TY - THES A1 - Hieke, Marie T1 - Synaptic arrangements and potential communication partners of \(Drosophila’s\) PDF-containing clock neurons within the accessory medulla T1 - Synaptische Konstellationen und potentielle Kommunikationspartner von \(Drosophila’s\) PDF-enthaltenden Uhrneuronen innerhalb der akzessorischen Medulla N2 - Endogenous clocks regulate physiological as well as behavioral rhythms within all organisms. They are well investigated in D. melanogaster on a molecular as well as anatomical level. The neuronal clock network within the brain represents the center for rhythmic activity control. One neuronal clock subgroup, the pigment dispersing factor (PDF) neurons, stands out for its importance in regulating rhythmic behavior. These neurons express the neuropeptide PDF (pigment dispersing factor). A small neuropil at the medulla’s edge, the accessory medulla (AME), is of special interest, as it has been determined as the main center for clock control. It is not only highly innervated by the PDF neurons but also by terminals of all other clock neuron subgroups. Furthermore, terminals of the photoreceptors provide light information to the AME. Many different types of neurons converge within the AME and afterward spread to their next target. Thereby the AME is supplied with information from a variety of brain regions. Among these neurons are the aminergic ones whose receptors’ are expressed in the PDF neurons. The present study sheds light onto putative synaptic partners and anatomical arrangements within the neuronal clock network, especially within the AME, as such knowledge is a prerequisite to understand circadian behavior. The aminergic neurons’ conspicuous vicinity to the PDF neurons suggests synaptic communication among them. Thus, based on former anatomical studies regarding this issue detailed light microscopic studies have been performed. Double immunolabellings, analyses of the spatial relation of pre- and postsynaptic sites of the individual neuron populations with respect to each other and the identification of putative synaptic partners using GRASP reenforce the hypothesis of synaptic interactions within the AME between dopaminergic/ serotonergic neurons and the PDF neurons. To shed light on the synaptic partners I performed first steps in array tomography, as it allows terrific informative analyses of fluorescent signals on an ultrastructural level. Therefore, I tested different ways of sample preparation in order to achieve and optimize fluorescent signals on 100 nm thin tissue sections and I made overlays with electron microscopic images. Furthermore, I made assumptions about synaptic modulations within the neuronal clock network via glial cells. I detected their cell bodies in close vicinity to the AME and PDFcontaining clock neurons. It has already been shown that glial cells modulate the release of PDF from s-LNvs’ terminals within the dorsal brain. On an anatomical level this modulation appears to exist also within the AME, as synaptic contacts that involve PDF-positive dendritic terminals are embedded into glial fibers. Intriguingly, these postsynaptic PDF fibers are often VIIAbstract part of dyadic or even multiple-contact sites in opposite to prolonged presynaptic active zonesimplicating complex neuronal interactions within the AME. To unravel possible mechanisms of such synaptic arrangements, I tried to localize the ABC transporter White. Its presence within glial cells would indicate a recycling mechanism of transmitted amines which allows their fast re-provision. Taken together, synapses accompanied by glial cells appear to be a common arrangement within the AME to regulate circadian behavior. The complexity of mechanisms that contribute in modulation of circadian information is reflected by the complex diversity of synaptic arrangements that involves obviously several types of neuron populations N2 - Endogene Uhren steuern sowohl physiologische als auch verhaltensbedingte Rhythmen bei allen Organismen. In D. melanogaster sind sie nicht nur auf molekularer sondern auch auf anatomischer Ebene bereits gut erforscht. Das neuronale Uhrnetzwerk im Gehirn stellt das Zentrum der Steuerung der rhythmischen Aktivität dar. Eine Uhrneuronengruppe sticht allein schon durch ihre besonderen anatomischen Eigenschaften hervor. Diese Neurone exprimieren das Neuropeptid PDF (pigment dispersing factor), welches zudem besonderen Einfluss auf die Lokomotionsaktivität der Fliege hat. Ein kleines Neuropil am Rande der Medulla, die akzessorische Medulla (AME) ist von besonderem Interesse, da neben seiner intensiven Innervation durch die PDF-Neurone auch Terminale aller anderen Uhrneuronengruppen zu finden sind. Zudem wird sie durch Terminale der Photorezeptoren mit Informatonen über die Lichtverhätnisse versorgt. Die AME erreichen des Weiteren Informationen aus vielen anderen Hirnregionen. Eine Vielzahl von Neuronentypen laufen in ihr zusammen, um sich anschließend wieder in verschiedenste Hirnareale zu verteilen. So wird die AME auch durchzogen von Fasern mit aminergem Inhalt, dessen Rezeptoren wiederum auf den PDF-Neuronen zu finden sind. Die vorliegende Arbeit gibt Aufschluss über vermutliche synaptische Partner und anatomische Anordnungen innerhalb des neuronalen Uhrnetzwerkes, insbesondere innerhalb der AME. Solch Wissen stellt eine Grundvoraussetzung dar, um zirkadianes Verhalten verstehen zu können. Die auffällige Nähe der aminergen Neurone zu den PDF Neuronen lässt eine synaptische Interaktion zwischen ihnen vermuten. Deshalb wurden basierend auf vorangegangen Studien detailiertere Untersuchungen dieser Thematik durchgeführt. So wird die Hypothese über synaptische Interaktionen innerhalb der AME zwischen dopaminergen/ serotonergen Neuronen und den PDF Neuronen bestärkt mittels Doppelimmunofärbungen, gegenüberstellende Analysen über die räumlichen Nähe von prä- und postsynaptischen Stellen der jeweiligen Neuronenpopulationen und durch die Identifikation vermutlicher synaptischer Partner unter Verwendung von GRASP. Zur möglichen Identifikation der synaptischen Partner unternahm ich erste Schritte in der Array Tomographie, welche hochinformative Analysen von fluoreszierenden Signalen auf einem ultrastrukturellen Level ermöglicht. Dazu testete ich verschieden Wege der Gewebepräparation, um Flureszenzsignale zu erhalten bzw. zu optimieren und bildete erste Überlagerungen der Fluoreszenz- und Elektronenmikrskopbilder. Die Auswertung der elektronenmikroskopischen Bilder erlaubten Mutmaßungen über mö- gliche synaptische Modulationen innerhalb des neuronalen Uhrnetzwerkes durch Gliazellen. Ihre Zellkörper fand ich in unmittelbarer Nähe zu den PDF Neuronen. Im dorsalen Hirn wurden neuronale Modulationen an den kleinen PDF Neuronen durch Gliazellen bereits festgestellt. Auf anatomischer Ebene scheint diese Modulation auch innerhalb der AME zu erfolgen, da synaptische Kontakte, welche PDF-positive Dendriten involvieren, von Gliafasern umgeben sind. Interessanterweise sind diese postsynaptischen PDF Fasern dabei oftmals Teil dyadischer oder sogar multipler Kontakte, die sich gegenüber einer ausgedehnten aktiven Zone befinden. Um mögliche Mechanismen solcher synaptischer Anordnungen zu erklären, versuchte ich den ABC Transporter White im Hirn von Drosophila zu lokalisieren. Seine Präsenz in Gliazellen würde auf einen Recyclingmechanismus hindeuten, welcher eine schnelle Wiederbereitstellung des Transmiters ermöglichen würde. Zusammengefasst scheinen Synapsen mit postsynaptischen PDF-Neuronen in Begleitung von Gliazellen, ein gebräuchliches synaptisches Arrangement innerhalb der AME dazustellen. Diese komplexe Diversität der synaptischen Anordnung reflektiert die komplexen Mechanismen, welche der Verarbeitung der zirkadianen Informationen zugrunde liegen KW - Taufliege KW - Chronobiologie KW - Endogene Rhythmik KW - PDF neurons KW - glia cells KW - circadian clock KW - accessory medulla KW - sleep KW - aminergic neurons KW - synapses KW - Gliazelle KW - Aminerge Nervenzelle KW - Pigmentdispergierender Faktor KW - Drosophila melanogaster Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-175988 ER - TY - JOUR A1 - Duan, Xiaodong A1 - Nagel, Georg A1 - Gao, Shiqiang T1 - Mutated channelrhodopsins with increased sodium and calcium permeability JF - Applied Sciences N2 - (1) Background: After the discovery and application of Chlamydomonas reinhardtii channelrhodopsins, the optogenetic toolbox has been greatly expanded with engineered and newly discovered natural channelrhodopsins. However, channelrhodopsins of higher Ca\(^{2+}\) conductance or more specific ion permeability are in demand. (2) Methods: In this study, we mutated the conserved aspartate of the transmembrane helix 4 (TM4) within Chronos and PsChR and compared them with published ChR2 aspartate mutants. (3) Results: We found that the ChR2 D156H mutant (XXM) showed enhanced Na\(^+\) and Ca\(^{2+}\) conductance, which was not noticed before, while the D156C mutation (XXL) influenced the Na\(^+\) and Ca\(^{2+}\) conductance only slightly. The aspartate to histidine and cysteine mutations of Chronos and PsChR also influenced their photocurrent, ion permeability, kinetics, and light sensitivity. Most interestingly, PsChR D139H showed a much-improved photocurrent, compared to wild type, and even higher Na+ selectivity to H\(^+\) than XXM. PsChR D139H also showed a strongly enhanced Ca\(^{2+}\) conductance, more than two-fold that of the CatCh. (4) Conclusions: We found that mutating the aspartate of the TM4 influences the ion selectivity of channelrhodopsins. With the large photocurrent and enhanced Na\(^+\) selectivity and Ca\(^{2+}\) conductance, XXM and PsChR D139H are promising powerful optogenetic tools, especially for Ca\(^{2+}\) manipulation. KW - optogenetics KW - channelrhodopsins KW - sodium KW - calcium KW - DC gate Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197435 SN - 2076-3417 VL - 9 IS - 4 ER - TY - JOUR A1 - Minev, Boris R. A1 - Lander, Elliot A1 - Feller, John F. A1 - Berman, Mark A1 - Greenwood, Bernadette M. A1 - Minev, Ivelina A1 - Santidrian, Antonio F. A1 - Nguyen, Duong A1 - Draganov, Dobrin A1 - Killinc, Mehmet O. A1 - Vyalkova, Anna A1 - Kesari, Santosh A1 - McClay, Edward A1 - Carabulea, Gabriel A1 - Marincola, Francesco M. A1 - Butterfield, Lisa H. A1 - Szalay, Aladar A. T1 - First-in-human study of TK-positive oncolytic vaccinia virus delivered by adipose stromal vascular fraction cells JF - Journal of Translational Medicine N2 - Background ACAM2000, a thymidine kinase (TK)-positive strain of vaccinia virus, is the current smallpox vaccine in the US. Preclinical testing demonstrated potent oncolytic activity of ACAM2000 against several tumor types. This Phase I clinical trial of ACAM2000 delivered by autologous adipose stromal vascular fraction (SVF) cells was conducted to determine the safety and feasibility of such a treatment in patients with advanced solid tumors or acute myeloid leukemia (AML). Methods Twenty-four patients with solid tumors and two patients with AML participated in this open-label, non-randomized dose-escalation trial. All patients were treated with SVF derived from autologous fat and incubated for 15 min to 1 h with ACAM2000 before application. Six patients received systemic intravenous application only, one patient received intra-tumoral application only, 15 patients received combination intravenous with intra-tumoral deployment, 3 patients received intravenous and intra-peritoneal injection and 1 patient received intravenous, intra-tumoral and intra-peritoneal injections. Safety at each dose level of ACAM2000 (1.4 × 106 plaque-forming units (PFU) to 1.8 × 107 PFU) was evaluated. Blood samples for PK assessments, flow cytometry and cytokine analysis were collected at baseline and 1 min, 1 h, 1 day, 1 week, 1 month, 3 months and 6 months following treatment. Results No serious toxicities (> grade 2) were reported. Seven patients reported an adverse event (AE) in this study: self-limiting skin rashes, lasting 7 to 18 days—an expected adverse reaction to ACAM2000. No AEs leading to study discontinuation were reported. Viral DNA was detected in all patients’ blood samples immediately following treatment. Interestingly, in 8 patients viral DNA disappeared 1 day and re-appeared 1 week post treatment, suggesting active viral replication at tumor sites, and correlating with longer survival of these patients. No major increase in cytokine levels or correlation between cytokine levels and skin rashes was noted. We were able to assess some initial efficacy signals, especially when the ACAM2000/SVF treatment was combined with checkpoint inhibition. Conclusions Treatment with ACAM2000/SVF in patients with advanced solid tumors or AML is safe and well tolerated, and several patients had signals of an anticancer effect. These promising initial clinical results merit further investigation of therapeutic utility. Trial registration Retrospectively registered (ISRCTN#10201650) on October 22, 2018. KW - clinical trial KW - oncolytic vaccinia virus KW - stromal vascular fraction KW - immunotherapy of cancer Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-224105 VL - 17 ER - TY - JOUR A1 - Breitenbach, Tim A1 - Lorenz, Kristina A1 - Dandekar, Thomas T1 - How to steer and control ERK and the ERK signaling cascade exemplified by looking at cardiac insufficiency JF - International Journal of Molecular Sciences N2 - Mathematical optimization framework allows the identification of certain nodes within a signaling network. In this work, we analyzed the complex extracellular-signal-regulated kinase 1 and 2 (ERK1/2) cascade in cardiomyocytes using the framework to find efficient adjustment screws for this cascade that is important for cardiomyocyte survival and maladaptive heart muscle growth. We modeled optimal pharmacological intervention points that are beneficial for the heart, but avoid the occurrence of a maladaptive ERK1/2 modification, the autophosphorylation of ERK at threonine 188 (ERK\(^{Thr188}\) phosphorylation), which causes cardiac hypertrophy. For this purpose, a network of a cardiomyocyte that was fitted to experimental data was equipped with external stimuli that model the pharmacological intervention points. Specifically, two situations were considered. In the first one, the cardiomyocyte was driven to a desired expression level with different treatment strategies. These strategies were quantified with respect to beneficial effects and maleficent side effects and then which one is the best treatment strategy was evaluated. In the second situation, it was shown how to model constitutively activated pathways and how to identify drug targets to obtain a desired activity level that is associated with a healthy state and in contrast to the maleficent expression pattern caused by the constitutively activated pathway. An implementation of the algorithms used for the calculations is also presented in this paper, which simplifies the application of the presented framework for drug targeting, optimal drug combinations and the systematic and automatic search for pharmacological intervention points. The codes were designed such that they can be combined with any mathematical model given by ordinary differential equations. KW - optimal pharmacological modulation KW - efficient intervention points KW - ERK signaling KW - optimal treatment strategies KW - optimal drug targeting KW - optimal drug combination Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285164 SN - 1422-0067 VL - 20 IS - 9 ER - TY - THES A1 - Baig, Ayesha Anjum T1 - Studies on platelet interactions with the coagulation system and on modulators of platelet (hem)ITAM signaling in genetically modified mice T1 - Studien zur Thrombozyteninteraktion mit der Gerinnungskaskade und Modulation des (hem)ITAM Signalwegs in genetisch veränderaten Mäusen N2 - Activated platelets and coagulation jointly contribute to physiological hemostasis. However, pathological conditions can also trigger unwanted platelet activation and initiation of coagulation resulting in thrombosis and precipitation of ischemic damage of vital organs such as the heart or brain. The specific contribution of procoagulant platelets, positioned at the interface of the processes of platelet activation and coagulation, in ischemic stroke had remained uninvestigated. The first section of the thesis addresses this aspect through experiments conducted in novel megakaryocyte- and platelet-specific TMEM16F conditional KO mice (cKO). cKO platelets phenocopied defects in platelets from Scott Syndrome patients and had severely impaired procoagulant characteristics. This led to decelerated platelet-driven thrombin generation and delayed fibrin formation. cKO mice displayed prolonged bleeding times and impaired arterial thrombosis. However, infarct volumes in cKO mice were comparable to wildtype (WT) mice in an experimental model of ischemic stroke. Therefore, while TMEM16F-regulated platelet procoagulant activity is critical for hemostasis and thrombosis, it is dispensable for cerebral thrombo-inflammation in mice. The second section describes the generation and initial characterization of a novel knockin mouse strain that expresses human coagulation factor XII (FXII) instead of endogenous murine FXII. These knockin mice had normal occlusion times in an experimental model of arterial thrombosis demonstrating that human FXII is functional in mice. Therefore, these mice constitute a valuable tool for testing novel pharmacological agents against human FXII – an attractive potential target for antithrombotic therapy. Glycoprotein (GP)VI and C-type lectin-like receptor 2 (CLEC-2)-mediated (hem)immunoreceptor tyrosine-based activation motif (ITAM) signaling represent a major pathway for platelet activation. The last section of the thesis provides experimental evidence for redundant functions between the two members of the Grb2 family of adapter proteins - Grb2 and Gads that lie downstream of GPVI and CLEC-2 stimulation. In vitro and in vivo studies in mice deficient in both Grb2 and Gads (DKO) revealed that DKO platelets had defects in (hem)ITAM-stimulation-specific activation, aggregation and signal transduction that were more severe than the defects observed in single Grb2 KO or Gads KO mice. Furthermore, the specific role of these adapters downstream of (hem)ITAM signaling was essential for maintenance of hemostasis but dispensable for the known CLEC-2 dependent regulation of blood-lymphatic vessel separation. N2 - Aktivierte Thrombozyten und die Gerinnungskaskade bilden gemeinsam die Grundlage der physiologischen Hämostase. Daneben können jedoch auch pathologische Bedingungen Thrombozytenaktivierung herbeiführen und die Gerinnungskaskade auslösen und somit zum Gefäßverschluss führen, was häufig ischämische Schäden lebenswichtiger Organe wie beispielsweise des Herzens oder des Gehirns verursachen kann. Prokoagulante Thrombozy-ten befinden sich an der Schnittstelle zwischen Thrombozytenaktivierung und der Gerin-nungskaskade, ihre Funktion bei der Pathogenese des ischämischen Schlaganfalls wurde jedoch bisher nicht im Detail untersucht. Der erste Teil dieser Doktorarbeit widmet sich dieser Fragestellung durch die Analyse von neu generierten konditionalen, Megakaryozyten- und Thrombozyten-spezifischen Tmem16f Knockout Mäusen. TMEM16F-defiziente Thrombozy-ten wiesen ähnliche Defekte wie die Thrombozyten von Scott-Syndrom-Patienten sowie stark beeinträchtigte prokoagulante Eigenschaften auf. Diese Defekte gingen mit signifikant verlangsamter thrombozytenabhängiger Thrombingenerierung und verzögerter Fibrinbildung einher. TMEM16F-Defizienz führte zu verlängerter Blutungszeit und beeinträchtigte in einem experimentellen Modell die Bildung arterieller Thromben. TMEM16F-defiziente Mäuse wiesen jedoch im Vergleich zu wildtypischen Mäusen keinerlei Unterschiede im experimentellen ischämischen Schlaganfall auf. TMEM16F-gesteuerte prokoagulante Thrombozytenfunktion ist demnach kritisch für Hämostase und Thrombose, während sie eine untergeordnete Rolle in zerebraler Thrombo-Inflammation spielt. Der zweite Teil dieser Arbeit befasst sich mit der Generierung und Erstbeschreibung einer neuen Mauslinie, welche den humanen Hageman-Faktor (FXII) anstelle des endogenen murinen FXII exprimiert. In den resultierenden Knock-in Mäusen war die Bildung okklusiver arterieller Thromben nach chemisch induzierter Gefäßverletzung nicht beeinträchtigt, was zeigt, dass der humane FXII im Maussystem voll funktionstüchtig ist. Somit können diese Mäuse in der Zukunft als ein wertvolles Werkzeug zum Testen neuer pharmakologischer Ansätze zur Herabsetzung der FXII-Aktivität eingesetzt werden, welche einen vielver-sprechenden Targets neuartiger antithrombotischer Behandlungsansätze darstellt. Die thrombozytären Rezeptoren Glykoprotein (GP)VI und C-type lectin-like receptor 2 (CLEC-2) lösen (hem)immunoreceptor tyrosine-based activation motif (ITAM)-gekoppelte Signalwege aus, welche eine eine Schlüsselrolle in der Thrombozytenaktivierung spielen. Der dritte Teil dieser Doktorarbeit liefert experimentelle Hinweise für überlappende Funkti-onen der Adapterproteine Grb2 und Gads in der (hem)ITAM-anhängigen Signalkaskade. In vitro und in vivo Studien zeigten, dass Grb2/Gads-doppeldefiziente Thrombozyten (hem)ITAM-spezifische Defekte in der Aktivierung, Aggregation und Signaltransduktion aufweisen, die im Vergleich zu einzeldefizienten Thrombozyten deutlich ausgeprägter sind und somit eine redundante Rolle der Adapterproteine offenbaren. Während Grb2 und Gads gemeinsam an der Aufrechterhaltung physiologischer Hämostase beteiligt sind, tragen sie nicht entscheidend zur bekannten CLEC-2-abhängigen Regulation der Trennung von Blut- und Lymphgefäßen bei. KW - Blutgerinnung KW - Thrombozyt KW - Signaltransduktion KW - Maus KW - Thrombosis KW - Thrombo-inflammation KW - TMEM16F KW - (hem)ITAM signaling Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-164888 ER - TY - THES A1 - Lotz, Christian T1 - Entwicklung eines Augenirritationstests zur Identifikation aller GHS-Kategorien für den Endpunkt Augenreizung T1 - Development of an eye irritation test to identify all GHS categories of eye irritation N2 - Die Risikobewertung von Chemikalien ist für die öffentliche Gesundheit von entschei-dender Bedeutung, weshalb strenge Testverfahren zu deren toxikologischer Begutach-tung angewandt werden. Die ursprünglich tierbasierten Testverfahren werden aufgrund von neuen wissenschaftlichen Erkenntnissen und wegen ökonomischer Ineffizienz sowie ethischer Fragwürdigkeit immer mehr durch alternative Methoden ohne Tiermodelle ersetzt. Für den toxikologischen Endpunkt der Augenreizung wurden bereits die ersten alternativen Testsysteme auf der Basis von ex vivo- oder in vitro-Modellen entwickelt. Jedoch ist bis dato kein alternatives Testsystem in der Lage, das gesamte Spektrum der verschiedenen Kategorien der Augenreizungen nach dem global harmonisierten System zur Einstufung und Kennzeichnung von Chemikalien (GHS) vorherzusagen und damit den tierbasierten Draize-Augenreizungstest vollends zu ersetzen. Gründe hierfür sind fehlende physiologische Merkmale im Modell sowie eine destruktive Analysemethode. Aufgrund dessen wurden in dieser Studie die Hypothesen getestet, ob ein verbessertes In-vitro-Modell oder eine zerstörungsfreie, hochsensitive Analysemethode die Vorher-sagekraft des Augenreizungstests verbessern können. Dafür wurden zunächst neue Mo-delle aus humanen Hornhaut- und Hautepithelzellen entwickelt. Die Modelle aus pri-mären cornealen Zellen zeigten eine gewebespezifische Expression der Marker Zytokera-tin 3 und 12 sowie Loricrin. In beiden Modellen konnte durch die Verkürzung der Kul-turdauer die Ausbildung einer Hornschicht verhindert werden. Die Modelle wiesen dadurch eine sensiblere Barriere vergleichbar der nativen Cornea auf. Darüber hinaus konnte durch die chemische Quervernetzung mit Polyethylenglykolsuccinimidylglutara-tester ein transparentes, nicht kontrahierendes Stroma-Äquivalent etabliert werden. Der Stroma-Ersatz konnte zur Generierung von Hemi- und Voll-Cornea-Äquivalenten einge-setzt werden und lieferte somit erste Ansatzpunkte für die Rekonstruktion der nativen Hornhaut. Parallel dazu konnte ein zerstörungsfreies Analyseverfahren basierend auf der Impe-danzspektroskopie entwickelt werden, das wiederholte Messungen der Gewebeintegri-tät zulässt. Zur verbesserten Messung der Barriere in dreidimensionalen Modelle wurde hierfür ein neuer Parameter, der transepitheliale elektrische Widerstand (TEER) bei der Frequenz von 1000 Hz, der TEER1000 Hz definiert, der eine genauere Aussage über die Integrität der Modelle zulässt. Durch die Kombination der entwickelten cornealen Epithelzellmodelle mit der TEER1000 Hz-Messung konnte die Prädikitivität des Augenrei-zungstests auf 78 - 100 % erhöht werden. Von besonderer Bedeutung ist dabei, dass die nicht destruktive Messung des TEER1000 Hz zum ersten Mal erlaubte, die Persistenz von Irritationen durch wiederholte Messungen in einem in vitro-Modell zu erkennen und somit die GHS-Kategorie 1 von GHS-Kategorie 2 zu unterscheiden. Der wissenschaftli-che Gewinn dieser Forschungsarbeit ist ein neues Testverfahren, das alle GHS-Kategorien in einem einzigen in vitro-Test nachweisen und den Draize-Augenreizungstest gänzlich ersetzen kann. N2 - The assessment of the risk of chemicals is of crucial importance for public health. Hence, strict test procedures have been developed for toxicological evaluation of consumer products. The original animal-based test methods are being replaced by alternative methods due to new scientific findings, economic inefficiency and ethical doubts. For the toxicological endpoint of eye irritation, the first alternative test systems based on ex vivo or in vitro models have been developed. However, to date no alternative test meth-od has been able to predict the entire spectrum of eye irritation categories specified in the globally harmonized system for the classification and labelling of chemicals (GHS). Thus, no stand-alone test methods can replace the animal-based Draize eye irritation test resulting in the need of complex integrated testing strategies. Reasons for this are the lack of key physiological characteristics of the implemented models, species specific differences and the employed destructive analysis method. Therefore, this study tested whether a refinement of the used models or a more sensitive analytical method could improve the predictive power of the eye irritation test. First, new models of human corneal and skin epithelial cells were developed. Since a key fea-ture of the human cornea is a lack of cornification, several parameters such as calcium and retinoic acid to reduce the cornification were investigated. In both models the for-mation of a stratum corneum could be prevented most effectively by shortening the cul-ture time. Hence, the models had a more sensitive barrier comparable to the native cor-nea. However, only the model based on primary cornea cells showed a cornea-specific expression of the markers cytokeratin 3 and 12 as well as loricrin. Models based on skin keratinocytes retained a skin-specific phenotype. In addition, a stromal matrix was de-veloped to allow for the generation of a full-thickness cornea model. For this a cell-seeded collagen hydrogel was chemically cross-linkined via a polyethylene glycol suc-cinimidyl glutarate generating a transparent, non-contracting stroma equivalent. In parallel, a non-destructive highly sensitive analysis method based on impedance spec-troscopy was developed that allows repeated measurements of the tissue integrity. To improve the measurement of the barrier in three-dimensional models, a new parameter, the transepithelial electrical resistance (TEER) at the frequency of 1000 Hz, the TEER1000 Hz was defined. By combining the developed corneal epithelial cell models with the TEER1000 Hz measurement, the predictivity of the eye irritation test could be increased to 78 - 100 %. Moreover, the TEER1000 Hz allowed for the first time to detect the persistence of irritative effects by repeated measurements in an in vitro model and thus to distinguish between all GHS categories. The scientific yield of this research work is therefore a new test method that can detect all GHS categories in a single in vitro test and holds the possibility to completely replace the Draize eye irritation test. KW - Tissue Engineering KW - Eye irritation Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170126 ER - TY - THES A1 - Tshitenge Tshitenge, Dieudonné T1 - Isolation and Structural Elucidation of Novel Anti-Infective Naphthylisoquinoline Alkaloids from Ancistrocladus ealaensis, and Phytochemical Analysis of Two Congolese Medicinal Plants T1 - Isolierung und Strukturaufklärung von neuen anti-infektiven Naphthylisochinolin-Alkaloiden aus Ancistrocladus ealaensis und phytochemische Analyse von zwei kongolesischen Heilpflanzen N2 - Herein described are the isolation, structural elucidation, and biological evaluation of highly thrilling monomeric and dimeric new naphthylisoquinoline alkaloids from A. ealaensis. The separation, chiral resolution, and characterization of a series of stereoisomeric 2,3-dihydrobenzofuran neolignans are also reported. The analytical and phytochemical analysis on two Congolese antimalarial herbal drugs is part of the last chapter of the results. In this last case, major concerns on widely used Congolese herbal drugs are discussed. N2 - Im Rahmen dieser Dissertation werden Einblicke in die strukturelle Vielfalt und das therapeutische Potenzial von pflanzlichen Sekundärmetaboliten gewährt KW - Isolation KW - Structural elucidation KW - Alkaloid KW - Naphthylisoquinoline KW - Anti-infective KW - Naphthylisochinolinalkaloide KW - Ancistrocladaceae KW - Kongo Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-154175 ER - TY - JOUR A1 - Schlegel, Jan A1 - Peters, Simon A1 - Doose, Sören A1 - Schubert-Unkmeir, Alexandra A1 - Sauer, Markus T1 - Super-resolution microscopy reveals local accumulation of plasma membrane gangliosides at Neisseria meningitidis Invasion Sites JF - Frontiers in Cell and Developmental Biology N2 - Neisseria meningitidis (meningococcus) is a Gram-negative bacterium responsible for epidemic meningitis and sepsis worldwide. A critical step in the development of meningitis is the interaction of bacteria with cells forming the blood-cerebrospinal fluid barrier, which requires tight adhesion of the pathogen to highly specialized brain endothelial cells. Two endothelial receptors, CD147 and the β2-adrenergic receptor, have been found to be sequentially recruited by meningococci involving the interaction with type IV pilus. Despite the identification of cellular key players in bacterial adhesion the detailed mechanism of invasion is still poorly understood. Here, we investigated cellular dynamics and mobility of the type IV pilus receptor CD147 upon treatment with pili enriched fractions and specific antibodies directed against two extracellular Ig-like domains in living human brain microvascular endothelial cells. Modulation of CD147 mobility after ligand binding revealed by single-molecule tracking experiments demonstrates receptor activation and indicates plasma membrane rearrangements. Exploiting the binding of Shiga (STxB) and Cholera toxin B (CTxB) subunits to the two native plasma membrane sphingolipids globotriaosylceramide (Gb3) and raft-associated monosialotetrahexosylganglioside GM1, respectively, we investigated their involvement in bacterial invasion by super-resolution microscopy. Structured illumination microscopy (SIM) and direct stochastic optical reconstruction microscopy (dSTORM) unraveled accumulation and coating of meningococci with GM1 upon cellular uptake. Blocking of CTxB binding sites did not impair bacterial adhesion but dramatically reduced bacterial invasion efficiency. In addition, cell cycle arrest in G1 phase induced by serum starvation led to an overall increase of GM1 molecules in the plasma membrane and consequently also in bacterial invasion efficiency. Our results will help to understand downstream signaling events after initial type IV pilus-host cell interactions and thus have general impact on the development of new therapeutics targeting key molecules involved in infection. KW - Neisseria meningitidis KW - sphingolipids KW - gangliosides and lipid rafts KW - super-resolution microscopy KW - single-molecule tracking Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-201639 VL - 7 IS - 194 ER - TY - JOUR A1 - Grebinyk, Anna A1 - Prylutska, Svitlana A1 - Grebinyk, Sergii A1 - Prylutskyy, Yuriy A1 - Ritter, Uwe A1 - Matyshevska, Olga A1 - Dandekar, Thomas A1 - Frohme, Marcus T1 - Complexation with C\(_{60}\) fullerene increases doxorubicin efficiency against leukemic cells in vitro JF - Nanoscale Research Letters N2 - Conventional anticancer chemotherapy is limited because of severe side effects as well as a quickly evolving multidrug resistance of the tumor cells. To address this problem, we have explored a C\(_{60}\) fullerene-based nanosized system as a carrier for anticancer drugs for an optimized drug delivery to leukemic cells.Here, we studied the physicochemical properties and anticancer activity of C\(_{60}\) fullerene noncovalent complexes with the commonly used anticancer drug doxorubicin. C\(_{60}\)-Doxorubicin complexes in a ratio 1:1 and 2:1 were characterized with UV/Vis spectrometry, dynamic light scattering, and high-performance liquid chromatography-tandem mass spectrometry (HPLC-MS/MS). The obtained analytical data indicated that the 140-nm complexes were stable and could be used for biological applications. In leukemic cell lines (CCRF-CEM, Jurkat, THP1 and Molt-16), the nanocomplexes revealed 3.5 higher cytotoxic potential in comparison with the free drug in a range of nanomolar concentrations. Also, the intracellular drug's level evidenced C\(_{60}\) fullerene considerable nanocarrier function.The results of this study indicated that C\(_{60}\) fullerene-based delivery nanocomplexes had a potential value for optimization of doxorubicin efficiency against leukemic cells. KW - C-60 fullerene KW - doxorubicin KW - noncovalent complex KW - leukemic cells KW - cytotoxicity KW - accumulation Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-228257 VL - 14 IS - 61 ER - TY - JOUR A1 - Grubisic, Maja A1 - Haim, Abraham A1 - Bhusal, Pramod A1 - Dominoni, Davide M. A1 - Gabriel, Katharina M. A. A1 - Jechow, Andreas A1 - Kupprat, Franziska A1 - Lerner, Amit A1 - Marchant, Paul A1 - Riley, William A1 - Stebelova, Katarina A1 - van Grunsven, Roy H. A. A1 - Zeman, Michal A1 - Zubidat, Abed E. A1 - Hölker, Franz T1 - Light Pollution, Circadian Photoreception, and Melatonin in Vertebrates JF - Sustainability N2 - Artificial light at night (ALAN) is increasing exponentially worldwide, accelerated by the transition to new efficient lighting technologies. However, ALAN and resulting light pollution can cause unintended physiological consequences. In vertebrates, production of melatonin—the “hormone of darkness” and a key player in circadian regulation—can be suppressed by ALAN. In this paper, we provide an overview of research on melatonin and ALAN in vertebrates. We discuss how ALAN disrupts natural photic environments, its effect on melatonin and circadian rhythms, and different photoreceptor systems across vertebrate taxa. We then present the results of a systematic review in which we identified studies on melatonin under typical light-polluted conditions in fishes, amphibians, reptiles, birds, and mammals, including humans. Melatonin is suppressed by extremely low light intensities in many vertebrates, ranging from 0.01–0.03 lx for fishes and rodents to 6 lx for sensitive humans. Even lower, wavelength-dependent intensities are implied by some studies and require rigorous testing in ecological contexts. In many studies, melatonin suppression occurs at the minimum light levels tested, and, in better-studied groups, melatonin suppression is reported to occur at lower light levels. We identify major research gaps and conclude that, for most groups, crucial information is lacking. No studies were identified for amphibians and reptiles and long-term impacts of low-level ALAN exposure are unknown. Given the high sensitivity of vertebrate melatonin production to ALAN and the paucity of available information, it is crucial to research impacts of ALAN further in order to inform effective mitigation strategies for human health and the wellbeing and fitness of vertebrates in natural ecosystems. KW - ALAN KW - artificial light at night KW - biological rhythm KW - circadian rhythm KW - melatonin Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193095 SN - 2071-1050 VL - 11 IS - 22 ER - TY - JOUR A1 - Heydarian, Motaharehsadat A1 - Yang, Tao A1 - Schweinlin, Matthias A1 - Steinke, Maria A1 - Walles, Heike A1 - Rudel, Thomas A1 - Kozjak-Pavlovic, Vera T1 - Biomimetic human tissue model for long-term study of Neisseria gonorrhoeae infection JF - Frontiers in Microbiology N2 - Gonorrhea is the second most common sexually transmitted infection in the world and is caused by Gram-negative diplococcus Neisseria gonorrhoeae. Since N. gonorrhoeae is a human-specific pathogen, animal infection models are only of limited use. Therefore, a suitable in vitro cell culture model for studying the complete infection including adhesion, transmigration and transport to deeper tissue layers is required. In the present study, we generated three independent 3D tissue models based on porcine small intestinal submucosa (SIS) scaffold by co-culturing human dermal fibroblasts with human colorectal carcinoma, endometrial epithelial, and male uroepithelial cells. Functional analyses such as transepithelial electrical resistance (TEER) and FITC-dextran assay indicated the high barrier integrity of the created monolayer. The histological, immunohistochemical, and ultra-structural analyses showed that the 3D SIS scaffold-based models closely mimic the main characteristics of the site of gonococcal infection in human host including the epithelial monolayer, the underlying connective tissue, mucus production, tight junction, and microvilli formation. We infected the established 3D tissue models with different N. gonorrhoeae strains and derivatives presenting various phenotypes regarding adhesion and invasion. The results indicated that the disruption of tight junctions and increase in interleukin production in response to the infection is strain and cell type-dependent. In addition, the models supported bacterial survival and proved to be better suitable for studying infection over the course of several days in comparison to commonly used Transwell® models. This was primarily due to increased resilience of the SIS scaffold models to infection in terms of changes in permeability, cell destruction and bacterial transmigration. In summary, the SIS scaffold-based 3D tissue models of human mucosal tissues represent promising tools for investigating N. gonorrhoeae infections under close-to-natural conditions. KW - 3D tissue model KW - small intestinal submucosa scaffold KW - co-culture KW - infection KW - Neisseria gonorrhoeae Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197912 SN - 1664-302X VL - 10 IS - 1740 ER - TY - JOUR A1 - Grebinyk, Anna A1 - Prylutska, Svitlana A1 - Chepurna, Oksana A1 - Grebinyk, Sergii A1 - Prylutskyy, Yuriy A1 - Ritter, Uwe A1 - Ohulchanskyy, Tymish Y. A1 - Matyshevska, Olga A1 - Dandekar, Thomas A1 - Frohme, Marcus T1 - Synergy of chemo- and photodynamic therapies with C\(_{60}\) Fullerene-Doxorubicin nanocomplex JF - Nanomaterials N2 - A nanosized drug complex was explored to improve the efficiency of cancer chemotherapy, complementing it with nanodelivery and photodynamic therapy. For this, nanomolar amounts of a non-covalent nanocomplex of Doxorubicin (Dox) with carbon nanoparticle C\(_{60}\) fullerene (C\(_{60}\)) were applied in 1:1 and 2:1 molar ratio, exploiting C\(_{60}\) both as a drug-carrier and as a photosensitizer. The fluorescence microscopy analysis of human leukemic CCRF-CEM cells, in vitro cancer model, treated with nanocomplexes showed Dox’s nuclear and C\(_{60}\)'s extranuclear localization. It gave an opportunity to realize a double hit strategy against cancer cells based on Dox's antiproliferative activity and C\(_{60}\)'s photoinduced pro-oxidant activity. When cells were treated with 2:1 C\(_{60}\)-Dox and irradiated at 405 nm the high cytotoxicity of photo-irradiated C\(_{60}\)-Dox enabled a nanomolar concentration of Dox and C\(_{60}\) to efficiently kill cancer cells in vitro. The high pro-oxidant and pro-apoptotic efficiency decreased IC\(_{50}\) 16, 9 and 7 × 10\(^3\)-fold, if compared with the action of Dox, non-irradiated nanocomplex, and C\(_{60}\)'s photodynamic effect, correspondingly. Hereafter, a strong synergy of therapy arising from the combination of C\(_{60}\)-mediated Dox delivery and C\(_{60}\) photoexcitation was revealed. Our data indicate that a combination of chemo- and photodynamic therapies with C\(_{60}\)-Dox nanoformulation provides a promising synergetic approach for cancer treatment. KW - photodynamic chemotherapy KW - synergistic effect KW - C\(_{60}\) fullerene KW - Doxorubicin KW - nanocomplex KW - leukemic cells KW - apoptosis Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193140 SN - 2079-4991 VL - 9 IS - 11 ER - TY - JOUR A1 - Villalobos, Alvaro S. A1 - Wiese, Jutta A1 - Imhoff, Johannes F. A1 - Dorador, Cristina A1 - Keller, Alexander A1 - Hentschel, Ute T1 - Systematic affiliation and genome analysis of Subtercola vilae DB165T with particular emphasis on cold adaptation of an isolate from a high-altitude cold volcano lake JF - Microorganisms N2 - Among the Microbacteriaceae the species of Subtercola and Agreia form closely associated clusters. Phylogenetic analysis demonstrated three major phylogenetic branches of these species. One of these branches contains the two psychrophilic species Subtercola frigoramans and Subtercola vilae, together with a larger number of isolates from various cold environments. Genomic evidence supports the separation of Agreia and Subtercola species. In order to gain insight into the ability of S. vilae to adapt to life in this extreme environment, we analyzed the genome with a particular focus on properties related to possible adaptation to a cold environment. General properties of the genome are presented, including carbon and energy metabolism, as well as secondary metabolite production. The repertoire of genes in the genome of S. vilae DB165\(^T\) linked to adaptations to the harsh conditions found in Llullaillaco Volcano Lake includes several mechanisms to transcribe proteins under low temperatures, such as a high number of tRNAs and cold shock proteins. In addition, S. vilae DB165\(^T\) is capable of producing a number of proteins to cope with oxidative stress, which is of particular relevance at low temperature environments, in which reactive oxygen species are more abundant. Most important, it obtains capacities to produce cryo-protectants, and to combat against ice crystal formation, it produces ice-binding proteins. Two new ice-binding proteins were identified which are unique to S. vilae DB165\(^T\). These results indicate that S. vilae has the capacity to employ different mechanisms to live under the extreme and cold conditions prevalent in Llullaillaco Volcano Lake. KW - cold adaptation KW - Subtercola vilae KW - genome analysis KW - systematic affiliation KW - Llullaillaco Volcano Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197394 SN - 2076-2607 VL - 7 IS - 4 ER - TY - JOUR A1 - Liu, Ruiqi A1 - Kinoshita, Masato A1 - Adolfi, Mateus C. A1 - Schartl, Manfred T1 - Analysis of the role of the Mc4r system in development, growth, and puberty of medaka JF - Frontiers in Endocrinology N2 - In mammals the melanocortin 4 receptor (Mc4r) signaling system has been mainly associated with the regulation of appetite and energy homeostasis. In fish of the genus Xiphophorus (platyfish and swordtails) puberty onset is genetically determined by a single locus, which encodes the mc4r. Wild populations of Xiphophorus are polymorphic for early and late-maturing individuals. Copy number variation of different mc4r alleles is responsible for the difference in puberty onset. To answer whether this is a special adaptation of the Mc4r signaling system in the lineage of Xiphophorus or a more widely conserved mechanism in teleosts, we studied the role of Mc4r in reproductive biology of medaka (Oryzias latipes), a close relative to Xiphophorus and a well-established model to study gonadal development. To understand the potential role of Mc4r in medaka, we characterized the major features of the Mc4r signaling system (mc4r, mrap2, pomc, agrp1). In medaka, all these genes are expressed before hatching. In adults, they are mainly expressed in the brain. The transcript of the receptor accessory protein mrap2 co-localizes with mc4r in the hypothalamus in adult brains indicating a conserved function of modulating Mc4r signaling. Comparing growth and puberty between wild-type and mc4r knockout medaka revealed that absence of Mc4r does not change puberty timing but significantly delays hatching. Embryonic development of knockout animals is retarded compared to wild-types. In conclusion, the Mc4r system in medaka is involved in regulation of growth rather than puberty. KW - medaka KW - Mc4r KW - knockout KW - puberty KW - growth Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-201472 VL - 10 ER - TY - JOUR A1 - Krebs, Markus A1 - Behrmann, Christoph A1 - Kalogirou, Charis A1 - Sokolakis, Ioannis A1 - Kneitz, Susanne A1 - Kruithof-de Julio, Marianna A1 - Zoni, Eugenio A1 - Rech, Anne A1 - Schilling, Bastian A1 - Kübler, Hubert A1 - Spahn, Martin A1 - Kneitz, Burkhard T1 - miR-221 Augments TRAIL-mediated apoptosis in prostate cancer cells by inducing endogenous TRAIL expression and targeting the functional repressors SOCS3 and PIK3R1 JF - BioMed Research International N2 - miR-221 is regarded as an oncogene in many malignancies, and miR-221-mediated resistance towards TRAIL was one of the first oncogenic roles shown for this small noncoding RNA. In contrast, miR-221 is downregulated in prostate cancer (PCa), thereby implying a tumour suppressive function. By using proliferation and apoptosis assays, we show a novel feature of miR-221 in PCa cells: instead of inducing TRAIL resistance, miR-221 sensitized cells towards TRAIL-induced proliferation inhibition and apoptosis induction. Partially responsible for this effect was the interferon-mediated gene signature, which among other things contained an endogenous overexpression of the TRAIL encoding gene TNFSF10. This TRAIL-friendly environment was provoked by downregulation of the established miR-221 target gene SOCS3. Moreover, we introduced PIK3R1 as a target gene of miR-221 in PCa cells. Proliferation assays showed that siRNA-mediated downregulation of SOCS3 and PIK3R1 mimicked the effect of miR-221 on TRAIL sensitivity. Finally, Western blotting experiments confirmed lower amounts of phospho-Akt after siRNA-mediated downregulation of PIK3R1 in PC3 cells. Our results further support the tumour suppressing role of miR-221 in PCa, since it sensitises PCa cells towards TRAIL by regulating the expression of the oncogenes SOCS3 and PIK3R1. Given the TRAIL-inhibiting effect of miR-221 in various cancer entities, our results suggest that the influence of miR-221 on TRAIL-mediated apoptosis is highly context- and entity-dependent. KW - Cancer Cell Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-202480 VL - 2019 ER - TY - JOUR A1 - Molinas-González, Carlos R. A1 - Castro, Jorge A1 - González-Megías, Adela A1 - Leverkus, Alexandro B. T1 - Effects of post-fire deadwood management on soil macroarthropod communities JF - Forests N2 - Dead wood comprises a vast amount of biological legacies that set the scene for ecological regeneration after wildfires, yet its removal is the most frequent management strategy worldwide. Soil-dwelling organisms are conspicuous, and they provide essential ecosystem functions, but their possible affection by different post-fire management strategies has so far been neglected. We analyzed the abundance, richness, and composition of belowground macroarthropod communities under two contrasting dead-wood management regimes after a large wildfire in the Sierra Nevada Natural and National Park (Southeast Spain). Two plots at different elevation were established, each containing three replicates of two experimental treatments: partial cut, where trees were cut and their branches lopped off and left over the ground, and salvage logging, where all the trees were cut, logs were piled, branches were mechanically masticated, and slash was spread on the ground. Ten years after the application of the treatments, soil cores were extracted from two types of microhabitat created by these treatments: bare-soil (in both treatments) and under-logs (in the partial cut treatment only). Soil macroarthropod assemblages were dominated by Hemiptera and Hymenoptera (mostly ants) and were more abundant and richer in the lowest plot. The differences between dead-wood treatments were most evident at the scale of management interventions: abundance and richness were lowest after salvage logging, even under similar microhabitats (bare-soil). However, there were no significant differences between microhabitat types on abundance and richness within the partial cut treatment. Higher abundance and richness in the partial cut treatment likely resulted from higher resource availability and higher plant diversity after natural regeneration. Our results suggest that belowground macroarthropod communities are sensitive to the manipulation of dead-wood legacies and that management through salvage logging could reduce soil macroarthropod recuperation compared to other treatments with less intense management even a decade after application. KW - forest fire KW - burnt-wood KW - species richness KW - soil fauna KW - post-fire management Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193079 SN - 1999-4907 VL - 10 IS - 11 ER - TY - JOUR A1 - Latifi, Hooman A1 - Valbuena, Ruben T1 - Current trends in forest ecological applications of three-dimensional remote sensing: Transition from experimental to operational solutions? JF - Forests N2 - The alarming increase in the magnitude and spatiotemporal patterns of changes in composition, structure and function of forest ecosystems during recent years calls for enhanced cross-border mitigation and adaption measures, which strongly entail intensified research to understand the underlying processes in the ecosystems as well as their dynamics. Remote sensing data and methods are nowadays the main complementary sources of synoptic, up-to-date and objective information to support field observations in forest ecology. In particular, analysis of three-dimensional (3D) remote sensing data is regarded as an appropriate complement, since they are hypothesized to resemble the 3D character of most forest attributes. Following their use in various small-scale forest structural analyses over the past two decades, these sources of data are now on their way to be integrated in novel applications in fields like citizen science, environmental impact assessment, forest fire analysis, and biodiversity assessment in remote areas. These and a number of other novel applications provide valuable material for the Forests special issue “3D Remote Sensing Applications in Forest Ecology: Composition, Structure and Function”, which shows the promising future of these technologies and improves our understanding of the potentials and challenges of 3D remote sensing in practical forest ecology worldwide. KW - 3D remote sensing KW - composition KW - forest ecology KW - function KW - structure Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193282 SN - 1999-4907 VL - 10 IS - 10 ER - TY - THES A1 - Derakhshani, Shaghayegh T1 - Measles virus infection enhances dendritic cell migration in a 3D environment T1 - Die Masernvirusinfektion verstärkt die Migration dendritischer Zellen in einer 3D-Umgebung N2 - The respiratory system is amongst the most important compartments in the human body. Due to its connection to the external environment, it is one of the most common portals of pathogen entry. Airborne pathogens like measles virus (MV) carried in liquid droplets exhaled from the infected individuals via a cough or sneeze enter the body from the upper respiratory tract and travel down to the lower respiratory tract and reach the alveoli. There, pathogens are captured by the resident dendritic cells (DCs) or macrophages and brought to the lymph node where immune responses or, as in case of MV, dissemination via the hematopoietic cell compartment are initiated. Basic mechanisms governing MV exit from the respiratory tract, especially virus transmission from infected immune cells to the epithelial cells have not been fully addressed before. Considering the importance of these factors in the viral spread, a complex close-to-in-vivo 3D human respiratory tract model was generated. This model was established using de-cellularized porcine intestine tissue as a biological scaffold and H358 cells as targets for infection. The scaffold was embedded with fibroblast cells, and later on, an endothelial cell layer seeded at the basolateral side. This provided an environment resembling the respiratory tract where MV infected DCs had to transmigrate through the collagen scaffold and transmit the virus to epithelial cells in a Nectin-4 dependent manner. For viral transmission, the access of infected DCs to the recipient epithelial cells is an essential prerequisite and therefore, this important factor which is reflected by cell migration was analyzed in this 3D system. The enhanced motility of specifically MV-infected DCs in the 3D models was observed, which occurred independently of factors released from the other cell types in the models. Enhanced motility of infected DCs in 3D collagen matrices suggested infection-induced cytoskeletal remodeling, as also verified by detection of cytoskeletal polarization, uropod formation. This enforced migration was sensitive to ROCK inhibition revealing that MV infection induces an amoeboid migration mode in DCs. In support of this, the formation of podosome structures and filopodia, as well as their activity, were reduced in infected DCs and retained in their uninfected siblings. Differential migration modes of uninfected and infected DCs did not cause differential maturation, which was found to be identical for both populations. As an underlying mechanism driving this enforced migration, the role of sphingosine kinase (SphK) and sphingosine-1-phosphate (S1P) was studied in MV-exposed cultures. It was shown in this thesis that MV-infection increased S1P production, and this was identified as a contributing factor as inhibition sphingosine kinase activity abolished enforced migration of MV-infected DCs. These findings revealed that MV infection induces a fast push-and-squeeze amoeboid mode of migration, which is supported by SphK/S1P axis. However, this push-and-squeeze amoeboid migration mode did not prevent the transendothelial migration of MV-infected DCs. Altogether, this 3D system has been proven to be a suitable model to study specific parameters of mechanisms involved in infections in an in vivo-like conditions. N2 - Die respiratorische System ist ein wesentlicher physiologischer Bestandteil. Durch die direkte und konstante Verbindung der Atemwege mit der äußeren Umgebung sind sie einer der häufigsten Pfade für den Eintritt von Krankheitserregern in den Körper. Luftübertragene Krankheitserreger wie das Masern-Virus (MV), das in Flüssigkeitströpfchen mitgeführt und von Patienten durch Husten oder Niesen ausgeatmet wird, können über die oberen Atemwege in den Körper gelangen und sich bis in die unteren Atemwege und bis zu den Alveolen ausbreiten. Dort werden diese Krankheitserreger von den dort residenten dendritischen Zellen (DC) oder Makrophagen erworben und zu sekundären lymphatischen Organen transportiert, in denen sowohl virus-spezifische Immunantworten, aber auch – wie im Falle von MV – die hämatogene Dissemination initiiert wird. Der Austrittsmechanismus des MV aus den Atemwegen, insbesondere dessen Übertragung von infizierten Immunzellen auf die Epithelzellen und die Faktoren, die diesen Ablauf bestimmen, wurden jedoch bisher unzureichend untersucht. In Anbetracht der Bedeutung dieser Faktoren für die Virusausbreitung wurde ein komplexes, realitätsnahes in-vivo 3D-Modell der menschlichen Atemwege erstellt. Dieses Modell wurde unter Verwendung von de-zellularisiertem Schweinedarmgewebe als biologischem Gerüst und H358 Epithelzellen als Empfänger etabliert. Dieses Grundgerüst wurde mit Fibroblastenzellen eingebettet. Später wurde auf der basolateralen Seite der Modelle eine Endothelzellschicht eingebracht, um eine Umgebung zu schaffen, die der der Atemwege ähnelt. Somit mussten die Virus-Donoren, MV-infizierte DC durch das Kollagengerüst wandern und das Virus auf Epithelzellen in einer Nektin-4 abhängigen Weise übertragen. Für die Virusübertragung ist der Zugang infizierter DC zu den Empfänger-Epithelzellen eine wesentliche Voraussetzung, weshalb dieser wichtige Faktor, der sich in der Zellmigration widerspiegelt, in diesem 3D-System analysiert wurde. Eine erhöhte Beweglichkeit spezifisch MV-infizierter DCs wurde in den 3D-Modellen beobachtet. Dies erwies sich als unabhängig von löslichen Faktoren der anderen Zelltypen in den Modellen. Erhöhte Beweglichkeit infizierten DCs wurde auch in 3D-Kollagenmatrizes gesehen, was auf einen infektionsvermittelten zytoskelettalen Umbau hindeutete, der auch anhand von Zytoskelettpolarisation und Uropodbildung bestätigt wurde. Die MV-Infektion induzierte einen schnellen amöboiden Migrationsmodus in den DCs, der sich als sensitiv gegenüber ROCK-Hemmung erwies. Im Gegensatz zu uninfizierten DCs gleichen Reifungsstadiums waren in infizierten DCs Podosomenstrukturen und Filopodien sowie deren Aktivität stark reduziert. Als potentiell zur verstärkten Motilität infizierter DCs beitragender Faktor wurde die Rolle der Sphingosinkinase (SphK) und des Sphingosin-1-phosphats (S1P) in MV-exponierten Kulturen untersucht. In dieser Arbeit wurde gezeigt, dass die S1P-Produktion durch eine MV-Infektion erhöht wurde, und in der Tat zur für infizierte DCs beobachteten erhöhten Geschwindigkeit beitrug, da diese sensitiv gegenüber Hemmung der Sphingosinkinase-Aktivität war. Diese Ergebnisse zeigen, dass die MV-Infektion einen schnellen amöboid-artigen Migrationsmodus induziert, der von der SphK/S1P-Achse unterstützt wird. Dieser Push-and-Squeeze-Amoeboid-Migrationsmodus verhinderte jedoch nicht die transendotheliale Migration von MV-infizierten DCs. Insgesamt hat sich dieses 3D-System als geeignetes Modell erwiesen, um die spezifische Parameter von Mechanismen von Infektionen in einem in-vivo-ähnlichen Zustand zu untersuchen. KW - Dendritische Zelle KW - Zell Migration KW - Masern-Virus KW - 3D-Modell KW - Sphingosine-1-phosphats KW - Dendritic cell KW - Cell migration KW - Measles virus KW - 3D tissue model KW - Tissue engineering KW - Sphingosine-1-phosphate Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189182 ER - TY - JOUR A1 - Hovestadt, Thomas A1 - Thomas, Jeremy A. A1 - Mitesser, Oliver A1 - Schönrogge, Karsten T1 - Multiple host use and the dynamics of host-switching in host-parasite systems JF - Insect Conservation and Diversity N2 - The link between multi‐host use and host switching in host–parasite interactions is a continuing area of debate. Lycaenid butterflies in the genus Maculinea, for example, exploit societies of different Myrmica ant species across their ranges, but there is only rare evidence that they simultaneously utilise multiple hosts at a local site, even where alternative hosts are present. We present a simple population‐genetic model accounting for the proportion of two alternative hosts and the fitness of parasite genotypes on each host. In agreement with standard models, we conclude that simultaneous host use is possible whenever fitness of heterozygotes on alternative hosts is not too low. We specifically focus on host‐shifting dynamics when the frequency of hosts changes. We find that (i) host shifting may proceed so rapidly that multiple host use is unlikely to be observed, (ii) back and forth transition in host use can exhibit a hysteresis loop, (iii) the parasites' host use may not be proportional to local host frequencies and be restricted to the rarer host under some conditions, and (iv) that a substantial decline in parasite abundance may typically precede a shift in host use. We conclude that focusing not just on possible equilibrium conditions but also considering the dynamics of host shifting in non‐equilibrium situations may provide added insights into host–parasite systems. KW - Host-parasite interaction KW - Maculinea butterfly KW - Myrmica ant non-equilibrium dynamics KW - population genetics Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-204747 VL - 12 IS - 6 ER - TY - THES A1 - Wilde, Sabrina T1 - Einsatz von mechanistischen Biomarkern zur Charakterisierung und Bewertung von \(in\) \(vitro\) Genotoxinen T1 - Use of mechanistic biomarkers for the characterization and evaluation of \(in\) \(vitro\) genotoxins N2 - Die verfügbaren in vitro Genotoxizitätstests weisen hinsichtlich ihrer Spezifität und ihres Informationsgehalts zum vorliegenden Wirkmechanismus (Mode of Action, MoA) Einschränkungen auf. Um diese Mängel zu überwinden, wurden in dieser Arbeit zwei Ziele verfolgt, die zu der Entwicklung und Etablierung neuer in vitro Methoden zur Prüfung auf Genotoxizität in der Arzneimittelentwicklung beitragen. 1. Etablierung und Bewertung einer neuen in vitro Genotoxizitätsmethode (MultiFlow Methode) Die MultiFlow Methode basiert auf DNA-schadensassoziierten Proteinantworten von γH2AX (DNA-Doppelstrangbrüche), phosphorylierten H3 (S10) (mitotische Zellen), nukleären Protein p53 (Genotoxizität) und cleaved PARP1 (Apoptose) in TK6-Zellen. Insgesamt wurden 31 Modellsubstanzen mit dem MultiFlow Assay und ergänzend mit dem etablierten Mikrokerntest (MicroFlow MNT), auf ihre Fähigkeit verschiedene MoA-Gruppen (Aneugene/Klastogene/Nicht-Genotoxine) zu differenzieren, untersucht. Die Performance der „neuen“ gegenüber der „alten“ Methode führte zu einer verbesserten Sensitivität von 95% gegenüber 90%, Spezifität von 90% gegenüber 72% und einer MoA-Klassifizierungsrate von 85% gegenüber 45% (Aneugen vs. Klastogen). 2. Identifizierung mechanistischer Biomarker zur Klassifizierung genotoxischer Substanzen Die Analyse 67 ausgewählter DNA-schadensassoziierter Gene in der QuantiGene Plex Methode zeigte, dass mehrere Gene gleichzeitig zur MoA-Klassifizierung beitragen können. Die Kombination der höchstrangierten Marker BIK, KIF20A, TP53I3, DDB2 und OGG1 ermöglichte die beste Identifizierungsrate der Modellsubstanzen. Das synergetische Modell kategorisierte 16 von 16 Substanzen korrekt in Aneugene, Klastogene und Nicht-Genotoxine. Unter Verwendung der Leave-One-Out-Kreuzvalidierung wurde das Modell evaluiert und erreichte eine Sensitivität, Spezifität und Prädiktivität von 86%, 83% und 85%. Ergebnisse der traditionellen qPCR Methode zeigten, dass Genotoxizität mit TP53I3, Klastogenität mit ATR und RAD17 und oxidativer Stress mit NFE2L2 detektiert werden kann. Durch die Untersuchungen von posttranslationalen Modifikationen unter Verwendung der High-Content-Imaging-Technologie wurden mechanistische Assoziationen für BubR1 (S670) und pH3 (S28) mit Aneugenität, 53BP1 (S1778) und FANCD2 (S1404) mit Klastogenität, p53 (K373) mit Genotoxizität und Nrf2 (S40) mit oxidativem Stress identifiziert. Diese Arbeit zeigt, dass (Geno)toxine unterschiedliche Gen- und Proteinveränderungen in TK6-Zellen induzieren, die zur Erfassung mechanistischer Aktivitäten und Einteilung (geno)toxischer MoA-Gruppen (Aneugen/Klastogen/ Reaktive Sauerstoffspezies) eingesetzt werden können und daher eine bessere Risikobewertung von Wirkstoffkandidaten ermöglichen. N2 - Available in vitro genotoxicity tests have limitations regarding their specificity and mode of action (MoA) information. To overcome these shortages, two objectives were pursued in this work to develop and establish new in vitro tools for genotoxicity testing. 1. Establishment and evaluation of a novel in vitro genotoxicity method (MultiFlow method) The MultiFlow method is based on DNA damage-related protein responses of γH2AX (DNA double-strand breaks), phosphorylated H3 (S10) (mitotic cells), nuclear protein p53 (genotoxicity) and cleaved PARP1 (apoptosis) in TK6 cells. In total, 31 model substances were studied flow cytometrically in the MultiFlow assay - and also with the well-established micronucleus test (MicroFlow MNT) - for their ability to classify across MoA groups: aneugens, clastogens and non-genotoxicants. The performance of the new method resulted in an improved sensitivity of 95% to 90%, specificity of 90% to 72% and a MoA classification rate of 85% to 45% (aneugen vs. clastogen). 2. Identification of mechanistic biomarkers for the characterization of genotoxicants The analysis of 67 selected DNA-damage associated genes using the QuantiGene Plex method showed that a combinaten of genes can contribute to MoA classification. The combination of the highest-ranked markers (BIK, KIF20A, TP53I3, DDB2 and OGG1) highlighted the best identification rate of model substances. The synergistic statistic tool correctly categorized 16 of 16 substances into aneugens, clastogens and non-genotoxicants. By using leave-one out cross validation, the model was evaluated and achieved a sensitivity, specificity and predictivity of 86%, 83%, 85% respectively. Follow-up with qPCR was conducted and revealed associations with TP53I3 for genotoxicity, ATR and RAD17 for clastogenicity and NFE2L2 for oxidative stress. By investigating posttranslational modifications using high-content imaging, associations for BubR1 (S670) and pH3 (S28) with aneugenicity, 53BP1 (S1778) and FANCD2 (S1404) with clastogenicity, p53 (K373) with genotoxicity and Nrf2 (S40) with oxidative stress were found to be further useful for MoA identification. This work demonstrates that genotoxicants and non-genotoxicants induce different gene- and protein expression changes in the TK6 cells that can be used to classify the MoA groups (aneugen/clastogen/non-genotoxicant/reactive oxygen species), thus enabling better risk assessment of potential drug candidates. KW - Genotoxizität KW - Genotoxicitiy KW - Klastogene KW - Aneugene KW - Biomarker KW - Klassifizierung KW - clastogens KW - aneugens KW - biomarker KW - classification Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-182782 ER -