@phdthesis{Grue1999, author = {Grue, Pernille}, title = {The physiological role of the two isoforms of DNA topoisomerase II in human cells}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-1369}, school = {Universit{\"a}t W{\"u}rzburg}, year = {1999}, abstract = {Unique functions of DNA topoisomerase IIalpha and IIbeta have been suggested. A human cell line which carries a homozygeous mutation of the nuclear localization sequence of the topoisomerase IIalpha gene expresses the isoform outside the nucleus at the onset of mitosis. At mitosis topoisomerase IIbeta diffused away from the chromatin despite the nuclear lack of the IIalpha-form. Chromosome condensation and disjunction was performed with the aid of cytosolic topoisomerase IIalpha which bound to the mitotic chromatin with low affinity. Consequently an increased rate of nondisjunction is observed in these cells. It is concluded that high affinity chromatin binding of topoisomerase IIalpha is essential for chromosome condensation/disjunction and that topoisomerase IIbeta does not adopt these functions. A centrosomal protein was recognized by topoisomerase IIalpha. This topoisomerase IIalpha-like protein resembles a modified form of topoisomerase IIalpha with an apparent size of 205 kDa compared to 170 kDa. The expression of the protein is constant in all stages of the cell cycle and it appears in proliferating as well as in resting cells. If there is not sufficient topoisomerase IIalpha present at mitosis the centrosomal proteins might adopt the function and a mitotic catastrophe in the cells could therefore be prevented.}, subject = {DNS-Gyrase}, language = {en} } @phdthesis{Christensen2003, author = {Christensen, Morten Overby}, title = {Dynamics of human DNA Topoisomerases I and II}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-4927}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2003}, abstract = {The first goal of this study was to develop cell lines with a stable expression of bio-fluorescent topo II and topo I. This was successfully achieved using a bicistronic vector system. Control experiments showed that proteins of expected size were expressed, and that GFP-tagged topos I, IIa, and IIb were active in the cells and fully integrated in the endogenous pools of the enzymes. These cell-lines provided a novel tool for investigating the cell biology of human DNA topoisomerases. Our most important finding was, that both types of mammalian topoisomerases are entirely mobile proteins that are in continuous and rapid flux between all compartments of the nucleus and between the cytososl and the chromosomes of mitotic cells. This was particularly surprising with regard to topo II, which is considered to be a structural component of the nuclear matrix and the chromosome scaffold. We must conclude that if this was the case, then these architectural structures appear to be much more dynamic than believed until now. In this context it should also be mentioned, that the alignment of topo II with the central axes of the chromosome arms, which has until now been considered a hall-mark of the enzyme's association with the chromosomal scaffold, is not seen in vivo and can be demonstrated to be to some extent an artefact of immunohistochemistry. Furthermore, we show that the two isoforms of topo II (a and b) have a different localisation during mitotic cell division, supporting the general concept that topo II functions at mitosis are exclusively assigned to the a-form, whereas at interphase the two isoenzymes work in concert. Despite unrestricted mobility within the entire nuclear space, topoisomerases I and II impose as mostly nucleolar proteins. We show that this is due to the fact that in the nucleoli they are moving slower than in the nucleoplasm. The decreased nucleolar mobility cannot be due to DNA-interactions, because compounds that fix topoisomerases to the DNA deplete them from the nucleoli. Interestingly, the subnucleolar distribution of topoisomerases I and II was complementary. The type II enzyme filled the entire nucleolar space, but excluded the fibrial centers, whereas topo I accumulated at the fibrial centers, an allocation directed by the enzyme's N-terminus. During mitosis, it also mediates association with the nucleolar organising regions of the acrocentric chromosomes. Thus, topo I stays associated with the rDNA during the entire cell-cycle and consistently colocalizes there with RNA-polymerase I. Finally, we show that certain cancer drugs believed to act by stabilising covalent catalytic DNA-intermediates of topoisomerases, do indeed immobilize the enzymes in living cells. Interestingly, these drugs do not target topoisomerases in the nucleoli but only in the nucleoplasm.}, subject = {Mensch}, language = {en} } @phdthesis{Visan2003, author = {Visan, Ioana Andreea}, title = {The CD23 receptor-regulation of expression and signal transduction}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-5556}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2003}, abstract = {Bisher sind zwei Isoformen des humanen CD23 (CD23a und CD23b) beschrieben. Beide unterscheiden sich lediglich in 6-7 Resten im N-terminalen, zytoplasmatischen Anteil. CD23a wird ausschließlich auf B-Zellen exprimiert, w{\"a}hrend CD23b sowohl auf B-Zellen als auch auf Monozyten, eosinophilen Granulozyten, Makrophagen und zahlreichen anderen Zelltypen durch Stimulation mit IL-4 induziert werden kann. Die beiden Isoformen vermitteln wahrscheinlich unterschiedliche Funktionen. CD23a gilt als Isoform, welche vornehmlich mit der Endozytose von IgE-Immunkomplexen und der Vermittlung von Antigen-Pr{\"a}sentation auf B-Zellen assoziiert ist. CD23b besitzt ein Phagozytose-Motiv und scheint bei der Phagozytose IgE besetzter Partikel, der Freisetzung von Zytokinen und der Bildung von Peroxiden eine Rolle zu spielen. Fr{\"u}here Untersuchungen legen die Vermutung nahe, dass die beiden Isoformen zwei getrennte Signal{\"u}bertragungswege miteinander verbinden. Die Gegen{\"u}berstellung von Ereignissen, welche in Zellen, die nur eine einer oder beide Isoformen von CD23 besitzen, stattfinden, legt die Vermutung nahe, dass CD23b cAMP und iNOS hochreguliert, wohingegen CD23a einen Anstieg des intrazellul{\"a}ren Kalziums vermittelt. Im ersten Teil unserer Untersuchungen haben wir die Regulation der B-Zell-spezifischen Expression von CD23a analysiert. Pax-5 ist ein auf B-Zellen beschr{\"a}nkter Transkriptionsfaktor, welcher f{\"u}r die fr{\"u}he und sp{\"a}te B-Zellentwicklung von entscheidender Bedeutung ist. M{\"o}gliche Pax-5 Bindungsstellen wurden in den proximalen Abschnitten des CD23a Promotors vermutet. Die Analyse des CD23a Promotors ergab drei mutmaßliche Pax-5 Bindungsstellen mit mehr als 50\% Homologie zur Konsensus-Sequenz. Eine dieser Bindungsstellen, namens CD23-1, kann mit einer hochaffinen Pax-5 Bindungsstelle konkurrieren oder direkt das Pax-5 Protein in Elektromobilit{\"a}ts Experimenten (EMSA) binden. Das Einf{\"u}gen von Mutationen an dieser Stelle verhindert die Bindung. Ein weiterer Versuch, bei dem die gesamte L{\"a}nge des CD23a Promotors durch {\"u}berlappende Peptide in einem kompetitiven Verfahren gegen{\"u}ber hoch affinen Bindungsstellen getestet wurde, zeigt ebenso CD23-1 als die einzige Stelle, welche direkt Pax-5 binden kann. In weiteren Experimenten f{\"u}hrte die Expression von Pax-5 in 293 Zellen zu einer 7fachen Aktivierung eines CD23a Kernpromotor Konstrukts. Die Kotransfektion zusammen mit STAT6 zeigte, dass Pax-5 mit diesem Transkriptionsfaktor kooperiert, indem es die Transkriptionsrate eines vergr{\"o}ßerten CD23a Promotorkonstrukts erh{\"o}ht. Von besonderer Bedeutung ist die Tatsache, dass die ektope Expression von Pax-5 in der monozyt{\"a}ren Zelllinie U-937, die normalerweise nur die CD23b Isoform exprimiert, dann zu einer Expression von CD23a nach Stimulation mit IL-4 und PMA f{\"u}hrte. Unsere Ergebnisse legen nahe, dass Pax-5 in der auf B-Zellen beschr{\"a}nkten Expression der CD23 Isoform eine Schl{\"u}sselrolle zukommt. Im zweiten Teil des Projekts haben wir ein "Zwei-Hefen-Hybrid-System" (Cyto-Trap von Stratagene) verwendet, um nach zytoplasmatischen Interaktionspartnern f{\"u}r den CD23 Rezeptor zu suchen. Das System wurde modifiziert um eine hohe Effizienz an Transformation zu erzielen. Unterschiedliche „K{\"o}der"-Vektorkonstrukte wurden hergestellt. Das Screening wurde mittels einer humanen Milzbibliothek mit dem Zielvektor des Systems durchgef{\"u}hrt. Die anfangs benutzten Konstrukte -pSosCD23a und pSosCD23b - exprimierten sehr kurze (22 Aminos{\"a}uren) zytoplasmatischen Reste der Isoformen am C-terminalen Ende des Fusionsproteins (humanes SOS). Verbesserte Konstrukte (pSos CD23a+Linker und pSosCD23b+Linker) exprimierten den zytoplasmatischen Anteil von CD23a/b am N-terminalen Ende des humanen SOS und hatten folglich den N-terminalen Anteil als Andockstelle frei, entsprechend den Bedingungen in vivo. Eine flexible Verbindungsregion trennte die Fusionsproteine, um auf diese Weise die kurze Aminos{\"a}urekette deutlich „sichtbar" werden zu lassen. Ann{\"a}hernd drei Millionen Klone wurden mittels der verschiedenen Konstrukte untersucht. Dabei konnte keine tats{\"a}chlich positive Interaktion gefunden werden. Stattdessen fand sich eine vergleichsweise hohe Zahl falsch-positiver Klone. Diese wiederum wurden in einem zweiten "Zwei-Hefen-Hybrid-System" getestet. In Zukunft wird ein neues Konstrukt als K{\"o}der verwendet werden. Hierbei wurde ein Tyrosin-Rest im zytoplasmatischen Anteil von CD23a durch Glutamat ersetzt. Das System wurde bereits dazu verwendet, die Interaktion zwischen CD23 und p59fyn - einem Mitglied der Src-Familie von Proteinkinasen, welches mit CD23a assoziiert sein soll - zu testen. Jedoch konnte im CytoTrap "Zwei-Hefen-Hybrid-System" keine Wechselwirkung nachgewiesen werden. Zusammenfassend zeigt das zentrale Ergebnis der Arbeit, dass Pax-5 der Schl{\"u}sselregulator ist, der die B-Zell-spezifische Expression von CD23a erm{\"o}glicht. Zus{\"a}tzlich wurde ein "Zwei-Hefen-Hybrid-System" etabliert, mit dem zytoplasmatische Interaktionspartner f{\"u}r die CD23 Isoformen gefunden werden k{\"o}nnen.}, subject = {Antigen CD23}, language = {en} } @phdthesis{Hallhuber2007, author = {Hallhuber, Matthias}, title = {Inhibition of Nuclear Import of Calcineurin Prevents the Development of Myocardial Hypertrophy}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-23536}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2007}, abstract = {The Calcineurin/NFAT signaling cascade is a crucial transducer of cellular function. It has recently been emerged that in addition to the transcription factor NFAT, the phosphatase Calcineurin is also translocated to the nucleus. Our traditional understanding of Calcineurin activation via sustained high Ca2+-levels was also advanced by recent findings from this working group (AG Ritter), which showed that Calcineurin is activated by proteolysis of the C-terminal autoinhibitory domain. This leads to the constitutive activation and nuclear translocation of Calcineurin. Therefore, Calcineurin is not only responsible for dephosphorylating of NFAT in the cytosol thus enabling its nuclear import, its presence in the nucleus is also significant in ensuring the full transcriptional activity of NFAT. Formation of complexes between transcription factors and DNA regulates the transcriptional process. Therefore, the time that transcription factors remain nuclear is a major determinant of transcriptional activity. The movement of proteins over ~40 kDa into and out of the nucleus is governed by the nuclear pore complex (NPC). Transcription factors and enzymes that regulate the activity of these proteins are shuttled across the nuclear envelope by proteins that recognize nuclear localization signals (NLS) and nuclear export signals (NES) within the amino acid sequence of these transcription factors. In this study, the precise mechanisms of Calcineurin nuclear import and export were identified. Additionally to the nuclear localization sequence (NLS) and the nuclear export sequence (NES) within the sequence of Calcineurin, the respective nuclear cargo proteins, responsible for nuclear import, Importin\&\#946;1, and for nuclear export, CRM1, were identified. Inhibition of the Calcineurin/importin interaction by a competitive peptide, called Import Blocking Peptide (IBP), which mimicked the Calcineurin NLS, prevented nuclear entry of Calcineurin. A non-inhibitory control peptide showed no effect. Using this approach, it was able to prevent the development of myocardial hypertrophy. In Angiotensin II stimulated cardiomyocytes, both the transcriptional and the translational level was suppressed. Additionally, cell size and expression of Brain natriuretic peptide (as molecular marker for hypertrophy) were significantly reduced compared untreated controls. IBP worked dose-dependent, but did not affect the Calcineurin phosphatase activity. In conclusion, Calcineurin is not only capable of dephosphorylating NFAT, thus enabling its nuclear import, its presence in the nucleus is also important for full NFAT transcriptional activity. Using IBP to prevent the nuclear import of Calcineurin is a completely new approach to prevent the development of myocardial hypertrophy.}, language = {en} } @phdthesis{Padmapriya2008, author = {Padmapriya, Ponnuswamy}, title = {Insight into oxidative stress mediated by nitric oxide synthase (NOS) isoforms in atherosclerosis}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-30659}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2008}, abstract = {The principle product of each NOS is nitric oxide. However, under conditions of substrate and cofactor deficiency the enzymes directly catalyze superoxide formation. Considering this alternative chemistry of each NOS, the effects of each single enzyme on key events of atherosclerosis are difficult to predict. Here, we evaluate nitric oxide and superoxide production by all three NOS isoforms in atherosclerosis. ESR measurements of circulating and vascular wall nitric oxide production showed significantly reduced nitric oxide levels in apoE/eNOS double knockout (dko) and apoE/iNOS dko animals but not in apoE/nNOS dko animals suggesting that eNOS and iNOS majorly contribute to vascular nitric oxide production in atherosclerosis. Pharmacological inhibition and genetic deletion of eNOS and iNOS reduced vascular superoxide production suggesting that eNOS and iNOS are uncoupled in atherosclerotic vessels. Though genetic deletion of nNOS did not alter superoxide production, acute inhibition of nNOS showed that nNOS contributes significantly to superoxide production. In conclusion, uncoupling of eNOS occurs in apoE ko atherosclerosis but eNOS mediated superoxide production does not outweigh the protective effects of eNOS mediated nitric oxide production. We show that although nNOS is not a major contributor of the vascular nitric oxide formation, it prevents atherosclerosis development. Acute inhibition of nNOS showed a significant reduction of superoxide formation suggesting that nNOS is uncoupled. The exact mechanism of action of nNOS in atheroprotection is yet to be elucidated. Genetic deletion of iNOS reduced NADPH oxidase activity. Thus, iNOS has both direct and indirect proatherosclerotic effects, as it directly generates both nitric oxide and superoxide simultaneously resulting in peroxynitrite formation and indirectly modulates NADPH oxidase activity. We hypothesize that eNOS is coupled in the disease free regions of the vessel and contributes to nitric oxide generation whereas in the diseased region of the vessel it is uncoupled to produce superoxide (Figure 16). nNOS expressed in the smooth muscle cells of the plaque contributes to the local superoxide generation. iNOS expressed in smooth muscle cells and leukocytes of the plaque generates superoxide and nitric oxide simultaneously to produce the strong oxidant peroxynitrite.}, subject = {atherosclerosis}, language = {en} } @phdthesis{Govindaraj2009, author = {Govindaraj, Vijayakumar}, title = {Improved Cardiac Glucose Uptake: A Potential Mechanism for Estrogens to Prevent the Development of Cardiac Hypertrophy}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-35911}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2009}, abstract = {The incidence of cardiovascular diseases including cardiac hypertrophy and failure in pre-menopausal women is lower compared to age-matched men but the risk of heart disease increases substantially after the onset of menopause. It has been postulated that female sex hormones play an important role in cardiovascular health in pre-menopausal women. In animal studies including spontaneously hypertensive (SHR) rats, the development of cardiac hypertrophy is attenuated by 17\&\#946;-estradiol treatment. Cardiac energy metabolism is crucial for normal function of the heart. In cardiac hypertrophy and heart failure, the myocardium undergoes a metabolic shift from fatty acid as primary cardiac energy source to glucose, which re-introduces the fetal type of metabolism that representing the glucose as a major source of energy. Many studies have reported that the disruption of the balance between glucose and fatty acid metabolism plays an important role in cardiac pathologies including hypertrophy, heart failure, diabetes, dilative cardiomyopathy and myocardial infarction. Glucose enters cardiomyocytes via GLUT1 and GLUT4 glucose transporters and GLUT4 is the major glucose transporter which is insulin-dependent. Cardiac-selective GLUT4 deficiency leads to cardiac hypertrophy. This shows that the decrease in cardiac glucose uptake may play a direct role in the pathogenesis of cardiac hypertrophy. Estrogens modulate glucose homeostasis in the liver and the skeletal muscle. But it is not known whether estrogens affect also cardiac glucose uptake which could provide another mechanism to explain the prevention of cardiac hypertrophy by female sex hormones. In the present study, SHR Rats were ovariectomized (OVX), not ovariectomized (sham) or ovariectomized and treated with subcutaneous 17\&\#946;-estradiol. After 6 weeks of treatment, body weight, the serum levels of estrogen, insulin, intra-peritoneal glucose tolerance test (IP-GTT), myocardial glucose uptake by FDG-PET (2-(18F)-fluoro-deoxyglucose (18FDG) and Positron Emission Tomography), cardiac glucose transporter expression and localization and cardiac hexokinase activity were analyzed. As results of this study, PET analysis of female SHR revealed decreased cardiac glucose uptake in OVX animals compared to intact that was normalized by estrogen supplementation. Interestingly, there was no change in global glucose tolerance among the treatment groups. Serum insulin levels and cardiac hexokinase activity were elevated by E2 substitution. The protein content of cardiac glucose transporters GLUT-4 and GLUT-1, and their translocation as determined by fractionation studies and immuno-staining did not show any significant change by ovariectomy and estrogen replacement. Also levels of insulin receptor substrate-1 (IRS-1) and its tyrosine phosphorylation, which is required for activation and translocation of GLUT4, was un-affected in all groups of SHR. Cardiac gene expression analysis in SHR heart showed that ei4Ebp1 and Frap1 genes which are involved in the mTOR signaling pathway, were differentially expressed upon estrogen treatment. These genes are known to be activated in presence of glucose in the heart. As a conclusion of this study, reduced myocardial FDG uptake in ovariectomized spontaneously hypertensive rat is normalized by 17\&\#946;-estradiol treatment. Increased myocardial hexokinase appears as a potential mechanism to explain increased myocardial glucose uptake by 17\&\#946;-estradiol. Increased cardiac glucose uptake in response to 17\&\#946;-estradiol in ovariectomized SHR may provide a novel mechanism to explain the reduction of cardiac hypertrophy in E2 treated SHR. Therefore, 17\&\#946;-estradiol improves cardiac glucose utilization in ovariectomized SHR which may give rise to possible mechanism for its protective effects against cardiac hypertrophy.}, subject = {estrogen}, language = {en} } @phdthesis{Fiedler2010, author = {Fiedler, Jan}, title = {Endothelial microRNA-24 contributes to capillary density in the infarcted heart}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-49809}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2010}, abstract = {Cardiovascular disease is the most common mortality risk in the industrialized world. Myocardial infarction (MI) results in the irreversible loss of cardiac muscle, triggering pathophysiological remodelling of the ventricle and development of heart failure. Insufficient myocardial capillary density within the surviving myocardium after MI has been identified as a critical event in this process, although the underlying molecular signalling pathways of cardiac angiogenesis are mechanistically not well understood. The discovery of microRNAs (miRNAs, miRs), small non-coding RNAs with 19-25 nucleotides in length, has introduced a new level of the regulation of cardiac signalling pathways. MiRNAs regulate gene expression post-transcriptionally by binding to their complementary target messenger RNAs (mRNAs) and represent promising therapeutic targets for gene therapy. Here, it is shown that cardiac miR-24 is primarily expressed in cardiac endothelial cells and upregulated following MI in mice and hypoxic conditions in vitro. Enhanced miR-24 expression induces endothelial cell apoptosis and impairs endothelial capillary network formation. These effects on endothelial cell biology are at least in part mediated through targeting of transcription factor GATA2, histone deacetylase H2A.X, p21-activated kinase PAK4 and Ras p21 protein activator RASA1. Mechanistically, target repression abolishes respective and secondary downstream signalling cascades. Here it is shown that endothelial GATA2 is an important mediator of cell cycle, apoptosis and angiogenesis at least in part by regulation of cytoprotective heme oxygenase 1 (HMOX1). Moreover, additional control of endothelial apoptosis is achieved by the direct miR-24 target PAK4. Its kinase function is essential for anti-apoptotic Bad phosphorylation in endothelial cells. In a mouse model of MI, blocking of endothelial miR-24 by systemic administration of a specific antagonist (antagomir) enhances capillary density in the infarcted heart and preserves cardiac function. The current findings indicate miR-24 to act as a critical regulator of endothelial cell apoptosis and angiogenesis. Modulation of miR-24 may be potentially a suitable strategy for therapeutic intervention in the setting of ischemic heart diseases.}, subject = {Herzinfarkt}, language = {en} } @article{BauerNadler2010, author = {Bauer, Wolfgang R. and Nadler, Walter}, title = {Thermodynamics of Competitive Molecular Channel Transport: Application to Artificial Nuclear Pores}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-68484}, year = {2010}, abstract = {In an analytical model channel transport is analyzed as a function of key parameters, determining efficiency and selectivity of particle transport in a competitive molecular environment. These key parameters are the concentration of particles, solvent-channel exchange dynamics, as well as particle-in-channel- and interparticle interaction. These parameters are explicitly related to translocation dynamics and channel occupation probability. Slowing down the exchange dynamics at the channel ends, or elevating the particle concentration reduces the in-channel binding strength necessary to maintain maximum transport. Optimized in-channel interaction may even shift from binding to repulsion. A simple equation gives the interrelation of access dynamics and concentration at this transition point. The model is readily transferred to competitive transport of different species, each of them having their individual in-channel affinity. Combinations of channel affinities are determined which differentially favor selectivity of certain species on the cost of others. Selectivity for a species increases if its in-channel binding enhances the species' translocation probablity when compared to that of the other species. Selectivity increases particularly for a wide binding site, long channels, and fast access dynamics. Recent experiments on competitive transport of in-channel binding and inert molecules through artificial nuclear pores serve as a paradigm for our model. It explains qualitatively and quantitatively how binding molecules are favored for transport at the cost of the transport of inert molecules.}, subject = {Thermodynamik}, language = {en} } @phdthesis{Burkard2010, author = {Burkard, Natalie}, title = {Signal{\"u}bertragungswege und Pr{\"a}ventionsm{\"o}glichkeiten der kardialen Hypertrophie : conditional overexpression of neuronal nitric oxide synthase is cardioprotective in ischemia-reperfusion}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-51832}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2010}, abstract = {Zusammenfassung: Wie fr{\"u}her schon gezeigt, wird der L-Typ Ca2+-Kanal durch eine induzierbare, myokardspezifische {\"U}berexpression der neuronalen Stickstoffmonoxidsynthase (nNOS) inhibiert. Gleichzeitig bewirkt diese {\"U}berexpression eine verminderte kardiale Kontraktilit{\"a}t1 (Burkard N. et al. (2007). Circ Res 100, 32-44). nNOS interagiert mit vielen verschiedenen Kompartimenten und Kan{\"a}len innerhalb der Zelle. In dieser Arbeit wurde gezeigt, dass eine nNOS {\"U}berexpression nach Isch{\"a}mie-Reperfusion kardioprotektiv wirkt. Dieses wird durch eine Inhibition der Mitochondrienfunktion und durch eine Verminderung der reaktiven Sauerstoffspezies (ROS) erm{\"o}glicht. In einer fr{\"u}heren Arbeit wurde der Effekt der induzierbaren und myokardspezifischen {\"U}berexpression von nNOS unter physiologischen Bedingungen am transgenen Tiermodell untersucht. Diese Arbeit besch{\"a}ftigt sich nun mit der {\"U}berexpression von nNOS unter pathophysiologischen (Isch{\"a}mie-Reperfusion) Bedingungen. Ein Isch{\"a}mie-Reperfusions-Schaden bewirkt bei Wildtyp-M{\"a}usen, sowie bei transgener nNOS {\"U}berexpression eine Anreicherung von nNOS in den Mitochondrien. Elektronenmikroskopische Aufnahmen von Mausmyokard haben gezeigt, dass bei {\"U}berexpression nNOS zus{\"a}tzlich in den Mitochondrien lokalisiert ist. Diese Translokation von nNOS in die Mitochondrien ist abh{\"a}ngig von HSP90. Isch{\"a}mie- Reperfusionsexperimente an isolierten M{\"a}useherzen zeigten einen kardioprotektiven Effekt der nNOS {\"U}berexpression (30min post ischemia, LVDP 27.0±2.5mmHg vs. 45.2±1.9mmHg, n=12, p<0.05). Dieser positive Effekt konnte bei der Bestimmung der Infarktgr{\"o}ße best{\"a}tigt werden. nNOS {\"u}berexprimierende M{\"a}use hatten eine kleinere Infarktgr{\"o}ße nach Isch{\"a}mie-Reperfusion (36.6±8.4 relative \% vs. 61.1±2.9 relative \%, n=8, p<0.05). Die {\"U}berexpression von nNOS bewirkte ebenfalls einen signifikanten Anstieg des mitochondrialen Nitrit-Levels, begleitet von einer Verminderung der Cytochrom C Oxidase Aktivit{\"a}t (72.0±8.9units/ml in nNOS overexpressing mice vs. 113.2±17.1units/ml in non-induced mice, n=12, p<0.01), was zu einer Hemmung der Mitochondrienfunktion f{\"u}hrt. Dementsprechend war der Sauerstoffverbrauch (gemessen an isolierten Herzmuskelstreifen) schon unter basalen Bedingungen beinNOS {\"U}berexpression vermindert (0.016±0.0015 vs. 0.024±0.006ml[O2] x mm-3 x min-1, n=13, p<0.05). Außerdem war die ROS Konzentration in Herzen von nNOS {\"u}berexprimierenden M{\"a}usen signifikant vermindert (6.14±0.685 vs. 14.53±1.7μM, n=8, p<0.01). Die Zugabe von verschiedenen Inhibitoren, Western Blot- und Aktivit{\"a}tsuntersuchungen zeigten schließlich, dass diese niedrigere ROS Konzentration durch eine verminderte Xanthin Oxidoreduktase Aktivit{\"a}t hervorgerufen wurde. Zusammenfassend hat diese Arbeit gezeigt, dass eine induzierbare und myokardspezifische {\"U}berexpression von nNOS unter pathophysiologischen Bedingungen (Isch{\"a}mie-Reperfusion) kardioprotektiv wirkt. Zus{\"a}tzlich zu der Verminderung des myokardialen Ca2+-{\"U}berschusses nach Reperfusion k{\"o}nnte dieser protektive Effekt durch eine Hemmung der Mitochondrienfunktion bedingt sein, schließlich wird der Sauerstoffverbrauch schon unter basalen Bedingungen reduziert}, subject = {Herzhypertrophie}, language = {en} } @article{JohanssenHahnerSaegeretal.2010, author = {Johanssen, Sarah and Hahner, Stefanie and Saeger, Wolfgang and Quinkler, Marcus and Beuschlein, Felix and Dralle, Henning and Haaf, Michaela and Kroiss, Matthias and Jurowich, Christian and Langer, Peter and Oelkers, Wolfgang and Spahn, Martin and Willenberg, Holger S. and Maeder, Uwe and Allolio, Bruno and Fassnacht, Martin}, title = {Deficits in the Management of Patients With Adrenocortical Carcinoma in Germany}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-85897}, year = {2010}, abstract = {Background: Adrenocortical carcinoma (ACC) is a rare tumor with a poor prognosis. Often, the physicians who first treat patients with ACC have no prior experience with the disease. The aim of our study was to evaluate the quality of medical care for patients with ACC in Germany. Methods: Data from the German ACC registry were analyzed with regard to the patients' preoperative diagnostic evaluation, histopathological reporting, and clinical followup. The findings were compared with the recommendations of the European Network for the Study of Adrenal Tumors (ENSAT). Results: Data were analyzed from 387 patients who had been given an initial diagnosis of ACC in the years 1998 to 2009. 21\% of them underwent no hormonal evaluation before surgery, and 59\% underwent an inadequate hormonal evaluation. This exposed the patients to unnecessary perioperative risks and impaired their follow-up. 48\% did not undergo CT scanning of the chest, even though the lungs are the most frequent site of metastases of ACC. For 13\% of the patients, the diagnosis of ACC was later revised by a reference pathologist. For 11\% of the patients, the histopathology report contained no information about resection status, even though this is an important determinant of further treatment and prognosis. Optimal management requires re-staging at three-month intervals, yet some patients underwent re-staging only after a longer delay, or not at all. Conclusion: We have identified significant deficits in the care of patients with ACC in Germany. We suspect that the situation is similar for other rare diseases. The prerequisite to better care is close and early cooperation of the treating physicians with specialized centers.}, language = {en} }