoch sind die Funktionen vieler Mitglieder dieser Phosphatasen Familie bis heute weitestgehend unbekannt. In der vorliegenden Arbeit wurden die zellbiologischen und physiologischen Funktionen der Phosphoglykolat-Phosphatase PGP, auch AUM genannt, charakterisiert. Zu diesem Zweck wurde mit gereinigtem Enzym nach potenziellen Protein-Substraten von PGP gesucht. Weiterhin wurden zellbiologische Studien mit der spermatogonialen GC1 Zelllinie sowie mit primären Endothelzellen und Lymphozyten durchgeführt. Mit biochemischen Methoden wurden zudem PGP-defiziente Mausembryonen charakterisiert. Es wurde zunächst die Rolle von PGP für RTK- und integrin- induzierte Zellmigration untersucht. Dabei zeigte sich, dass PGP Inaktivierung die Zelladhäsion und Zellmigration steigerte. Gleichzeitig wurde eine vermehrte Bildung von RTK- und integrinvermittelten ringförmigen Plasmamembranausstülpungen, sogenannten Circular Dorsal Ruffles (CDR) auf der dorsalen Zelloberfläche beobachtet. PGP wurde zudem als negativer Regulator integrinund GPCR-induzierter gerichteter Lymphozytenmigration identifiziert. Der zugrundeliegende molekulare Mechanismus wurde näher untersucht. Es konnte gezeigt werden, dass PGP die Bildung von CDRs und die gerichtetete Zellmigration in Abhängigkeit der Phospholipase C- (PLC-), Proteinkinase C- (PKC-) sowie Src Kinase-Aktivität steuert. Nach Integrin- und RTKAktivierung waren die Tyrosinreste 1068 und 1173 des EGF-Rezeptors in PGP-depletierten Zellen vermehrt phosphoryliert und PLCγ1 in diesen Zellen hyperaktiviert. Interessanterweise wurde zudem eine beschleunigte PKC-vermittelte Reorganisation des Zytoskeletts beobachtet. In stimulierten Lymphozyten führte PGP-Inaktivierung zu einer erhöhten PKCAktivität. Durch massenspektrometrische Analysen konnten erhöhte Spiegel des Membranlipids Phosphatidylserin (PS) in PGP-defizienten Zellen nachgewiesen werden. Diese Ergebnisse sind konsistent mit der Hypothese, dass die Anreicherung von PS in der Plasmamembran PGP-defizienter Zellen zu einer Vor-Rekrutierung von Signalproteinen führt, die die Aktivierung von Integrinen, EGF-Rezeptoren und GPCRs mit einer beschleunigten Zytoskelett-Reorganisation verbindet. Hierdurch konnte gezeigt werden, dass PGP durch die Dephosphorylierung von Phosphoglykolat die Zelladhäsion und Zellmigration reguliert. Um die physiologischen Funktionen von PGP zu verstehen, wurden konditional PGPinaktivierte Mäuse untersucht. Die Inaktivierung von PGP im gesamten Organismus führte zu einem Wachstumsdefekt ab Tag E8.5 und dem Tod der Embryonen im Uterus zwischen Tag E9.5 und E11.5. Die beobachtete embryonale Letalität war nicht durch einen Defekt des (kardio-)vaskulären Systems zu erklären. PGP-inaktivierte Embryonen starben zu einem Zeitpunkt, an dem der intrauterine Übergang von einem hypoxischen zu einem normoxischen Millieu stattfindet. Der Einfluss von Sauerstoff wurde deshalb weiter untersucht. Zellwachstumsanalysen unter normoxischen und hypoxischen Bedingungen mit GC1 Zellen und embryonalen Maus-Fibroblasten, die aus E8.5 Embryonen gewonnen wurden zeigten, dass normoxische Bedingungen (~20% O2) einen Wachstumsdefekt PGP-inaktivierter Zellen verursacht, wohingegen dies unter hypoxischen Bedingungen (~1% O2) nicht der Fall war. Mechanistisch konnte gezeigt werden, dass die Aktivität der Triosephosphatisomerase (TPI), ein durch PG in vitro gehemmtes Enzym, in PGP inaktivierten Zellen und Embryonen vermindert war. TPI stellt einen entscheidenden Verzweigungspunkt des Glukose- und Lipidstoffwechsels dar. TPI katalysiert die Isomerisierung der aus der Glykolyse stammenden Intermediate Dihydroxyacetonphosphat (DHAP, eine Vorstufe des für die Triglycerid-Biosynthese benötigten Glycerol-Grundgerüsts) und Glyceraldehyd-3’-phosphat (GADP). Eine Verringerung der TPI-Aktivität in PGPinaktivierten Zellen resultierte in erhöhten Glycerol-3-phosphat Spiegeln und einer gesteigerten Triglycerid-Biosynthese. Die Analyse des zellulären ATP Gehalts und des Sauerstoffverbrauchs bei der mitochondrialen Atmung zeigte, dass sowohl die ATP Produktion als auch die mitochondriale Atmung in Abhängikeit der Lipolyse in PGP-defizienten Zellen erhöht waren. Unter hypoxischen Bedingungen, die zu einer Normalisierung der Zellproliferation führten, wiesen PGP-profiziente und -defiziente Zellen keinen Unterschied bezüglich ATP Produktion und mitochondrialer Atmung auf. Wir vermuten deswegen, dass die Inhibierung der TPI-Aktivität durch PG-Anreicherung aufgrund ausbleibender Hydrolyse durch PGP zu einer Verschiebung des zellulären Energiehaushaltes von Seiten eines pro-proliferativ glykolytischen auf die Seite eines lipogenetisch/lipolytischen Metabolismus führt. Zusammenfassend konnte gezeigt werden, dass PGP als eine metabolische Phosphatase Zellmigration, Zellproliferation wie auch den zellulären Energiehaushalt reguliert. Die vorliegende Arbeit stellt somit die Grundlage für weitere Untersuchungen an der Schnittschnelle dieser zellulären Prozesse dar und lässt auf eine wichtige Rolle von PGP im Glukose- und Lipidstoffwechsel im adulten Organismus schließen. KW - Phosphoglykolatphosphatase KW - Phosphoglykolat-Phosphatase KW - Maus KW - Cytologie KW - Physiologie KW - Phosphatasen Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-123847 ER -