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Africa meets Frankfurt
(2012)
The canonical Wnt pathway, also known as Wnt/β-‐catenin pathway, comprises a network of proteins which control diverse developmental and adult processes in all metazoan organisms. The binding of canonical Wnt ligands to a cell surface receptor complex, consisting of frizzled family members and low density lipoprotein receptor-‐ related protein 5 or 6 co‐receptors, triggers a signaling cascade which results in a β-catenin-‐mediated transcriptional activation of different target genes, implicated in cellular proliferation, apoptosis, migration and differentiation. A couple of years ago, several groups including us, iden2fied transient activation of the canonical Wnt-pathway in endothelial cells (ECs) of the developing central nervous system (CNS). In this context, Wnt/β-‐catenin signaling could be demonstrated to be crucial for brain angio genesis as well as for the establishment of the blood-brain barrier (BBB) phenotype in the newly formed vessels.
Gliomas, in particular the glioblastoma (GBM), belong to the group of highly vascularized solid tumors which gain their vascularization due to an angiogenic switch occurring during tumor progression. Interestingly, nuclear localized β-‐catenin could be exclusively detected in the activated endothelium of induced rat gliomas and of human GBM, suggesting a so far unknown and not further characterized involvement of the canonical Wnt pathway in pathological angiogenesis. In order to systematically decipher the precise role of endothelial Wnt/β-‐catenin signaling in tumor angiogenesis, I established
murine GL261 glioma cell lines overexpressing either Wnt1 or Dickkopf (Dkk) 1 in a doxycycline-‐dependent manner, an activator and potent inhibitor of Wnt/β-‐catenin signaling, respectively. In subcutaneous and intracranial transplantations, tumor-derived Wnt1 reduced, while Dkk1 increased GL261 tumor growth without affecting in vitro proliferation, cell cycle or cell death of the established cell lines. Nowadays, it is well accepted that solid tumors are dependent on vascular support allowing them to grow beyond a certain size. In my work I could show that tumor-‐derived Wnt1 targets the tumor vasculature by increasing endothelial Wnt/β-‐catenin signaling, which reduced tumor vessel density and resulted in a more quiescent tumor vasculature. Furthermore, Wnt1-‐expression mediated tight association of smooth muscle cells (SMCs) and pericytes to the tumor endothelium, a phenotype which is unusual for tumor vessels and a described hallmark of tumor vessel normalization. In contrast, inhibition of endothelial Wnt/β-‐catenin signaling by Dkk1 mediated an opposing effect, characterized by endothelial hyper-proliferation and a tumor vasculature with a rough basal lamina distribution and loosely anached mural cells, indicative of a strong angiogenic activity. The described vascular effects in Wnt1-expressing GL261 tumors could be verified by subcutaneous transplantations of a rat glioma cell line constitutively expressing Wnt1. Furthermore, an applied in vivo MatrigelTM plug assay uncovered the reduction in vessel density upon Wnt1 simulation to be tumor cell independent, suggesting an EC-‐autonomous effect. This hypothesis was confirmed by subcutaneous transplantations of parental GL261 cells into mice with genetically generated endothelial β-‐catenin gain-of-function (GOF). The derived GOF tumor from this experiment comprised a quiescent and normalized tumor vasculature and phenocopied the vascular effects observed in Wnt1-expressing tumors.
Our previous work provided evidence that Wnt/β-‐catenin signaling contributes to the BBB phenotype of the developing CNS through the transcriptional regulation of the tight junction protein claudin-‐3. Furthermore, the coverage of pericytes to brain vessels has been described to correlate with BBB integrity. In agreement with these publications, vessels of intracranial Wnt1-‐expressing GL261 tumors retained or regained barrier properties, indicated by a reduced leakage of the tracer Evans blue and endogenous mouse immunoglobulin G and increased junctional localiza2on of the tight junction proteins claudin-‐3, -‐5 and zonula occludens-‐1.
Overall, we detected sustained endothelial Wnt/β-‐catenin signaling to induce a quiescent and normalized tumor vascularization. Interestingly, the Notch signaling pathway has been shown to inhibit the angiogenic tip cell and to promote the quiescent stalk cell phenotype via its ligand Delta-like ligand 4 (Dll4) and the receptors Notch1 and 4. Mechanistically, my work demonstrated for the first time that overactivation of endothelial Wnt/β-‐catenin signaling reactivated expression of Dll4 in the tumor endothelium, which could be shown in vitro to increase Notch signaling and to favor a stalk cell-like gene signature. Furthermore, we uncovered the platelet-derived growth factor subunit B (pdgm) as a novel transcriptional target of Wnt/β-catenin signaling in ECs. Hence endothelial-‐derived PDGF-‐B is known to promote the recruitment of mural cells, the upregulation of this factor might explain the increased SMC/pericyte coverage observed in the tumor vasculature upon sustained endothelial Wnt/β-‐catenin signaling which additionally might promote a cycle of vascular normalization.
Taken together, my work reveals several vascular effects, being mediated by reinforced endothelial Wnt/β-‐catenin signaling during tumor angiogenesis. While a moderate level of canonical Wnt signaling, observed in vessels of human astrocytomas and murine control tumors, is considered to be associated with tumor angiogenesis, dominant activation of this pathway in ECs is shown to limit angiogenesis and to promote a quiescent and normalized tumor vasculature with increased barrier properties. Furthermore, my work discovers pdgm as a novel target of canonical Wnt signaling in ECs.
The work presented in this dissertation therefore not only uncovers the role of endothelial Wnt/β-‐catenin signaling in tumor angiogenesis but additionally reveals this pathway to be a novel modulator in pathological vessel development which might proof to be a valuable therapeutic target for anti-angiogenic and edema glioma therapy.
The brain is characterized by its immune privileged state. However, recent studies suggest an extended contribution of hematopoietic cells to the brain. After transplantation of genetically labeled bone marrow into bone marrow depleted mice, not only labeled blood cells but also labeled neurons and other non-hematopoietic cells can be observed. Initially interpreted as transdifferentiated hematopoietic stem cells, this contribution later was identified as cell fusion of hematopoietic cells and neurons. Our lab previously addressed the question whether these fusion events also occur under non-invasive conditions. A Cre-LoxP based transgenic mouse line was used to irreversibly label all hematopoietic cells. In these mice, Cre expression is controlled by a hematopoietic promoter, thus causing recombination and subsequent marker gene expression restricted to blood cells. Interestingly, contribution of these hematopoietic cells to non-hematopoietic tissues was observed, but fusion could be excluded as the underlying mechanism. The Cre mRNA or protein seems to reach the non-hematopoietic cells from an external source. Extracellular vesicles, specifically exosomes, are increasingly recognized as a vehicle for the intercellular transfer of cellular components such as proteins or mRNAs. However, if they contribute to signaling between tissues in vivo is completely unknown and would represent a major paradigm shift for intercellular communication. Therefore, the aim of this PhD study is to investigate whether an exosomal transfer between the hematopoietic system and the brain exists. To confirm the previous results, a second Cre-LoxP mouse line that expresses the Cre recombinase under a different hematopoietic promoter is used additionally. Both mouse lines are screened for recombination and show comparable numbers and types of different non-hematopoietic cells. Besides hepatocytes and cells in lung and intestine, recombined Purkinje neurons in the cerebellum are detectable. To assess the influence of inflammation on these recombination events, different lesions such as peripheral tumors or peritonitis are applied to the mice. Inflammatory stimuli strongly increase the numbers of recombined Purkinje neurons. These neurons remain mononuclear, indicating that fusion does not occur. Also in human cerebellar material, no evidence for inflammation induced cell fusion is detectable. To screen for Cre recombinase containing exosomes, exosome purification protocols such as differential ultracentrifugation and sucrose gradient fractioning, are applied. The exosomal content is analyzed with nested PCR and western blot. Hematopoietically expressed Cre mRNA is detectable in blood plasma and hematopoietic cell culture conditioned medium. Further analysis reveals that this Cre mRNA but no Cre protein is contained in exosomes. The exosomal ability to induce recombination is investigated by injections into Cre reporter mice. After direct cerebellar injection, exosomes are sufficient to induce recombination of Purkinje neurons. Brain tissue of mice that received an inflammation is analyzed further to reveal other recombined cell types. The main immune cells of the brain, microglia, are not recombined. Mainly neuronal cell types are recombined in different areas of the brain. The observations made in this study are consistent with the hypothesis that a previously unrecognized way to communicate RNA based signals between the immune system and the brain exists. Specifically neurons are target cells for the uptake of hematopoietic exosomes and seem able to translate exosomal mRNA into functional protein. Microglial cells are neither involved as target cells, nor do they release Cre containing exosomes. By using the Cre-LoxP system, in vivo tracing of exosomes could be achieved for the first time. With this knowledge, other exosomal routes can be uncovered in future. The discovery of the exosomal transfer between the blood and the brain enables further research about the relevance of this signaling pathway. It will be important to investigate its role especially in the context of neural malfunctions and further studies might help to find new therapeutical approaches.
Die Arbeit entstand im Rahmen des Förderprogramms ”Profil NT” und war Bestandteil des BMBF–Projektes ”NANOTHERM” (FKZ17PNT005). Dabei sollte die Möglichkeit der Integration und Verwendung von Nanodrähten als funktionsbestimmende Komponente im thermoelektrischen Sensorelement untersucht werden. Eine wichtige Aufgabe bestand darin die thermoelektrischen Eigenschaften der einzelnen Nanodrähte, insbesondere den Seebeck–Koeffizienten, zu untersuchen. Im Hinblick auf die weitere Entwicklung der Nanotechnologie ist es sehr wichtig, geeignete Messplattformen zu generieren und der Wissenschaftlichen Gemeinschaft zur Verfügung zu stellen für die Charakterisierung von Nanostrukturen. Für die Forschung bedeutet dies, dass man immer präziser die ”Physik im kleinen” studieren kann. Im Bezug auf die Anwendungen stellen die ausgeführten Untersuchungen eine wesentliche Basis für die Bauelemente–Optimierung und ihren späteren industriellen Einsatz dar.
In dieser Arbeit werden zwei Chipdesigns vorgestellt für die Bestimmung des Seebeck–Koeffizienten, die eine ausreichend hohe Temperaturdifferenz in Nanostrukturen erzeugen. Für beide Chips wird die mikromechanische Fertigung im einzelnen erläutert. Zusätzlich wurden die Chips in FEM–Simulationen analysiert. Eine messtechnische Charakterisierung der Chips bestätigt die Simulationen und die Funktionsweise der Chips für Untersuchungen des Seebeck–Koeffizienten an Nanostrukturen. Erstmals wurden Wolfram bzw. Platin FEBID–Deponate hinsichtlich des Seebeck–Koeffizienten untersucht. Für die Wolfram–Deponate ergab sich ein negativer Seebeck–Koeffizient. Der gemessenen Seebeck–Koeffizient war über mehrere Tage stabil. Als Ergebnis temperaturabhängiger Messungen des Seebeck–Koeffizienten konnte eine Wurzel-T Abhängigkeit beobachtet werden, die in der Theorie beschrieben wird.
Eine Untersuchung des Seebeck–Koeffizienten an Pt–FEBID–Deponaten zeigt einen Vorzeichenwechsel für Proben mit geringer elektrischer Leitfähigkeit (isolierender Charakter, schwache Kopplung). In der Literatur wird dieser Vorzeichenwechsel allerdings für Proben mit metallischer elektrischer Leitfähigkeit beschrieben. Aufgrund der Messergebnisse ist zu prüfen inwiefern die Theorie des Seebeck–Koeffizienten auf Proben mit schwacher Kopplung zu übertragen ist. Da die gemessenen Seebeck–Koeffizienten bei einigen nanoskaligen Proben sehr klein waren, wurde der Seebeck–Koeffizient des Kontaktmaterials in separaten Versuchen untersucht. Für das hier verwendete Schichtsystem Ti(40nm)/Au(120nm) kann ein Seebeck–Koeffizient von -0,22µV/K angegeben werden. Bei der Charakterisierung der Pt–FEBID–Deponaten wurde dieser Beitrag des Kontaktschichtsystems zur Thermospannung berücksichtigt.
Untersuchungen an BiTe–Nanodrähten mit dem Seebeck–Chip ergaben einen negativen Seebeck–Koeffizienten. Die ersten Untersuchungen wurden mit Kupfer als Kontaktmaterial durchgeführt, weil dieses sehr gute Lift–Off Eigenschaften besaß. Trotz der Kupferdiffusion in den Nanodraht hinein, wird der negative Seebeck–Koeffizient einem Tellur–Überschuss zugeschrieben, denn an Proben mit einer geeigneten Diffusionsbarriere war in nachfolgenden Untersuchungen ebenso ein negativer Seebeck–Koeffizient zu messen. Die ermittelten Beweglichkeiten sind niedriger als die von Bulkmaterial und können durch klassische Size–Effekte erklärt werden. Die gemessenen Ladungsträgerkonzentrationen liegen in typischen Bereichen für Halbmetalle. Die Charakterisierung des Seebeck–Koeffizienten mit Hilfe des hier vorgestellten Z–Chip ergab einen negativen Seebeck–Koeffizienten für die BiTe–Nanodrähte, die wie oben erläutert auf einen Tellur–Überschuss zurückzuführen sind. Eine Abschätzung eines mit Nanodrähten aufgebauten Sensors zeigt, dass im Vergleich zu konventionellen Dünnschicht–Thermopiles deutlich höhere Empfindlichkeiten zu erzielen sind. Erste technologische Konzepte für den Aufbau von Nanodraht–Arrays wurden erarbeitet und durch entsprechende Untersuchungen verifiziert.
Grundsätzlich ist der Z–Chip für die Charakterisierung aller drei Transportkoeffizienten geeignet und bietet die Option, anderen Arbeitsgruppen eine universelle thermoelektrische Messplattform zur Verfügung zu stellen.