TY - JOUR A1 - Schartl, Manfred A1 - Shen, Yingjia A1 - Maurus, Katja A1 - Walter, Ron A1 - Tomlinson, Chad A1 - Wilson, Richard K. A1 - Postlethwait, John A1 - Warren, Wesley C. T1 - Whole body melanoma transcriptome response in medaka JF - PLoS ONE N2 - The incidence of malignant melanoma continues to increase each year with poor prognosis for survival in many relapse cases. To reverse this trend, whole body response measures are needed to discover collaborative paths to primary and secondary malignancy. Several species of fish provide excellent melanoma models because fish and human melanocytes both appear in the epidermis, and fish and human pigment cell tumors share conserved gene expression signatures. For the first time, we have examined the whole body transcriptome response to invasive melanoma as a prelude to using transcriptome profiling to screen for drugs in a medaka (Oryzias latipes) model. We generated RNA-seq data from whole body RNA isolates for controls and melanoma fish. After testing for differential expression, 396 genes had significantly different expression (adjusted p-value <0.02) in the whole body transcriptome between melanoma and control fish; 379 of these genes were matched to human orthologs with 233 having annotated human gene symbols and 14 matched genes that contain putative deleterious variants in human melanoma at varying levels of recurrence. A detailed canonical pathway evaluation for significant enrichment showed the top scoring pathway to be antigen presentation but also included the expected melanocyte development and pigmentation signaling pathway. Results revealed a profound down-regulation of genes involved in the immune response, especially the innate immune system. We hypothesize that the developing melanoma actively suppresses the immune system responses of the body in reacting to the invasive malignancy, and that this mal-adaptive response contributes to disease progression, a result that suggests our whole-body transcriptomic approach merits further use. In these findings, we also observed novel genes not yet identified in human melanoma expression studies and uncovered known and new candidate drug targets for further testing in this malignant melanoma medaka model. KW - metastatic melanoma KW - expression KW - fish KW - cancer KW - stage III KW - melanogenesis KW - genome cells KW - gene KW - contributes Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-144714 VL - 10 IS - 12 ER - TY - THES A1 - Gnamlin, Prisca T1 - Use of Tumor Vasculature for Successful Treatment of Carcinomas by Oncolytic Vaccinia Virus T1 - Die Tumorvasulatur in der erfolgreichen Therapie von Carcinomen durch onkolytische Vaccinia Viren N2 - Tumor-induced angiogenesis is of major interest for oncology research. Vascular endothelial growth factor (VEGF) is the most potent angiogenic factor characterized so far. VEGF blockade was shown to be sufficient for angiogenesis inhibition and subsequent tumor regression in several preclinical tumor models. Bevacizumab was the first treatment targeting specifically tumor-induced angiogenesis through VEGF blockade to be approved by the Food and Drugs Administration (FDA) for cancer treatment. However, after very promising results in preclinical evaluations, VEGF blockade did not show the expected success in patients. Some tumors became resistant to VEGF blockade. Several factors have been accounted responsible, the over-expression of other angiogenic factors, the noxious influence of VEFG blockade on normal tissues, the selection of hypoxia resistant neoplastic cells, the recruitment of hematopoietic progenitor cells and finally the transient nature of angiogenesis inhibition by VEGF blockade. The development of blocking agents against other angiogenic factors like placental growth factor (PlGF) and Angiopoietin-2 (Ang-2) allows the development of an anti-angiogenesis strategy adapted to the profile of the tumor. Oncolytic virotherapy uses the natural propensity of viruses to colonize tumors to treat cancer. The recombinant vaccinia virus GLV-1h68 was shown to infect, colonize and lyse several tumor types. Its descendant GLV-1h108, expressing an anti-VEGF antibody, was proved in previous studies to inhibit efficiently tumor induced angiogenesis. Additional VACVs expressing single chain antibodies (scAb) antibodies against PlGF and Ang-2 alone or in combination with anti VEGF scAb were designed. In this study, VACV-mediated anti-angiogenesis treatments have been evaluated in several preclinical tumor models. The efficiency of PlGF blockade, alone or in combination with VEGF, mediated by VACV has been established and confirmed. PlGF inhibition alone or with VEGF reduced tumor burden 5- and 2-folds more efficiently than the control virus, respectively. Ang-2 blockade efficiency for cancer treatment gave controversial results when tested in different laboratories. Here we demonstrated that unlike VEGF, the success of Ang-2 blockade is not only correlated to the strength of the blockade. A particular balance between Ang-2, VEGF and Ang-1 needs to be induced by the treatment to see a regression of the tumor and an improved survival. We saw that Ang-2 inhibition delayed tumor growth up to 3-folds compared to the control virus. These same viruses induced statistically significant tumor growth delays. This study unveiled the need to establish an angiogenic profile of the tumor to be treated as well as the necessity to better understand the synergic effects of VEGF and Ang-2. In addition angiogenesis inhibition by VACV-mediated PlGF and Ang-2 blockade was able to reduce the number of metastases and migrating tumor cells (even more efficiently than VEGF blockade). VACV colonization of tumor cells, in vitro, was limited by VEGF, when the use of the anti-VEGF VACV GLV-1h108 drastically improved the colonization efficiency up to 2-fold, 72 hours post-infection. These in vitro data were confirmed by in vivo analysis of tumors. Fourteen days post-treatment, the anti-VEGF virus GLV-1h108 was colonizing 78.8% of the tumors when GLV-1h68 colonization rate was 49.6%. These data confirmed the synergistic effect of VEGF blockade and VACV replication for tumor regression. Three of the tumor cell lines used to assess VACV-mediated angiogenesis inhibition were found, in certain conditions, to mimic either endothelial cell or pericyte functions, and participate directly to the vascular structure. The expression by these tumor cells of e-selectin, p-selectin, ICAM-1 and VCAM-1, normally expressed on activated endothelial cells, corroborates our findings. These proteins play an important role in immune cell recruitment, and there amount vary in presence of VEGF, PlGF and Ang-2, confirming the involvement of angiogenic factors in the immuno-modulatory abilities of tumors. In this study VACV-mediated angiogenesis blockade proved its potential as a therapeutic agent able to treat different tumor types and prevent resistance observed during bevacizumab treatment by acting on different factors. First, the expression of several antibodies by VACV would prevent another angiogenic factor to take over VEGF and stimulate angiogenesis. Then, the ability of VACV to infect tumor cells would prevent them to form blood vessel-like structures to sustain tumor growth, and the localized delivery of the antibody would decrease the risk of adverse effects. Next, the blockade of angiogenic factors would improve VACV replication and decrease the immune-modulatory effect of tumors. Finally the fact that angiogenesis blockade lasts until total regression of the tumor would prevent the recovery of the tumor-associated vasculature and the relapse of patients. N2 - Ein Hauptinteresse der onkologischen Forschung liegt auf dem Verständnis der Tumor-induzierten Angiogenese. Es wurde bereits festgestellt, dass die meisten Tumortypen eine abnorme Expression angiogener Faktoren zeigen. Der vascular endothelial growth factor (VEGF) wurde als der effektivste angiogene Faktor beschrieben. Es wurde gezeigt, dass die Hemmung des VEGF zur Inhibition der Angiogenese führt, das wiederum zu Tumorregression in vorklinischen Tumormodellen führte. Bevacizumab ist das erste FDA zugelassene Krebs-Therapeutikum, welches spezifisch auf die Tumor-induzierte Angiogenese durch VEGF-Inhibition abzielt. Der erwartete Erfolg durch VEGF-Hemmung konnte im Patienten allerdings nicht erzielt werden. Die Entwicklung von neuen Angiogenese hemmenden Stoffen wie gegen den placental growth factor (PIGF) oder Angiopoietin-2 (Ang-2), ermöglichen eine an das Tumor-Profil angepasste anti-angiogene Strategie. Die onkolytische Virustherapie die natürliche Eigenschaft der Viren Tumore zu kolonisieren. Das Vaccinia-Virus (VACV) gehört zur Familie der Poxviridae und wurde bereits lange Zeit als Vakzin zur Immunisierung gegen Pocken eingesetzt. Es konnte gezeigt werden, dass das rekombinante VACV GLV-1h68 effizient verschiedene Tumortypen infiziert, kolonisiert und lysiert. Das VACV GLV-1h108, welches auf der Basis des GLV-1h68 generiert wurde, kodiert einen anti-VEGF Antikörper. Dieses Virus ist in der Lage ist die Tumor-induzierte Angiogenese effizient zu inhibieren. Zusätzlich zu diesem VACV wurden weitere Konstrukte kloniert, welche für Antikörper gegen PIGF und Ang-2 kodieren. Zusätzlich wurden Virusstämme konstruiert, die gleichzeitig zwei Angiogenesefaktoren anzielen. Es wurde verschiedene VACV-vermittelte anti-Angiogenese Therapien in vorklinischen Tumormodellen wie Lungenadenokarzinome, KolonKarzinom, Melanom und Lungenadenokarzinome evaluiert. Die Effizienz der VACV-vermittelten Hemmung von PIGF und Ang-2, singulär oder in Kombination mit VEGF, wurde mit Tumor-Xenotransplantaten ermittelt. Die Inhibition von PlGF alleine oder in Kombination mit VEGF reduzierten die Tumorbelastung bis zu fünf, beziehungsweise zwei mal effizienter als GLV-1h68. Weiterhin wurde gezeigt, dass anders als VEGF, der Erfolg der Ang-2 Hemmung nicht nur mit der Stärke der Hemmung korreliert. Um Tumorregression sowie eine verbesserte Überlebensrate zu verursachen muss eine Balance zwischen Ang-2, VEGF und Ang-1 induziert werden. GLV-1h68 behandelte Tumore waren drei mal gröβer als Tumore, die mit den anti-Ang2 exprimierenden Viren behandelt wurden. Dieselben Virusstämme verursachten eine erhebliche Verspätung des Wachstums der Tumoren. Ausserdem hat diese Arbeit die Notwendigkeit enthüllt, ein angiogenes Profil des zu behandelnden Tumors zu etablieren sowie den Bedarf die synergistischen Effekte von VEGF und Ang-2 besser zu verstehen. Durch die Inhibition der Angiogenese durch VACV-verursachte PIGF und Ang-2 Hemmung wurde die Anzahl der Metastasen und der migrierenden Tumorzellen reduziert. Es wurde gezeigt, dass VEGF die VACV-Kolonisierung von Tumorzellen limitiert, da der Einsatz eines anti-VEGF VACV zu einer Verbesserung der Kolonisierung führt. In vivo Analysen bestätigten diese in vitro Daten. Nach vierzehn Tagen kolonisierte das anti-VEGF Virus 78,85% der Tumoren während die Kolonizationsquote des Kontrollviruses 49,64 % war. Dies resultierte in Tumorregression. Drei der getesteten Tumorzelllinien, in welchen die VACV-vermittelte Angiogenese-Inhibition untersucht wurde, waren in der Lage als Teil der Vaskulatur zu fungieren. Die Expression von Adhäsionsproteinen in diesen Tumorzellen untermauert die Ergebnisse. Weiterhin konnte ein unterschiedliches Expressionsmuster in Anwesenheit von VEGF, PIGF und Ang-2 festgestellt werden, wodurch die Beteiligung angiogener Faktoren bei den immunmodulatorischen Eigenschaften von Tumoren gezeigt werden konnte. In dieser Arbeit konnte gezeigt werden, dass eine VACV-vermittelte anti-angiogene Behandlung für verschiedene Tumorvarianten erfolgsversprechend ist. Die Möglichkeit verschiedene Antikörper gegen unterschiedliche angiogene Faktoren zu exprimieren würde verhindern, dass diese die Angiogenese stimulierende Wirkung des VEGF übernehmen. Die Eigenschaft von VACV Tumorzellen zu infizieren verhindert, dass diese Blutgefäß-ähnliche Strukturen bilden, welche das Tumorwachstum gewährleisten würde. Weiterhin würde die lokal begrenzte Antikörper-Freisetzung das Risiko von Nebenwirkungen senken. Die Inhibition angiogener Faktoren würde die VACV Replikationsrate steigern und den immunmodulatorischen Effekt der Tumore abschwächen. Letztlich würde die Hemmung der Angiogenese bis zur völligen Regression des Tumors aufrechterhalten, die Neubildung Tumor-assoziierter Vaskulatur verhindern und somit den Rückfall des Patienten. KW - Vaccinia-Virus KW - cancer KW - vaccinia virus KW - virotherapy KW - tumor vascularization KW - oncolytic virotherapy KW - Onkolyse KW - Angiogenese Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119019 ER - TY - JOUR A1 - Paschke, Ralf A1 - Lincke, Thomas A1 - Müller, Stefan P. A1 - Kreissl, Michael C. A1 - Dralle, Henning A1 - Fassnacht, Martin T1 - The Treatment of Well-Differentiated Thyroid Carcinoma JF - Deutsches Ärzteblatt International N2 - Background: Recent decades have seen a rise in the incidence of well-differentiated (mainly papillary) thyroid carcinoma around the world. In Germany, the age-adjusted incidence of well-differentiated thyroid carcinoma in 2010 was 3.5 per 100 000 men and 8.7 per 100 000 women per year. Method: This review is based on randomized, controlled trials and multicenter trials on the treatment of well-differentiated thyroid carcinoma that were retrieved by a selective literature search, as well as on three updated guidelines issued in the past two years. Results: The recommended extent of surgical resection depends on whether the tumor is classified as low-risk or high-risk, so that papillary microcar cinomas, which carry a highly favorable prognosis, will not be overtreated. More than 90% of localized, well-differentiated thyroid carcinomas can be cured with a combination of surgery and radioactive iodine therapy. Radio active iodine therapy is also effective in the treatment of well-differentiated thyroid carcinomas with distant metastases, yielding a 10-year survival rate of 90%, as long as there is good iodine uptake and the tumor goes into remission after treatment; otherwise, the 10-year survival rate is only 10%. In the past two years, better treatment options have become available for radioactive-iodine-resistant thyroid carcinoma. Phase 3 studies of two different tyrosine kinase inhibitors have shown that either one can markedly prolong progression-free survival, but not overall survival. Their more common clinically significant side effects are hand-foot syndrome, hypertension, diarrhea, proteinuria, and weight loss. Conclusion: Slow tumor growth, good resectability, and susceptibility to radioactive iodine therapy lend a favorable prognosis to most cases of well-differentiated thyroid carcinoma. The treatment should be risk-adjusted and interdisciplinary, in accordance with the current treatment guidelines. Even metastatic thyroid carcinoma has a favorable prognosis as long as there is good iodine uptake. The newly available medical treatment options for radioactive-iodine-resistant disease need to be further studied. KW - BRAF(V600E) mutation KW - distant metastases KW - papillary KW - guidelines KW - surgery KW - dissection KW - management KW - association KW - cancer KW - radioiodine therapy Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151636 VL - 112 SP - 452 EP - 458 ER - TY - JOUR A1 - Adelfinger, Marion A1 - Bessler, Simon A1 - Cecil, Alexander A1 - Langbein-Laugwitz, Johanna A1 - Frentzen, Alexa A1 - Gentschev, Ivaylo A1 - Szalay, Aladar A. T1 - Preclinical Testing Oncolytic Vaccinia Virus Strain GLV-5b451 Expressing an Anti-VEGF Single-Chain Antibody for Canine Cancer Therapy JF - Viruses N2 - Virotherapy on the basis of oncolytic vaccinia virus (VACV) strains is a novel approach for canine cancer therapy. Here we describe, for the first time, the characterization and the use of VACV strain GLV-5b451 expressing the anti-vascular endothelial growth factor (VEGF) single-chain antibody (scAb) GLAF-2 as therapeutic agent against different canine cancers. Cell culture data demonstrated that GLV-5b451 efficiently infected and destroyed all four tested canine cancer cell lines including: mammary carcinoma (MTH52c), mammary adenoma (ZMTH3), prostate carcinoma (CT1258), and soft tissue sarcoma (STSA-1). The GLV-5b451 virus-mediated production of GLAF-2 antibody was observed in all four cancer cell lines. In addition, this antibody specifically recognized canine VEGF. Finally, in canine soft tissue sarcoma (CSTS) xenografted mice, a single systemic administration of GLV-5b451 was found to be safe and led to anti-tumor effects resulting in the significant reduction and substantial long-term inhibition of tumor growth. A CD31-based immuno-staining showed significantly decreased neo-angiogenesis in GLV-5b451-treated tumors compared to the controls. In summary, these findings indicate that GLV-5b451 has potential for use as a therapeutic agent in the treatment of CSTS. KW - canine cancer therapy KW - canine soft tissue sarcoma (CSTS) KW - oncolytic virus KW - cancer KW - canine cancer cell lines KW - antibody production KW - angiogenesis Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125705 VL - 7 ER - TY - JOUR A1 - Elkon, Ran A1 - Loayza-Puch, Fabricio A1 - Korkmaz, Gozde A1 - Lopes, Rui A1 - van Breugel, Pieter C A1 - Bleijerveld, Onno B A1 - Altelaar, AF Maarten A1 - Wolf, Elmar A1 - Lorenzin, Francesca A1 - Eilers, Martin A1 - Agami, Reuven T1 - Myc coordinates transcription and translation to enhance transformation and suppress invasiveness JF - EMBO reports N2 - c‐Myc is one of the major human proto‐oncogenes and is often associated with tumor aggression and poor clinical outcome. Paradoxically, Myc was also reported as a suppressor of cell motility, invasiveness, and metastasis. Among the direct targets of Myc are many components of the protein synthesis machinery whose induction results in an overall increase in protein synthesis that empowers tumor cell growth. At present, it is largely unknown whether beyond the global enhancement of protein synthesis, Myc activation results in translation modulation of specific genes. Here, we measured Myc‐induced global changes in gene expression at the transcription, translation, and protein levels and uncovered extensive transcript‐specific regulation of protein translation. Particularly, we detected a broad coordination between regulation of transcription and translation upon modulation of Myc activity and showed the connection of these responses to mTOR signaling to enhance oncogenic transformation and to the TGFβ pathway to modulate cell migration and invasiveness. Our results elucidate novel facets of Myc‐induced cellular responses and provide a more comprehensive view of the consequences of its activation in cancer cells. KW - c‐Myc KW - transcriptional responses KW - translational regulation KW - transcription KW - transformation KW - metastasis KW - cancer KW - protein biosynthesis & quality control Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-150373 VL - 16 IS - 12 ER - TY - JOUR A1 - Hausmann, Stefan A1 - Brandt, Evelyn A1 - Köchel, Carolin A1 - Einsele, Hermann A1 - Bargou, Ralf C. A1 - Seggewiss-Bernhardt, Ruth A1 - Stühmer, Thorsten T1 - Loss of serum and glucocorticoid-regulated kinase 3 (SGK3) does not affect proliferation and survival of multiple myeloma cell lines JF - PLoS ONE N2 - Multiple myeloma (MM) is a generally fatal plasma cell cancer that often shows activation of the phosphoinositide 3-kinase/Akt (PI3K/Akt) pathway. Targeted pharmacologic therapies, however, have not yet progressed beyond the clinical trial stage, and given the complexity of the PI3K/Akt signalling system (e.g. multiple protein isoforms, diverse feedback regulation mechanisms, strong variability between patients) it is mandatory to characterise its ramifications in order to better guide informed decisions about the best therapeutic approaches. Here we explore whether serum and glucocorticoid-regulated kinase 3 (SGK3), a potential downstream effector of PI3K, plays a role in oncogenic signalling in MM cells-either in concert with or independent of Akt. SGK3 was expressed in all MM cell lines and in all primary MM samples tested. Four MM cell lines representing a broad range of intrinsic Akt activation (very strong: MM. 1s, moderate: L 363 and JJN-3, absent: AMO-1) were chosen to test the effects of transient SGK3 knockdown alone and in combination with pharmacological inhibition of Akt, PI3K-p110\(\alpha\), or in the context of serum starvation. Although the electroporation protocol led to strong SGK3 depletion for at least 5 days its absence had no substantial effect on the activation status of potential downstream substrates, or on the survival, viability or proliferation of MM cells in all experimental contexts tested. We conclude that it is unlikely that SGK3 plays a significant role for oncogenic signalling in multiple myeloma. KW - Akt KW - phosphorylation KW - downstream KW - mechanism KW - pathway KW - isoforms KW - activation KW - cancer KW - inhibition KW - phosphatidylinositol 3-kinase/Akt Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148708 VL - 10 IS - 4 ER - TY - JOUR A1 - Philipp-Abbrederis, Kathrin A1 - Herrmann, Ken A1 - Knop, Stefan A1 - Schottelius, Margret A1 - Eiber, Matthias A1 - Lückerath, Katharina A1 - Pietschmann, Elke A1 - Habringer, Stefan A1 - Gerngroß, Carlos A1 - Franke, Katharina A1 - Rudelius, Martina A1 - Schirbel, Andreas A1 - Lapa, Constantin A1 - Schwamborn, Kristina A1 - Steidle, Sabine A1 - Hartmann, Elena A1 - Rosenwald, Andreas A1 - Kropf, Saskia A1 - Beer, Ambros J A1 - Peschel, Christian A1 - Einsele, Hermann A1 - Buck, Andreas K A1 - Schwaiger, Markus A1 - Götze, Katharina A1 - Wester, Hans-Jürgen A1 - Keller, Ulrich T1 - In vivo molecular imaging of chemokine receptor CXCR4 expression in patients with advanced multiple myeloma JF - EMBO Molecular Medicine N2 - CXCR4 is a G-protein-coupled receptor that mediates recruitment of blood cells toward its ligand SDF-1. In cancer, high CXCR4 expression is frequently associated with tumor dissemination andpoor prognosis. We evaluated the novel CXCR4 probe [\(^{68}\)Ga]Pentixafor for invivo mapping of CXCR4 expression density in mice xenografted with human CXCR4-positive MM cell lines and patients with advanced MM by means of positron emission tomography (PET). [\(^{68}\)Ga]Pentixafor PET provided images with excellent specificity and contrast. In 10 of 14 patients with advanced MM [\(^{68}\)Ga]Pentixafor PET/CT scans revealed MM manifestations, whereas only nine of 14 standard [\(^{18}\)F]fluorodeoxyglucose PET/CT scans were rated visually positive. Assessment of blood counts and standard CD34\(^{+}\) flow cytometry did not reveal significant blood count changes associated with tracer application. Based on these highly encouraging data on clinical PET imaging of CXCR4 expression in a cohort of MM patients, we conclude that [\(^{68}\)Ga]Pentixafor PET opens a broad field for clinical investigations on CXCR4 expression and for CXCR4-directed therapeutic approaches in MM and other diseases. KW - FDG PET/CT KW - cells KW - CXCR4/SDF-1 KW - CXCR4 KW - multiple myeloma KW - positron emission tomography KW - chemokine receptor KW - in vivo imaging KW - malignancies KW - involvement KW - microenvironment KW - survival KW - cancer KW - autologous transplantation KW - bone disease Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148738 VL - 7 IS - 4 ER - TY - JOUR A1 - Leikam, C A1 - Hufnagel, AL A1 - Otto, C A1 - Murphy, DJ A1 - Mühling, B A1 - Kneitz, S A1 - Nanda, I A1 - Schmid, M A1 - Wagner, TU A1 - Haferkamp, S A1 - Bröcker, E-B A1 - Schartl, M A1 - Meierjohann, S T1 - In vitro evidence for senescent multinucleated melanocytes as a source for tumor-initiating cells JF - Cell Death and Disease N2 - Oncogenic signaling in melanocytes results in oncogene-induced senescence (OIS), a stable cell-cycle arrest frequently characterized by a bi-or multinuclear phenotype that is considered as a barrier to cancer progression. However, the long-sustained conviction that senescence is a truly irreversible process has recently been challenged. Still, it is not known whether cells driven into OIS can progress to cancer and thereby pose a potential threat. Here, we show that prolonged expression of the melanoma oncogene N-RAS\(^{61K}\) in pigment cells overcomes OIS by triggering the emergence of tumor-initiating mononucleated stem-like cells from senescent cells. This progeny is dedifferentiated, highly proliferative, anoikis-resistant and induces fast growing, metastatic tumors. Our data describe that differentiated cells, which are driven into senescence by an oncogene, use this senescence state as trigger for tumor transformation, giving rise to highly aggressive tumor-initiating cells. These observations provide the first experimental in vitro evidence for the evasion of OIS on the cellular level and ensuing transformation. KW - reactive oxygen KW - human melanoma KW - MITF KW - cancer KW - skin KW - DNA damage KW - kappa-B KW - oncogene-induced senescence KW - cellular senescence Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148718 VL - 6 IS - e1711 ER - TY - JOUR A1 - Kumar, Praveen A1 - Naumann, Ulrike A1 - Aigner, Ludwig A1 - Wischhusen, Joerg A1 - Beier, Christoph P A1 - Beier, Dagmar T1 - Impaired TGF-β induced growth inhibition contributes to the increased proliferation rate of neural stem cells harboring mutant p53 JF - American Journal of Cancer Research N2 - Gliomas have been classified according to their histological properties. However, their respective cells of origin are still unknown. Neural progenitor cells (NPC) from the subventricular zone (SVZ) can initiate tumors in murine models of glioma and are likely cells of origin in the human disease. In both, p53 signaling is often functionally impaired which may contribute to tumor formation. Also, TGF-beta, which under physiological conditions exerts a strong control on the proliferation of NPCs in the SVZ, is a potent mitogen on glioma cells. Here, we approach on the crosstalk between p53 and TGF-beta by loss of function experiments using NPCs derived from p53 mutant mice, as well as pharmacological inhibition of TGF-beta signaling using TGF-beta receptor inhibitors. NPC derived from p53 mutant mice showed increased clonogenicity and more rapid proliferation than their wildtype counterparts. Further, NPC derived from p53\(^{mut/mut}\) mice were insensitive to TGF-beta induced growth arrest. Still, the canonical TGF-beta signaling pathway remained functional in the absence of p53 signaling and expression of key proteins as well as phosphorylation and nuclear translocation of SMAD2 were unaltered. TGF-beta-induced p21 expression could, in contrast, only be detected in p53\(^{wt/wt}\) but not in p53\(^{mut/mut}\) NPC. Conversely, inhibition of TGF-beta signaling using SB431542 increased proliferation of p53\(^{wt/wt}\) but not of p53\(^{mut/mut}\) NPC. In conclusion, our data suggest that the TGF-beta induced growth arrest in NPC depends on functional p53. Mutational inactivation of p53 hence contributes to increased proliferation of NPC and likely to the formation of hyperplasia of the SVZ observed in p53 deficient mice in vivo. KW - mouse brain KW - tumors KW - cancer KW - TGF-beta KW - glioblastoma stem cell KW - pathways KW - expression KW - astrocytoma KW - glioblastoma KW - transforming growth factor-beta-1 KW - neurogenesis KW - gliomas KW - neural stem cell KW - p53 KW - subventricular zone KW - premalignant lesion Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-144262 VL - 5 IS - 11 ER - TY - THES A1 - Wolter, Patrick T1 - Characterization of the mitotic localization and function of the novel DREAM target GAS2L3 and Mitotic kinesins are regulated by the DREAM complex, often up-regulated in cancer cells, and are potential targets for anti-cancer therapy T1 - Charakterisierung der mitotischen Lokalisation und Funktion von GAS2L3, eines kürzlich gefundenen Zielgens des DREAM Komplexes und Mitotische Kinesine werden vom DREAM Komplex reguliert, sind in Krebszellen häufig hochreguliert und sind potentielle Zielle für die Krebstherapie N2 - The recently discovered human DREAM complex (for DP, RB-like, E2F and MuvB complex) is a chromatin-associated pocket protein complex involved in cell cycle- dependent gene expression. DREAM consists of five core subunits and forms a complex either with the pocket protein p130 and the transcription factor E2F4 to repress gene expression or with the transcription factors B-MYB and FOXM1 to promote gene expression. Gas2l3 was recently identified by our group as a novel DREAM target gene. Subsequent characterization in human cell lines revealed that GAS2L3 is a microtubule and F-actin cross-linking protein, expressed in G2/M, plays a role in cytokinesis, and is important for chromosomal stability. The aim of the first part of the study was to analyze how expression of GAS2L3 is regulated by DREAM and to provide a better understanding of the function of GAS2L3 in mitosis and cytokinesis. ChIP assays revealed that the repressive and the activating form of DREAM bind to the GAS2L3 promoter. RNA interference (RNAi) mediated GAS2L3 depletion demonstrated the requirement of GAS2L3 for proper cleavage furrow ingression in cytokinesis. Immunofluorescence-based localization studies showed a localization of GAS2L3 at the mitotic spindle in mitosis and at the midbody in cytokinesis. Additional experiments demonstrated that the GAS2L3 GAR domain, a putative microtubule- binding domain, is responsible for GAS2L3 localization to the constriction zones in cytokinesis suggesting a function for GAS2L3 in the abscission process. DREAM is known to promote G2/M gene expression. DREAM target genes include several mitotic kinesins and mitotic microtubule-associated proteins (mitotic MAPs). However, it is not clear to what extent DREAM regulates mitotic kinesins and MAPs, so far. Furthermore, a comprehensive study of mitotic kinesin expression in cancer cell lines is still missing. Therefore, the second major aim of the thesis was to characterize the regulation of mitotic kinesins and MAPs by DREAM, to investigate the expression of mitotic kinesins in cancer cell line panels and to evaluate them as possible anti-cancer targets. ChIP assays together with RNAi mediated DREAM subunit depletion experiments demonstrated that DREAM is a master regulator of mitotic kinesins. Furthermore, expression analyses in a panel of breast and lung cancer cell lines revealed that mitotic kinesins are up-regulated in the majority of cancer cell lines in contrast to non-transformed controls. Finally, an inducible lentiviral-based shRNA system was developed to effectively deplete mitotic kinesins. Depletion of selected mitotic kinesins resulted in cytokinesis failures and strong anti-proliferative effects in several human cancer cell lines. Thus, this system will provide a robust tool for future investigation of mitotic kinesin function in cancer cells. N2 - Der vor kurzem entdeckte humane DREAM Komplex (für DP,RB ähnlich, E2F und MuvB Komplex) ist ein Chromatin bindender Pocket-Protein-Komplex involviert in Zellzyklusphase abhängiger Genregulation. DREAM besteht aus fünf Kernproteinen, die entweder zusammen mit dem Pocket-Protein p130 und dem Transkriptionsfaktor E2F4 die Genexpression reprimieren oder zusammen mit den Transkriptionsfaktoren B-MYB und FOXM1 die Genexpression fördern. GAS2L3 wurde vor kurzem als neues Zielgen des DREAM Komplexes identifiziert. Eine anschließende Charakterisierung in humanen Zelllinien offenbarte, dass GAS2L3 in der Lage ist, das F-Aktin und das Mikrotubuli Cytoskelett zu binden und zu vernetzen. Außerdem ist GAS2L3 speziell während der G2/M Phase exprimiert, spielt eine Rolle in der Cytokinese und ist wichtig für die genomische Integrität. Der erste Teil der Arbeit hatte zum Ziel zu ergründen in welcher Art und Weise DREAM GAS2L3 reguliert. Außerdem sollte das Verständnis der Rolle von GAS2L3 in der Cytokinese erweitert werden. Hierzu durchgeführte ChIP Analysen zeigten, dass sowohl der reprimierende als auch der aktivierende DREAM Komplex an den Promoter von GAS2L3 bindet. Experimente, in denen GAS2L3 durch RNA-Interferenz (RNAi) depletiert wurde, demonstrierten, dass GAS2L3 in der Cytokinese am Prozess der Einschnürung der Teilungsfurche beteiligt ist. Anschließende auf Immunfluoreszenzmikroskopie basierende Lokalisationsstudien zeigten, dass GAS2L3 an der mitotischen Spindel in der Mitose und am Midbody in der Cytokinese lokalisiert ist. Weiterführende Studien zeigten, dass die GAR Domäne von GAS2L3, eine mutmaßliche Mikrotubuli- Bindedomäne, für die Lokalisierung von GAS2L3 in der für die Abszission wichtigen Konstriktionszone verantwortlich ist. Dieses Ergebnis lässt vermuten, dass GAS2L3 eine Rolle in diesem Prozess spielt. Der DREAM Komplex ist bekannt dafür G2/M Genexpression zu fördern. G2/M Zielgene des Komplexes sind unter anderem mehrere mitotische Kinesine und mitotische Mikrotubuli-Bindeproteine. Bisher ist die Art und Weise und das Ausmaß der Regulierung dieser Proteingruppen durch DREAM aber nur ungenügend untersucht worden. Des Weiteren fehlt bisher eine umfassende Charakterisierung der Expression von mitotischen Kinesinen in Krebszellen. Deswegen befasste sich der zweite Teil der Arbeit mit der Charakterisierung der Regulation von mitotischen Kinesinen und Mikrotubuli-Bindeproteinen durch DREAM, untersuchte die Expression dieser beiden Proteingruppen in Krebszelllinien und evaluierte diese anschließend als potentielle Ziele für die Krebstherapie. Eine Kombination aus ChIP Analysen und RNAi Experimenten zeigte, dass DREAM eine zentrale Rolle in der Regulierung von mitotischen Kinesinen spielt. Expressions- analysen deckten auf, dass mitotische Kinesine in der Mehrheit der Krebszelllinien hochreguliert sind im Gegensatz zu den nicht entarteten Kontrollzelllinien. Schließlich wurde ein auf Lentiviren basierendes induzierbares shRNA System etabliert, welches mitotische Kinesine effektiv herunterregulieren konnte. Depletion ausgewählter mitotischer Kinesine führte zu Fehlern in der Cytokinese und hatte starke Auswirkungen auf das Wachstumsverhalten von mehreren Krebszelllinien. Aufgrund dieser Erkenntnisse wird das lentivirale System eine solide Ausgangsbasis für zukünftige Untersuchungen von mitotischen Kinesinen in Krebszellen bilden. KW - Zellzyklus KW - GAS2L3 KW - B-MYB KW - DREAM KW - cytokinesis KW - mitosis KW - kinesin KW - cancer KW - FOXM1 KW - regulation KW - Zellteilung KW - Regulation KW - Krebs KW - Biologie / Zellbiologie Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122531 ER -