TY - JOUR A1 - Budich, Jan Carl A1 - Trauzettel, Björn T1 - Z(2) Green's function topology of Majorana wires JF - New Journal of Physics N2 - We represent the Z2 topological invariant characterizing a one-dimensional topological superconductor using a Wess–Zumino–Witten dimensional extension. The invariant is formulated in terms of the single-particle Green’s function which allows us to classify interacting systems. Employing a recently proposed generalized Berry curvature method, the topological invariant is represented independent of the extra dimension requiring only the single-particle Green’s function at zero frequency of the interacting system. Furthermore, a modified twisted boundary conditions approach is used to rigorously define the topological invariant for disordered interacting systems. KW - Green's function Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129751 VL - 15 IS - 065006 ER - TY - JOUR A1 - Herbert, Cornelia A1 - Sfärlea, Anca A1 - Blumenthal, Terry T1 - Your emotion or mine: labeling feelings alters emotional face perception—an ERP study on automatic and intentional affect labeling JF - Frontiers in Human Neuroscience N2 - Empirical evidence suggests that words are powerful regulators of emotion processing. Although a number of studies have used words as contextual cues for emotion processing, the role of what is being labeled by the words (i.e., one's own emotion as compared to the emotion expressed by the sender) is poorly understood. The present study reports results from two experiments which used ERP methodology to evaluate the impact of emotional faces and self- vs. sender-related emotional pronoun-noun pairs (e.g., my fear vs. his fear) as cues for emotional face processing. The influence of self- and sender-related cues on the processing of fearful, angry and happy faces was investigated in two contexts: an automatic (experiment 1) and intentional affect labeling task (experiment 2), along with control conditions of passive face processing. ERP patterns varied as a function of the label's reference (self vs. sender) and the intentionality of the labeling task (experiment 1 vs. experiment 2). In experiment 1, self-related labels increased the motivational relevance of the emotional faces in the time-window of the EPN component. Processing of sender-related labels improved emotion recognition specifically for fearful faces in the N170 time-window. Spontaneous processing of affective labels modulated later stages of face processing as well. Amplitudes of the late positive potential (LPP) were reduced for fearful, happy, and angry faces relative to the control condition of passive viewing. During intentional regulation (experiment 2) amplitudes of the LPP were enhanced for emotional faces when subjects used the self-related emotion labels to label their own emotion during face processing, and they rated the faces as higher in arousal than the emotional faces that had been presented in the “label sender's emotion” condition or the passive viewing condition. The present results argue in favor of a differentiated view of language-as-context for emotion processing. KW - emotion regulation KW - language-as-context KW - affect labeling KW - face processing KW - event-related brain potentials KW - social context KW - social cognition KW - perspective taking Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97065 ER - TY - JOUR A1 - Schwarz, Katharina A. A1 - Wieser, Matthias J. A1 - Gerdes, Antje B. M. A1 - Mühlberger, Andreas A1 - Pauli, Paul T1 - Why are you looking like that? How the context influences evaluation and processing of human faces JF - Social Cognitive and Affective Neuroscience N2 - Perception and evaluation of facial expressions are known to be heavily modulated by emotional features of contextual information. Such contextual effects, however, might also be driven by non-emotional aspects of contextual information, an interaction of emotional and non-emotional factors, and by the observers’ inherent traits. Therefore, we sought to assess whether contextual information about self-reference in addition to information about valence influences the evaluation and neural processing of neutral faces. Furthermore, we investigated whether social anxiety moderates these effects. In the present functional magnetic resonance imaging (fMRI) study, participants viewed neutral facial expressions preceded by a contextual sentence conveying either positive or negative evaluations about the participant or about somebody else. Contextual influences were reflected in rating and fMRI measures, with strong effects of self-reference on brain activity in the medial prefrontal cortex and right fusiform gyrus. Additionally, social anxiety strongly affected the response to faces conveying negative, self-related evaluations as revealed by the participants’ rating patterns and brain activity in cortical midline structures and regions of interest in the left and right middle frontal gyrus. These results suggest that face perception and processing are highly individual processes influenced by emotional and non-emotional aspects of contextual information and further modulated by individual personality traits. KW - social anxiety KW - facial expression KW - context KW - self-reference Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132126 VL - 8 IS - 4 ER - TY - JOUR A1 - Gageik, Nils A1 - Strohmeier, Michael A1 - Montenegro, Sergio T1 - Waypoint flight parameter comparison of an autonomous UAV JF - International Journal of Artificial Intelligence & Applications (IJAIA) N2 - The present paper compares the effect of different waypoint parameters on the flight performance of a special autonomous indoor UAV (unmanned aerial vehicle) fusing ultrasonic, inertial, pressure and optical sensors for 3D positioning and controlling. The investigated parameters are the acceptance threshold for reaching a waypoint as well as the maximal waypoint step size or block size. The effect of these parameters on the flight time and accuracy of the flight path is investigated. Therefore the paper addresses how the acceptance threshold and step size influence the speed and accuracy of the autonomous flight and thus influence the performance of the presented autonomous quadrocopter under real indoor navigation circumstances. Furthermore the paper demonstrates a drawback of the standard potential field method for navigation of such autonomous quadrocopters and points to an improvement. KW - autonomous UAV KW - Quadrocopter KW - Quadrotor KW - waypoint parameter KW - navigation Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96833 ER - TY - JOUR A1 - Camago-Molina, J.E. A1 - O'Leary, B. A1 - Porod, W. A1 - Staub, F. T1 - Vevacious: a tool for finding the global minima of one-loop effective potentials with many scalars JF - European Physical Journal C N2 - Several extensions of the Standard Model of particle physics contain additional scalars implying a more complex scalar potential compared to that of the Standard Model. In general these potentials allow for charge- and/or color-breaking minima besides the desired one with correctly broken SU(2) L ×U(1) Y . Even if one assumes that a metastable local minimum is realized, one has to ensure that its lifetime exceeds that of our universe. We introduce a new program called Vevacious which takes a generic expression for a one-loop effective potential energy function and finds all the tree-level extrema, which are then used as the starting points for gradient-based minimization of the one-loop effective potential. The tunneling time from a given input vacuum to the deepest minimum, if different from the input vacuum, can be calculated. The parameter points are given as files in the SLHA format (though is not restricted to supersymmetric models), and new model files can be easily generated automatically by the Mathematica package SARAH. This code uses HOM4PS2 to find all the minima of the tree-level potential, PyMinuit to follow gradients to the minima of the one-loop potential, and CosmoTransitions to calculate tunneling times. KW - True Vacuum KW - One-loop Effective Potential KW - Saddle Point KW - Minimal Surface Tension KW - CMSSM Point KW - SM Gauge Group KW - Renormalization Scale KW - Landau Gauge KW - Homotopy Continuation Method KW - Gauge-dependent Quantity KW - False Vacuum KW - Spectrum Generator KW - SLHA File KW - Tunneling Time KW - Charged Scalar Field Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132110 VL - 73 IS - 2588 ER - TY - JOUR A1 - Matlach, Juliane A1 - Freiberg, Florentina J. A1 - Gadeholt, Ottar A1 - Göbel, Winfried T1 - Vasculitis-like hemorrhagic retinal angiopathy in Wegener’s granulomatosis JF - BMC Research Notes N2 - Background: Granulomatosis with polyangiitis, also known as Wegener’s granulomatosis, is a chronic systemic inflammatory disease that can also involve the eyes. We report a case of massive retinal and preretinal hemorrhages with perivascular changes as the initial signs in granulomatosis with polyangiitis (Wegener’s granulomatosis). Case presentation: A 39-year-old Caucasian male presented with blurred vision in his right eye, myalgia and arthralgia, recurrent nose bleeds and anosmia. Fundus image of his right eye showed massive retinal hemorrhages and vasculitis-like angiopathy, although no fluorescein extravasation was present in fluorescein angiography. Laboratory investigations revealed an inflammation with increased C-reactive protein, elevated erythrocyte sedimentation rate and neutrophil count. Tests for antineutrophil cytoplasmic antibodies (ANCA) were positive for c-ANCA (cytoplasmatic ANCA) and PR3-ANCA (proteinase 3-ANCA). Renal biopsy demonstrated a focal segmental necrotizing glomerulonephritis. Granulomatosis with polyangiitis (Wegener’s granulomatosis) was diagnosed and a combined systemic therapy of cyclophosphamide and corticosteroids was initiated. During 3 months of follow-up, complete resorption of retinal hemorrhages was seen and general complaints as well as visual acuity improved during therapy. Conclusion: Vasculitis-like retinal changes can occur in Wegener’s granulomatosis. Despite massive retinal and preretinal hemorrhages that cause visual impairment, immunosuppressive therapy can improve ocular symptoms. KW - cyclophosphamide KW - Wegener’s granulomatosis KW - granulomatosis with polyangiitis KW - retinal vasculitis KW - hemorrhages Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-128744 VL - 6 IS - 364 ER - TY - JOUR A1 - Streng, Andrea A1 - Grote, Veit A1 - Carr, David A1 - Hagemann, Christine A1 - Liese, Johannes G. T1 - Varicella routine vaccination and the effects on varicella epidemiology – results from the Bavarian Varicella Surveillance Project (BaVariPro), 2006-2011 JF - BMC Infectious Diseases N2 - Background In 2004, routine varicella vaccination was recommended in Germany for children 11-14 months of age with one dose, and since 2009, with a second dose at 15-23 months of age. The effects on varicella epidemiology were investigated. Methods Data on varicella vaccinations, cases and complications were collected from annual parent surveys (2006-2011), monthly paediatric practice surveillance (Oct 2006 - Sep 2011; five varicella seasons) and paediatric hospital databases (2005-2009) in the area of Munich (about 238,000 paediatric inhabitants); annual incidences of cases and hospitalisations were estimated. Results Varicella vaccination coverage (1st dose) in children 18-36 months of age increased in two steps (38%, 51%, 53%, 53%, 66% and 68%); second-dose coverage reached 59% in the 2011 survey. A monthly mean of 82 (62%) practices participated; they applied a total of 50,059 first-dose and 40,541 second-dose varicella vaccinations, with preferential use of combined MMR-varicella vaccine after recommendation of two doses, and reported a total of 16,054 varicella cases <17 years of age. The mean number of cases decreased by 67% in two steps, from 6.6 (95%CI 6.1-7.0) per 1,000 patient contacts in season 2006/07 to 4.2 (95%CI 3.9-4.6) in 2007/08 and 4.0 (95%CI 3.6-4.3) in 2008/09, and further to 2.3 (95%CI 2.0-2.6) in 2009/10 and 2.2 (95%CI 1.9-2.5) in 2010/11. The decrease occurred in all paediatric age groups, indicating herd protection effects. Incidence of varicella was estimated as 78/1,000 children <17 years of age in 2006/07, and 19/1,000 in 2010/11. Vaccinated cases increased from 0.3 (95%0.2-0.3) per 1,000 patient contacts in 2006/07 to 0.4 (95%CI 0.3-0.5) until 2008/09 and decreased to 0.2 (95%CI 0.2-0.3) until 2010/11. The practices treated a total of 134 complicated cases, mainly with skin complications. The paediatric hospitals recorded a total of 178 varicella patients, including 40 (22.5%) with neurological complications and one (0.6%) fatality due to varicella pneumonia. Incidence of hospitalisations decreased from 7.6 per 100,000 children <17 years of age in 2005 to 4.3 in 2009, and from 21.0 to 4.7 in children <5 years of age. Conclusions Overall, the results show increasing acceptance and a strong impact of the varicella vaccination program, even with still suboptimal vaccination coverage. KW - Varicella KW - Surveillance KW - Coverage KW - Vaccination KW - Hospitalisation KW - Paediatric KW - Incidence Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96297 UR - http://www.biomedcentral.com/1471-2334/13/303 ER - TY - THES A1 - Christ, Thomas T1 - Value-distribution of the Riemann zeta-function and related functions near the critical line T1 - Werteverteilung der Riemannschen Zetafunktion und verwandter Funktionen nahe der kritischen Geraden N2 - The Riemann zeta-function forms a central object in multiplicative number theory; its value-distribution encodes deep arithmetic properties of the prime numbers. Here, a crucial role is assigned to the analytic behavior of the zeta-function on the so called critical line. In this thesis we study the value-distribution of the Riemann zeta-function near and on the critical line. Amongst others we focus on the following. PART I: A modified concept of universality, a-points near the critical line and a denseness conjecture attributed to Ramachandra. The critical line is a natural boundary of the Voronin-type universality property of the Riemann zeta-function. We modify Voronin's concept by adding a scaling factor to the vertical shifts that appear in Voronin's universality theorem and investigate whether this modified concept is appropriate to keep up a certain universality property of the Riemann zeta-function near and on the critical line. It turns out that it is mainly the functional equation of the Riemann zeta-function that restricts the set of functions which can be approximated by this modified concept around the critical line. Levinson showed that almost all a-points of the Riemann zeta-function lie in a certain funnel-shaped region around the critical line. We complement Levinson's result: Relying on arguments of the theory of normal families and the notion of filling discs, we detect a-points in this region which are very close to the critical line. According to a folklore conjecture (often attributed to Ramachandra) one expects that the values of the Riemann zeta-function on the critical line lie dense in the complex numbers. We show that there are certain curves which approach the critical line asymptotically and have the property that the values of the zeta-function on these curves are dense in the complex numbers. Many of our results in part I are independent of the Euler product representation of the Riemann zeta-function and apply for meromorphic functions that satisfy a Riemann-type functional equation in general. PART II: Discrete and continuous moments. The Lindelöf hypothesis deals with the growth behavior of the Riemann zeta-function on the critical line. Due to classical works by Hardy and Littlewood, the Lindelöf hypothesis can be reformulated in terms of power moments to the right of the critical line. Tanaka showed recently that the expected asymptotic formulas for these power moments are true in a certain measure-theoretical sense; roughly speaking he omits a set of Banach density zero from the path of integration of these moments. We provide a discrete and integrated version of Tanaka's result and extend it to a large class of Dirichlet series connected to the Riemann zeta-function. N2 - Die Riemannsche Zetafunktion ist ein zentraler Gegenstand der multiplikativen Zahlentheorie; in ihrer Werteverteilung liegen wichtige arithmetische Eigenschaften der Primzahlen kodiert. Besondere Bedeutung kommt hierbei dem analytischen Verhalten der Zetafunktion auf der sog. kritischen Geraden zu. Wir untersuchen in dieser Arbeit die Werteverteilung der Riemannschen Zetafunktion auf und nahe der kritischen Geraden. Wir fokusieren wir uns dabei u.a. auf folgende Punkte. TEIL I: Ein modifiziertes Universalitätskonzept, a-Stellen nahe der kritischen Geraden und eine Dichtheitsvermutung nach Ramachandra. Die kritische Gerade fungiert als natürliche Grenze für die Voroninsche Universalitätseigenschaft der Riemannschen Zetafunktion. Wir modifizieren Voronins Universalitätskonzept dahingehend, dass wir die vertikalen Translationen aus Voronins Universalitätssatz mit einer zusätzlichen Skalierung versehen. Wir untersuchen, ob durch dieses modifizierte Konzept eine abgeschwächte Universalitätseigenschaft der Riemannschen Zetafunktion um die kritschen Gerade aufrecht erhalten werden kann. Es stellt sich heraus, dass die Gestalt der Funktionen, die sich auf diese Weise durch die Zetafunktion approximieren lassen, stark von der Funktionalgleichung und der Wahl des skalierenden Faktors abhängt. Nach einem Resultat von Levinson liegen fast alle a-Stellen der Riemannschen Zetafunktion in einem trichterförmigen Bereich um die kritische Gerade. Gewisse Normalitätsargumenten sowie das Konzept der 'filling discs' erlauben uns Levinsons Resultat zu ergänzen und a-Stellen in diesem trichterförmigen Bereich aufzuspüren, die sehr nahe an der kritischen Geraden liegen. Man vermutet, dass die Werte der Riemannschen Zetafunktion auf der kritischen Geraden dicht in den komplexen Zahlen liegen. Wir nähern uns dieser Vermutung (die man oft Ramachandra zuschreibt), indem wir die Existenz gewisser Kurven nachweisen, die sich asymptotisch an die kritische Gerade anschmiegen und die Eigenschaft besitzen, dass die Werte der Zetafunktion auf diesen Kurven dicht in den komplexen Zahlen liegen. Viele unserer Ergebnisse in Teil I sind unabhängig von der Eulerproduktdarstellung der Zetafunktion und gelten allgemein für beliebige meromorphe Funktionen, die einer Funktionalgleichung vom Riemann-Typ genügen. TEIL II: Diskrete und kontinuierliche Momente. Die Lindelöf Vermutung trifft eine Aussage über das Wachstumsverhalten der Zetafunktion auf der kritischen Geraden. Nach klassischen Arbeiten von Hardy und Littlewood lässt sie sich mittels Potenzmomente der Zetafunktion rechts von der kritischen Geraden umformulieren. Tanaka konnte kürzlich nachweisen, dass die asymptotischen Formeln, die man für diese Potenzmomente erwartet in einem gewissen maßtheoretischem Sinne Gülitgkeit besitzen: grob gesprochen wird heibei eine Menge mit Banachdichte null vom Integrationsweg der Potenzmomente ausgespart. Wir stellen eine diskrete und eine integrierte Version von Tanakas Resultat zur Verfügung. Zudem verallgemeinern wir Tanakas Ergebnis auf eine große Klasse von Dirichletreihen. KW - Riemannsche Zetafunktion KW - Riemann zeta-function KW - universality KW - a-point distribution Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97763 ER - TY - THES A1 - Huang, Ting T1 - Vaccinia Virus-mediated Therapy of Solid Tumor Xenografts: Intra-tumoral Delivery of Therapeutic Antibodies T1 - Vaccini-Virus-vermittelte Therapie solider Tumoren: Intra-tumoraler Transport therapeutischer Antikörper N2 - Over the past 30 years, much effort and financial support have been invested in the fight against cancer, yet cancer still represents the leading cause of death in the world. Conventional therapies for treatment of cancer are predominantly directed against tumor cells. Recently however, new treatments options have paid more attention to exploiting the advantage of targeting the tumor stroma instead. Vaccinia virus (VACV) has played an important role in human medicine since the 18th century as a vaccination against smallpox. In our laboratory, the recombinant, replication-competent vaccinia virus, GLV-1h68, was shown to enter, colonize and destroy cancer cells both in cell culture, and in vivo, in xenograft models (Zhang, Yu et al. 2007). In addition, combined therapy of GLV-1h68 and anti-VEGF immunotherapy significantly enhanced antitumor therapy in vivo (Frentzen, Yu et al. 2009). In this study, we constructed several new recombinant VACVs carrying genes encoding different antibodies against fibroblast activation protein (FAP) in stroma (GLV-1h282), nanobody against the extracellular domain of epidermal growth factor receptor (EGFR, GLV-1h442) or antibodies targeting both vascular endothelial growth factor (VEGF) and EGFR (GLV-1h444) or targeting both VEGF and FAP (GLV-1h446). The expression of the recombinant proteins was first verified using protein analytical methods, SDS-gel electrophoresis, Western blot analysis, immunoprecipitation (IP) assays and ELISA assays. The proteins were detected after infection of the cells with the different VACVs and the recombinant proteins purified by affinity adsorption. The purified antibodies were shown to specifically bind to their respective antigens. Secondly, the infection and replication capability of all the virus strains was analyzed in cell culture using several human tumor cell lines (A549, FaDu or DU145), revealing that all the new recombinant VACVs were able to infect cancer cells with comparable efficiency to the parental viruses from which they were derived. Thirdly, the antitumor efficacy of the new recombinant VACVs was evaluated in vivo using several human cancer xenograft models in mice. In A549 and DU145 xenografts, the new recombinant VACVs exhibited an enhanced therapeutic efficacy compared to GLV-1h68 with no change in toxicity in mice. In the FaDu xenograft, treatment with GLV-1h282 (anti-FAP) significantly slowed down the speed of tumor growth compared to GLV-1h68. Additionally, treatment with the recombinant VACVs expressed the various antibodies achieved comparable or superior therapeutic effects compared to treatment with a combination of GLV-1h68 and the commercial therapeutic antibodies, Avastin, Erbitux or both. Next, the virus distribution in tumors and organs of treated mice was evaluated. For most of the viruses, the virus titer in tumors was not signficantly diffferent than GLV-1h68. However, for animals treated with GLV-1h282, the virus titer in tumors was significantly higher than with GLV-1h68. This may be the reason for enhanced antitumor efficacy of GLV-1h282 in vivo. Lastly, the underlying mechanisms of therapeutic antibody-enhanced antitumor effects were investigated by immunohistochemistry. Blood vessels density and cell proliferation in tumors were suppressed after treatment with the antibody-encoded VACVs. The results indicated that the suppression of angiogenesis or cell proliferation in tumors may cause the observed therapeutic effect. In conclusion, the results of the studies presented here support the hypothesis that the treatment of solid tumors with a combination of oncolytic virotherapy and immunotherapy has an additive effect over each treatment alone. Moreover, expression of the immunotherapeutic antibody by the oncolytic VACV locally in the tumor enhances the antitumor effect over systemic treatment with the same antibody. Combined, these results indicate that therapy with oncolytic VACVs expressing-therapeutic antibodies may be a promising approach for the treatment of cancer. N2 - In den letzten 30 Jahren wurde viel Aufwand und finanzielle Unterstützung in den Kampf gegen Krebs investiert, doch das Resultat ist limitiert, da Krebs immer noch die zweithöchste Todesursache in der Welt darstellt. Zusätzlich zu gegenwärtig verwendeten Therapien, die vorwiegend gegen Tumorzellen gerichtet sind, wird neuen Therapien mehr Aufmerksamkeit gewidmet, die stattdessen direkt auf das Tumorstroma zielen. Onkolytische Vaccinia Viren haben seit dem 18ten Jahrhundert als Impfstoff gegen Pocken in der Humanmedizin eine wichtige Rolle gespielt. In unserem Labor hat das rekombinante, replikationskompetente Vaccinia Virus GLV-1h68 gezeigt, dass es in Zellkultur und in Xenograft Modellen in Krebszellen eindringen sowie diese kolonisieren und zerstören kann (Zhang, Yu et al. 2007). Zusätzlich verbessert die kombinierte Therapie von GLV-1h68 und anti-VEGF Immunotherapy signifikant die Antitumortherapie in vivo (Frentzen, Yu et al. 2009). In dieser Studie haben wir mehrere neue rekombinante VACVs konstruiert, die die Gene für verschiedene Antikörper gegen das Fibroblasten Aktivierungs Protein (FAP) im Stroma (GLV-1h282) oder einen Nanobody gegen die extrazelluläre Domäne des Epidermalen Wachstumsfaktor (EGFR; GLV-1h442) kodieren. Ausserdem wurden Viren konstruiert, die eine Ko-Expression von Antikörpern gegen sowohl vaskulären Endothelwachstumsfaktor (VEGF) als auch EGFR (GLV-1h444) oder gegen sowohl VEGF als auch FAP (GLV-1h446) erlauben. Zunächst wurden SDS-Gelelektrophorese, Western Blot Analyse, Immunprezipitation (IP) und ELISA Assays durchgeführt, um die Expression der rekombinanten Proteine in Zellen mit proteinanalytischen Methoden zu untersuchen. Die Proteine waren nach Infektion der Zellen mit den verschiedenen VACVs nachweisbar und wurden mittles des FLAG Tags mit einem IP Kit aufgereinigt. Es konnte gezeigt werden, dass die aufgereinigten Antikörper spezifisch an ihr jeweiliges Antigen binden. Zweitens wurde die Infektion und Replikationsfähigkeit aller Virusstämme in Zellkultur untersucht (A549, FaDu oder DU145) und mit ihrem jeweiligen Ausgangsstamm GLV-1h68, GLV-1h164, GLV-1h282 oder GLV-1h442 verglichen. Die Ergebnisse zeigten, dass alle neuen rekombinanten VACVs Zellen mit vergleichbarer Effizienz infizieren konnten wie ihre Ausgangsstämme. Drittens, um die Antitumoreffizienz der neuen rekombinanten Stämme in vivo zu testen, wurden verschiedene humane Tumor Xenotransplantat-tragende Nacktmäuse mit verschiedenen VACVs behandelt. In A549 und DU145 Xenotransplantaten zeigten die neuen rekombinanten VACVs erhöhte therapeutische Effizienz verglichen mit dem Ausgangsstamm GLV-1h68, ohne Veränderung der Toxizität in Mäusen. Im FaDu Xenotransplantat verursachte die Behandlung mit GLV-1h68 keine Tumorregression, wohingegen die Behandlung mit GLV-1h282 (anti-FAP) die Geschwindigkeit des Tumorwachstums signifikant verlangsamte sowie das Überleben verlängerte. Zusätzlich haben wir herausgefunden, dass die Behandlung mit Antikörpern, die mittels Virus geliefert wurden, einen identischen oder sogar erhöhten inhibitorischen Effekt erzielen können, wie in einer Kombinationstherapie von GLV-1h68 und kommerziell erhältlichen Antikörpern, wie Avastin, Erbitux oder beidem. Um die virale Verteilung in vivo zu untersuchen, wurden Tumore und Organe von Mäusen seziert und homogenisiert, gefolgt von Titration der Virusmenge. Die Virus-Titer in Tumoren waren signifikant höher in Tieren, die mit GLV-1h282 behandelt wurden als solche, die mit GLV-1h68 behandelt wurden. Dies mag den Grund für die erhöhte Antitumoreffizienz von GLV-1h282 in vivo darstellen. Die Virus-Titer in allen anderen Gruppen zeigten keinen signifikanten Unterschied. Um den Mechanismus der durch therapeutische Antikörper erhöhten Antitumortherapie zu untersuchen, wurde Immunohistochemie durchgeführt. Nach Behandlung mit den Antikörper-kodierenden VACVs waren die Blutgefäβdichte und Zellproliferation in Tumoren reduziert, nachgewiesen durch die jeweilige CD31 and Ki67 Färbung. Die Resultate deuteten an, dass die Suppression der Angiogenese oder der Zellproliferation in Tumoren den beobachteten Effekt verursachen könnte. Zusammenfassend zeigen die hier präsentierten Daten dass die Kombination der Behandlung von onkolytischer Virotherapie mit Immunotherapie durch Virus-gelieferte Antikörper einen vielversprechenden Ansatz für Krebstherapie darstellt. KW - Vaccinia-Virus KW - therapeutic antibody KW - oncolytic virus KW - Krebs KW - Therapie KW - Antikörper KW - Tumor Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-91327 ER - TY - THES A1 - Heß, Michael T1 - Vaccinia virus-encoded bacterial beta-glucuronidase as a diagnostic biomarker for oncolytic virotherapy T1 - Vaccinia Virus-codierte bakterielle Beta-Glucuronidase als diagnostischer Biomarker in der onkolytischen Virotherapie N2 - Oncolytic virotherapy represents a promising approach to revolutionize cancer therapy. Several preclinical and clinical trials display the safety of oncolytic viruses as wells as their efficiency against solid tumors. The development of complementary diagnosis and monitoring concepts as well as the optimization of anti-tumor activity are key points of current virotherapy research. Within the framework of this thesis, the diagnostic and therapeutic prospects of beta-glucuronidase expressed by the oncolytic vaccinia virus strain GLV-1h68 were evaluated. In this regard, a beta-glucuronidase-based, therapy-accompanying biomarker test was established which is currently under clinical validation. By using fluorescent substrates, the activity of virally expressed beta-glucuronidase could be detected and quantified. Thereby conclusions about the replication kinetics of oncolytic viruses in animal models and virus-induced cancer cell lysis could be drawn. These findings finally led to the elaboration and establishment of a versatile biomarker assay which allows statements regarding the replication of oncolytic viruses in mice based on serum samples. Besides the analysis of retrospective conditions, this test is able to serve as therapy-accompanying monitoring tool for virotherapy approaches with beta-glucuronidase-expressing viruses. The newly developed assay also served as complement to routinely used plaque assays as well as reference for virally expressed anti-angiogenic antibodies in additional preclinical studies. Further validation of this biomarker test is currently taking place in the context of clinical trials with GL-ONC1 (clinical grade GLV-1h68) and has already shown promising preliminary results. It was furthermore demonstrated that fluorogenic substrates in combination with beta-glucuronidase expressed by oncolytic viruses facilitated the optical detection of solid tumors in preclinical models. In addition to diagnostic purposes, virus-encoded enzymes could also be combined with prodrugs resulting in an improved therapeutic outcome of oncolytic virotherapy. In further studies, the visualization of virus-induced immune reactions as well as the establishment of innovative concepts to improve the therapeutic outcome of oncolytic virotherapy could be accomplished. In conclusion, the results of this thesis provide crucial findings about the influence of virally expressed beta-glucuronidase on various diagnostic concepts in the context of oncolytic virotherapy. In addition, innovative monitoring and therapeutic strategies could be established. Our preclinical findings have important clinical influence, particularly by the development of a therapy-associated biomarker assay which is currently used in different clinical trials. N2 - Onkolytische Viren stellen einen vielversprechenden Therapieansatz dar, der die Behandlung von Krebserkrankungen revolutionieren könnte. Intensive präklinische und klinische Studien zeigen sowohl die körperliche Verträglichkeit von onkolytischen Viren, als auch deren Wirksamkeit gegenüber soliden Tumoren. Die Entwicklung von therapiebegleitenden Diagnose- und Monitoringkonzepten sowie eine Optimierung der Antitumorwirkung onkolytischer Viren stellen Eckpunkte der aktuellen Forschung auf dem Gebiet der Virotherapie dar. Im Rahmen dieser Arbeit wurde untersucht, welche diagnostischen und therapeutischen Möglichkeiten die virale Expression von beta-Glucuronidase durch den onkolytischen Vaccinia-Virus-Stamm GLV-1h68 eröffnet. In diesem Zusammenhang wurde ein, auf beta-Glucuronidase basierender, therapiebegleitender Biomarkertest entwickelt, dessen klinische Validierung derzeit stattfindet. Mit Hilfe von fluorogenen Substraten konnte die Aktivität viral exprimierter beta-Glucuronidase detektiert und quantifiziert werden. Dies lies direkte Rückschlüsse auf das Replikationsverhalten von onkolytischen Viren im Tiermodell zu und ermöglichte zudem Aussagen über die Zelllyse Virus-infizierter Krebszellen. Diese Erkenntnisse führten letztendlich zur Ausarbeitung und Etablierung eines vielseitig anwendbaren Biomarker-Assays, der es ermöglicht anhand von Blutproben Aussagen über das Replikationsverhalten onkolytischer Viren in Mäusen zu machen. Neben retrospektiven Analysen erlaubt dieser Test auch ein therapiebegleitendes Monitoring der onkolytischen Virotherapie mit beta-Glucuronidase-exprimierenden Viren. In weiteren präklinischen Untersuchungen diente der entwickelte Assay zudem als Ergänzung zum viralen Plaque Assays sowie als Referenz für Virus-exprimierte anti-angiogene Antikörper. Eine fortführende Validierung dieses neuartigen Biomarkertests findet derzeit im Rahmen humaner Studien mit der klinischen Formulierung von GLV-1h68, GL-ONC1, statt und zeigte bereits erste positive Resultate. Weiterhin konnte im Rahmen dieser Arbeit gezeigt werden, dass die Expression von beta-Glucuronidase durch onkolytische Viren in Verbindung mit fluoreszierenden Substraten eine optische Detektion von Karzinomen im präklinischen Tiermodell ermöglicht. Neben diagnostischen Zwecken, konnten Virus-kodierte Enzyme in Kombination mit Prodrugs genutzt werden, um den Therapieerfolg der onkolytischen Virotherapie zu verbessern. In zusätzlichen Studien konnten zudem Methoden zur Visualisierung der Virus-induzierten Immunantwort sowie neuartige Konzepte zur Therapieverbesserung etabliert werden. Zusammenfassend liefern die Ergebnisse der vorliegenden Arbeit wichtige Erkenntnisse über den Einfluss Virus-exprimierter beta-Glucuronidase auf unterschiedliche Diagnosekonzepte im Rahmen der onkolytischen Virotherapie. Daneben konnten entscheidende Erkenntnisse über den möglichen Einsatz neuer Monitoring- und Therapieansätze erzielt werden. Insbesondere durch die Entwicklung eines therapiebegleitenden Biomarkertests haben diese Resultate erheblichen Einfluss auf die weitere klinische Anwendung von onkolytischen Vaccinia-Viren. KW - Vaccinia-Virus KW - Glucuronidase KW - Krebs KW - cancer KW - oncolytic virus KW - biomarker KW - beta-glucuronidase Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-86789 ER - TY - JOUR A1 - Gholami, Sepideh A1 - Chen, Chun-Hao A1 - Belin, Laurence J. A1 - Lou, Emil A1 - Fujisawa, Sho A1 - Antonacci, Caroline A1 - Carew, Amanda A1 - Chen, Nanhai G. A1 - De Brot, Marina A1 - Zanzonico, Pat B. A1 - Szalay, Aladar A. A1 - Fong, Yuman T1 - Vaccinia virus GLV-1h153 is a novel agent for detection and effective local control of positive surgical margins for breast cancer JF - Breast Cancer Research N2 - Introduction: Surgery is currently the definitive treatment for early-stage breast cancer. However, the rate of positive surgical margins remains unacceptably high. The human sodium iodide symporter (hNIS) is a naturally occurring protein in human thyroid tissue, which enables cells to concentrate radionuclides. The hNIS has been exploited to image and treat thyroid cancer. We therefore investigated the potential of a novel oncolytic vaccinia virus GLV1h-153 engineered to express the hNIS gene for identifying positive surgical margins after tumor resection via positron emission tomography (PET). Furthermore, we studied its role as an adjuvant therapeutic agent in achieving local control of remaining tumors in an orthotopic breast cancer model. Methods: GLV-1h153, a replication-competent vaccinia virus, was tested against breast cancer cell lines at various multiplicities of infection (MOIs). Cytotoxicity and viral replication were determined. Mammary fat pad tumors were generated in athymic nude mice. To determine the utility of GLV-1h153 in identifying positive surgical margins, 90% of the mammary fat pad tumors were surgically resected and subsequently injected with GLV-1h153 or phosphate buffered saline (PBS) in the surgical wound. Serial Focus 120 microPET images were obtained six hours post-tail vein injection of approximately 600 mu Ci of I-124-iodide. Results: Viral infectivity, measured by green fluorescent protein (GFP) expression, was time-and concentrationdependent. All cell lines showed less than 10% of cell survival five days after treatment at an MOI of 5. GLV-1h153 replicated efficiently in all cell lines with a peak titer of 27 million viral plaque forming units (PFU) ( < 10,000-fold increase from the initial viral dose) by Day 4. Administration of GLV-1h153 into the surgical wound allowed positive surgical margins to be identified via PET scanning. In vivo, mean volume of infected surgically resected residual tumors four weeks after treatment was 14 mm(3) versus 168 mm(3) in untreated controls (P < 0.05). Conclusions: This is the first study to our knowledge to demonstrate a novel vaccinia virus carrying hNIS as an imaging tool in identifying positive surgical margins of breast cancers in an orthotopic murine model. Moreover, our results suggest that GLV-1h153 is a promising therapeutic agent in achieving local control for positive surgical margins in resected breast tumors. KW - conservation KW - carcinoma KW - mastectomy KW - metastases KW - stage-i KW - thyroid-cancer KW - radiation-therapy KW - conserving surgery KW - sodium-iodide symporter Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122140 VL - 15 IS - R26 ER - TY - JOUR A1 - Duggal, Rohit A1 - Geissinger, Ulrike A1 - Zhang, Qian A1 - Aguilar, Jason A1 - Chen, Nanhai G. A1 - Binda, Elena A1 - Vescovi, Angelo L. A1 - Szalay, Aladar A. T1 - Vaccinia virus expressing bone morphogenetic protein-4 in novel glioblastoma orthotopic models facilitates enhanced tumor regression and long-term survival JF - Journal of Translational Medicine N2 - No abstract availableBackground: Glioblastoma multiforme (GBM) is one of the most aggressive forms of cancer with a high rate of recurrence. We propose a novel oncolytic vaccinia virus (VACV)-based therapy using expression of the bone morphogenetic protein (BMP)-4 for treating GBM and preventing recurrence. Methods: We have utilized clinically relevant, orthotopic xenograft models of GBM based on tumor-biopsy derived, primary cancer stem cell (CSC) lines. One of the cell lines, after being transduced with a cDNA encoding firefly luciferase, could be used for real time tumor imaging. A VACV that expresses BMP-4 was constructed and utilized for infecting several primary glioma cultures besides conventional serum-grown glioma cell lines. This virus was also delivered intracranially upon implantation of the GBM CSCs in mice to determine effects on tumor growth. Results: We found that the VACV that overexpresses BMP-4 demonstrated heightened replication and cytotoxic activity in GBM CSC cultures with a broad spectrum of activity across several different patient-biopsy cultures. Intracranial inoculation of mice with this virus resulted in a tumor size equal to or below that at the time of injection. This resulted in survival of 100% of the treated mice up to 84 days post inoculation, significantly superior to that of a VACV lacking BMP-4 expression. When mice with a higher tumor burden were injected with the VACV lacking BMP-4, 80% of the mice showed tumor recurrence. In contrast, no recurrence was seen when mice were injected with the VACV expressing BMP-4, possibly due to induction of differentiation in the CSC population and subsequently serving as a better host for VACV infection and oncolysis. This lack of recurrence resulted in superior survival in the BMP-4 VACV treated group. Conclusions: Based on these findings we propose a novel VACV therapy for treating GBM, which would allow tumor specific production of drugs in the future in combination with BMPs which would simultaneously control tumor maintenance and facilitate CSC differentiation, respectively, thereby causing sustained tumor regression without recurrence. KW - cancer stem cells (CSCs) and differentiation KW - glioblastoma multiforme (GBM) KW - vaccinia virus (VACV) KW - bone morphogenetic protein (BMP) Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129626 VL - 11 IS - 155 ER - TY - JOUR A1 - Prelog, Martina T1 - Vaccination in Patients with Rheumatoid Arthritis Receiving Immunotherapies JF - Clinical & Cellular Immunology N2 - Patients with rheumatoid arthritis (RA) are at higher risk to suffer from morbidity due to vaccine-preventable diseases and, thus, display an important target population to receive vaccines for protection from infectious complications. There have been only a few studies focusing on the administration of vaccines in RA patients with immunotherapy. Overall, antibody response rates against influenza or pneumococcal disease appeared to be only slightly lower than expected in healthy individuals. Crucial problems in the interpretation of data from studies in RA patients vaccinated against influenza and pneumococcal disease are the impaired comparability of studies due to different study designs and type of vaccines used, different health states among RA patients, heterogeneity in treatments including concomitant therapy with conventional DMARDs and glucocorticoids in addition to biological agents. Assessment of vaccination status should be performed in the initial work-up of patients with RA and should ideally be administered before initiation of immunotherapies or during stable disease. Due to differences in antibody responses and uncertainty regarding maintenance of protective antibodies, routine controls for antibody titers and specific strategies for earlier re-vaccination might be scheduled for patients with RA. KW - Immunotherapy KW - Anti-TNF-alpha agents KW - Rituximab KW - Tocilizumab KW - Abatacept KW - Pneumococcal vaccination KW - Influenza vaccination Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96446 ER - TY - JOUR A1 - Bárcena-Uribarri, Iván A1 - Thein, Marcus A1 - Maier, Elke A1 - Bonde, Mari A1 - Bergström, Sven A1 - Benz, Roland T1 - Use of Nonelectrolytes Reveals the Channel Size and Oligomeric Constitution of the Borrelia burgdorferi P66 Porin JF - PLoS ONE N2 - In the Lyme disease spirochete Borrelia burgdorferi, the outer membrane protein P66 is capable of pore formation with an atypical high single-channel conductance of 11 nS in 1 M KCl, which suggested that it could have a larger diameter than ‘normal’ Gram-negative bacterial porins. We studied the diameter of the P66 channel by analyzing its single-channel conductance in black lipid bilayers in the presence of different nonelectrolytes with known hydrodynamic radii. We calculated the filling of the channel with these nonelectrolytes and the results suggested that nonelectrolytes (NEs) with hydrodynamic radii of 0.34 nm or smaller pass through the pore, whereas neutral molecules with greater radii only partially filled the channel or were not able to enter it at all. The diameter of the entrance of the P66 channel was determined to be \(\leq\)1.9 nm and the channel has a central constriction of about 0.8 nm. The size of the channel appeared to be symmetrical as judged from one-sidedness of addition of NEs. Furthermore, the P66-induced membrane conductance could be blocked by 80–90% by the addition of the nonelectrolytes PEG 400, PEG 600 and maltohexaose to the aqueous phase in the low millimolar range. The analysis of the power density spectra of ion current through P66 after blockage with these NEs revealed no chemical reaction responsible for channel block. Interestingly, the blockage of the single-channel conductance of P66 by these NEs occurred in about eight subconductance states, indicating that the P66 channel could be an oligomer of about eight individual channels. The organization of P66 as a possible octamer was confirmed by Blue Native PAGE and immunoblot analysis, which both demonstrated that P66 forms a complex with a mass of approximately 460 kDa. Two dimension SDS PAGE revealed that P66 is the only polypeptide in the complex. KW - radii KW - hydrodynamics KW - SDS polyacrylamide gel electrophoresis KW - molecular mass KW - outer membrane proteins KW - single channel recording KW - blue native polyacrylamide gel electrophoresis KW - borrelia burgdorferi Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129965 VL - 8 IS - 11 ER - TY - JOUR A1 - Mayer, Matthias A1 - Rabindranath, Raman A1 - Börner, Juliane A1 - Hörner, Eva A1 - Bentz, Alexander A1 - Salgado, Josefina A1 - Han, Hong A1 - Böse, Holger A1 - Probst, Jörn A1 - Shamonin, Mikhail A1 - Monkman, Gereth J. A1 - Schlunck, Günther T1 - Ultra-Soft PDMS-Based Magnetoactive Elastomers as Dynamic Cell Culture Substrata JF - PLOS ONE N2 - Mechanical cues such as extracellular matrix stiffness and movement have a major impact on cell differentiation and function. To replicate these biological features in vitro, soft substrata with tunable elasticity and the possibility for controlled surface translocation are desirable. Here we report on the use of ultra-soft (Young's modulus <100 kPa) PDMS-based magnetoactive elastomers (MAE) as suitable cell culture substrata. Soft non-viscous PDMS (<18 kPa) is produced using a modified extended crosslinker. MAEs are generated by embedding magnetic microparticles into a soft PDMS matrix. Both substrata yield an elasticity-dependent (14 vs. 100 kPa) modulation of alpha-smooth muscle actin expression in primary human fibroblasts. To allow for static or dynamic control of MAE material properties, we devise low magnetic field (approximate to 40 mT) stimulation systems compatible with cell-culture environments. Magnetic field-instigated stiffening (14 to 200 kPa) of soft MAE enhances the spreading of primary human fibroblasts and decreases PAX-7 transcription in human mesenchymal stem cells. Pulsatile MAE movements are generated using oscillating magnetic fields and are well tolerated by adherent human fibroblasts. This MAE system provides spatial and temporal control of substratum material characteristics and permits novel designs when used as dynamic cell culture substrata or cell culture-coated actuator in tissue engineering applications or biomedical devices. KW - elastic magnetic-materials KW - smooth muscle actin KW - magnetorheological elastomers KW - adhesion KW - mechanotransduction KW - stiffness KW - tension KW - mechanics KW - hydrogels KW - behavior Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-128246 SN - 1932-6203 VL - 8 IS - 10 ER - TY - JOUR A1 - Bodem, Jochen A1 - Schrom, Eva-Maria A1 - Moschall, Rebecca A1 - Hartl, Maximilian J. A1 - Weitner, Helena A1 - Fecher, David A1 - Langemeier, Jörg A1 - Wöhrl, Brigitta M. T1 - U1snRNP-mediated suppression of polyadenylation in conjunction with the RNA structure controls poly (A) site selection in foamy viruses JF - Retrovirology N2 - Background During reverse transcription, retroviruses duplicate the long terminal repeats (LTRs). These identical LTRs carry both promoter regions and functional polyadenylation sites. To express full-length transcripts, retroviruses have to suppress polyadenylation in the 5′LTR and activate polyadenylation in the 3′LTR. Foamy viruses have a unique LTR structure with respect to the location of the major splice donor (MSD), which is located upstream of the polyadenylation signal. Results Here, we describe the mechanisms of foamy viruses regulating polyadenylation. We show that binding of the U1 small nuclear ribonucleoprotein (U1snRNP) to the MSD suppresses polyadenylation at the 5′LTR. In contrast, polyadenylation at the 3′LTR is achieved by adoption of a different RNA structure at the MSD region, which blocks U1snRNP binding and furthers RNA cleavage and subsequent polyadenylation. Conclusion Recently, it was shown that U1snRNP is able to suppress the usage of intronic cryptic polyadenylation sites in the cellular genome. Foamy viruses take advantage of this surveillance mechanism to suppress premature polyadenylation at the 5’end of their RNA. At the 3’end, Foamy viruses use a secondary structure to presumably block access of U1snRNP and thereby activate polyadenylation at the end of the genome. Our data reveal a contribution of U1snRNP to cellular polyadenylation site selection and to the regulation of gene expression. KW - Polyadenylation KW - foamy virus KW - RNA structure KW - Major splice donor KW - Polyadenylierung KW - RNS Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96085 UR - http://www.retrovirology.com/content/10/1/55 ER - TY - JOUR A1 - Engel, Volker A1 - Albert, Julian A1 - Schubert, Alexander T1 - Two-dimensional vibronic spectroscopy of molecular predissociation JF - New Journal of Physics N2 - We calculate two-dimensional (2D) spectra reflecting the time-dependent electronic predissociation of a diatomic molecule. The laser-excited electronic state is coupled non-adiabatically to a fragment channel, leading to the decay of the prepared quasi-bound states. This decay can be monitored by the three-pulse configuration employed in optical 2D spectroscopy. It is shown that in this way it is possible to state-selectively characterize the time-dependent population of resonance states with different lifetimes. A model of the NaI molecule serves as a numerical example. KW - computational physics KW - atomic physics KW - molecular physics Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96199 ER - TY - JOUR A1 - Chopra, Martin A1 - Lang, Isabell A1 - Salzmann, Steffen A1 - Pachel, Christina A1 - Kraus, Sabrina A1 - Bäuerlein, Carina A. A1 - Brede, Christian A1 - Jordán Garrote, Ana-Laura A1 - Mattenheimer, Katharina A1 - Ritz, Miriam A1 - Schwinn, Stefanie A1 - Graf, Carolin A1 - Schäfer, Viktoria A1 - Frantz, Stefan A1 - Einsele, Hermann A1 - Wajant, Harald A1 - Beilhack, Andreas T1 - Tumor Necrosis Factor Induces Tumor Promoting and Anti-Tumoral Effects on Pancreatic Cancer via TNFR1 JF - PLoS ONE N2 - Multiple activities are ascribed to the cytokine tumor necrosis factor (TNF) in health and disease. In particular, TNF was shown to affect carcinogenesis in multiple ways. This cytokine acts via the activation of two cell surface receptors, TNFR1, which is associated with inflammation, and TNFR2, which was shown to cause anti-inflammatory signaling. We assessed the effects of TNF and its two receptors on the progression of pancreatic cancer by in vivo bioluminescence imaging in a syngeneic orthotopic tumor mouse model with Panc02 cells. Mice deficient for TNFR1 were unable to spontaneously reject Panc02 tumors and furthermore displayed enhanced tumor progression. In contrast, a fraction of wild type (37.5%), TNF deficient (12.5%), and TNFR2 deficient mice (22.2%) were able to fully reject the tumor within two weeks. Pancreatic tumors in TNFR1 deficient mice displayed increased vascular density, enhanced infiltration of CD4+ T cells and CD4+ forkhead box P3 (FoxP3)+ regulatory T cells (Treg) but reduced numbers of CD8+ T cells. These alterations were further accompanied by transcriptional upregulation of IL4. Thus, TNF and TNFR1 are required in pancreatic ductal carcinoma to ensure optimal CD8+ T cell-mediated immunosurveillance and tumor rejection. Exogenous systemic administration of human TNF, however, which only interacts with murine TNFR1, accelerated tumor progression. This suggests that TNFR1 has basically the capability in the Panc02 model to trigger pro-and anti-tumoral effects but the spatiotemporal availability of TNF seems to determine finally the overall outcome. KW - Bioluminescence KW - cancer treatment KW - cell staining KW - cytokines KW - immune cells KW - metastasis KW - regulatory T cells KW - T cells Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97246 ER - TY - JOUR A1 - Shannon, Graver A1 - Hein, Melanie T1 - Tumor cell response to bevacizumab single agent therapy in vitro JF - Cancer Cell International N2 - Background Angiogenesis represents a highly multi-factorial and multi-cellular complex (patho-) physiologic event involving endothelial cells, tumor cells in malignant conditions, as well as bone marrow derived cells and stromal cells. One main driver is vascular endothelial growth factor (VEGFA), which is known to interact with endothelial cells as a survival and mitogenic signal. The role of VEGFA on tumor cells and /or tumor stromal cell interaction is less clear. Condition specific (e.g. hypoxia) or tumor specific expression of VEGFA, VEGF receptors and co-receptors on tumor cells has been reported, in addition to the expression on the endothelium. This suggests a potential paracrine/autocrine loop that could affect changes specific to tumor cells. Methods We used the monoclonal antibody against VEGFA, bevacizumab, in various in vitro experiments using cell lines derived from different tumor entities (non small cell lung cancer (NSCLC), colorectal cancer (CRC), breast cancer (BC) and renal cell carcinoma (RCC)) in order to determine if potential VEGFA signaling could be blocked in tumor cells. The experiments were done under hypoxia, a major inducer of VEGFA and angiogenesis, in an attempt to mimic the physiological tumor condition. Known VEGFA induced endothelial biological responses such as proliferation, migration, survival and gene expression changes were evaluated. Results Our study was able to demonstrate expression of VEGF receptors on tumor cells as well as hypoxia regulated angiogenic gene expression. In addition, there was a cell line specific effect in tumor cells by VEGFA blockade with bevacizumab in terms of proliferation; however overall, there was a limited measurable consequence of bevacizumab therapy detected by migration and survival. Conclusion The present study showed in a variety of in vitro experiments with several tumor cell lines from different tumor origins, that by blocking VEGFA with bevacizumab, there was a limited autocrine or cell-autonomous function of VEGFA signaling in tumor cells, when evaluating VEGFA induced downstream outputs known in endothelial cells. KW - Bevacizumab KW - NCI-60 KW - Tumor angiogenesis KW - VEGFA KW - Hypoxia KW - In vitro Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-97185 UR - http://www.cancerci.com/content/13/1/94 ER - TY - JOUR A1 - Muturi, Harrison T. A1 - Dreesen, Janine D. A1 - Nilewski, Elena A1 - Jastrow, Holger A1 - Giebel, Bernd A1 - Ergun, Suleyman A1 - Singer, Berhard B. T1 - Tumor and Endothelial Cell-Derived Microvesicles Carry Distinct CEACAMs and Influence T-Cell Behavior JF - PLOS ONE N2 - Normal and malignant cells release a variety of different vesicles into their extracellular environment. The most prominent vesicles are the microvesicles (MVs, 100-1 000 nm in diameter), which are shed of the plasma membrane, and the exosomes (70-120 nm in diameter), derivates of the endosomal system. MVs have been associated with intercellular communication processes and transport numerous proteins, lipids and RNAs. As essential component of immune-escape mechanisms tumor-derived MVs suppress immune responses. Additionally, tumor-derived MVs have been found to promote metastasis, tumor-stroma interactions and angiogenesis. Since members of the carcinoembryonic antigen related cell adhesion molecule (CEACAM)-family have been associated with similar processes, we studied the distribution and function of CEACAMs in MV fractions of different human epithelial tumor cells and of human and murine endothelial cells. Here we demonstrate that in association to their cell surface phenotype, MVs released from different human epithelial tumor cells contain CEACAM1, CEACAM5 and CEACAM6, while human and murine endothelial cells were positive for CEACAM1 only. Furthermore, MVs derived from CEACAM1 transfected CHO cells carried CEACAM1. In terms of their secretion kinetics, we show that MVs are permanently released in low doses, which are extensively increased upon cellular starvation stress. Although CEACAM1 did not transmit signals into MVs it served as ligand for CEACAM expressing cell types. We gained evidence that CEACAM1-positive MVs significantly increase the CD3 and CD3/CD28-induced T-cell proliferation. All together, our data demonstrate that MV-bound forms of CEACAMs play important roles in intercellular communication processes, which can modulate immune response, tumor progression, metastasis and angiogenesis. KW - carcinoembryonic anitgen family KW - biliary glycoprotein CD66A KW - adhesion molecule-1 KW - epithelial cells KW - membrane vesicles KW - growth-factor KW - cancer KW - expression KW - proliferation Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-128373 SN - 1932-6203 VL - 8 IS - 9 ER - TY - JOUR A1 - Spitznagel, N. A1 - Durig, T. A1 - Zimanowski, B. T1 - Trigger - and heat-transfer times measured during experimental molten-fuel-interactions JF - AIP Advances N2 - A modified setup featuring high speed high resolution data and video recording was developed to obtain detailed information on trigger and heat transfer times during explosive molten fuel-coolant-interaction (MFCI). MFCI occurs predominantly in configurations where water is entrapped by hot melt. The setup was modified to allow direct observation of the trigger and explosion onset. In addition the influences of experimental control and data acquisition can now be more clearly distinguished from the pure phenomena. More precise experimental studies will facilitate the description of MFCI thermodynamics. KW - temperature measurement KW - data acquisition KW - heat transfer KW - expolsions KW - shock waves Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-128625 VL - 3 IS - 102126 ER - TY - JOUR A1 - Szalay, Aladar A A1 - Weibel, Stephanie A1 - Hofmann, Elisabeth A1 - Basse-Luesebrink, Thomas Christian A1 - Donat, Ulrike A1 - Seubert, Carolin A1 - Adelfinger, Marion A1 - Gnamlin, Prisca A1 - Kober, Christina A1 - Frentzen, Alexa A1 - Gentschev, Ivaylo A1 - Jakob, Peter Michael T1 - Treatment of malignant effusion by oncolytic virotherapy in an experimental subcutaneous xenograft model of lung cancer JF - Journal of Translational Medicine N2 - Background Malignant pleural effusion (MPE) is associated with advanced stages of lung cancer and is mainly dependent on invasion of the pleura and expression of vascular endothelial growth factor (VEGF) by cancer cells. As MPE indicates an incurable disease with limited palliative treatment options and poor outcome, there is an urgent need for new and efficient treatment options. Methods In this study, we used subcutaneously generated PC14PE6 lung adenocarcinoma xenografts in athymic mice that developed subcutaneous malignant effusions (ME) which mimic pleural effusions of the orthotopic model. Using this approach monitoring of therapeutic intervention was facilitated by direct observation of subcutaneous ME formation without the need of sacrificing mice or special imaging equipment as in case of MPE. Further, we tested oncolytic virotherapy using Vaccinia virus as a novel treatment modality against ME in this subcutaneous PC14PE6 xenograft model of advanced lung adenocarcinoma. Results We demonstrated significant therapeutic efficacy of Vaccinia virus treatment of both advanced lung adenocarcinoma and tumor-associated ME. We attribute the efficacy to the virus-mediated reduction of tumor cell-derived VEGF levels in tumors, decreased invasion of tumor cells into the peritumoral tissue, and to viral infection of the blood vessel-invading tumor cells. Moreover, we showed that the use of oncolytic Vaccinia virus encoding for a single-chain antibody (scAb) against VEGF (GLAF-1) significantly enhanced mono-therapy of oncolytic treatment. Conclusions Here, we demonstrate for the first time that oncolytic virotherapy using tumor-specific Vaccinia virus represents a novel and promising treatment modality for therapy of ME associated with advanced lung cancer. KW - Oncolytic virotherapy KW - Malignant effusion KW - Lung cancer KW - VEGF KW - Lungenkrebs KW - Vascular endothelial Growth Factor Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96016 UR - http://www.translational-medicine.com/content/11/1/106 ER - TY - JOUR A1 - Ablin, Jacob A1 - Fitzcharles, Mary-Ann A1 - Buskila, Dan A1 - Shir, Yoram A1 - Sommer, Claudia A1 - Häuser, Winfried T1 - Treatment of Fibromyalgia Syndrome: Recommendations of Recent Evidence-Based Interdisciplinary Guidelines with Special Emphasis on Complementary and Alternative Therapies JF - Evidence-Bayed Complementary and Alternative Medicine N2 - Objective. Current evidence indicates that there is no single ideal treatment for fibromyalgia syndrome (FMS). First choice treatment options remain debatable, especially concerning the importance of complementary and alternative medicine (CAM) treatments. Methods. Three evidence-based interdisciplinary guidelines on FMS in Canada, Germany, and Israel were compared for their first choice and CAM-recommendations. Results. All three guidelines emphasized a patient-tailored approach according to the key symptoms. Aerobic exercise, cognitive behavioral therapy, and multicomponent therapy were first choice treatments. The guidelines differed in the grade of recommendation for drug treatment. Anticonvulsants (gabapentin, pregabalin) and serotonin noradrenaline reuptake inhibitors (duloxetine, milnacipran) were strongly recommended by the Canadian and the Israeli guidelines. These drugs received only a weak recommendation by the German guideline. In consideration of CAM-treatments, acupuncture, hypnosis/guided imagery, and Tai Chi were recommended by the German and Israeli guidelines. The Canadian guidelines did not recommend any CAM therapy. Discussion. Recent evidence-based interdisciplinary guidelines concur on the importance of treatment tailored to the individual patient and further emphasize the need of self-management strategies (exercise, and psychological techniques). KW - metaanalysis KW - management KW - care Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122235 SN - 1741-427X ER - TY - JOUR A1 - Walter, Maggie C. A1 - Reilich, Peter A1 - Thiele, Simone A1 - Schessl, Joachim A1 - Schreiber, Herbert A1 - Reiners, Karlheinz A1 - Kress, Wolfram A1 - Müller-Reible, Clemens A1 - Vorgerd, Matthias A1 - Urban, Peter A1 - Schrank, Bertold A1 - Deschauer, Marcus A1 - Schlotter-Weigel, Beate A1 - Kohnen, Ralf A1 - Lochmüller, Hans T1 - Treatment of dysferlinopathy with deflazacort: a double-blind, placebo-controlled clinical trial JF - Orphanet Journal of Rare Diseases N2 - Background: Dysferlinopathies are autosomal recessive disorders caused by mutations in the dysferlin (DYSF) gene encoding the dysferlin protein. DYSF mutations lead to a wide range of muscular phenotypes, with the most prominent being Miyoshi myopathy (MM) and limb girdle muscular dystrophy type 2B (LGMD2B). Methods: We assessed the one-year-natural course of dysferlinopathy, and the safety and efficacy of deflazacort treatment in a double-blind, placebo-controlled cross-over trial. After one year of natural course without intervention, 25 patients with genetically defined dysferlinopathy were randomized to receive deflazacort and placebo for six months each (1 mg/kg/day in month one, 1 mg/kg every 2nd day during months two to six) in one of two treatment sequences. Results: During one year of natural course, muscle strength declined about 2% as measured by CIDD (Clinical Investigation of Duchenne Dystrophy) score, and 76 Newton as measured by hand-held dynamometry. Deflazacort did not improve muscle strength. In contrast, there is a trend of worsening muscle strength under deflazacort treatment, which recovers after discontinuation of the study drug. During deflazacort treatment, patients showed a broad spectrum of steroid side effects. Conclusion: Deflazacort is not an effective therapy for dysferlinopathies, and off-label use is not warranted. This is an important finding, since steroid treatment should not be administered in patients with dysferlinopathy, who may be often misdiagnosed as polymyositis. KW - Deflazacort KW - muscle strength KW - gridle muscular-dystrophy KW - Duchenne dystrphy KW - Miyoshi myopathy KW - mutation KW - prednisone KW - gene KW - 2B KW - children KW - design KW - steroids KW - therapy KW - dysferlinopathy KW - Limb girdle muscular dystrophy (LGMD) Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125663 SN - 1750-1172 VL - 8 IS - 26 ER - TY - THES A1 - Regneri, Janine T1 - Transcriptional regulation of cancer genes in the Xiphophorus melanoma system T1 - Transkriptionelle Regulation von Krebsgenen im Xiphophorus-Melanommodell N2 - The Xiphophorus melanoma system is a useful animal model for the study of the genetic basis of tumor formation. The development of hereditary melanomas in interspecific hybrids of Xiphophorus is connected to pigment cell specific overexpression of the mutationally activated receptor tyrosine kinase Xmrk. In purebred fish the oncogenic function of xmrk is suppressed by the molecularly still unidentified locus R. The xmrk oncogene was generated by a gene duplication event from the Xiphophorus egfrb gene and thereby has acquired a new 5’ regulatory sequence, which has probably altered the transcriptional control of the oncogene. So far, the xmrk promoter region was still poorly characterized and the molecular mechanism by which R controls xmrk-induced melanoma formation in Xiphophorus still remained to be elucidated. To test the hypothesis that R controls melanoma development in Xiphophorus on the transcriptional level, the first aim of the thesis was to gain a deeper insight into the transcriptional regulation of the xmrk oncogene. To this end, a quantitative analysis of xmrk transcript levels in different Xiphophorus genotypes carrying either the highly tumorigenic xmrkB or the non-tumorigenic xmrkA allele was performed. I was able to demonstrate that expression of the tumorigenic xmrkB allele is strongly increased in malignant melanomas of R-free backcross hybrids compared to benign lesions, macromelanophore spots, and healthy skin. The expression level of the non-tumorigenic xmrkA allele, in contrast, is not influenced by the presence or absence of R. These findings strongly indicate that differential transcriptional regulation of the xmrk promoter triggers the tumorigenic potential of these xmrk alleles. To functionally characterize the xmrk promoter region, I established a luciferase assay using BAC clones containing the genomic regions where xmrk and egfrb are located for generation of reporter constructs. This approach showed for the first time a melanoma cell specific transcriptional activation of xmrkB by its flanking regions, thereby providing the first functional evidence that the xmrk oncogene is controlled by a pigment cell specific promoter region. Subsequent analysis of different deletion constructs of the xmrkB BAC reporter construct strongly indicated that the regulatory elements responsible for the tumor-inducing overexpression of xmrkB in melanoma cells are located within 67 kb upstream of the xmrk oncogene. Taken together, these data indicate that melanoma formation in Xiphophorus is regulated by a tight transcriptional control of the xmrk oncogene and that the R locus acts through this mechanism. As the identification of the R-encoded gene(s) is necessary to fully understand how melanoma formation in Xiphophorus is regulated, I furthermore searched for alternative R candidate genes in this study. To this end, three genes, which are located in the genomic region where R has been mapped, were evaluated for their potential to be a crucial constituent of the regulator locus R. Among these genes, I identified pdcd4a, the ortholog of the human tumor suppressor gene PDCD4, as promising new candidate, because this gene showed the expression pattern expected from the crucial tumor suppressor gene encoded at the R locus. N2 - Fische der Gattung Xiphophorus sind ein gut etabliertes Modellsystem zur Analyse der genetischen Grundlagen der Tumorentwicklung. Die Entwicklung hereditärer Melanome in bestimmten interspezifischen Xiphophorus-Hybriden wird durch die pigmentzellspezifische Überexpression des Onkogens xmrk ausgelöst. Dieses Gen codiert für eine durch Mutationen aktivierte Rezeptortyrosinkinase. In den reinerbigen Elterntieren wird die onkogene Funktion von xmrk durch den Regulator-Locus R unterdrückt, welcher jedoch auf molekularer Ebene noch nicht identifiziert wurde. Das Onkogen xmrk ist durch eine Genduplikation aus dem Protoonkogen egfrb entstanden und hat dabei eine neue regulatorische 5‘ Region erhalten, welche mit hoher Wahrscheinlichkeit die transkriptionelle Regulation des Onkogens verändert hat. Die Promotorregion von xmrk war allerdings bisher nur unzureichend charakterisiert und der molekulare Mechanismus, durch den der R-Locus die xmrk-induzierte Melanomentwicklung kontrolliert, war noch weitgehend unbekannt. Um zu analysieren, ob der R-Locus die Melanomentwicklung in Xiphophorus auf transkriptioneller Ebene kontrolliert, war das erste Ziel dieser Arbeit die transkriptionelle Regulation des xmrk Onkogens genauer zu untersuchen. Zu diesem Zweck habe ich eine quantitative Analyse der xmrk Expressionslevel in Geweben verschiedener Xiphophorus-Genotypen durchgeführt, welche entweder das stark tumorigene xmrkB oder das nicht tumorigene xmrkA Allel besitzen. Ich konnte zeigen, dass im Vergleich zu benignen Läsionen, Macromelanophoren und gesunder Haut, die Expression des tumorigenen xmrkB Allels in den malignen Melanomen der R-defizienten Rückkreuzungshybride stark erhöht ist. Das Expressionslevel des xmrkA Allels wird hingegen nicht durch den R-Locus beeinflusst. Dieses Ergebnis deutet darauf hin, dass eine differenzielle transkriptionelle Regulierung des xmrk Promotors für die Unterschiede im onkogenen Potential dieser Allele verantwortlich ist. Um die xmrk Promotorregion funktional zu charakterisieren, habe ich in der hier vorliegenden Studie einen Luciferase-Assay etabliert, für den BAC-Klone, welche die xmrk- oder egfrb-Region enthalten, zur Herstellung von Reporterkonstrukten verwendet wurden. Mit Hilfe dieses Ansatzes konnte ich zum ersten Mal eine melanomzellspezifische Aktivierung des xmrkB Gens durch seine regulatorischen Regionen zeigen. Dies liefert den ersten funktionalen Beweis, dass das xmrk Onkogen tatsächlich durch einen pigmentzellspezifischen Promotor kontrolliert wird. Durch die nachfolgende Analyse einer Deletionsserie des xmrkB Reporterkonstrukts konnte gezeigt werden, dass die regulatorischen Elemente, welche die starke Überexpression von xmrk in Melanomzellen steuern, in den proximalen 67 kb der xmrk 5‘ Region lokalisiert sind. Zusammengefasst deuten diese Ergebnisse darauf hin, dass die Melanomentwicklung in Xiphophorus durch eine strikte transkriptionelle Kontrolle des xmrk Onkogens reguliert wird und dass der Regulator-Locus R seine tumorsuppressive Funktion über diesen Mechanismus ausübt. Da die Identifizierung des R-Locus-Gens entscheidend ist, um die Melanomentwicklung in Xiphophorus vollständig zu verstehen, habe ich im zweiten Teil dieser Arbeit drei Gene, welche in derselben genomischen Region liegen in der R lokalisiert wurde, genauer untersucht, um zu testen, ob es sich bei einem dieser Gene um eine entscheidende tumorsuppressive Komponente des R-Locus handelt. Von diesen Genen wurde pdcd4a, welches das Ortholog zum humanen Tumorsuppressorgen PDCD4 ist, als vielversprechendes neues Kandidatengen identifiziert, da das Expressionsmuster von pdcd4a mit dem zu erwartenden Expressionsmuster des am R-Locus codierten Tumorsuppressorgens übereinstimmt. KW - Melanom KW - Schwertkärpfling KW - Chromatophor KW - Epidermaler Wachstumsfaktor KW - Onkogen KW - Tumorsuppressorgen KW - Hybrid KW - transkriptionelle Regulation KW - melanoma KW - Xiphophorus KW - xmrk KW - transcriptional control KW - pigment cell KW - Hautkrebs KW - Epidermaler Wachstumsfaktor-Rezeptor Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-82319 ER - TY - THES A1 - Rudolf, Ronald T1 - Transcriptional Regulation of and by NFATc1 in Lymphocytes T1 - Transkriptionelle Regulation von und durch NFATc1 in Lymphozyten N2 - The transcription factor NFATc1 has been shown to regulate the activation and differentiation of T-cells and B-cells, of DCs and megakaryocytes. Dysregulation of NFAT signaling was shown to be associated with the generation of autoimmune diseases, malignant transformation and the development of cancer [71]. The primary goal of this work was to gain insights on Nfatc1 induction and regulation in lymphocytes and to find new direct NFATc1 target genes. Three new BAC -transgenic reporter mouse strains (tgNfatc1/Egfp, tgNfatc1/DE1 and tgNfatc1/DE2) were applied to analyze Nfatc1 induction and regulation in primary murine B- and T-cells. As a result, we were able to show the persistent requirement of immunoreceptor-signaling for constant Nfatc1 induction, particularly, for NFATc1/αA expression. Furthermore, we showed that NF-κB inducing agents, such as LPS, CpG or CD40 receptor engagement, in combination with primary receptor-signals, positively contributed to Nfact1 induction in B-cells [137]. We sought to establish a new system which could help to identify direct NFATc1 target genes by means of ChIP and NGS in genom-wide approaches. We were able to successfully generate a new BAC-transgene encoding a biotinylatable short isoform of NFATc1, which is currently injected into mice oocyte at the TFM in Mainz. In addition, in vivo biotinylatable NFATc1–isoforms were cloned and stably expressed in the murine B-cell lymphoma line WEHI-231. The successful use of these cells stably overexpressing either the short NFATc1/αA or the long NFATc1/βC isoform along with the bacterial BirA biotin ligase was confirmed by intracellular stainings, FACS analysis, confocal microscopy and protein IP. By NGS, we detected 2185 genes which are specifically controlled by NFATc1/αA, and 1306 genes which are exclusively controlled by NFATc1/βC. This shows that the Nfatc1 locus encodes “two genes” which exhibit alternate, in part opposite functions. Studies on the induction of apoptosis and cell-death revealed opposed roles for the highly inducible short isoform NFATc1/αA and the constantly expressed long isoform NFATc1/βC. These findings were confirmed by whole transcriptome-sequencing performed with cells overexpressing NFATc1/αA and NFATc1/βC. Several thousand genes were found to be significantly altered in their expression profile, preferentially genes involved in apoptosis and PCD for NFATc1/βC or genes involved in transcriptional regulation and cell-cycle processes for NFATc1/αA. In addition we were able to perform ChIP-seq for NFATc1/αA and NFATc1/βC in an ab-independent approach. We found potential new target-sites, but further studies will have to address this ambitious goal in the future. In individual ChIP assays, we showed direct binding of NFATc1/αA and NFATc1/βC to the Prdm1 and Aicda promoter regions which are individually controlled by the NFATc1 isoforms. N2 - Der Transkriptionsfaktor NFATc1 wurde als Regulator der Aktivierung und Differenzierung für T-Zellen, B-Zellen, Dendritische-Zellen und Megakaryozyten beschrieben. Autoimmunerkrankungen und die Entstehung von Krebs wurden mit Fehlregulationen der NFAT-Signalwege in Verbindung gebracht [71]. Ziel dieser Arbeit war der Gewinn neuer Erkenntnisse über die Induktion und Regulation von NFATc1 in Lymphozyten. Darüber hinaus sollten Gene, welche direkt durch NFATc1 gebunden und reguliert werden, identifiziert werden. Um die Induktion und Regulation von NFATc1 in primären T- und B-Zellen untersuchen zu können, wurden drei BAC transgene Reporter Maus Linien (tgNfatc1/Egfp, tgNfatc1/DE1 and tgNfatc1/DE2) verwendet. Dadurch war es uns möglich zu zeigen, dass es einer ununterbrochenen Antigen-Rezeptor Stimulation bedarf, um NFATc1, im Besonderen die Transkription der kurzen Isoform NFATc1/αA, dauerhaft zu induzieren. Zusätzlich konnten wir zeigen, dass Induktoren wie LPS, CpG oder auch die Stimulation des CD40-Rezeptors, die die Expression des Transkriptionsfaktors NF-B zur Folge haben, einen positiven Einfluss auf die Nfatc1-Induktion haben [137]. Unser Interesse lag darin, ein System zu etablieren, dass es uns ermöglichen sollte, neue NFATc1-Zielgene durch ChIP assays und Genom-weite Sequenzierungen zu ermitteln. Es ist uns gelungen, ein neues BAC-Transgen, welches für eine in vivo biotinylierbare Variante des NFATc1/αA Proteins kodiert, zu erzeugen. Dieses Konstrukt wird zum gegenwärtigen Zeitpunkt - in Zusammenarbeit mit der Universität Mainz (TFM) - in die Vorkerne von Maus-Eizellen injiziert. Ferner wurden biotinylierbare NFATc1-Isoformen kloniert und mit Hilfe retroviraler Plasmide stabil in WEHI-231 B-Lymphom-Zellen integriert. Durch intrazellulare Färbungen, FACS-Analysen, Konfokalmikroskopie und Immunpräzipitationen konnten wir eine erfolgreiche in vivo Biotinylierung in NFATc1/αA- und NFATc1/βC-exprimierenden WEHI-231 Zellen nachweisen. Mittels Next-Generation-Sequencing, in Kollaboration mit TRON, Univ. Mainz, konnten wir 2185 Gene, die spezifisch durch NFATc1/αA kontrolliert wurden, und 1306 Gene, die ausschließlich durch die Überexpression von NFATc1/βC reguliert wurden, identifizieren. Diese Ergebnisse zeigen, dass im Nfatc1 Locus „zwei Gene“ mit alternativer, zum Teil gegensätzlicher Funktion, kodiert sind. Untersuchungen zu Apoptose und Zelltod haben entgegengesetzte Eigenschaften der stark induzierbaren, kurzen Isoform NFATc1/αA und der stetig exprimierten langen Isoform NFATc1/βC aufgezeigt. Daten von Sequenzierungen des gesamten Transkriptoms, die mit NFATc1/αA und -βC überexprimierenden WEHI-231 Zellen durchgeführt wurden (TRON, Mainz), bestätigten diese Befunde. Es zeigte sich, dass es wesentliche Veränderungen der Expressionsprofile Tausender von Genen gab. In WEHI-231-Zellen, die NFATc1/βC überexprimierten, waren viele dieser Gene an Apoptose und Zelltod beteiligt. Demgegenüber waren in NFATc1/αA-Zellen vor allem Gene betroffen, die an transkriptionaler Regulation und dem Zellzyklus beteiligt waren. Überdies war es uns möglich, ChIPseq Assays für NFATc1/αA und NFATc1/βC in einem Antikörper-unabhängigen Ansatz durchzuführen. Dadurch konnten wir neue NFATc1-Bindungstellen identifizieren. Es bedarf jedoch noch weiterer Untersuchungen, um diese Ergebnisse der Genom-weiten ChIPseq Assays zu bestätigen. Durch weitere ChIP Experimente konnten wir eine direkte Bindung von NFATc1/αA und NFATc1/βC an die regulatorischen Regionen der Prdm1- und Aicda-Gene nachweisen. Die Transkription beider Gene wurde durch die Überexpression von NFATc1/αA und -βC deutlich reguliert und spielt offenbar bei der Bildung von Plasma-B-Zellen, die für die Antikörper-Produktion verantwortlich sind, eine wesentliche Rolle. KW - Lymphozyt KW - Transkriptionsfaktor KW - Lymphozyten KW - NFATc1 KW - Lymphocytes KW - NFATc1 KW - Genregulation KW - Maus Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-83993 ER - TY - THES A1 - Kullmann, Martin Armin T1 - Tracing Excited-State Photochemistry by Multidimensional Electronic Spectroscopy T1 - Auflösung der Photochemie von angeregten Zuständen mittels multidimensionaler elektronischer Spektroskopie N2 - Light-induced excitation of matter proceeds within femtoseconds, resulting in excited states. Originating from these states chemical reaction mechanisms, like isomerization or bond formation, set in. Photophysical mechanisms like energy distribution and excitonic delocalization also occur. Thus, the reaction scheme has to be disentangled by assessing the importance of each process. Spectroscopic methods based on fs laser pulses have emerged as a versatile tool to study these reactions. Within this thesis time-resolved experiments with fs laser pulses on various molecular systems were performed. Novel photosystems, with possible applications ranging from ultrathin molecular wires to molecular switches, were extensively characterized. To resolve the complex kinetics of the investigated systems, time-resolved techniques had to be newly developed. By combining a visible excitation pulse pair with an additional pulse and a continuum probe electronic triggered-exchange two-dimensional spectroscopy (TE2D) was demonstrated for the first time. This goal was accomplished by combining a three-color transient-absorption setup with a pulse shaper. Hence, 2D spectroscopy with a continuum probe was also implemented. Using these methods two different molecular systems in solution were characterized in a comprehensive manner. (ZnTPP)2, a directly beta,beta’-linked Zn-metallated bisporphyrin, and a spiropyran-merocyanine photosystem, 6,8-dinitro BIPS, were characterized. (ZnTPP)2 is a homodimer, featuring strong excitonic effects. These manifest themselves in a twofold splitting of the Soret band (S2). 6,8-Dinitro BIPS exists in one of two possible conformations. The ring closed spiropyran absorbs only in the UV, while the ring open merocyanine also absorbs in the visible. For both molecular systems photodynamics upon illumination were monitored using transient-absorption. However, the obtained results were ambiguous, necessitating more complex methods. In the case of (ZnTPP)2 first the monomeric building block was characterized. There, population transfer from the S2 state into S1 within 2 ps was identified. Afterwards, intersystem crossing proceeds within 2 ns. For (ZnTPP)2 similar pathways were found, albeit the relaxation is faster. The intersystem crossing with 1.5 ns was not only indirectly deduced but directly measured by probing in the NIR spectral range. The excitonic influence of was investigated by coherent 2D spectroscopy in the Soret band. Population transfer within S2 was directly visualized on a time-scale of 100 fs. Calculation of the 2D spectra of a simple homodimer confirmed the results. After this analysis of the distinct excitonic character, this molecule may serve as a building block for larger porphyrin arrays with applications ranging from asymmetric catalysis over biomimicry of electron-transfer to organic optical devices. The second photosystem was the molecular switch 6,8-dinitro BIPS, existing in two conformations. Merocyanine is the more stable form in thermal equilibrium. Transient-absorption measurements uncovered that the sample consisted of a mixture of two merocyanine isomers, referred to as TTC and TTT. However, both isomers are capable of ring-closure forming spiropyran. The remaining excited molecules return to the ground state radiatively. Conducting 2D measurements utilizing a continuum probe the differing photochemistry of both isomers was examined in a single measurement. No isomerization between these conformations was detected. Therefore, 6,8-dinitro BIPS performs a concerted switching without long-living intermediates. This was confirmed by a pump-repump-probe scan. 6,8-DinitroBIPS can be closed by visible and opened by UV pulses using subsequent pulses and vice versa. These mechanisms via singlet pathways satisfy an important criterion for a unimolecular switching device. A second pump-repump-probe experiment showed that the sample is ionized, resulting in a merocyanine radical cation, when the first excited state is resonantly excited. Furthermore, by implementing TE2Dspectroscopy, it was elucidated that only TTC was ionized. Taking all this into account new techniques were developed and complex molecular systems were characterized within this thesis. Deeper insight into the photodynamics of (ZnTPP)2and 6,8-dinitro BIPS was gained by adapting transient absorption for the NIR spectral range, constructing a 2D setup in pump-probe geometry, and combining it with multipulse excitation to coherent TE2D. All techniques solved the questions for which they were constructed, but they are not limited to these cases. Especially TE2D opens new roads in photochemistry. By connecting reactant, product and the corresponding intermediates, a chemical reaction can be tracked through all stages, making unambiguous identification of the reactive states feasible. Thus, fundamental insight into the photochemistry of molecular compounds is gained. N2 - Über Lichtanregung erreichen Moleküle innerhalb von Femtosekunden angeregte Zustände. Aus diesen können photochemische Reaktionen wie Isomerisierungen einsetzen. Zusätzlich treten photophysikalische Effekte wie exzitonische Delokalisierungen auf. Daher ist es wichtig, die auftretenden Relaxationspfade zu analysieren um das Reaktionsschema des Systems zu erhalten. Ultrakurzzeitspektroskopie mit Femtosekundenlaserpulsen hat sich als nützliches Werkzeug erwiesen um lichtinduzierte Reaktionen auf ihrer intrinsischen Zeitskala zu studieren. In dieser Arbeit sind zeitaufgelöste Experimente an unterschiedlichen Verbindungen durchgeführt worden. Einerseits wurden neuartige Molekülklassen umfassend photodynamisch untersucht. Andererseits sind neue breitbandige Spektroskopiemethoden entwickelt worden. Durch die Kombination eines Anregungspulspaars mit einem weiteren Laserpuls sowie einem Weißlichtkontinuum wurde zum ersten Mal elektronische zweidimensionale Spektroskopie mit ausgelöster Umwandlung ("triggered-exchange 2D“, TE2D) demonstriert. Dies war durch die Implementierung eines Pulsformers in ein transientes Absorptionsspektrometer möglich. In einem ersten Experiment wurde die prinzipielle Eignung des Aufbaus getestet indem 2D Spektroskopie mit Weißlichtabfrage implementiert wurde. Diese Methoden wurden dazu genutzt zwei verschiedene Verbindungen zu untersuchen, ein direkt beta,beta'-verknüpftes, Zn-metalliertes Bisporphyrin [(ZnTPP)2] und ein Spiropyran-Merocyanin Photoschalter (6,8-dinitro BIPS). (ZnTPP)2 ist ein Homodimer, in welchem sich starke exzitonische Einflüsse, z. B. das Aufspalten der Soret-Bande (S2), zeigen. 6,8-Dinitro BIPS hingegen besteht aus zwei Konformeren. Zum einen liegt das nur im UV absorbierende Spiropyran vor. Das zweite Konformer ist Merocyanin, welches zusätzlich im sichtbaren absorbiert. Zuerst sind die Relaxationsdynamiken beider Moleküle mittels transienter Absorption untersucht worden. Allerdings waren die Resultate nicht eindeutig, so dass im Anschluss komplexere Messmethoden angewandt wurden. Für das Studium des Bisporphyrins (ZnTPP)2 wurde das zugehörige Monomer untersucht. Nach Anregung relaxiert die Population aus dem S2 in den S1 Zustand. Anschließend tritt Intersystem Crossing in T1 ein. Für das Dimer selbst ergaben sich die gleichen Reaktionswege. Das Intersystem Crossing wurde nicht nur abgeleitet, sondern durch Abfrage im nahinfraroten Spektralbereich direkt gemessen. Der Einfluss der Exzitonen auf das Bisporphyrin wurde durch kohärente 2D Spektroskopie innerhalb der Soret-Bande untersucht. Dies ermöglichte die Visualisierung von Populationstransfer innerhalb von 100 fs. Eine Berechnung der 2D Spektren eines einfachen Homodimers unterstützt dieses Resultat. Indem die hier vorgestellten Ergebnisse genutzt werden, könnte (ZnTPP)2 als Baustein für Porphyrinsysteme dienen. Deren denkbare Anwendungen reichen von asymmetrischer Katalyse über die Nachahmung von biologischem Elektronentransfer hinzu organo-optischen Geräten. Das zweite untersuchte System war der molekulare Schalter 6,8-dinitro BIPS mit Merocyanin als stabile Form im thermischen Gleichgewicht. Transiente Absorptionsmessungen deckten auf, dass die Lösung aus zwei Merocyanin-Isomeren besteht (TTC oder TTT). Es ergab sich ebenso, dass beide eine elektrozyklische Ringschlussreaktion zum Spiropyran durchführen. Mittels eines 2D Spektrums konnte die unterschiedliche Photochemie beider Isomere innerhalb einer einzigen Messung aufgezeigt werden. Zusätzlich wurde keine Isomerisierung zwischen ihnen beobachtet. Damit steht fest, dass 6,8-dinitro BIPS eine konzertierte Reaktion zum Spiropyran durchführt. Der direkte Schaltvorgang wurde eindeutig über Anrege-Wiederanrege-Abfrage Spektroskopie nachgewiesen. Hierfür wurde 6,8-dinitro BIPS mit sichtbarem gefolgt von ultraviolettem Licht bestrahlt. Der resultierende zweifache Schaltvorgang ist ein wichtiges Kriterium für einen Photoschalter. Ein ähnliches Experiment zeigte, dass 6,8-dinitro BIPS ionisiert wird, wenn die angeregte Population resonant bestrahlt wird. Das neugebildete langlebige Produkt konnte einem Kation zugeordnet werden. Durch die Verwendung der neuen elektronischen TE2D Methode ist aufgezeigt worden, dass lediglich TTC ionisiert werden kann. Zusammengefasst gilt, dass sowohl Fortschritte in der Methodenentwicklung als auch in der Charakterisierung von Verbindungen erzielt wurden. Ein tieferes Verständnis über die Dynamiken des Bisporphyrins (ZnTPP)2 und des molekularen Schalters 6,8-dinitro BIPS wurden durch Erweiterungen an einem transienten Absorptionsspektrometers, den Aufbau eines 2D Spektrometers in Anrege-Abfrage-Geometrie und durch die Kombination von letzterem mit Mehrfachanregung zu TE2D Spektroskopie gewonnen. Insbesondere letztere eröffnet neue Möglichkeiten in der Photochemie, da Edukte, Produkte und die zugehörigen Zwischenzustände miteinander verknüpft werden, wodurch lichtinduzierte Reaktionen schrittweise nachvollzogen werden können. KW - Femtosekundenspektroskopie KW - Fotochemie KW - Angeregter Zustand KW - Elektronenspektroskopie KW - femtosecond spectroscopy KW - pericyclic reaction KW - porphyrin KW - merocyanine KW - optical spectroscopy KW - Pericyclische Reaktion KW - Porphyrin KW - Photonenecho KW - Optische Spektroskopie KW - Merocyanine Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-81276 ER - TY - JOUR A1 - Holubyev, Konstyantyn A1 - Bratengeier, Klaus A1 - Gainey, Mark A1 - Polat, Bülent A1 - Flentje, Michael T1 - Towards automated on-line adaptation of 2-Step IMRT plans: QUASIMODO phantom and prostate cancer cases JF - Radiation Oncology N2 - Background The standard clinical protocol of image-guided IMRT for prostate carcinoma introduces isocenter relocation to restore the conformity of the multi-leaf collimator (MLC) segments to the target as seen in the cone-beam CT on the day of treatment. The large interfractional deformations of the clinical target volume (CTV) still require introduction of safety margins which leads to undesirably high rectum toxicity. Here we present further results from the 2-Step IMRT method which generates adaptable prostate IMRT plans using Beam Eye View (BEV) and 3D information. Methods Intermediate/high-risk prostate carcinoma cases are treated using Simultaneous Integrated Boost at the Universitätsklinkum Würzburg (UKW). Based on the planning CT a CTV is defined as the prostate and the base of seminal vesicles. The CTV is expanded by 10 mm resulting in the PTV; the posterior margin is limited to 7 mm. The Boost is obtained by expanding the CTV by 5 mm, overlap with rectum is not allowed. Prescription doses to PTV and Boost are 60.1 and 74 Gy respectively given in 33 fractions. We analyse the geometry of the structures of interest (SOIs): PTV, Boost, and rectum, and generate 2-Step IMRT plans to deliver three fluence steps: conformal to the target SOIs (S0), sparing the rectum (S1), and narrow segments compensating the underdosage in the target SOIs due to the rectum sparing (S2). The width of S2 segments is calculated for every MLC leaf pair based on the target and rectum geometry in the corresponding CT layer to have best target coverage. The resulting segments are then fed into the DMPO optimizer of the Pinnacle treatment planning system for weight optimization and fine-tuning of the form, prior to final dose calculation using the collapsed cone algorithm. We adapt 2-Step IMRT plans to changed geometry whilst simultaneously preserving the number of initially planned Monitor Units (MU). The adaptation adds three further steps to the previous isocenter relocation: 1) 2-Step generation for the geometry of the day using the relocated isocenter, MU transfer from the planning geometry; 2) Adaptation of the widths of S2 segments to the geometry of the day; 3) Imitation of DMPO fine-tuning for the geometry of the day. Results and conclusion We have performed automated 2-Step IMRT adaptation for ten prostate adaptation cases. The adapted plans show statistically significant improvement of the target coverage and of the rectum sparing compared to those plans in which only the isocenter is relocated. The 2-Step IMRT method may become a core of the automated adaptive radiation therapy system at our department. KW - Prostate carcinoma KW - IMRT KW - IGRT KW - Adaptation Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96818 UR - http://www.ro-journal.com/content/8/1/263 ER - TY - JOUR A1 - Assaad, F. F. A1 - Bercx, M. A1 - Hohenadler, M. T1 - Topological Invariant and Quantum Spin Models from Magnetic pi Fluxes in Correlated Topological Insulators JF - Physical Review X N2 - The adiabatic insertion of a \(\pi\) flux into a quantum spin Hall insulator gives rise to localized spin and charge fluxon states. We demonstrate that \(\pi\) fluxes can be used in exact quantum Monte Carlo simulations to identify a correlated \(Z_2\) topological insulator using the example of the Kane-Mele-Hubbard model. In the presence of repulsive interactions, a \(\pi\) flux gives rise to a Kramers doublet of spin-fluxon states with a Curie-law signature in the magnetic susceptibility. Electronic correlations also provide a bosonic mode of magnetic excitons with tunable energy that act as exchange particles and mediate a dynamical interaction of adjustable range and strength between spin fluxons. \(\pi\) fluxes can therefore be used to build models of interacting spins. This idea is applied to a three-spin ring and to one-dimensional spin chains. Because of the freedom to create almost arbitrary spin lattices, correlated topological insulators with \(\pi\) fluxes represent a novel kind of quantum simulator, potentially useful for numerical simulations and experiments. KW - topological insulators KW - strongly correlated materials Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129849 VL - 3 IS - 1 ER - TY - JOUR A1 - Kato, Hiroki A1 - Lu, Qiping A1 - Rapaport, Doron A1 - Kozjak-Pavlovic, Vera T1 - Tom70 Is Essential for PINK1 Import into Mitochondria JF - PLoS ONE N2 - PTEN induced kinase 1 (PINK1) is a serine/threonine kinase in the outer membrane of mitochondria (OMM), and known as a responsible gene of Parkinson's disease (PD). The precursor of PINK1 is synthesized in the cytosol and then imported into the mitochondria via the translocase of the OMM (TOM) complex. However, a large part of PINK1 import mechanism remains unclear. In this study, we examined using cell-free system the mechanism by which PINK1 is targeted to and assembled into mitochondria. Surprisingly, the main component of the import channel, Tom40 was not necessary for PINK1 import. Furthermore, we revealed that the import receptor Tom70 is essential for PINK1 import. In addition, we observed that although PINK1 has predicted mitochondrial targeting signal, it was not processed by the mitochondrial processing peptidase. Thus, our results suggest that PINK1 is imported into mitochondria by a unique pathway that is independent of the TOM core complex but crucially depends on the import receptor Tom70. KW - binding KW - outer-membrane proteins KW - Parkinsons diesease KW - intracellular membranes KW - quality control KW - pathway KW - recruitment KW - biogenesis KW - mechanisms KW - complex Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131061 VL - 8 IS - 3 ER - TY - JOUR A1 - Moll, Corinna A1 - Reboredo, Jenny A1 - Schwarz, Thomas A1 - Appelt, Antje A1 - Schürlein, Sebastian A1 - Walles, Heike A1 - Nietzer, Sarah T1 - Tissue Engineering of a Human 3D in vitro Tumor Test System JF - Journal of Visualized Experiments N2 - Cancer is one of the leading causes of death worldwide. Current therapeutic strategies are predominantly developed in 2D culture systems, which inadequately reflect physiological conditions in vivo. Biological 3D matrices provide cells an environment in which cells can self-organize, allowing the study of tissue organization and cell differentiation. Such scaffolds can be seeded with a mixture of different cell types to study direct 3D cell-cell-interactions. To mimic the 3D complexity of cancer tumors, our group has developed a 3D in vitro tumor test system. Our 3D tissue test system models the in vivo situation of malignant peripheral nerve sheath tumors (MPNSTs), which we established with our decellularized porcine jejunal segment derived biological vascularized scaffold (BioVaSc). In our model, we reseeded a modified BioVaSc matrix with primary fibroblasts, microvascular endothelial cells (mvECs) and the S462 tumor cell line For static culture, the vascular structure of the BioVaSc is removed and the remaining scaffold is cut open on one side (Small Intestinal Submucosa SIS-Muc). The resulting matrix is then fixed between two metal rings (cell crowns). Another option is to culture the cell-seeded SIS-Muc in a flow bioreactor system that exposes the cells to shear stress. Here, the bioreactor is connected to a peristaltic pump in a self-constructed incubator. A computer regulates the arterial oxygen and nutrient supply via parameters such as blood pressure, temperature, and flow rate. This setup allows for a dynamic culture with either pressure-regulated pulsatile or constant flow. In this study, we could successfully establish both a static and dynamic 3D culture system for MPNSTs. The ability to model cancer tumors in a more natural 3D environment will enable the discovery, testing, and validation of future pharmaceuticals in a human-like model. KW - bioengineering KW - biomedical engineering KW - tissue engineering KW - biotechnology KW - cultured KW - tumor cells KW - cell culture KW - 3D in vitro models KW - bioreactor KW - dynamic culture conditions KW - tumor test system KW - primary cell isolation KW - BioVaSc KW - decellularization KW - equipment and supplies KW - cellular microenvironment KW - culture techniques KW - cell engineering KW - anatomy KW - physiology KW - molecular biology KW - cellular biology Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132277 UR - http://www.jove.com/video/50460 VL - 78 IS - e50460 ER - TY - JOUR A1 - Falge, M. A1 - Engel, V. A1 - Gräfe, S. T1 - Time-resolved photoelectron spectroscopy of coupled nuclear-electronic dynamics JF - EPJ Web of Conferences N2 - We study the effect of nuclear-electron coupling on time-resolved photo-electron spectra, employing a model system which allows to directly comparing spectra resulting from the adiabatic approximation with those obtained within a non-Born-Oppenheimer description. Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-121812 SN - 2100-014X VL - 41 ER - TY - JOUR A1 - Meule, Adrian A1 - Kübler, Andrea A1 - Blechert, Jens T1 - Time course of electrocortical food-cue responses during cognitive regulation of craving JF - Frontiers in Psychology N2 - In our current obesogenic environment, exposure to visual food-cues can easily lead to craving and overeating because short-term, pleasurable effects of food intake dominate over the anticipated long-term adverse effects such as weight gain and associated health problems. Here we contrasted these two conditions during food-cue presentation while acquiring event-related potentials (ERPs) and subjective craving ratings. Female participants (n = 25) were presented with either high-calorie (HC) or low-calorie (LC) food images under instructions to imagine either immediate (NOW) or long-term effects (LATER) of consumption. On subjective ratings for HC foods, the LATER perspective reduced cravings as compared to the NOW perspective. For LC foods, by contrast, craving increased under the LATER perspective. Early ERPs (occipital N1, 150-200 ms) were sensitive to food type but not to perspective. Late ERPs (late positive potential, LPP, 350-550 ms) were larger in the HC-LATER condition than in all other conditions, possibly indicating that a cognitive focus on negative long-term consequences induced negative arousal. This enhancement for HC-LATER attenuated to the level of the LC conditions during the later slow wave (550-3000 ms), but amplitude in the HC-NOW condition was larger than in all other conditions, possibly due to a delayed appetitive response. Across all conditions, LPP amplitudes were positively correlated with self-reported emotional eating. In sum, results reveal that regulation effects are secondary to an early attentional analysis of food type and dynamically evolve over time. Adopting a long-term perspective on eating might promote a healthier food choice across a range of food types. KW - EEG KW - disorder examination questionnaire KW - eating disorder KW - emotion regulation KW - future directions KW - attention KW - brain KW - high-calorie KW - german version KW - bulimia nervosa KW - chocolate images KW - event-related potentials KW - eating KW - calorie content KW - food-cues KW - food craving KW - LPP KW - slow wave Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122566 SN - 1664-1078 VL - 4 IS - 669 ER - TY - JOUR A1 - Luxenhofer, Robert A1 - Fetsch, Corinna T1 - Thermal Properties of Aliphatic Polypeptoids JF - Polymers N2 - A series of polypeptoid homopolymers bearing short (C1–C5) side chains of degrees of polymerization of 10–100 are studied with respect to thermal stability, glass transition and melting points. Thermogravimetric analysis of polypeptoids suggests stability to >200 °C. The study of the glass transition temperatures by differential scanning calorimetry revealed two dependencies. On the one hand an extension of the side chain by constant degree of polymerization decrease the glass transition temperatures (Tg) and on the other hand a raise of the degree of polymerization by constant side chain length leads to an increase of the Tg to a constant value. Melting points were observed for polypeptoids with a side chain comprising not less than three methyl carbon atoms. X-ray diffraction of polysarcosine and poly(N-ethylglycine) corroborates the observed lack of melting points and thus, their amorphous nature. Diffractograms of the other investigated polypeptoids imply that crystalline domains exist in the polymer powder. KW - peptoid KW - biomaterials KW - glass transition temperature KW - DSC KW - TGA KW - XRD Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96333 ER - TY - JOUR A1 - Gross, Hans J. A1 - Samhita, Laasya T1 - The “Clever Hans Phenomenon” revisited N2 - In the first decade of the 20th century, a horse named Hans drew worldwide attention in Berlin as the first and most famous “speaking” and thinking animal. Hans solved calculations by tapping numbers or letters with his hoof in order to answer questions. Later on, it turned out that the horse was able to give the correct answer by reading the microscopic signals in the face of the questioning person. This observation caused a revolution and as a consequence, experimenters avoided strictly any face-to-face contact in studies about cognitive abilities of animals—a fundamental lesson that is still not applied rigorously. KW - Clever Hans Phenomenon Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-112626 ER - TY - JOUR A1 - Mussel, Patrick A1 - Göritz, Anja S. A1 - Hewig, Johannes T1 - The value of a smile: Facial expression affects ultimatum-game responses JF - Judgment and Decision Making N2 - In social interaction, the facial expression of an opponent contains information that may influence the interaction. We asked whether facial expression affects decision-making in the ultimatum game. In this two-person game, the proposer divides a sum of money into two parts, one for each player, and then the responder decides whether to accept the offer or reject it. Rejection means that neither player gets any money. Results of a large-sample study support our hypothesis that offers from proposers with a smiling facial expression are more often accepted, compared to a neutral facial expression. Moreover, we found lower acceptance rates for offers from proposers with an angry facial expression. KW - ultimatum game KW - emotions KW - decision-making KW - facial expressions Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129639 VL - 8 IS - 3 ER - TY - THES A1 - Onyenali, Rowland T1 - The Trilogy of Parables in Mt 21:28-22:14 from a Matthean Perspective T1 - Die Gleichnistrilogie im Mt 21,28-22,14 im Kontext des Mt-Evangeliums N2 - The parables of Jesus have undergone different transmutations in the long history of their transmission. The events surrounding his death and resurrection as well as the new situations his followers were confronted with after these events, led to the parables being given new accentuation according to the needs of the reflecting community. This is evident in Matthew's treatment of the parable trilogy of Mt 21:28-22:14. The work tries to show how Matthew has used the dominical parables and sayings found in his tradition to serve the needs of his community, especially in her struggles with the official Jewish leaders of his time. Through these parables, which he presented as a three-pronged attack against the Jewish leaders, he shows his community as the true Israel, called to produce the fruits of righteousness. N2 - Die Gleichnisse Jesu haben verschiedene Wandlungen in der langen Geschichte ihrer Überlieferung unterzogen. Die Ereignisse rund um seinen Tod und seine Auferstehung sowie die neuen Situationen, mit denen seine Jünger nach diesen Ereignissen konfrontiert wurden, führte dazu, dass die Gleichnisse neue Akzentuierung bekammen. Dies ist evident von der Gleichnistrilogie im Matthäus Mt 21,28-22,14. Die Arbeit versucht zu zeigen, wie Matthäus die Jesuanische Gleichnisse und Sprüche, die er in seiner Tradition gefunden hat verwendet, um die Bedürfnisse seiner Gemeinde zu dienen, besonders in den Ausseinandersetzungen mit den jüdischen Autoritäten seiner Zeit. Durch diesen Gleichnissen, die er als einen dreifachen Angriff gegen den jüdischen Autoritäten umdeutet, zeigt er seine Gemeinde als das wahre Israel, aufgerufen, um die Früchte der Gerechtigkeit zu bringen. KW - Matthäusevangelium 21 KW - 28-22 KW - 14 KW - Matthew KW - Parables KW - Jewish leaders Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-74971 ER - TY - THES A1 - Wetzel, Andrea T1 - The role of TrkB and NaV1.9 in activity-dependent axon growth in motoneurons T1 - Die Rolle von TrkB und NaV1.9 in aktivitätsabhängigem Axonwachstum von Motoneuronen N2 - Während der Entwicklung des Nervensystems lassen sich bei Motoneuronen aktivitätsabhängige Kalziumströme eobachten, die das Axonwachstum regulieren. Diese Form der neuronalen Spontanaktivität sowie das Auswachsen von Axonen sind bei Motoneuronen, die aus Tiermodellen der Spinalen Muskelatrophie isoliert werden, gestört. Experimente aus unserer Arbeitsgruppe haben gezeigt, dass spontane Erregbarkeit und aktivitätsabhängiges Axonwachstum von kultivierten Motoneuronen auch unter Verwendung von Toxinen beeinträchtigt sind, welche die Aktivität von spannungsabhängigen Natriumkanälen blockieren. In diesen Versuchen war die Wirkung von Saxitoxin effizienter als die Wirkung von Tetrodotoxin. Wir identifizierten den Saxitoxin-sensitiven/Tetrodotoxin-insensitiven spannungsabhängigen Natriumkanal NaV1.9 als Trigger für das Öffnen spannungsabhängiger Kalziumkanäle. Die Expression von NaV1.9 in Motoneuronen konnte über quantitative RT-PCR nachgewiesen werden und antikörperfärbungen offenbarten eine Anreicherung des Kanals im axonalen Wachstumskegel sowie an Ranvier'schen Schnürringen von isolierten Nervenfasern wildtypischer Mäuse. Motoneurone von NaV1.9 knock-out Mäusen zeigen reduzierte Spontanaktivität und eine Reduktion des Axonwachstums, welche durch NaV1.9 Überexpression normalisiert werden kann. In Motoneuronen von Smn-defizienten Mäusen konnte keine Abweichung der NaV1.9 Proteinverteilung nachgewiesen werden. Kürzlich wurden Patienten identifiziert, die eine missense-Mutation im NaV1.9 kodierenden SCN11A Gen tragen. Diese Patienten können keinerlei Schmerz empfinden und leiden zudem an Muskelschwäche in Kombination mit einer verzögerten motorischen Entwicklung. Im Rahmen dieser Doktorarbeit konnten molekularbiologische Untersuchungen an Mäusen, welche die Mutation im orthologen Scn11a Gen tragen, zur Aufklärung des Krankheitsmechanismus beitragen. Die Kooperationsstudie zeigte, dass eine gesteigerte Funktion von NaV1.9 diese spezifische Kanalerkrankung auslöst, was die Wichtigkeit von NaV1.9 in menschlichen Motoneuronen unterstreicht. Eine frühere Studie beschrieb an hippocampalen Neuronen, dass die Rezeptortyrosinkinase tropomyosin receptor kinase B (TrkB) den NaV1.9 Kanal öffnen kann. Im Wachstumskegel von Motoneuronen ist TrkB nachweisbar und folglich in räumlicher Nähe zu NaV1.9 zu finden. Um zu prüfen, ob TrkB in die spontane Erregbarkeit von Motoneuronen involviert ist, wurden TrkB knock-out Mäuse untersucht. Isolierte Motoneurone von TrkB knock-out Mäusen weisen eine Reduktion der Spontanaktivität und eine Verringerung des Axonwachstums auf. Ob TrkB und NaV1.9 hierbei funktionell gekoppelt sind, ist Gegenstand künftiger Forschung. N2 - During development of the nervous system, spontaneous Ca2+ transients are observed that regulate the axon growth of motoneurons. This form of spontaneous neuronal activity is reduced in motoneurons from a mouse model of spinal muscular atrophy and this defect correlates with reduced axon elongation. Experiments from our group demonstrated that voltage-gated sodium channel pore blockers decrease spontaneous neuronal activity and axon growth in cultured motoneurons, too. In these experiments, saxitoxin was more potent than tetrodotoxin. We identified the saxitoxin-sensitive/tetrodotoxin-insensitive voltage-gated sodium channel NaV1.9 as trigger for the opening of voltage-gated calcium channels. In motoneurons, expression of NaV1.9 was verified via quantitative RT-PCR. Immuno labelling experiments revealed enrichment of the channel in axonal growth cones and at the nodes of Ranvier of isolated nerve fibres from wild type mice. Motoneurons from NaV1.9 knock-out mice show decreased spontaneous activity and reduced axonal elongation. This growth defect can be rescued by NaV1.9 overexpression. In motoneurons from Smn-deficient mice, NaV1.9 distribution appeared to be normal. Recently, patients carrying a missense mutation in the NaV1.9-encoding gene SCN11A were identified. These patients are not able to feel pain and suffer from muscular weakness and a delayed motor development. Molecular biological work during this dissertation supported the analysis of this mutation in a mouse model carrying the orthologous alteration in the Scn11a locus. The cooperation study confirmed that a gain-of-function mechanism underlies the NaV1.9-mediated channelopathy, thus suggesting a functional role of NaV1.9 in human motoneurons. An earlier study showed in hippocampal neurons that the receptor tyrosine kinase tropomyosin receptor kinase B (TrkB) can open the NaV1.9 channel. TrkB is localized in growth cones of motoneurons and subsequently found in close proximity to NaV1.9. In order to proof whether TrkB is involved in spontaneous excitability in motoneurons, TrkB knock-out mice were analysed. Isolated motoneurons from TrkB knock-out mice show a reduced spontaneous activity and axon elongation. It remains to be studied whether TrkB and NaV1.9 are functionally connected. KW - Motoneuron KW - Neurotrophic factors KW - NaV1.9 KW - motoneuron KW - spontaneous neuronal activity KW - Axon KW - Wachstum KW - Natriumkanal KW - TrkB Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-92877 ER - TY - THES A1 - Link, Jana T1 - The role of meiotic nuclear envelope components in chromosome dynamics and meiotic progression T1 - Die Rolle meiotischer Kernhüllenkomponenten für Chromosomendynamiken und den meiotischen Ablauf N2 - Meiosis is the specialised cell division which produces haploid germ cells, capable of developing into fertile gametes, from diploid progenitor cells. During meiosis, chromosomes undergo strictly regulated and strongly conserved dynamic processes, at the beginning of which the telomeres are actively tethered and intimately attached to the nuclear envelope (NE). The attached telomeres are then moved within the NE through cytoskeletal forces to cluster within a restricted region, forming the highly conserved bouquet stage. Subsequently, the bouquet is released simultaneously to the completion of the synaptonemal complex assembly tightly linking homologous chromosome pairs together. In combination these processes are essential for the successful completion of meiosis. Because the meiotic NE serves as a platform for telomere attachment and movement it can be assumed to be critically involved in these events crucial for fertility. However, the precise roles of many meiotic NE proteins in the attachment and movement of telomeres still remain elusive. Therefore, it was the aim of this thesis to investigate the functions of two mammalian meiotic NE components in telomere attachment and dynamics. The first part of this thesis is concerned with the meiosis-specific lamin C2. Lamin C2 is the only A-type lamin expressed during meiosis and has in previous studies shown to feature altered meiosis-specific properties, clearly distinguishing it from somatic lamins. Because lamin C2 is enriched at sites of telomere attachment, exhibits a high mobility within the nuclear lamina and influences NE integrity, it has been postulated that it may locally increase NE flexibility to allow efficient meiotic telomere movement. Therefore, possible functions of lamin C2 in the movement of attached telomeres were investigated in this thesis by studying the bouquet formation and release of pubertal mice specifically lacking lamin C2. This revealed that lamin C2 deficient mice show a delayed bouquet release, leading to severe defects in the synaptic pairing of homologous chromosomes, which in turn results in infertility of the males. Therefore, the efficient repositioning of attached meiotic telomeres, facilitated by lamin C2, seems essential for completing meiosis. The second part of this thesis focuses on the protein complex responsible for the attachment of meiotic telomeres to the NE and their coupling to the cytoskeleton. The so-called LINC complex is composed of SUN domain proteins in the inner nuclear membrane interacting with KASH domain proteins of the outer nuclear membrane. In previous studies it had been shown that SUN1, SUN2 and KASH5 localise to the attached meiotic telomeres. Regarding the meiotic role of SUN2, however, contradicting results have recently been discussed, showing the need for further investigations. Using an available SUN1 deficient mouse strain, this thesis was able to show that SUN2 is sufficient for telomere attachment per se although telomere attachment is impaired in SUN1 deficient mice leading to infertility. It is also demonstrated that SUN2 forms a functional LINC complex together with KASH5 to mediate this telomere attachment. This LINC complex in the absence of SUN1 is able to move attached telomeres into a bouquet-like cluster formation. Therefore, this demonstrates that SUN2 is involved in the functional attachment and movement of meiotic telomeres. In summary, this thesis has shown SUN2 and the meiotic nuclear lamina to be directly involved in or essential for the highly conserved attachment and movement of telomeres, making them critical for a successful meiosis. The meiotic NE is therefore in this thesis demonstrated to be a determinant of mammalian fertility. N2 - Die Meiose, eine spezialisierte Zellteilung, produziert aus diploiden Vorläuferzellen haploide Keimzellen, welche sich zu befruchtungsfähigen Gameten entwickeln können. Chromosomen durchlaufen während der Meiose stark regulierte, evolutionär hochkonservierte Bewegungen. Zunächst werden die Telomere aktiv und stabil an der Kernhülle verankert. Angeheftete Telomere werden durch das Cytoskelett entlang der Kernhülle bewegt um sich in einer begrenzten Region anzureichern und das chromosomale Bouquet bilden. Das Bouquet wird durch gerichtete Telomerbewegungen anschließend wieder aufgelöst während die finalen Schritte des Zusammenbaus des Synaptonemalkomplexes stattfinden. Diese Prozesse sind in ihrer Summe essentiell für den erfolgreichen Ablauf der Meiose. Da die meiotische Kernhülle als Plattform für die Anheftung und Bewegung der Telomere dient, kann angenommen werden, dass sie in diese für die Fertilität kritischen Prozesse involviert ist. Die genaue Funktion von Kernhüllenproteinen in der Anheftung und Bewegung meiotischer Telomere ist trotzdem zu großen Teilen noch unverstanden. Deshalb war es Ziel dieser Arbeit zwei Komponenten der meiotische Kernhülle und deren Rolle in Telomeranheftung und –dynamik zu untersuchen. Der erste Teil dieser Arbeit beschäftigt sich mit dem meiosespezifischen Lamin C2, welches das einzige während der Meiose exprimierte A-typ Lamin ist. Weil Lamin C2 in Bereichen der Telomeranheftung angereichter ist, eine hohe Mobilität in der Kernhülle aufweist und Kernhülleneigenschaften verändern kann, wurde postuliert dass es lokal die Flexibilität der Kernhülle steigern könnte um leichtere Bewegungen der Telomere zu ermöglichen. Demzufolge sollte in dieser Arbeit eine mögliche Rolle von Lamin C2 in der effizienten Bewegung angehefteter Telomere anhand von jungen Lamin C2-defizienten Mäuse untersucht werden. Dies ergab, dass Lamin C2-defiziente Mäuse eine verlangsamte Auflösung des meiotische Bouquets zeigten, was Defekte in der Homologenpaarung verursacht und letztlich zur Infertilität der Männchen führt. Schlussendlich, scheint die effiziente Bewegung angehefteter Telomere, ermöglicht durch Lamin C2, damit essentiell für einen erfolgreichen Ablauf der Meiose. Der zweite Teil dieser Arbeit ist auf einen Proteinkomplex fokussiert welcher für die Anheftung meiotische Telomere und deren Verbindung zum Cytoskelett verantwortlich ist. Dieser LINC complex besteht aus SUN-domänenproteinen der inneren Kernmembran welche mit KASH-domänenproteinen der äußeren Kernmembran interagieren. Aus früheren Studien ist bekannt, dass SUN1, SUN2 und KASH5 an angehefteten Telomeren lokalisieren. Die meiotische Funktion von SUN2, jedoch, wird aktuell anhand widersprüchlicher Ergebnisse diskutiert. Durch die Verwendung SUN1-defizienter Mäuse konnte diese Arbeit zeigen, dass obwohl die partiell unvollständige Telomeranheftung in der Abwesenheit von SUN1 zu Infertilität führt, SUN2 dennoch für Telomeranheftung an sich ausreichend ist. Um diese Anheftung zu vermitteln, bildet SUN2 einen funktionellen LINC complex mit KASH5 welcher angeheftete Telomere in der Abwesenheit von SUN1 in bouquet-ähnliche Konformationen führt. Demzufolge demonstriert diese Arbeit, dass SUN2 an der funktionellen Telomeranheftung und –bewegung beteiligt ist. Zusammenfassend hat diese Arbeit gezeigt, dass SUN2 und die meiotische Lamina in die hochkonservierte Anheftung und Bewegung von Telomeren direkt involviert oder für sie essentiell sind, und somit unabdingbar für eine erfolgreiche Meiose. Damit definiert diese Arbeit die meiotische Kernhülle als eine Determinante für die Fertilität von Säugern. KW - Meiose KW - Kernhülle KW - Meiosis KW - Nuclear envelope Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-83540 ER - TY - THES A1 - Kannen Cardoso, Vinicius T1 - The role of Fluoxetine against preneoplastic lesions and tumors in colon tissue T1 - Die Rolle von Fluoxetin gegen präneoplastische Läsionen und Tumoren im Darmgewebe N2 - Introduction: Colon cancer is one of the major human malignancies worldwide, and much effort has been applied to understand the process of colon carcinogenesis, as well as the role of potential treatments and co-therapeutical agents against it. A growing body of evidence suggests that the use of fluoxetine (FLX), an antidepressant belonging to the selective serotonin reuptake inhibitors (SSRIs), may be associated with a reduced colon cancer risk. However, controversial opinions have been published and an identification of the mechanisms of the activity of FLX on colon cells would help in the clarification of this controversy. Objectives: Using several in vitro and in vivo-based methods and analyses, we aimed to verify whether FLX has antioxidant, pro-oxidant or DNA-damaging potential in standard toxicological assays; to check whether and how FLX could prevent and reduce colon preneoplastic lesions; to ascertain whether FLX has any oncostatic potential against colon tumors; and, to investigate whether FLX activity could be comparable with a known and current applied chemotherapeutic agent against colon cancer. Results: FLX did not have any antioxidant potential in our experiments. Although it did not induce reactive oxygen species (ROS) generation or DNA-damage in fibroblast and colon tumor cell lines, FLX reduced dysplasia and proliferation in two different carcinogen models. Further, a significant decrease in colon stromal reactivity and angiogenesis was found in both carcinogen-induced preneoplasia models. In a xenograft model of colon cancer, FLX shrank tumors, reduced tumor proliferation, arrested cancer cells at the G0/G1 cell-cycle phase, and took ROS generation under control. Such effects were detected together with an intracellular acidification and loss of mitochondrial membrane potential in FLX-treated cells. Modulating mitochondrial respiratory chain, HIF-1 expression and Akt/mTOR signaling pathway, FLX was found to reduce colon tumors similar to the widely used chemotherapeutic agent 5-Fluoracil activity. Conclusion: Our collective data suggest that FLX is a remarkable chemopreventive and oncostatic agent against colon preneoplastic lesions and tumors, acting without DNA-damage or ROS generation. N2 - Einleitung: Darmkrebs ist eine der wichtigsten menschlichen Tumorarten weltweit und viel Aufwand wurde unternommen, um den Prozess der Colonkarzinogenese, sowie die Rolle der möglichen Behandlungen und Co-therapeutische Mittel zu verstehen. Eine wachsende Zahl von Hinweisen deuted darauf hin, dass die Verwendung von Fluoxetin (FLX), einem Antidepressivum aus der Klasse der selektiven Serotonin-Wiederaufnahmehemmer (SSRIs), mit einem reduzierten Dickdarmkrebs-Risiko verbunden sein kann. Allerdings sind auch kontroverse Meinungen veröffentlicht worden und eine Identifizierung der Mechanismen der Aktivität von FLX auf Darmzellen würde bei der Klärung dieser Kontroverse helfen. Ziele: Mit in vitro-und in vivo-Methoden wollten wir prüfen, ob FLX antioxidatives, prooxidatives oder DNA-schädigendes Potential in Standard-toxikologischen Untersuchungen hat; des weiteren sollte analysiert werden, ob und wie FLX präneoplastischen Läsionen verhindern und reduzieren kann, sowie ob FLX onkostatisches Potenzial gegen Darmtumoren hat. Letzteres sollte im direkten Vergleich mit dem etablierten Chemotherapeutikum 5-Fluoruracil untersucht werden. Ergebnisse: FLX zeigte keine direkte antioxidative Kapazität in unseren Testsystemen. Obwohl es keine Bildung reaktiver Sauerstoffspecies (ROS) und keine Induktion von DNA-Schaden in Fibroblasten und Kolon Tumorzellinien verursachte, reduzierte FLX Dysplasien und Proliferation in zwei verschiedenen Kanzerogen-Modellen in vivo. Ferner wurde eine signifikante Abnahme der Reaktivität der Stromazellen und von Angiogenese in beiden Karzinogen-induzierten Präneoplasie-Modellen gefunden. In einem Xenograft Modell des Kolonkarzinoms brachte FLX die Tumoren durch verringerte Proliferation zum Schrumpfen. In vitro wurde in den entsprechenden Zellinien eine Anreicherung der Zellen in der Ga0/G1 Zellzyklus-Phase, eine Reduktion Hypoxie-verursachter ROS-Bildung, intrazelluläre Ansäuerung und Velust des mitochondrialen Membranpotentials nach FLX-Behandlung gefunden. Weitere Aktivitäten waren auf die mitochondriale Atmungskette, HIF-1 Expression und den Akt/mTOR-Sinalweg zu beobachten. Die Reduktion der Kolontumoren war der mit 5-Fluoruracil erzielten vergleichbar. Schlussfolgerung: Unsere Daten deuten darauf hin, dass FLX eine bemerkenswerte chemopräventive und onkostatischen Aktivität gegen präneoplastische Läsionen und Tumore im Darm aufweist, die ohne Induktion von DNA-Schäden ROS stattfindet. KW - Fluoxetin KW - Magenkrebs KW - Fluoxetine KW - Colon cancer Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-77589 ER - TY - JOUR A1 - Meule, Adrian A1 - Vögele, Claus T1 - The psychology of eating JF - Frontiers in Psychology N2 - No abstract available. Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190460 SN - 1664-1078 VL - 4 ER - TY - JOUR A1 - Chatterjee, Manik A1 - Andrulis, Mindaugas A1 - Stühmer, Thorsten A1 - Müller, Elisabeth A1 - Hofmann, Claudia A1 - Steinbrunn, Torsten A1 - Heimberger, Tanja A1 - Schraud, Heike A1 - Kressmann, Stefanie A1 - Einsele, Hermann A1 - Bargou, Ralf C. T1 - The PI3K/Akt signaling pathway regulates the expression of Hsp70, which critically contributes to Hsp90-chaperone function and tumor cell survival in multiple myeloma JF - Haematologica N2 - Despite therapeutic advances multiple myeloma remains largely incurable, and novel therapeutic concepts are needed. The Hsp90-chaperone is a reasonable therapeutic target, because it maintains oncogenic signaling of multiple deregulated pathways. However, in contrast to promising pre-clinical results, only limited clinical efficacy has been achieved through pharmacological Hsp90 inhibition. Because Hsp70 has been described to interact functionally with the Hsp90-complex, we analyzed the suitability of Hsp72 and Hsp73 as potential additional target sites. Expression of Hsp72 and Hsp73 in myeloma cells was analyzed by immunohistochemical staining and western blotting. Short interfering RNA-mediated knockdown or pharmacological inhibition of Hsp72 and Hsp73 was performed to evaluate the role of these proteins in myeloma cell survival and for Hsp90-chaperone function. Furthermore, the role of PI3K-dependent signaling in constitutive and inducible Hsp70 expression was investigated using short interfering RNA-mediated and pharmacological PI3K inhibition. Hsp72 and Hsp73 were frequently overexpressed in multiple myeloma. Knockdown of Hsp72 and/or Hsp73 or treatment with VER-155008 induced apoptosis of myeloma cells. Hsp72/Hsp73 inhibition decreased protein levels of Hsp90-chaperone clients affecting multiple oncogenic signaling pathways, and acted synergistically with the Hsp90 inhibitor NVP-AUY922 in the induction of death of myeloma cells. Inhibition of the PI3K/Akt/GSK3b pathway with short interfering RNA or PI103 decreased expression of the heat shock transcription factor 1 and down-regulated constitutive and inducible Hsp70 expression. Treatment of myeloma cells with a combination of NVP-AUY922 and PI103 resulted in additive to synergistic cytotoxicity. In conclusion, Hsp72 and Hsp73 sustain Hsp90-haperone function and critically contribute to the survival of myeloma cells. Translation of Hsp70 inhibition into the clinic is therefore highly desirable. Treatment with PI3K inhibitors might represent an alternative therapeutic strategy to target Hsp70. KW - Haematology Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130574 VL - 98 IS - 7 ER - TY - THES A1 - Dreykluft, Angela T1 - The PD-1/B7-H1 Pathway in a Transgenic Mouse Model for Spontaneous Autoimmune Neuroinflammation: Immunological Studies on Devic B7-H1-/- Mice T1 - Der PD-1/B7-H1 Signalweg in einem transgenen Mausmodell für spontane autoimmune Neuroinflammation: Immunologische Studien an Devic B7-H1-/- Mäusen N2 - Multiple sclerosis is an autoimmune disease of the central nervous system characterized by inflammatory, demyelinating lesions and neuronal death. Formerly regarded as a variant of MS, neuromyelitis optica (NMO)/Devic’s disease is now recognized as a distinct neurological disorder exhibiting characteristic inflammatory and demyelinated foci in the optic nerves and the spinal cord sparing the brain. With the introduction of the double-transgenic “Devic mouse” model featuring spontaneous, adjuvant-free incidence of autoimmune neuroinflammation due to the interaction of transgenic MOG-specific T and B cells, a promising tool was found for the analysis of factors triggering or preventing autoimmunity. The co-inhibitory molecule B7-H1 has been proposed to contribute to the maintenance of peripheral tolerance and to confine autoimmune inflammatory damage via the PD-1/B7-H1 pathway. Compared to Devic B7-H1+/+ mice, Devic B7-H1-/- mice developed clinical symptoms with a remarkably higher incidence rate and faster kinetics emphasized by deteriorated disease courses and a nearly quadrupled mortality rate. Remarkably enlarged immune-cell accumulation in the CNS of Devic B7-H1-/- mice, in particular of activated MOG-specific CD4+ T cells, correlated with the more severe clinical features. Our studies showed that the CNS not only was the major site of myelin-specific CD4+ T-cell activation but also that B7-H1 expression within the target organ significantly influenced T-cell activation and differentiation levels. Analysis at disease maximum revealed augmented accumulation of MOG-specific CD4+ T cells in the peripheral lymphoid organs of Devic B7-H1-/- mice partly due to increased T-cell proliferation rates. Transgenic MOG-specific B cells of Devic B7-H1-/- mice activated MOG-specific CD4+ T cells more efficiently than B cells of Devic B7-H1+/+ mice. This observation indicated a relevant immune-modulating role of B7-H1 on APCs (antigen-presenting cells) in this mouse model. We also assumed altered thymic selection processes to be involved in increased peripheral CD4+ T-cell numbers of Devic B7-H1-/- mice as we found more thymocytes expressing the transgenic MOG-specific T-cell receptor (TCR). Moreover, preliminary in vitro experiments hinted on an enhanced survival of TCRMOG-transgenic CD4+ T cells of Devic B7-H1-/- mice; a mechanism that might as well have led to higher peripheral T-cell accumulation. Elevated levels of MOG-specific CD4+ T cells in the periphery of Devic B7-H1-/- mice could have entailed the higher quantities in the CNS. However, mechanisms such as CNS-specific proliferation and/or apoptosis/survival could also have contributed. This should be addressed in future investigations. Judging from in vitro migration assays and adoptive transfer experiments on RAG-1-/- recipient mice, migratory behavior of MOG-specific CD4+ T cells of Devic B7-H1+/+ and Devic B7-H1-/- mice seemed not to differ. However, enhanced expression of the transmigration-relevant integrin LFA-1 on CD4+ T cells in young symptom-free Devic B7-H1-/- mice might hint on temporally differently pronounced transmigration capacities during the disease course. Moreover, we attributed the earlier conversion of CD4+ T cells into Th1 effector cells in Devic B7-H1-/- mice during the initiation phase to the lack of co-inhibitory signaling via PD-1/B7-H1 possibly leading to an accelerated disease onset. Full blown autoimmune inflammatory processes could have masked these slight effects of B7-H1 in the clinical phase. Accordingly, at peak of the disease, Th1 and Th17 effector functions of peripheral CD4+ T cells were comparable in both mouse groups. Moreover, judging from titers of MOG-specific IgG1 and IgM antibodies, alterations in humoral immunity were not detected. Therefore, clinical differences could not be explained by altered T-cell or B-cell effector functions at disease maximum. B7-H1 rather seemed to take inhibitory effect in the periphery during the initiation phase only and consistently within the target organ by parenchymal expression. Our observations indicate that B7-H1 plays a relevant role in the regulation of T-cell responses in this mouse model for spontaneous CNS autoimmunity. By exerting immune-modulating effects in the preclinical as well as the clinical phase of the disease, B7-H1 contributed to the confinement of the immunopathological tissue damage in Devic B7-H1+/+ mice mirrored by later disease onsets and lower disease scores. As a model for spontaneous autoimmunity featuring a close to 100 % incidence rate, the Devic B7-H1-/- mouse may prove instrumental in clarifying disease-triggering and -limiting factors and in validating novel therapeutic approaches in the field of autoimmune neuroinflammation, in particular the human Devic’s disease. N2 - Multiple Sklerose ist eine Autoimmunerkrankung des zentralen Nervensystems, die durch entzündliche, demyelinisierende Läsionen und neuronalen Tod gekennzeichnet ist. Einst als Variante der MS betrachtet, gilt die Neuromyelitis optica (NMO) / Devic-Krankheit heute als eigenständige neurologische Erkrankung, bei der charakteristische Läsionen in den Sehnerven und im Rückenmark jedoch nicht im Gehirn auftreten. Mit der Einführung des doppelt-transgenen "Devic Maus"-Modells, bei dem es zur spontanen, Adjuvans-freien Inzidenz von autoimmuner Neuroinflammation durch Expression transgener MOG-spezifischer T- und B-Zellen kommt, wurde ein vielversprechendes Werkzeug für die Analyse von Faktoren gefunden, die Autoimmunität auslösen bzw. hemmen können. Das ko-inhibitorische Molekül B7-H1 trägt über den PD-1/B7-H1 Signalweg vermeintlich zur Aufrechterhaltung peripherer Toleranz bei. Devic B7-H1-/ - Mäuse entwickelten im Vergleich zu Devic B7-H1+/ + Mäusen Symptome, die mit deutlich höherer Inzidenz und schnellerer Kinetik einhergingen, unterstrichen von verstärkten Krankheitsverläufen und einer nahezu vervierfachten Sterblichkeit. Die verstärkte Akkumulierung von Immunzellen im ZNS, insbesondere von aktivierten MOG-spezifischen CD4+ T-Zellen, korrelierte mit den schwerwiegenderen klinischen Merkmalen. Unsere Untersuchungen zeigten nicht nur, dass die Aktivierung von myelin-spezifischen CD4+ T-Zellen hauptsächlich im ZNS stattfand, sondern auch, dass im Zielorgan exprimiertes B7-H1 maßgeblich den T-Zell-Aktivierungs- und -Differenzierungsgrad beeinflusste. Analysen am Krankheitsmaximum zeigten eine verstärkte Akkumulierung von MOG-spezifischen CD4+ T-Zellen in den Lymphorganen von Devic B7-H1-/- Mäusen, die wir teils auf erhöhte T-Zell-Proliferation zurückzuführten. Transgene MOG-spezifische B-Zellen der Devic B7-H1-/- Mäuse aktivierten effizienter als B-Zellen der Devic B7-H1+/+ Mäuse MOG-spezifische CD4+ T-Zellen. Dies deutet auf eine wichtige immunmodulierende Rolle von B7-H1 auf Antigen-präsentierenden Zellen in diesem Mausmodell hin. Veränderte Selektionsprozesse im Thymus trugen wohlmöglich zu den höheren CD4+ T-Zellzahlen in der Peripherie bei. Vorläufige in vitro Experimente deuteten auf ein verbessertes Überleben von TCRMOG-transgenen CD4+ T-Zellen aus Devic B7-H1-/- Mäusen hin. Eine erhöhte Anzahl von peripheren MOG-spezifischen CD4+ T-Zellen könnte zu den größeren Mengen im ZNS von Devic B7-H1-/- Mäusen geführt haben. Jedoch sind zusätzliche Mechanismen wie ZNS-spezifische Proliferation und/oder Apoptose bzw. Überleben denkbar. Dies sollte in zukünftigen Untersuchungen genauer analysiert werden. Anhand von in vitro-Migrationsassays und Adoptiver Transfer-Experimenten in RAG-1-/- Mäusen schlossen wir, dass das Migrationsverhalten von MOG-spezifischen CD4+ T-Zellen von Devic B7-H1-/- Mäusen nicht verändert war. Allerdings deutet die verstärkte Expression des transmigrationsrelevanten Intergins LFA-1 auf CD4+ T-Zellen in jungen, symptomfreien Devic B7-H1-/- Mäusen auf im Krankheitsverlauf zeitlich verschieden ausgeprägte Transmigrationskapazitäten hin. Die frühere Differenzierung von peripheren CD4+ T-Zellen in Th1-Effektorzellen in Devic B7-H1-/- Mäusen während der Initiationsphase schrieben wir der fehlenden inhibierenden Wirkung des PD-1/B7-H1 Signalwegs zu, was den früheren Krankheitsbeginn bedingt haben könnte. Stark ausgeprägte autoimmune Entzündungsreaktionen am Krankheitsmaximum maskierten jedoch wahrscheinlich diese schwachen Effekte von B7-H1. Dies wurde durch die Tatsache untermauert, dass am Krankheitsmaximum Th1- und Th17-Effektorfunktionen von peripheren CD4+ T-Zellen in beiden Mausgruppen vergleichbar ausgeprägt waren. Des Weiteren bestanden am Krankheitsmaximum keine Unterschiede in der humoralen Immunität. Die beobachteten klinischen Unterschiede waren demnach nicht durch veränderte periphere T-Zell- oder B-Zell-Effektorfunktionen in dieser Krankheitsphase erklärbar. Vielmehr scheint B7-H1 in der Peripherie ausschließlich während der Initiationsphase der Krankheit und fortwährend im Zielorgan durch seine parenchymale Expression immuninhibierend zu wirken. Unsere Beobachtungen zeigen, dass B7-H1 eine relevante Rolle bei der Immunregulierung im vorliegenden Mausmodell für spontane ZNS-Autoimmunität spielt. Durch immunmodulierende Effekte in der präklinischen sowie der klinischen Phase der Krankheit trug B7-H1 zu der Begrenzung der immunpathologischen Gewebeschädigung in Devic B7-H1+/+ Mäusen bei, sichtbar an einem späteren Krankheitsbeginn und leichteren -verlauf. Als Tiermodell für spontane ZNS-Autoimmunität mit nahezu 100 %iger Inzidenz könnte sich die Devic B7-H1-/- Maus als hilfreich bei der Klärung krankheitsauslösender und -limitierender Faktoren erweisen sowie bei der Validierung neuer therapeutischer Ansätze im Bereich der autoimmunen Neuroinflammation, insbesondere der Devic-Krankheit im Menschen. KW - Autoimmunität KW - Zentralnervensystem KW - Neuroinflammation KW - B7-H1 KW - Ko-inhibitorischer Signalweg KW - Devic Maus KW - autoimmunity KW - neuroinflammation KW - B7-H1 KW - co-inhibitory signalling KW - Devic mice KW - Maus KW - Entzündung KW - Signaltransduktion Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-83288 ER - TY - JOUR A1 - Poppe, Lidia M. A1 - Bröcker, Eva-Bettina A1 - Trautmann, Axel T1 - The One-nail Brown Band: Macro- and Micro-morphology JF - Acta Dermato-Venereologica N2 - No abstract available. KW - brown band KW - macro-morphology KW - micro-morphology Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-128566 VL - 93 IS - 4 ER - TY - JOUR A1 - Hohenauer, Tobias A1 - Berking, Carola A1 - Schmidt, Andreas A1 - Haferkamp, Sebastian A1 - Senft, Daniela A1 - Kammerbauer, Claudia A1 - Fraschka, Sabine A1 - Graf, Saskia Anna A1 - Irmler, Martin A1 - Beckers, Johannes A1 - Flaig, Michael A1 - Aigner, Achim A1 - Höbel, Sabrina A1 - Hoffmann, Franziska A1 - Hermeking, Heiko A1 - Rothenfusser, Simon A1 - Endres, Stefan A1 - Ruzicka, Thomas A1 - Besch, Robert T1 - The neural crest transcription factor Brn3a is expressed in melanoma and required for cell cycle progression and survival JF - EMBO Molecular Medicine N2 - Pigment cells and neuronal cells both are derived from the neural crest. Here, we describe the Pit-Oct-Unc (POU) domain transcription factor Brn3a, normally involved in neuronal development, to be frequently expressed in melanoma, but not in melanocytes and nevi. RNAi-mediated silencing of Brn3a strongly reduced the viability of melanoma cell lines and decreased tumour growth in vivo. In melanoma cell lines, inhibition of Brn3a caused DNA double-strand breaks as evidenced by Mre11/Rad50-containing nuclear foci. Activated DNA damage signalling caused stabilization of the tumour suppressor p53, which resulted in cell cycle arrest and apoptosis. When Brn3a was ectopically expressed in primary melanocytes and fibroblasts, anchorage-independent growth was increased. In tumourigenic melanocytes and fibroblasts, Brn3a accelerated tumour growth in vivo. Furthermore, Brn3a cooperated with proliferation pathways such as oncogenic BRAF, by reducing oncogene-induced senescence in non-malignant melanocytes. Together, these results identify Brn3a as a new factor in melanoma that is essential for melanoma cell survival and that promotes melanocytic transformation and tumourigenesis. KW - oncogene-induced senescence KW - BRN-3A KW - DNA KW - DNA damage KW - tumourigenesis KW - P53 KW - in-vitro KW - neural crest factors KW - family KW - apoptosis KW - melanoma KW - BRAF mutations KW - domain Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122193 SN - 1757-4676 VL - 5 ER - TY - JOUR A1 - Rasche, Leo A1 - Duell, Johannes A1 - Morgner, Charlotte A1 - Chatterjee, Manik A1 - Hensel, Frank A1 - Rosenwald, Andreas A1 - Einsele, Hermann A1 - Topp, Max S. A1 - Brändlein, Stephanie T1 - The Natural Human IgM Antibody PAT-SM6 Induces Apoptosis in Primary Human Multiple Myeloma Cells by Targeting Heat Shock Protein GRP78 JF - PLoS ONE N2 - In contrast to other haematological malignancies, targeted immunotherapy has not entered standard treatment regimens for de novo or relapsed multiple myeloma (MM) yet. While a number of IgG-formatted monoclonal antibodies are currently being evaluated in clinical trials in MM, our study aimed to investigate whether the fully human IgM monoclonal antibody PAT-SM6 that targets a tumour-specific variant of the heat shock protein GRP78 might be an attractive candidate for future immunotherapeutic approaches. We here show that GRP78 is stably and consistently expressed on the surface on tumour cells from patients with de novo, but also relapsed MM and that binding of PAT-SM6 to MM cells can specifically exert cytotoxic effects on malignant plasma cells, whereas non-malignant cells are not targeted. We demonstrate that the induction of apoptosis and, to a lesser extent, complement dependent cytotoxicity is the main mode of action of PAT-SM6, whereas antibody dependent cellular cytotoxicity does not appear to contribute to the cytotoxic properties of this antibody. Given the favourable safety profile of PAT-SM6 in monkeys, but also in a recent phase I trial in patients with malignant melanoma, our results form the basis for a planned phase I study in patients with relapsed MM. KW - cytotoxicity KW - apoptosis KW - immunohistochemistry techniques KW - enzyme-linked immunoassays KW - multiple myeloma KW - cell staining KW - cell binding KW - complement system Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130125 VL - 8 IS - 5 ER - TY - THES A1 - Ngwa, Che Julius T1 - The mosquito midgut-specific stages of the malaria parasite as targets for transmission blocking interventions T1 - Die Moskitomitteldarmstadien des Malariaparasiten als Ziele für übertragungsblockierende Eingriffe N2 - Die Tropenkrankheit Malaria, wird durch eine Infektion mit einzelligen Parasiten der Gattung Plasmodium verursacht und durch den Stich der weiblichen Anopheles-Mücke von Mensch zu Mensch verbreitet. Dabei kann eine erfolgreiche Übertragung des Parasiten auf den Menschen nur dann stattfinden, wenn der Parasit seine sexuelle Entwicklungsphase im Mitteldarm der Mücke erfolgreich durchläuft. Ziel dieser Arbeit war es daher, die Wechselwirkungen des Malariaparasiten im Mitteldarm der Mücke in Hinblick auf die Identifizierung möglicher neuer transmissionsblockierender Strategien zu untersuchen. Der Zweck von transmissionsblockierende Strategien ist es, der Verbreitung der Malaria durch die Mücke entgegenzuwirken, indem die Entwicklung des Parasiten in der Mücke unterbunden und dadurch der Lebenszyklus des Parasiten unterbrochen wird. Der Schwerpunkt der vorliegenden Arbeit lag auf insgesamt drei Aspekten. Der erste Aspekt der Arbeit befasste sich mit der Wechselwirkung zwischen dem Para-siten und der mikrobiellen Darmflora der Mücke. Dabei sollte der mögliche Einfluss des Parasiten auf die Darmflora untersucht werden und weiterführend die potentielle Verwendung von Darmbakterien als Vehikel für die Herstellung paratransgener Mücken erforscht werden. Vergleichende16S-rRNA- und DGGE-Analysen an der Darmflora des asiatischen Malariavektors Anopheles stephensi zeigten eine deutliche Reduktion der mikrobiellen Diversität während der Entwicklung vom Ei zur adulten Mücke. Zudem konnte das gram-negative Bakterium Elizabethkingia meningoseptica, das sich stadien- und generationsübergreifend verbreitet, als dominante Darmspezies bei im Labor aufgezogenen weiblichen und männlichen An. stephensi festgestellt werden. Die Dominanz von E. meningoseptica wurde zudem nicht durch die Aufnahme von infiziertem Blut oder einer veränderten Nahrung beeinflusst. Für die Studien wurde sowohl der humanpathogene Parasit P. falciparum als auch der Nagermalariaerreger P. berghei verwendet. Weiterführende Versuche zeigten, dass Extrakte von E. meningoseptica antibakterielle, antifungale und antiplasmodiale Aktivitäten aufwiesen, die ein möglicher Grund für die Dominanz dieser Spezies im Mitteldarm des Vektors waren. Isolate von E. meningoseptica sind im Labor kultivierbar; dadurch stellt das Bakterium einen potentiellen Kandidaten zur Generierung von paratransgenen Anopheles-Mücken dar. Ein zweites Ziel dieser Arbeit war es, mögliche Unterschiede in der Genexpression von P. falciparum darzustellen, die in den ersten 30 Minuten nach dessen Übertragung auf die Mücke erfolgen. Dies hatte zum einen zum Zweck, die durch den Wirtswechsel hervorgerufenen Genregulationen besser zu verstehen, und bot zum anderen die Möglichkeit, neue Proteine zu identifizieren, die als potentielle transmissionsblockierende Ziele genutzt werden können. Mittels supression substractive hybridization (SSH) konnten insgesamt 126 Gene identifiziert werden, deren Expression sich während der Gametogenese verändert. Die identifizierten Gene konnten einer Vielzahl von putativen Funktionen wie zum Beispiel in der Signaltransduktion (17,5%), im Zellzyklus (14,3%) oder im Zytoskelett (8,7%) zugeordnet werden. Des Weiteren wurden 7,9% der Gene eine Funktion in der Proteastase und 6,4% in metabolischen Prozessen zugeordnet. 12,7% der Gene kodierten für zelloberflächenassoziierte Proteine. 11,9% der Gene hatten anderen Funktionen, während 20% der Gene keine putative Funktion zugeordnet werden konnte. Etwa 40% der identifizierten Genprodukte waren bisher nicht in Proteomstudien nachgewiesen worden. In weiterführenden Analysen wurden 34 Gene aus jeder ontologischen Gruppe ausgewählt und deren Expressionsveränderung per quantitativer real time RT-PCR im Detail untersucht. Für 29 Gene konnte dabei eine Transkriptexpression in Gametozyten nachgewiesen werden. Zudem wiesen 20 Gene eine erhöhte Expression in Gametozyten im Vergleich asexuellen Stadien auf. Insgesamt zeigten 8 Gene besonders hohe Transkriptlevel in aktivierten Gametozyten, was auf eine Funktion dieser Proteine während der Übertragung des Parasiten auf die Mücke hindeutet und diese somit potentielle Angriffspunkte für transmissionsblockierende Strategien darstellen könnten. Im letzten Teil dieser Arbeit stand die Untersuchung verschiedener antimikrobieller Substanzen in Bezug auf ihre transmissionsblockierenden Eigenschaften im Vordergrund. Die Substanzen waren entweder direkt aus der Hämolymphe verschiedener Insekten isoliert oder rekombinant in transgenem Tabak exprimiert worden. Dabei wurden die rekombinanten Peptide so ausgewählt, dass sie entweder gegen die Mitteldarmstadien des Parasiten wirken oder mückenspezifische Rezeptoren blockieren, die der Parasit für seine weitere Entwicklung benötigt. Dabei konnte gezeigt werden, dass das antimikrobielle Molekül Harmonin, ein Abwehrmolekül aus der Hämolymphe des asiatischen Marienkäfers Harmonia axyridis, antiplasmodiale als auch transmissions-blockierende Eigenschaften besitzt. Harmonin stellt daher eine potentielle Leitstruktur für die Entwicklung neuer Malariawirkstoffe dar N2 - Malaria is a vector-borne disease caused by the protozoan parasite of the genus Plasmodium and it is transmitted from human to human by female Anopheles mosquitoes during a blood meal. For malaria transmission to occur, the malaria parasite must undergo a crucial developmental sexual phase inside the mosquito midgut. In this study, we sought to investigate the interplay of the malaria parasite in the mosquito midgut with regard to the identification of novel types of transmission blocking intervention strategies. These strategies are aimed at reducing the spread of malaria by blocking the development of the mosquito midgut-specific stages of Plasmodium. We focused on three aspects. The first aspect was to investigate the interplay between mosquito midgut bacteria and malaria parasites in order to determine the potential influence of malaria parasites on the composition of the mosquito gut microbiota and also determine midgut bacteria which could be exploited as vehicles for the generation of paratransgenic Anopheles mosquitoes. We analyzed the microbial diversity of gut bacteria of the Asian malaria vector Anopheles stephensi during development and under different feeding regimes, including feeds on malaria parasite-infected blood, using the human pathogenic P. falciparum as well as the rodent malaria model P. berghei. 16S rRNA and DGGE analyses demonstrated a reduction in the microbial diversity during mosquito development from egg to adult and identified the gram-negative bacterium Elizabethkingia meningoseptica as the dominant species in the midgut of laboratory-reared male and female mosquitoes. E. meningoseptica is transmitted between generations and its predominance in the mosquito midgut was not altered by diet, when the gut microbiota was compared between sugar-fed and blood-fed female mosquitoes. Furthermore, feeds on blood infected with malaria parasites did not impact the presence of E. men-ingoseptica in the gut. Interestingly, extracts from E. meningoseptica exhibited antibacterial, antifungal and antiplasmodial activities, which may account for its dominance in the midgut of the malaria vector. Isolates of E. meningoseptica were cultivable, making the bacterium a potential candidate vehicle for the generation of paratransgenic Anopheles mosquitoes. The second aspect of this thesis was to determine transcriptome changes that occur during the first half hour following transmission of P. falciparum to the mosquito vector in order to better understand gene regulation mechanisms important for the change of hosts and determine novel proteins which could be exploited in malaria transmission blocking interventions. We initially used suppression subtractive hybridization (SSH) to compare mRNA levels of P. falciparum gametocytes before and 30 min fol-lowing activation. We identified a total of 126 genes for which transcript expression changed during gametogenesis. Among these, 17.5% had putative functions in signaling, 14.3% were assigned to cell cycle and gene expression, 8.7% were linked to the cytoskeleton or motor complex, 7.9% were involved in proteostasis and 6.4% in metabolism, 12.7% were genes encoding for cell surface associated proteins, 11.9% were assigned to other functions, and 20.6% represented genes of unknown function. For 40% of the identified genes there has as yet not been any protein evidence. We further selected a subset of 34 genes from all the above ontology groups and analyzed the transcript changes during gametogenesis in detail by quantitative realtime RT-PCR. Of these, 29 genes were expressed in gametocytes, and for 20 genes transcript expres-sion in gametocytes was increased compared to asexual blood stage parasites. Transcript levels of eight genes were particularly high in activated gametocytes, pointing at functions downstream of gametocyte transmission to the mosquito which could be exploited in malaria transmission blocking strategies. The last aspect of this thesis was to determine the transmission blocking effect of a range of antimicrobial molecules as transmission blocking agents. The molecules were either isolated from insect hemolymph or recombinantly expressed in tobacco and designed to act either directly on the mosquito midgut stages or cover receptors on mosquito tissues like the midgut epithelium which the parasite would need for transit. We were able to show an antiplasmodial and transmission blocking effect of the anti-microbial molecule harmonine, a defense compound isolated from the hemolymph of the Asian ladybug Harmonia axyridis. Harmonine thus represents a potential lead structure for the development of novel antimalarials. KW - Malariamücke KW - Anopheles stephensi KW - Mitteldarm KW - Malaria KW - Mosquito KW - midgut KW - transmission KW - Malaria KW - Krankheitsübertragung KW - Mücke KW - Mitteldarm Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-83594 ER - TY - THES A1 - Kühn, Andrea T1 - The molecular interplay of proteins expressed in the sexual stages and the induction of gamete formation in the malaria parasite Plasmodium falciparum T1 - Molekulare Wechselwirkungen in den Sexualstadien exprimierter Proteine und die Induktion der Gametenbildung im Malariaerreger Plasmodium falciparum N2 - Transmission of the malaria parasite from man to the mosquito requires the formation of sexual parasite stages, the gametocytes. The gametocytes are the only parasite stage that is able to survive in the mosquito midgut and to undergo further development – gamete formation and fertilization. Numerous sexual stage-specific proteins have been discovered, some of which play crucial roles for parasite transmission. However, the functions of many sexual stage proteins remain elusive. Amongst the sexual stage-specific proteins are the proteins of the PfCCp proteins family, which exhibit numerous adhesion domains in their protein structures. For four members of the protein family, PfCCp1 to PfCCp4 gene-disruptant parasite lines had been already studied. Amongst these, PfCCp2 and PfCCp3 showed an important role for development of the parasites in the mosquito. In the present work the study of gene-disrupted parasites of the PfCCp Protein family was completed. PfCCp5-KO and PfFNPA-KO parasite lines were characterized to a great extent and many properties were similar to those of other PfCCp proteins. The co-dependent expression previously reported to be a phenomenon of PfCCp proteins was also observed in these two mutants, although to lesser extent. When either PfCCp5 or PfFNPA were absent, all other proteins were detected in reduced abundance only. Co-dependent expression manifests exclusively on the protein level. Transcript levels were not altered as RT-PCR showed. Amongst PfCCp proteins numerous proteinproteins interactions are taking place. The previously described multimeric protein complexes also include further sexual stage-specific proteins like Pfs230, Pfs48/45 and Pfs25. Recently, a new component of PfCCp-based multimeric protein complexes had been identified. The protein was named PfWLP1 (WD repeat protein-like protein 1) due to its possession of several WD40 repeats. In the present study expression of this uncharacterized protein was investigated via indirect IFA. It was expressed in asexual blood stages and gametocytes. Upon gamete formation and fertilization its expression ceased. Another sexual stage protein studied in this work was PfactinII. It was shown to be exclusively expressed in sexual stages. In gametocytes it co-localizes with Pfs230 and correct localization of PfactinII depends on presence of Pfs230. Transcript analysis by means of RT-PCR revealed the expression of several components of the IMC in gametocytes. Furthermore, five or six myosin genes encoded in the P. falciparum genome were detected in gametocytes. Gametocyte egress was studied on the ultrastructural level via transmission electron microscopy and an inside-out type of egress was observed. Firstly, the membrane of the parasitophorous vacuole (PVM) was lysed and only thereafter the membrane of the red blood cell (RBCM) ruptured. Furthermore, a new inductor of gametogenesis was identified: The K+/H+ ionophore nigericin induced gametocytes activation in the absence of xanthurenic acid (XA), which is responsible for gamtetocyte activation in the mosquito midgut. Selective permeabilization of RBCM and PVM by the mild detergent saponin, showed that in the absence of these membranes male gametocytes were still able to perceive both XA and the drop in temperature. Thus, the receptors for both factors signaling the parasite transmission to the mosquito, seem to be of parasitic origin. LC/MS/MS analysis confirmed the ability of RBCs to take up XA. With malaria eradication on the agenda of malaria research targeting the sexual stages becomes a crucial part of intervention strategies. The sexual stages are especially attractive target as they represent a population bottleneck. The here reported findings on P. falciparum gametocytes provide several potential candidate proteins for developing tools to interrupt transmission from man to mosquito. Such tools might include Transmission blocking vaccines and drugs. N2 - Die Übertragung der Malaria vom menschlichen Wirt auf die Überträgermücke erfordert die Bildung von Sexualstadien, der Gametozyten. Dieses Parasitenstadium ist in der Lage im Mitteldarm der Mücke zu überleben und sich zu Gameten zu entwickeln, gefolgt von Befruchtung und ygotenbildung. Eine Vielzahl von in den Sexualstadien exprimierter Proteine wurde bereits entdeckt. Einige von diesen haben essentielle Funktionen für die Transmission der Parasiten auf die Mücke. Die Rolle der meisten dieser spezifisch exprimierter Protein ist jedoch ungeklärt. Zu den sexualstadienspezifischen Proteinen gehören die Proteine der PfCCp-Proteinfamilie. Für vier Proteine diese Proteinfamilie wurden bereits KO-Mutanten untersucht. Zwei Mutanten, PfCCp2-KO und PfCCp3-KO besitzen eine wichtige Funktion während der Entwicklung der Parasiten in der Mücke. In der vorliegenden Arbeit wurde die Studie der PfCCp-Proteine komplettiert. PfCCp5- und PfFNPA-defiziente Parasitenlinien wurden zu einem Großteil charakterisiert. Viele Eigenschaften dieser beiden Parasitenlinien wiesen Ähnlichkeiten zu den bisher untersuchten PfCCp-KO-Mutanten auf. Die ko-abhängige Expression welche in der PfCCp-Proteinfamilie vorkommt, wurde auch in diesen beiden Mutanten beobachtet, wenngleich in geringerem Ausmaß. In den Mutanten, in welchem entweder PfCCp5 oder PfFNPA fehlten, waren alle übrigen PfCCp-Proteine nur in reduzierter Menge nachzuweisen. Diese ko-abhängige Expression ist ausschließlich auf dem Proteinlevel zu beobachten. Die Transkription der jeweiligen Gene hingegen ist unbeeinflusst. Zahlreiche Protein-Protein-Interaktionen finden zwischen den Proteinen der Proteinfamilie statt. The zuvor beschriebenen multimeren Proteinkomplexe schließen auch weitere sexualstadienspezifische Proteine ein, wie Pfs230, Pfs48/45 und Pfs25. Kürzlich wurde eine neue Komponente der PfCCp-basierten Multiproteinkomplexe identifiziert. Dieses Protein wurde PfWLP1 (WD repeat protein-like protein 1) genannt, da es mehrere WD40 repeat Domänen besitzt. In der vorliegenden Arbeit wurde das bisher unbeschriebene Protein mittels indirekter immunfluoreszenzstudien charakterisiert. PfWLP1 ist sowohl in asexuellen Blutstadien als auch in Gametozyten exprimiert. Nach der Gametenbildung und Fertilisation nimmt die Expression des Proteins ab. Ein weiteres Protein der Sexualstadien, welches in dieser Arbeit untersucht wurde, ist PfactinII. Es wurde gezeigt, dass dieses Protein ausschließlich in den Sexualstadien vorliegt. In Gametozyten ko-lokalisiert es mit Pfs230 und die korrekte Lokalisierung ist abhängig von der Anwesenheit von Pfs230. Mittels RT-PCR wurden mehrere Komponenten des inneren Membrankomplexes in Gametozyten nachgewiesen. Weiterhin wurden Transkripte für fünf der sechs Myosin-Gene, welche im Genom von P. falciparum exprimiert sind, nachgewiesen. Der Austritt der Gametozyten aus der Wirtszelle wurde auf ultrastruktureller Ebene mittels Transmissionselektronenmikroskopie untersucht. Hierbei wurde gezeigt, dass die Lyse der den Parasiten umgebenden Membranen von innen nach außen geschieht. Das heißt, dass zunächst die Membran der parasitophoren Vakuole (PVM) lysiert wird, und erst anschließend die Erythrozyten-Plasmamembran (RBCM). Als neuer Induktor der Gametozytenaktivierung wurde Nigericin identifiziert. Nigericin ist ein K+/H+-Ionophor, welcher in Abwesenheit von XA in der Lage ist, die Gametenbildung zu identifizieren. Die selektive Permeabilisierung der beiden den Gametozyten umgebenden Membranen, PVM und RBCM, zeigte, dass männliche Gametozyten nach Entfernung der beiden Membranen, in der Lage sind, den Temperaturabfall und XA zu perzipieren. Somit kann geschlussfolgert werden, dass die Rezeptoren beider Stimuli parasitischen Ursprungs sind. LC/MS/MS-Analysen bestätigten, dass Erythrozyten in der Lage sind, XA aufzunehmen. Die Sexualstadien des Malariaparasiten nehmen mehr und mehr an Bedeutung zu, da langfristig nicht nur eine Eindämmung der Malaria in endemischen Gebieten sondern die Auslöschung der Malaria angestrebt wird. Die Sexualstadien sind ein attraktiver Angriffspunkt aufgrund ihrer Bedeutung für die Transmission der Krankheit. Zum anderen ist die auf den Vektor übertragene Parasitenanzahl vergleichsweise gering. Die Ergebnisse der vorliegenden Arbeit zeigen mehrere potentielle Kandidatenproteine auf, welche für die Entwicklung von Interventionsstrategien von Bedeutung sein könnten. Als Interventionsstrategien wären sowohl transmissionsblockierenden Vakzine als auch transmissionsblockierende Wirkstoffe denkbar. KW - Malaria KW - Multiproteinkomplex KW - Gametocyt KW - Gametogenese KW - Plasmodium falciparum KW - malaria KW - Plasmodium falciparum KW - gametogenesis KW - co-dependent expression KW - gametocyt Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-98028 ER - TY - JOUR A1 - Alsheimer, Manfred A1 - Link, Jana A1 - Jahn, Daniel A1 - Schmitt, Johannes A1 - Göb, Eva A1 - Baar, Johannes A1 - Ortega, Sagrario A1 - Benavente, Ricardo T1 - The Meiotic Nuclear Lamina Regulates Chromosome Dynamics and Promotes Efficient Homologous Recombination in the Mouse JF - PLoS Genetics N2 - The nuclear lamina is the structural scaffold of the nuclear envelope and is well known for its central role in nuclear organization and maintaining nuclear stability and shape. In the past, a number of severe human disorders have been identified to be associated with mutations in lamins. Extensive research on this topic has provided novel important clues about nuclear lamina function. These studies have contributed to the knowledge that the lamina constitutes a complex multifunctional platform combining both structural and regulatory functions. Here, we report that, in addition to the previously demonstrated significance for somatic cell differentiation and maintenance, the nuclear lamina is also an essential determinant for germ cell development. Both male and female mice lacking the short meiosis-specific A-type lamin C2 have a severely defective meiosis, which at least in the male results in infertility. Detailed analysis revealed that lamin C2 is required for telomere-driven dynamic repositioning of meiotic chromosomes. Loss of lamin C2 affects precise synapsis of the homologs and interferes with meiotic double-strand break repair. Taken together, our data explain how the nuclear lamina contributes to meiotic chromosome behaviour and accurate genome haploidization on a mechanistic level. KW - homologous chromosomes KW - homologous recombination KW - lamins KW - Oocytes KW - spermatocytes KW - synapsis KW - telomeres KW - testes Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96285 ER - TY - THES A1 - Reuß, Heiko T1 - The interplay of unconscious processing and cognitive control T1 - Das Zusammenspiel unbewusster Verarbeitung und kognitiver Kontrolle N2 - The aim of this study was both to investigate the influence of cognitive control on unconscious processing, and to investigate the influence of unconscious processing on cognitive control. At first, different mechanisms and accounts to explain unconscious priming are presented. Here, perceptual and motor processes, as well as stimulus-response learning, semantic categorization, and the action trigger account as theories to explain motor priming are discussed. Then, the issue of the potential limits of unconscious processing is presented. Findings that indicate that active current intentions and expertise modulate unconscious processing are illustrated. Subsequently, results that imply an influence of unconsciously presented stimuli that goes beyond motor processes are discussed, with a special focus on inhibition processes, orienting of attention, task set activation, and conflict adaptation. Then I present the results of my own empirical work. Experiment 1 shows that the effective processing of unconsciously presented stimuli depends on expertise, even when potentially confounding difference between the expert and novice groups are controlled. The results of Experiments 2 and 3 indicate that the intention to use particular stimuli is a crucial factor for the effectiveness of these stimuli when they are presented unconsciously. Additionally, these findings show that shifts of attention can be triggered by centrally presented masked arrow cues. Experiments 4 and 5 broaden these results to cue stimuli that are not inherently associated with a spatial meaning. The finding corroborate that typically endogenously controlled shifts of attention can also be induced by unconscious stimuli. Experiments 6 and 7 demonstrate that even a central cognitive control process like task set activation is not contingent on conscious awareness, but can in contrast be triggered through unconscious stimulation. Finally, these results are integrated and I discuss how the concept of cognitive control and the limits of unconscious processing may have to be reconsidered. Furthermore, potential future research possibilities in this field are presented. N2 - Das Ziel dieser Arbeit war es, sowohl den Einfluss von kognitiver Kontrolle auf unbewusste Verarbeitung, als auch den Einfluss unbewusster Verarbeitung auf kognitive Kontrolle zu untersuchen. Zunächst werden verschiedene Mechanismen und Ansätze zur Erklärung unbewusster Bahnung vorgestellt. Dabei werden perzeptuelle Prozesse sowie motorische Prozesse beleuchtet und mit Reiz-Reaktions-Verbindungen, semantischer Kategorisierung und dem Ansatz handlungsdeterminierender Reizerwartungen drei verschiedene Ansätze zur Erklärung motorischer Bahnung besprochen. Danach wird die Problematik der Grenzen unbewusster Verarbeitung dargestellt. Es werden Befunde vorgestellt, die Hinweise auf den Einfluss von aktiven Aufgabeneinstellungen sowie von Expertise auf unbewusste Verarbeitung geben. Als nächstes werden Ergebnisse besprochen, die einen über motorische Prozesse hinausgehenden Einfluss unbewusster Reize nahelegen. Dabei wird insbesondere auf den Einfluss auf Hemmprozesse, Aufmerksamkeitsausrichtung, die Aktivierung von Aufgabeneinstellungen und Konfliktadaptation eingegangen. Dann werden die Ergebnisse eigener empirischer Arbeiten vorgestellt. In Experiment 1 wurde gezeigt, dass die effektive Verarbeitung unbewusster Reize von Expertise abhängt, auch wenn sonstige Unterschiede zwischen Experten- und Novizen-Gruppen kontrolliert sind. Die Ergebnisse von Experiment 2 und 3 zeigten, dass die Absicht, bestimmte Reize zu nutzen, ein entscheidender Faktor dabei ist, ob diese Reize auch unbewusst einen Effekt entfalten können. Zudem wurde hier gezeigt, dass Aufmerksamkeitsverschiebungen durch zentral präsentierte, maskierte Pfeile ausgelöst werden können. Die Experimente 4 und 5 erweiterten diesen Befund auf Hinweisreize, die keine inhärente räumliche Bedeutung haben. Hier konnte bestätigt werden, dass eigentlich endogen gesteuerte Aufmerksamkeitsverschiebungen durch unbewusste Reize induziert werden können. Die Experimente 6 und 7 zeigten, dass selbst ein zentraler kognitiver Kontrollprozess wie die Aktivierung verschiedener Aufgabeneinstellungen nicht bewusstseinspflichtig ist, sondern im Gegenteil durch unbewusste Stimulation in Gang gesetzt werden kann. Letztendlich werden diese Ergebnisse zueinander in Beziehung gesetzt. Es wird diskutiert, inwiefern das Konzept kognitiver Kontrolle und die Grenzen unbewusster Verarbeitung neu betrachtet werden müssen. Außerdem werden mögliche zukünftige Forschungsfelder in diesem Bereich aufgezeigt. KW - Bewusstsein KW - unconscious processing KW - cognitive control KW - Kognitiver Prozess KW - Allgemeine Psychologie Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-76950 ER -