TY - JOUR A1 - Rossow, Leonie A1 - Veitl, Simona A1 - Vorlová, Sandra A1 - Wax, Jacqueline K. A1 - Kuhn, Anja E. A1 - Maltzahn, Verena A1 - Upcin, Berin A1 - Karl, Franziska A1 - Hoffmann, Helene A1 - Gätzner, Sabine A1 - Kallius, Matthias A1 - Nandigama, Rajender A1 - Scheld, Daniela A1 - Irmak, Ster A1 - Herterich, Sabine A1 - Zernecke, Alma A1 - Ergün, Süleyman A1 - Henke, Erik T1 - LOX-catalyzed collagen stabilization is a proximal cause for intrinsic resistance to chemotherapy JF - Oncogene N2 - The potential of altering the tumor ECM to improve drug response remains fairly unexplored. To identify targets for modification of the ECM aiming to improve drug response and overcome resistance, we analyzed expression data sets from pre-treatment patient cohorts. Cross-evaluation identified a subset of chemoresistant tumors characterized by increased expression of collagens and collagen-stabilizing enzymes. We demonstrate that strong collagen expression and stabilization sets off a vicious circle of self-propagating hypoxia, malignant signaling, and aberrant angiogenesis that can be broken by an appropriate auxiliary intervention: Interfering with collagen stabilization by inhibition of lysyl oxidases significantly enhanced response to chemotherapy in various tumor models, even in metastatic disease. Inhibition of collagen stabilization by itself can reduce or enhance tumor growth depending on the tumor type. The mechanistical basis for this behavior is the dependence of the individual tumor on nutritional supply on one hand and on high tissue stiffness for FAK signaling on the other. KW - Cancer models KW - Cancer therapeutic resistance KW - Targeted therapies KW - Tumour angiogenesis Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-227008 VL - 37 ER - TY - JOUR A1 - Jansch, Charline A1 - Günther, Katharina A1 - Waider, Jonas A1 - Ziegler, Georg C. A1 - Forero, Andrea A1 - Kollert, Sina A1 - Svirin, Evgeniy A1 - Pühringer, Dirk A1 - Kwok, Chee Keong A1 - Ullmann, Reinhard A1 - Maierhofer, Anna A1 - Flunkert, Julia A1 - Haaf, Thomas A1 - Edenhofer, Frank A1 - Lesch, Klaus-Peter T1 - Generation of a human induced pluripotent stem cell (iPSC) line from a 51-year-old female with attention-deficit/hyperactivity disorder (ADHD) carrying a duplication of SLC2A3 JF - Stem Cell Research N2 - Fibroblasts were isolated from a skin biopsy of a clinically diagnosed 51-year-old female attention-deficit/hyperactivity disorder (ADHD) patient carrying a duplication of SLC2A3, a gene encoding neuronal glucose transporter-3 (GLUT3). Patient fibroblasts were infected with Sendai virus, a single-stranded RNA virus, to generate transgene-free human induced pluripotent stem cells (iPSCs). SLC2A3-D2-iPSCs showed expression of pluripotency-associated markers, were able to differentiate into cells of the three germ layers in vitro and had a normal female karyotype. This in vitro cellular model can be used to study the role of risk genes in the pathogenesis of ADHD, in a patient-specific manner. KW - ADHD KW - SLC2A3 KW - induced pluripotent stem cells Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176654 VL - 28 ER - TY - JOUR A1 - Simon, Micha A1 - Ipek, Rojda A1 - Homola, György A. A1 - Rovituso, Damiano M. A1 - Schampel, Andrea A1 - Kleinschnitz, Christoph A1 - Kuerten, Stefanie T1 - Anti-CD52 antibody treatment depletes B cell aggregates in the central nervous system in a mouse model of multiple sclerosis JF - Journal of Neuroinflammation N2 - Background: Multiple sclerosis (MS) is a chronic autoimmune disease of the central nervous system (CNS) for which several new treatment options were recently introduced. Among them is the monoclonal anti-CD52 antibody alemtuzumab that depletes mainly B cells and T cells in the immune periphery. Considering the ongoing controversy about the involvement of B cells and in particular the formation of B cell aggregates in the brains of progressive MS patients, an in-depth understanding of the effects of anti-CD52 antibody treatment on the B cell compartment in the CNS itself is desirable. Methods: We used myelin basic protein (MBP)-proteolipid protein (PLP)-induced experimental autoimmune encephalomyelitis (EAE) in C57BL/6 (B6) mice as B cell-dependent model of MS. Mice were treated intraperitoneally either at the peak of EAE or at 60 days after onset with 200 μg murine anti-CD52 vs. IgG2a isotype control antibody for five consecutive days. Disease was subsequently monitored for 10 days. The antigen-specific B cell/antibody response was measured by ELISPOT and ELISA. Effects on CNS infiltration and B cell aggregation were determined by immunohistochemistry. Neurodegeneration was evaluated by Luxol Fast Blue, SMI-32, and Olig2/APC staining as well as by electron microscopy and phosphorylated heavy neurofilament serum ELISA. Results: Treatment with anti-CD52 antibody attenuated EAE only when administered at the peak of disease. While there was no effect on the production of MP4-specific IgG, the treatment almost completely depleted CNS infiltrates and B cell aggregates even when given as late as 60 days after onset. On the ultrastructural level, we observed significantly less axonal damage in the spinal cord and cerebellum in chronic EAE after anti-CD52 treatment. Conclusion: Anti-CD52 treatment abrogated B cell infiltration and disrupted existing B cell aggregates in the CNS. KW - Alemtuzumab KW - B cells KW - CD52 KW - CNS KW - EAE KW - MS Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-176120 VL - 15 IS - 225 ER - TY - JOUR A1 - Drenckhahn, Detlev A1 - Jansen, Werner A1 - Weber, Heinrich E. T1 - Rubus pseudoglotta Drenckhahn & W. Jansen, eine neue deutsch-dänische Brombeerart aus dem Formenkreis des Rubus phylloglotta (Frid.) Å. Gust. T1 - Rubus pseudoglotta Drenckhahn & W. Jansen, a new bramble species with German-Danish distribution related to R. phylloglotta (Frid.) Å. Gust. JF - Forum Geobotanicum N2 - Rubus pseudoglotta Drenckhahn & W. Jansen ist eine tetraploide Brombeerart aus der Sektion Corylifolii (Serie Subradula), die bisher zum Variabilitäts-Spektrum von R. phylloglotta (Frid.) Å. Gust. gezählt wurde. Charakteristische Merkmale sind die 4 (3–5)-zähligen Blätter mit obovaten Endblättchen mit kurzer (ca. 1 cm) abgesetzter Spitze, kurzhaariger Blattoberseite und fühlbar behaarter grüner Blattunterseite. Die flach bogigen, teils klimmenden Schösslinge sind überwiegend stumpfkantig, grün bis rötlichbraun, schwach behaart und reichlich mit 2–4 (5) mm langen, geraden bis schwach gekrümmten Stacheln und kleineren Stacheln, Stachelhöckern, Stieldrüsen und Borsten besetzt. Die Blütenstiele sind mit 2–8 (pro cm) schlanken, geraden bis leicht gekrümmten Stacheln (1–2 mm lang) und zahlreichen Stieldrüsen (teils bis 0,6 mm lang) besetzt. Die Sippe wächst bevorzugt an Straßen- und Wegrändern und in Hecken. Die bekannt gewordenen Fundstellen erstrecken sich von Rendsburg bis in das Umfeld von Kiel, nordwärts bis zu den dänischen Inseln Alsen und Fünen. Unsere Untersuchungen zeigen weiterhin, dass R. phylloglotta bisher nicht in Schleswig-Holstein/Deutschland nachgewiesen wurde. Ob R. phylloglotta überhaupt außerhalb der Insel Tåsinge in Dänemark vorkommt, bedarf weiterer Nachforschungen. N2 - Rubus pseudoglotta Drenckhahn & W. Jansen is a tetraploid new member of the Rubus section Corylifolii, series Subradula, which was formerly included in the variability spectrum of R. phylloglotta (Frid.) Å. Gust.. This new species is distinguished by 4 (3–5)-nate leaves with obovate acuminate to cuspidate terminal leaflets with short-haired upper side and light greenish tangibly hairy under side. Stems grow arcuate, partly climbing, are obtusely angled, moderately hairy, green to reddish brown coloured, and armed with 10–20 straight, slender prickles, 2–4 (5) mm long, numerous pricklets, stalked glands and bristlets. Pedicels of inflorescence are armed with 2–8 (per cm) slender straight to slightly curved prickles (1–2 mm long) and studded with numerous stalked glands (up to 0.6 mm long) and some bristles. The species prefers road sides and hedgerows. The distribution area of R. pseudoglotta, known so far, extends from the area between Rendsburg and the surroundings of the city of Kiel in Schleswig-Holstein and reaches north to the Danish islands of Als and Fyn. A further outcome of this study is that there is no safe record of R. phylloglotta in Schleswig-Holstein/Deutschland and that it is questionable whether R. phylloglotta occurs outside the island Tåsinge in Denmark at all. KW - Rubus pseudoglotta KW - Rubus phylloglotta KW - Sektion Corylifolii KW - Rubus KW - Species novum KW - false tongue-leaf blackberry KW - new species KW - genome size KW - distribution Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-174599 UR - http://www.forum-geobotanicum.net/articles/vol_8-2018/drenckhahn-jansen-weber_r_pseudoglotta/drenckhahn-jansen-weber_r_pseudoglotta.pdf SN - 1867-9315 VL - 8 ER - TY - JOUR A1 - Weber, Heinrich E. T1 - Nomenklatorische Korrektur in der Gattung Rubus T1 - Nomenclatural correction in the genus Rubus JF - Forum Geobotanicum N2 - Wegen des älteren Homonyms Rubus tilioides Gand. 1884 wird für Rubus tilioides W. Jansen & H. E. Weber 2010 der neue Name Rubus tiliifrons W. Jansen & H. E. Weber veröffentlicht. N2 - Because of the older homonym Rubus tilioides Gand. 1884 the name Rubus tiliifrons W. Jansen & H. E. Weber is established as new name for Rubus tilioides W. Jansen & H. E. Weber 2010. KW - Rubus L. sectio Corylifolii KW - Botanische Nomenklatur KW - Nomen novum KW - new name Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-174587 UR - http://www.forum-geobotanicum.net/articles/vol_8-2018/weber_rubus/weber_rubus-tiliifrons.pdf SN - 1867-9315 VL - 8 ER - TY - JOUR A1 - Nose, Naoko A1 - Werner, Rudolf A. A1 - Ueda, Yuichiro A1 - Günther, Katharina A1 - Lapa, Constantin A1 - Javadi, Mehrbod S. A1 - Fukushima, Kazuhito A1 - Edenhofer, Frank A1 - Higuchi, Takahiro T1 - Metabolic substrate shift in human induced pluripotent stem cells during cardiac differentiation: Functional assessment using in vitro radionuclide uptake assay JF - International Journal of Cardiology N2 - BACKGROUND: Recent developments in cellular reprogramming technology enable the production of virtually unlimited numbers of human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CM). Although hiPSC-CM share various characteristic hallmarks with endogenous cardiomyocytes, it remains a question as to what extent metabolic characteristics are equivalent to mature mammalian cardiomyocytes. Here we set out to functionally characterize the metabolic status of hiPSC-CM in vitro by employing a radionuclide tracer uptake assay. MATERIAL AND METHODS: Cardiac differentiation of hiPSC was induced using a combination of well-orchestrated extrinsic stimuli such as WNT activation (by CHIR99021) and BMP signalling followed by WNT inhibition and lactate based cardiomyocyte enrichment. For characterization of metabolic substrates, dual tracer uptake studies were performed with \(^{18}\)F‑2‑fluoro‑2‑deoxy‑d‑glucose (\(^{18}\)F-FDG) and \(^{125}\)I‑β‑methyl‑iodophenyl‑pentadecanoic acid (\(^{125}\)I-BMIPP) as transport markers of glucose and fatty acids, respectively. RESULTS: After cardiac differentiation of hiPSCs, in vitro tracer uptake assays confirmed metabolic substrate shift from glucose to fatty acids that was comparable to those observed in native isolated human cardiomyocytes. Immunostaining further confirmed expression of fatty acid transport and binding proteins on hiPSC-CM. CONCLUSIONS: During in vitro cardiac maturation, we observed a metabolic shift to fatty acids, which are known as a main energy source of mammalian hearts, suggesting hi-PSC-CM as a potential functional phenotype to investigate alteration of cardiac metabolism in cardiac diseases. Results also highlight the use of available clinical nuclear medicine tracers as functional assays in stem cell research for improved generation of autologous differentiated cells for numerous biomedical applications. KW - tracer KW - Stammzelle KW - induced pluripotent stem cells KW - cardiomyocytes KW - fatty acid KW - stem cell therapy KW - hiPSC-CM Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170699 VL - 269 ER - TY - THES A1 - Rehman, Saba T1 - Identification of accessible and closed substrate binding sites in the outward open cleft of rat Organic Cation Transporter 1 (rOCT1) T1 - Identifizierung von zugänglichen und unzugänglichen Substratbindungsstellen in der nach außen offenen Konformation des organischen Kationentransporters rOCT1 N2 - The present study was conducted on the rOCT1, a member of SLC22 family. Structurally, it consists of 12 membrane spanning α-helices with both N- and C-termini intracellular. Studies done so far, through tracer uptake and inhibition, reconstitution of rOCT1 in nanodiscs and proteoliposomes and voltage-clamp fluorometry, have identified the main amino acids in the cleft of rOCT1 that interact in a critical manner with the substrates/inhibitors either directly or indirectly. Homology modeling studies have also supported these observations. In the present study we aimed at measuring the binding of substrates MPP+ and TEA+ to rOCT1 at 0oC in order to establish the amino acids in the cleft region that interact with the substrate when the transporter is frozen in the outward-open conformation. Previously identified crucial amino acids (Asp475, Phe160, Leu447, Arg440, Trp218 and Tyr222) were selected for the study. rOCT1 wild-type and its mutants were stably expressed in HEK293 cells and these cells were used for the binding measurements with the radioactive substrate (MPP+ or TEA+) at 0°C in Mg-Ca-PBS buffer as described in “Materials and Methods” section in detail. rOCT1 wild-type revealed for MPP+-binding a KD which was not significantly different from the corresponding Km value. Also, after addition of 10 nM non-radioactive MPP+, an initial increase of about 20% in bound MPP+ was observed. The results indicate that the Km for transport is dependent on the binding of MPP+ to the outward-open conformation and hints at the possibility of allosteric interaction between the binding sites. Mutations at position Trp218, Phe160 and Asp475 resulted in a change in the KD value. Trp218 mutations also showed an allosteric increase similar to the rOCT1 wild-type. This study suggests that these amino acids are located at a critical position in the outward-open conformation for MPP+ transport. TEA+-binding could not be observed in rOCT1 wild-type, indicating that the binding site is perhaps inaccessible for TEA+ in frozen outward-open state. The mutants D475E, F160A, L447F, R440K and Y222F showed a very low affinity binding with a very high KD value as compared to the corresponding Km values indicating that the transporter might have different affinities for extra-cellular binding alone and for the complete transport process especially if temperature is the limiting factor. Substrate inhibition studies done using both MPP+ and TEA+ have confirmed the existence of overlapping binding sites for these two ligands. This study has confirmed the direct interaction of Trp218, Phe160, Asp475 with MPP+ and Phe160, Asp475, Leu447, Arg440 and Tyr222 with TEA+ in the outward-open conformation. N2 - In der vorgelegten Arbeit werden Untersuchungen am organischen Transporter rOCT1, einem Mitglied der SLC22 Familie, berichtet. Frühere Untersuchungen beinhalteten Transportmessungen mit radioaktiven Substanzen und Hemmstoffen, Transport- und Bindungsmessungen nach Rekonstitution in Nanodisken und Proteo¬liposomen und Voltage-Clamp-Fluorimetrie-Analysen an rOCT1 und rOCT1 Mutanten. Sie führten zur Identifizierung wichtiger Aminosäuren im Bindungsspalt von rOCT1, welche für die Interaktion mit Substraten oder Hemmstoffen wichtig sind. Homologiemodelle wurden zur Interpretationen der Ergebnisse herangezogen. In der vorgelegten Arbeit haben wir die Binding der Substrate MPP+ und TEA+ an rOCT1 bei 0°C gemessen um herauszufinden welche Aminosäuren in der Spaltregion von rOCT1 mit diesen Substraten interagieren, wenn der Transporter in der nach außen offenen Konfor¬mation „eingefroren“ ist. Für die Untersuchungen wurden Aminosäuren ausgewählt, deren Relevanz für den Transport von MPP+ und TEA+ in früheren Untersuchungen erkannt worden war. Es handelt sich um die Aminosäuren Asp475, Phe160, Leu447, Arg440, Trp218 und Tyr222. rOCT1 Wildtyp und rOCT1 Mutanten wurden stabil in HEK293 Zellen exprimiert. Mit diesen Zellen wurden bei 0oC Bindungsmessungen mit radioaktiv markiertem MPP+ und TEA+ unter Verwendung eines Magnesium und Calcium erhaltenen Puffers. Für die MPP+-Bindung an den rOCT1 Wildtyp ergab sich eine µmolare Dissoziationskonstante (KD), die keinen signifikanten Unterschied zum früher gemessenen Km Wert aufweist. Dieses Ergebnis zeigt, dass der Km von der MPP+-Bindung an die nach außen offene Konformation abhängig ist. Bei der Zugabe von 10 nM nicht-radioaktivem MPP+ war beim rOCT1 Wildtyp die Bindung von radioaktiv markiertem MPP+ um 20% erhöht. Dies deutet auf einen allosterischen Effekt einer hochaffinen MPP+ Bindungsstelle auf die direkt am Transport beteiligte µmolare Bindungsstelle hin. Mutationen der Aminosäuren Trp218, Phe160 und Asp475 führten zu Änderungen des KD Wertes für die MPP+ Bindung. Für die Mutanten von Trp218 wurde ein ähnlicher allosterischer MPP+ Effekt wie beim rOCT1 Wildtyp beobachtet. Die Unter¬suchungen weisen darauf hin, dass diese drei Aminosäuren in kritischen Positionen für die MPP+-Bindung von außen befinden. Bei 00C konnte beim rOCT1 Wildtyp keine TEA+-Bindung nachgewiesen werden. Dies legt den Schluss nahe, dass die TEA+-Bindungsstelle in der „eingefrorenen“ nach außen gerichteten Konformation unzugänglich ist. In Gegensatz dazu zeigen die Mutanten D475E, F160A, L447F, R440K und Y222F eine sehr niederaffine TEA+-Bindung mit hohen KD Werten, die sich stark von den entsprechenden Km Werten unterscheiden. Durch Experimente, bei denen die Bindung von MPP+ durch TEA+ bzw. die Bindung von TEA+ durch MPP+ gehemmt wurde, wurde die Hypothese bestätigt, dass sich die Bindungsstellen für MPP+ und TEA+ überlappen. Unsere Untersuchungen deuten darauf hin, dass in der nach außen gerichteten Konformation von rOCT1 Trp218, Phe160 und Asp475 direkt mit MPP+ und Phe160, Asp475, Leu447, Arg440 und Tyr222 direkt mit TEA+ interagieren. KW - Kation KW - Transporters KW - Stofftransport KW - OCT1 Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-169992 ER - TY - JOUR A1 - Werner, Rudolf A1 - Wakabayashi, Hiroshi A1 - Bauer, Jochen A1 - Schütz, Claudia A1 - Zechmeister, Christina A1 - Hayakawa, Nobuyuki A1 - Javadi, Mehrbod S. A1 - Lapa, Constantin A1 - Jahns, Roland A1 - Ergün, Süleyman A1 - Jahns, Valerie A1 - Higuchi, Takahiro T1 - Longitudinal \(^{18}\)F-FDG PET imaging in a Rat Model of Autoimmune Myocarditis JF - European Heart Journal Cardiovascular Imaging N2 - Aims: Although mortality rate is very high, diagnosis of acute myocarditis remains challenging with conventional tests. We aimed to elucidate the potential role of longitudinal 2-Deoxy-2-\(^{18}\)F-fluoro-D-glucose (\(^{18}\)F-FDG) positron emission tomography (PET) inflammation monitoring in a rat model of experimental autoimmune myocarditis. Methods and results: Autoimmune myocarditis was induced in Lewis rats by immunizing with porcine cardiac myosin emulsified in complete Freund’s adjuvant. Time course of disease was assessed by longitudinal \(^{18}\)F-FDG PET imaging. A correlative analysis between in- and ex vivo \(^{18}\)F-FDG signalling and macrophage infiltration using CD68 staining was conducted. Finally, immunohistochemistry analysis of the cell-adhesion markers CD34 and CD44 was performed at different disease stages determined by longitudinal \(^{18}\)F-FDG PET imaging. After immunization, myocarditis rats revealed a temporal increase in 18F-FDG uptake (peaked at week 3), which was followed by a rapid decline thereafter. Localization of CD68 positive cells was well correlated with in vivo \(^{18}\)F-FDG PET signalling (R\(^2\) = 0.92) as well as with ex vivo 18F-FDG autoradiography (R\(^2\) = 0.9, P < 0.001, respectively). CD44 positivity was primarily observed at tissue samples obtained at acute phase (i.e. at peak 18F-FDG uptake), while CD34-positive staining areas were predominantly identified in samples harvested at both sub-acute and chronic phases (i.e. at \(^{18}\)F-FDG decrease). Conclusion: \(^{18}\)F-FDG PET imaging can provide non-invasive serial monitoring of cardiac inflammation in a rat model of acute myocarditis. KW - positron emission tomography KW - Myokarditis KW - myocarditis KW - inflammation KW - 18F-FDG KW - PET KW - personalized treatment Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-165601 SN - 2047-2404 ER - TY - INPR A1 - Nose, Naoko A1 - Werner, Rudolf A. A1 - Ueda, Yuichiro A1 - Günther, Katharina A1 - Lapa, Constantin A1 - Javadi, Mehrbod S. A1 - Fukushima, Kazuhito A1 - Edenhofer, Frank A1 - Higuchi, Takahiro T1 - Metabolic substrate shift in human induced pluripotent stem cells during cardiac differentiation: Functional assessment using in vitro radionuclide uptake assay T2 - International Journal of Cardiology N2 - Background: Recent developments in cellular reprogramming technology enable the production of virtually unlimited numbers of human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CM). Although hiPSC-CM share various characteristic hallmarks with endogenous cardiomyocytes, it remains a question as to what extent metabolic characteristics are equivalent to mature mammalian cardiomyocytes. Here we set out to functionally characterize the metabolic status of hiPSC-CM in vitro by employing a radionuclide tracer uptake assay. Material and Methods: Cardiac differentiation of hiPSC was induced using a combination of well-orchestrated extrinsic stimuli such as WNT activation (by CHIR99021) and BMP signalling followed by WNT inhibition and lactate based cardiomyocyte enrichment. For characterization of metabolic substrates, dual tracer uptake studies were performed with \(^{18}\)F-2-fluoro-2-deoxy-D-glucose (\(^{18}\)F-FDG) and \(^{125}\)I-β-methyl-iodophenyl-pentadecanoic acid (\(^{125}\)I-BMIPP) as transport markers of glucose and fatty acids, respectively. Results: After cardiac differentiation of hiPSC, in vitro tracer uptake assays confirmed metabolic substrate shift from glucose to fatty acids that was comparable to those observed in native isolated human cardiomyocytes. Immunostaining further confirmed expression of fatty acid transport and binding proteins on hiPSC-CM. Conclusions: During in vitro cardiac maturation, we observed a metabolic shift to fatty acids, which are known as a main energy source of mammalian hearts, suggesting hi-PSC-CM as a potential functional phenotype to investigate alteration of cardiac metabolism in cardiac diseases. Results also highlight the use of available clinical nuclear medicine tracers as functional assays in stem cell research for improved generation of autologous differentiated cells for numerous biomedical applications. KW - tracer KW - Stammzelle KW - induced pluripotent stem cells KW - cardiomyocytes KW - fatty acid KW - stem cell therapy KW - hiPSC-CM Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-163320 SN - 0167-5273 ER - TY - THES A1 - Günther, Katharina T1 - Generation of early human neuroepithelial progenitors from primary cells for biomedical applications T1 - Generierung früher humaner neuroepithelialer Vorläufer aus primären Zellen für biomedizinische Anwendungen N2 - Patient-specific induced pluripotent stem cells (iPSCs) emerged as a promising cell source for disease modeling and drug screening as well as a virtually unlimited source for restorative therapy. The thesis deals with three major topics to help realizing biomedical applications with neural stem cells. To enable the generation of transgene-free iPSCs, alternatives to retroviral reprogramming were developed. Hence, the adaptation and evaluation of reprogramming using excisable lentiviral constructs, Sendai virus (SeV) and synthetic mRNA-based methods was assessed in the first part of this thesis. hiPSCs exhibit the pluripotency markers OCT4, SSEA-4, TRA1-60 which were confirmed by immunofluorescence and flow cytometry. Besides, the potential to differentiate in cell types of all three germ layers was detected, confirming pluripotent identity of proliferating colonies resulting from various reprogramming strategies. However, major differences such as high efficiency with SeV in contrast to a relatively low efficiency with mRNA in regard to passage number and the phenotype of starting fibroblasts were observed. Furthermore, a prolonged clone- and passage-dependent residual presence of viral RNA genes was identified in SeV-iPSCs for up to 23 passages using RT-PCR underlining the importance of careful monitoring of clone selection. In contrast, viral-free reprogramming by synthetic mRNA represents a fully non-integrative approach but requires further refinement to be efficiently applicable to all fibroblasts. The second part of this thesis deals with the establishment of a rapid monolayer approach to differentiate neural progenitor cells from iPSCs. To achieve this, a two-step protocol was developed allowing first the formation of a stable, primitive NPC line within 7 days which was expanded for 2-3 passages. In a second step, a subsequent adaptation to conditions yielding neural rosette-like NPCs followed. Both neural lines were demonstrated to be expandable, cryopreservable and negative for the pluripotency marker OCT4. Furthermore, a neural precursor identity including SOX1, SOX2, PAX6, Nestin was confirmed by immunofluorescence and quantitative RT-PCR. Moreover, the differentiation resulted in TUJ1-positive neurons and GFAP-positive astrocytes. Nonetheless, the outcome of glial differentiation from primitive NSCs remained low, whereas FGF/EGF-NPCs were efficiently differentiated into GFAP-positive astrocytes which were implicated in a cellular model of the blood brain barrier. The third and major objective of this study was to generate human early neural progenitor cells from fetal brain tissue with a wide neural differentiation capacity. Therefore, a defined medium composition including small molecules and growth factors capable of modulation of crucial signaling pathways orchestrating early human development such as SHH and FGF was assessed. Indeed, specific culture conditions containing TGFβ inhibitor SB431542, SHH agonist Purmorphamine, GSK3β inhibitor CHIR99021 and basic FGF, but no EGF enabled robust formation of early neuroepithelial progenitor (eNEP) colonies displaying a homogeneous morphology and a high proliferation rate. Moreover, primary eNEPs exhibit a relatively high clonogenicity of more than 23 % and can be monoclonally expanded for more than 45 passages carrying a normal karyotype. Characterization by immunofluorescence, flow cytometry and quantitative RT-PCR revealed a distinct NPC profile including SOX1, PAX6, Nestin and SOX2 and Prominin. Furthermore, primary eNEPs show NOTCH and HES5 activation in combination with non-polarized morphology, indicative of an early neuroepithelial identity. Microarray analysis unraveled SOX11, BRN2 and other HES-genes as characteristic upregulated genes. Interestingly, eNEPs were detected to display ventral midbrain/hindbrain regional identity. The validation of yielded cell types upon differentiation indicates a strong neurogenic potential with more than 90 % of TUJ1-positive neurons. Moreover, astrocytes marked by GFAP and putative myelin structures indicating oligodendrocytes were identified. Electrophysiological recordings revealed functionally active neurons and immunofluorescence indicate GABAergic, glutamatergic, dopaminergic and serotonergic subtypes. Additionally, putative physiological synapse formation was observed by the presence of Synapsin and PSD-95 as well as by ultrastructural examination. Notably, rare neurons stained positive for the peripheral neuronal marker Peripherin suggesting the potential of eNEPS to give rise to cells of neural tube and neural crest origin. By the application of specific differentiation protocols an increase of TH-positive neurons or neural crest-derivatives such as putative A- and C-sensory neurons and mesenchymal cells was identified. Taken together, primary eNEPs might help to elucidate mechanisms of early human neurodevelopment and will serve as a novel source for cell replacement and further biomedical applications. N2 - Patientenspezifische induziert pluripotente Zellen (iPSZ) haben sich als eine vielversprechende Möglichkeit erwiesen Zellen zu gewinnen, die für Krankheitsmodellierung, Arzneimitteltests und Zellersatztherapie in Frage kommen. In dieser Arbeit wurden drei wichtige Fragestellungen adressiert, die für potenzielle biomedizinische Anwendungen von neuralen Stammzellen von großem Interesse sind. Um die Generierung von transgenfreien iPSZ zu ermöglichen, wurden Alternativen zur retroviralen Reprogrammierung entwickelt. Im ersten Teil dieser Arbeit wurden Reprogrammierungsmethoden, die auf deletierbaren, lentiviralen Konstrukten oder nichtintegrativen Verfahren wie Sendaivirus (SeV)-Transduktion und Transfektion synthetischer mRNA basieren, adaptiert und evaluiert. Die daraus resultierenden iPSZ exprimieren die Pluripotenzmarker OCT4, SSEA-4 und TRA1-60. Weiterhin wurde das Potenzial in Zelltypen aller drei Keimblätter zu differenzieren nachgewiesen. Dadurch konnte die pluripotente Identität der proliferativen Kolonien bestätigt werden. Beim Vergleich der angewandten Methoden fielen, bezüglich der generierten iPSZ-Linien, sowohl qualitative als auch quantitative Unterschiede auf. Bei der Verwendung von SeV-Partikeln wurde eine hohe Reprogrammierungseffizienz festgestellt. Bei der Transfektion von mRNAs hingegen war die Reprogrammierungseffizienz deutlich niedriger. Diese war darüber hinaus abhängig von der Passage und dem Genotyp der Ausgangsfibroblasten. Des Weiteren konnte eine klon- und passagenabhängige Präsenz viraler Gene in SeV-iPSZ bis zu 23 Passagen lang beobachtet werden, während bei der mRNA-Transfektion keine Spuren der genetischen Manipulation zurückblieben. Dies verdeutlicht die Bedeutung einer sorgfältigen Qualitätskontrolle bei der Klonselektion im Falle der SeV-iPSZ. Im Gegensatz dazu stellt die Reprogrammierung durch Transfektion synthetischer mRNAs eine völlig nicht-integrative Strategie dar, erfordert allerdings weitere Verfeinerung um das Verfahren effizient und vor allem für alle Fibroblastenpräparationen anwendbar zu machen. Der zweite Teil der Arbeit behandelt die Etablierung eines schnellen, adhärenten Protokolls, um neurale Vorläuferpopulation aus iPSZ zu differenzieren. Um dies zu erreichen, wurde ein zweiphasiges Protokoll entwickelt, welches zunächst die Generierung einer primitiven neuralen Vorläuferzellpopulation innerhalb von 7 Tagen erlaubt. In einem zweiten Schritt erfolgte die Adaptierung an Kulturbedingungen, die eine neurale, rosettenähnliche Zellpopulation induzieren. Beide neuralen Zellpopulationen konnten weiter expandiert und eingefroren werden und waren negativ für den Pluripotenz-assoziierten Transkriptionsfaktor OCT4. Darüber hinaus konnte die neurale Vorläuferidentität mittels positiver Expression von SOX1, SOX2, PAX6 und Nestin bestätigt werden. Eine weitere Differenzierung dieser Zellen resultierte in TUJ1-positiven Neuronen und GFAP-positiven Astrozyten, die die Verwendung der Zellpopulation beispielsweise in einem zellulären Modell der Blut-Hirn-Schranke erlaubten. Das Hauptprojekt dieser Dissertation war es, frühe humane neurale Vorläuferzellen aus fetalem Hirngewebe zu isolieren und in Kultur zu stabilisieren. Diese Population sollte eine breite Differenzierungskapazität aufweisen. Zu diesem Zweck wurde eine chemisch definierte Medienzusammensetzung gewählt, die zusätzlich pharmakologisch wirksame Verbindungen und Wachstumsfaktoren beinhaltet. Hierdurch konnten Signaltransduktionswege wie zum Beispiel der Sonic-Hedgehog- (SHH) oder FGF-Signalweg, die bei der frühen neuralen Entwicklung eine bedeutende Rolle spielen, moduliert werden. In der Tat ermöglichten spezifische Kultivierungsbedingungen, die den TGFβ-Inhibitor SB431542, den SHH-Agonisten Purmorphamin, den GSK3β-Inhibitor CHIR99021 und basisches FGF, jedoch kein EGF enthielten, die robuste Bildung einer früheren neuroepithelialen Vorläuferpopulation (eNEP). Die so stabilisierten Kolonien wiesen eine homogene Morphologie und eine hohe Proliferationsrate auf. Außerdem zeigten sie eine hohe Klonogenitätsrate von 23%, die es ermöglichte monoklonale Zelllinien zu isolieren und für mehr als 45 Passagen zu expandieren. Dabei blieb ein normaler Karyotyp erhalten. Die Zellen zeigten ein eindeutiges neurales Profil, gekennzeichnet durch SOX1, PAX6, Nestin, SOX2 und Prominin-Expression. Weiterhin wiesen eNEPs NOTCH und HES5-Aktivierung in Kombination mit nicht-polarisierter Morphologie auf, was auf eine frühe neuropitheliale Identität hinweist. Eine Microarray-Analyse demonstrierte weiterhin SOX11, BRN2 und einige HES-Gene als charakteristisch hochregulierte Gene. Interessanterweise zeigen eNEPs eine regionale Identität, die auf eine Mittelhirn/Hinterhirn-Regionalisierung hinweist. Die Validierung ungerichtet ausdifferenzierter Zelltypen offenbarte mit einem Kulturanteil von 90% TUJ1-positiven Neuronen ein stark neurogenes Potenzial. Zusätzlich konnten GFAPpositive Astrozyten sowie mögliche Myelinstrukturen, die auf Oligodendrozyten hinweisen, nachgewiesen werden. Elektrophysiologische Aufzeichnungen deuten auf funktionell aktive Neurone hin und Immunofluoreszenzfärbungen zeigten GABAerge, glutamaterge, dopaminerge und serotonerge neuronale Subtypen. Außerdem wurden mittels Immunfluoreszenzanalyse Synapsin- und PSD-95- positive synaptische Strukturen nachgewiesen. Ultrastrukturelle Analysen mittels Transmissionselektronenmikroskopie bestätigten das Ergebnis. Hervorzuheben ist, dass einige Neurone positiv für den peripheren Neuronenmarker Peripherin gefärbt wurden, was darauf hinweist, dass eNEPs das Potenzial besitzen, in Zellen der Neuralleiste zu differenzieren. Durch die Verwendung von spezifischen Differenzierungsprotokollen konnte das Vorkommen TH-positiver und auch möglicher A- und C-sensorischer Fasern, sowie mesenchymaler Zellen nachgewiesen werden. Zusammenfassend lässt sich sagen, dass primäre eNEPs dazu beitragen könnten, die frühe humane Gehirnentwicklung zu verstehen. Darüber hinaus stellen eNEPs eine potentielle zelluläre Quelle für Zellersatztherapien und weitere biomedizinische Anwendungen dar. KW - progenitors KW - stem cells KW - biomedicine KW - human primary cells KW - biomedical applications KW - neuroepithelial progenitors KW - neuroepitheliale Vorläufer KW - early neural precursors KW - frühe neurale Vorläufer Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-150348 ER - TY - JOUR A1 - Drenckhahn, Detlev A1 - Drenckhahn, Helga T1 - Trifolium micranthum Viv. an Nordseedeichen von Schleswig-Holstein – Charakterisierung der Pflanzen und ihrer Habitate, Status in Deutschland und Nachbargebieten T1 - Trifolium micranthum Viv. at the North Sea dikes of Schleswig-Holstein – characterization of plants and their habitats, status in Germany and neighbouring countries JF - Forum Geobotanicum N2 - In der vorliegenden Arbeit wird ein neues Teilareal von T. micranthum mit zahlreichen Vorkommen an den Nordseedeichen von Schleswig-Holstein zwischen der Elbeästuar und der Insel Nordstrand mit Schwerpunkt auf der Halbinsel Eiderstedt mitgeteilt, das geographisch zwischen dem Vorkommen in den Niederlanden und dem Ostsee-Areal in Dänemark vermittelt. Es handelt sich um die einzigen weitgehend naturnahen Wuchsorte der Art in Deutschland. Die anderen beiden aktuellen deutschen Vorkommen befinden sich auf Friedhöfen in Nordrhein-Westfalen. T. micranthum wächst bevorzugt an den steilen und artenreicheren Innenböschungen der Seedeiche, deren Vegetation durch intensive Schafbeweidung und Trittspuren kurz und lückig gehalten wird. Die Beweidung bewirkt eine signifikante Größenreduktion (Miniaturisierung) verschiedener Pflanzenteile. Widersprüchliche Angaben zu bestimmungskritischen Merkmalen werden durch morphometrische Untersuchungen überprüft. Unter anderem beträgt die Länge der Blütenstiele 0,6–1,1 mm (im Mittel 0,8 mm) und die Blüten mit Kelch sind deutlich unter 3 mm lang (im Mittel 2,4 mm). Die Zahl der Blüten der Infloreszenz beträgt (1)2–6(8). Eine graphische Darstellung soll bei Artbestimmung und Auffinden neuer Wuchsorte behilflich sein. N2 - A new distribution area with numerous growth sites of Trifolium micranthum has been discovered at the sea dikes of the North Sea coast of Schleswig-Holstein in Germany between the estuary of river Elbe and the island of Nordstrand with main occurrence on the peninsula Eiderstedt. Geographically this area links the Dutch population with the West Baltic population in Denmark and is the only semi natural growth site of this tiny clover in Germany. The other current growth sites in Germany are located on cemeteries in Nordrhein-Westfalen. T. micranthum prefers the steep inner slopes of sea dikes (30% gradient) with their higher diversity of vegetation and open ground sites created by grazing and tracks of sheep. Grazing creates significant reduction of the size of various parts of the clover (miniaturization). The paper also provides morphometric data on distinguishing features that are controversially treated in the literature, e.g. the length of pedicels with 0.6–1.1 mm (mean 0.8 mm), flower size (corolla with calyx) below 3 mm (mean 2.4 mm) and number of flowers per inflorescence of (1)2–6(8). A drawing of T. micranthum is provided that may help to discover new growth sites. KW - Trifolium micranthum KW - distribution range KW - Klee KW - anatomy KW - ecology KW - Trifolium dubium Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-159163 UR - http://www.forum-geobotanicum.net/articles/vol_8-2018/drenckhahn_trifolium/drenckhahn-drenckhahn_Trifolium_micranthum.pdf SN - 1867-9315 VL - 8 ER -