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B cell development in bone marrow is a precisely regulated complex process. Through successive stages of differentiation, which are regulated by a multitude of signaling pathways and an array of lineage-specific transcription factors, the common lymphoid progenitors ultimately give rise to mature B cells. Similar to early thymocyte development in the thymus, early B cell development in bone marrow is critically dependent on IL-7 signaling. During this IL-7-dependent stage of differentiation, several transcription factors, such as E2A, EBF1, and Pax5, among others, play indispensable roles in B lineage specification and maintenance. Although recent studies have implicated several other transcription factors in B cell development, the role of NFATc1 in early B cell developmental stages is not known. Here, using multiple gene-manipulated mouse models and applying various experimental methods, we show that NFATc1 activity is vital for early B cell differentiation. Lack of NFATc1 activity in pro-B cells suppresses EBF1 expression, impairs immunoglobulin gene rearrangement, and thereby preBCR formation, resulting in defective B cell development. Overall, deficiency in NFATc1 activity arrested the pro-B cell transition to the pre-B cell stage, leading to severe B cell lymphopenia. Our findings suggest that, along with other transcription factors, NFATc1 is a critical component of the signaling mechanism that facilitates early B cell differentiation.
The potential of human-induced pluripotent stem cells (hiPSCs) to be differentiated into cardiomyocytes (CMs) mimicking adult CMs functional morphology, marker genes and signaling characteristics has been investigated since over a decade. The evolution of the membrane localization of CM-specific G protein-coupled receptors throughout differentiation has received, however, only limited attention to date. We employ here advanced fluorescent spectroscopy, namely linescan Fluorescence Correlation Spectroscopy (FCS), to observe how the plasma membrane abundance of the β\(_1\)- and β\(_2\)-adrenergic receptors (β\(_{1/2}\)-ARs), labelled using a bright and photostable fluorescent antagonist, evolves during the long-term monolayer culture of hiPSC-derived CMs. We compare it to the kinetics of observed mRNA levels in wildtype (WT) hiPSCs and in two CRISPR/Cas9 knock-in clones. We conduct these observations against the backdrop of our recent report of cell-to-cell expression variability, as well as of the subcellular localization heterogeneity of β-ARs in adult CMs.
Hypophosphatasia (HPP) is a rare genetic disease with diverse symptoms and a heterogeneous severity of onset with underlying mutations in the ALPL gene encoding the ectoenzyme Tissue-nonspecific alkaline phosphatase (TNAP). Considering the establishment of zebrafish (Danio rerio) as a new model organism for HPP, the aim of the study was the spatial and temporal analysis of alpl expression in embryos and adult brains. Additionally, we determined functional consequences of Tnap inhibition on neural and skeletal development in zebrafish. We show that expression of alpl is present during embryonic stages and in adult neuronal tissues. Analyses of enzyme function reveal zones of pronounced Tnap-activity within the telencephalon and the mesencephalon. Treatment of zebrafish embryos with chemical Tnap inhibitors followed by axonal and cartilage/mineralized tissue staining imply functional consequences of Tnap deficiency on neuronal and skeletal development. Based on the results from neuronal and skeletal tissue analyses, which demonstrate an evolutionary conserved role of this enzyme, we consider zebrafish as a promising species for modeling HPP in order to discover new potential therapy strategies in the long-term.
The eukaryotic parasite Trypanosoma brucei has evolved sophisticated strategies to persist within its mammalian host. Trypanosomes evade the hosts' immune system by antigenic variation of their surface coat, consisting of variant surface glycoproteins (VSGs). Out of a repertoire of thousands of VSG genes, only one is expressed at any given time from one of the 15 telomeric expression sites (ES). The VSG is stochastically exchanged either by a transcriptional switch of the active ES (in situ switch) or by a recombinational exchange of the VSG within the active ES. However, for infections to persist, the parasite burden has to be limited. The slender (sl) bloodstream form secretes the stumpy induction factor (SIF), which accumulates with rising parasitemia. SIF induces the irreversible developmental transition from the proliferative sl to the cell cycle-arrested but fly-infective stumpy (st) stage once a concentration threshold is reached. Thus, antigenic variation and st development ensure persistent infections and transmissibility. A previous study in monomorphic cells indicated that the attenuation of the active ES could be relevant for the development of trypanosomes. The present thesis investigated this hypothesis using the inducible overexpression of an ectopic VSG in pleomorphic trypanosomes, which possess full developmental competence. These studies revealed a surprising phenotypic plasticity: while the endogenous VSG was always down-regulated upon induction, the ESactivity determined whether the VSG overexpressors arrested in growth or kept proliferating. Full ES-attenuation induced the differentiation of bona fide st parasites independent of the cell density and thus represents the sole natural SIF-independent differentiation trigger to date. A milder decrease of the ES-activity did not induce phenotypic changes, but appeared to prime the parasites for SIF-induced differentiation. These results demonstrate that antigenic variation and development are linked and indicated that the ES and the VSG are independently regulated. Therefore, I investigated in the second part of my thesis how ES-attenuation and VSG-silencing can be mediated. Integration of reporters with a functional or defective VSG 3'UTR into different genomic loci showed that the maintenance of the active state of the ES depends on a conserved motif within the VSG 3'UTR. In situ switching was only triggered when the telomere-proximal motif was partially deleted, suggesting that it serves as a DNA-binding motif for a telomere-associated protein. The VSG levels seem to be additionally regulated in trans based on the VSG 3'UTR independent of the genomic context, which was reinforced by the regulation of a constitutively expressed reporter with VSG 3' UTR upon ectopic VSG overexpression.
Adipocytes play a central role in maintaining metabolic homeostasis in the body. Differentiation of adipocyte precursor cells requires the transcriptional activity of peroxisome proliferator-activated receptor-γ (Pparγ) and CCAAT/enhancer binding proteins (C/Ebps). Transcriptional activity is regulated by signaling modules activated by a plethora of hormones and nutrients. Mechanistic target of rapamacin complexes (mTORC) 1 and 2 are central for the coordination of hormonal and nutritional inputs in cells and are essential for adipogenesis. Serum glucocorticoid kinase 1 (Sgk1)-dependent phosphorylation of N-Myc downstream-regulated gene 1 (Ndrg1) is a hallmark of mTORC2 activation in cells. Moreover, Pparγ activation promotes Ndrg1 expression. However, the impact of Ndrg1 on adipocyte differentiation and function has not yet been defined. Here, we show that Ndrg1 expression and its Sgk1-dependent phosphorylation are induced during adipogenesis. Consistently, we demonstrate that Ndrg1 promotes adipocyte differentiation and function by inducing Pparγ expression. Additionally, our results indicate that Ndrg1 is required for C/Ebpα phosphorylation. Moreover, we found that Ndrg1 phosphorylation by Sgk1 promotes adipocyte formation. Taken together, we show that induction of Ndrg1 expression by Pparγ and its phosphorylation by Sgk1 kinase are required for the acquisition of adipocyte characteristics by precursor cells.
Rats intracerebroventricularily (icv) treated with streptozotocin (STZ), shown to generate an insulin resistant brain state, were used as an animal model for the sporadic form of Alzheimer's disease (sAD). Previously, we showed in an in vivo study that 3 months after STZ icv treatment hippocampal adult neurogenesis (AN) is impaired. In the present study, we examined the effects of STZ on isolated adult hippocampal neural stem cells (NSCs) using an in vitro approach. We revealed that 2.5 mM STZ inhibits the proliferation of NSCs as indicated by reduced number and size of neurospheres as well as by less BrdU-immunoreactive NSCs. Double immunofluorescence stainings of NSCs already being triggered to start with their differentiation showed that STZ primarily impairs the generation of new neurons, but not of astrocytes. For revealing mechanisms possibly involved in mediating STZ effects we analyzed expression levels of insulin/glucose system-related molecules such as the glucose transporter (GLUT) 1 and 3, the insulin receptor (IR) and the insulin-like growth factor (IGF) 1 receptor. Applying quantitative Real time-PCR (qRT-PCR) and immunofluorescence stainings we showed that STZ exerts its strongest effects on GLUT3 expression, as GLUT3 mRNA levels were found to be reduced in NSCs, and less GLUT3-immunoreactive NSCs as well as differentiating cells were detected after STZ treatment. These findings suggest that cultured NSCs are a good model for developing new strategies to treat nerve cell loss in AD and other degenerative disorders.
Control of genetic regulatory networks is challenging to define and quantify. Previous control centrality metrics, which aim to capture the ability of individual nodes to control the system, have been found to suffer from plausibility and applicability problems. Here we present a new approach to control centrality based on network convergence behaviour, implemented as an extension of our genetic regulatory network simulation framework Jimena (http://stefan-karl.de/jimena). We distinguish three types of network control, and show how these mathematical concepts correspond to experimentally verified node functions and signalling pathways in immunity and cell differentiation: Total control centrality quantifies the impact of node mutations and identifies potential pharmacological targets such as genes involved in oncogenesis (e.g. zinc finger protein GLI2 or bone morphogenetic proteins in chondrocytes). Dynamic control centrality describes relaying functions as observed in signalling cascades (e.g. src kinase or Jak/Stat pathways). Value control centrality measures the direct influence of the value of the node on the network (e.g. Indian hedgehog as an essential regulator of proliferation in chondrocytes). Surveying random scale-free networks and biological networks, we find that control of the network resides in few high degree driver nodes and networks can be controlled best if they are sparsely connected.
Oligodendrocytes are the myelinating glia of the central nervous system and ensure rapid saltatory conduction. Shortage or loss of these cells leads to severe malfunctions as observed in human leukodystrophies and multiple sclerosis, and their replenishment by reprogramming or cell conversion strategies is an important research aim. Using a transgenic approach we increased levels of the transcription factor Sox10 throughout the mouse embryo and thereby prompted Fabp7-positive glial cells in dorsal root ganglia of the peripheral nervous system to convert into cells with oligodendrocyte characteristics including myelin gene expression. These rarely studied and poorly characterized satellite glia did not go through a classic oligodendrocyte precursor cell stage. Instead, Sox10 directly induced key elements of the regulatory network of differentiating oligodendrocytes, including Olig2, Olig1, Nkx2.2 and Myrf. An upstream enhancer mediated the direct induction of the Olig2 gene. Unlike Sox10, Olig2 was not capable of generating oligodendrocyte-like cells in dorsal root ganglia. Our findings provide proof-of-concept that Sox10 can convert conducive cells into oligodendrocyte-like cells in vivo and delineates options for future therapeutic strategies.
Stimulating the immune system to attack cancer is a promising approach, even for the control of advanced cancers. Several cytokines that promote interferon-γ-dominated immune responses show antitumor activity, with interleukin 12 (IL-12) being of major importance. Here, we used an antibody-IL-12 fusion protein (NHS-IL12) that binds histones of necrotic cells to treat human sarcoma in humanized mice. Following sarcoma engraftment, NHS-IL12 therapy was combined with either engineered IL-7 (FcIL-7) or IL-2 (IL-2MAB602) for continuous cytokine bioavailability. NHS-IL12 strongly induced innate and adaptive antitumor immunity when combined with IL-7 or IL-2. NHS-IL12 therapy significantly improved survival of sarcoma-bearing mice and caused long-term remissions when combined with IL-2. NHS-IL12 induced pronounced cancer cell senescence, as documented by strong expression of senescence-associated p16\(^{INK4a}\) and nuclear translocation of p-HP1γ, and permanent arrest of cancer cell proliferation. In addition, this cancer immunotherapy initiated the induction of myogenic differentiation, further promoting the hypothesis that efficient antitumor immunity includes mechanisms different from cytotoxicity for efficient cancer control in vivo.
Elektromagnetische Felder (EMF) sind in der Umwelt des Menschen allgegenwärtig. Unter Verwendung unterschiedlicher Frequenzen bilden sie die Grundlage zahlreicher Technologien und begegnen uns im Alltag in einer Vielzahl von Anwendungen. Eine sehr wichtige Anwendung von EMF ist die mobile Kommunikation. Die hierfür verwendeten Frequenzen liegen im hochfrequenten Bereich und variieren mit dem Mobilfunkstandard. Weit verbreitet ist die GSM- und UMTS-Modulation der zweiten (2G) und dritten Generation (3G). Zum neuesten Mobilfunkstandard zählt LTE (4G).
Aus statistischen Daten geht hervor, dass derzeit weltweit mehr als sieben Milliarden Mobilfunk-Endgeräte existieren. Die weitverbreitete und stetig ansteigende Verwendung dieser Technologien verdeutlicht, dass viele Menschen, darunter auch zunehmend Kinder und Jugendliche, regelmäßig einer Exposition gegenüber EMF ausgesetzt sind. Die wichtigste Expositionsquelle stellt dabei das Mobiltelefon dar, da sich in diesem Szenario die Quelle sehr nah am menschlichen Körper befindet. In der Vergangenheit wurden zahlreiche in-vitro- und in-vivo-Untersuchungen sowie epidemiologische Studien durchgeführt, um potentielle, nicht-thermische Effekte von Mobilfunkstrahlung auf biologische Systeme beurteilen zu können. Ein vollständiger Konsens konnte auf der Basis der erhaltenen Ergebnisse jedoch nicht erzielt werden, sodass weiterhin Bedenken zum schädlichen Potential dieser nichtionisierenden Strahlung bestehen. Insbesondere wurden Fragestellungen zu Langzeiteffekten sowie zu Effekten, die speziell bei Kindern eine besondere Rolle spielen, bisher nicht ausreichend adressiert. Kinder können empfindlicher auf Umwelteinflüsse reagieren und sind im Vergleich zu Erwachsenen teilweise höher gegenüber EMF exponiert. Dies gilt vor allem für Kopfregionen, in denen sich das aktive, für die Hämatopoese verantwortliche Knochenmark befindet.
Vor diesem Hintergrund war es das Ziel der vorliegenden Arbeit, den Einfluss von Mobilfunkstrahlung auf das humane blutbildende System zu untersuchen. Im Fokus standen dabei humane hämatopoetische Stammzellen, die mit Frequenzen der Mobilfunkstandards GSM (900 MHz), UMTS (1.950 MHz) und LTE (2.535 MHz) jeweils über einen kurzen (4 h) und einen langen (20 h) Zeitraum und mit unterschiedlichen Intensitäten (0 W/kg, 0,5 W/kg, 1 W/kg, 2 W/kg und 4 W/kg) exponiert wurden. Vergleichende Experimente erfolgten mit Zellen der Promyelozyten-Zelllinie HL-60. Mögliche Effekte wurden mit den Endpunkten Apoptose, oxidativer Stress, Zellzyklus, DNA-Schaden und –Reparatur sowie Differenzierung und Epigenetik in Form von Histonacetylierung bewertet. In keinem der genannten Endpunkte konnten klare Effekte durch Mobilfunkstrahlung ausgemacht werden, weder für die hämatopoetischen Stammzellen, noch für die Zelllinie HL-60. Die einzige Veränderung wurde bei der Quantifizierung von DNA-Schäden beobachtet. Hier zeigte sich nach der Kurzzeitexposition der Stammzellen mit der Modulation GSM eine kleine, aber statistisch signifikante Abnahme der DNA-Schäden verglichen mit der Scheinexposition. Diese Beobachtung ließ sich in weiteren Replikaten jedoch nicht reproduzieren und wurde daher als nicht biologisch relevant eingestuft.
Insgesamt konnte mit dieser Arbeit gezeigt werden, dass durch Mobilfunkstrahlung mit Frequenzen der verbreiteten Modulationen GSM, UMTS und LTE sowie SAR-Werten, die unterhalb und oberhalb des empfohlenen Sicherheitsstandards liegen und typischerweise bei Handytelefonaten auftreten, keine Effekte in Zellen des blutbildenden Systems unter den gegebenen Versuchsbedingungen induziert wurden. Ein besonderer Fokus lag hierbei auf der Reproduzierbarkeit der Ergebnisse. Weiterhin wurden zum ersten Mal humane hämatopoetische Stammzellen für derartige Untersuchungen eingesetzt. Dies hat insofern eine besondere Bedeutung, als hämatopoetische Stammzellen aufgrund ihrer multipotenten Eigenschaften eine breitere Analyse mit Hinblick auf die Kanzerogenese und auf das Immunsystem ermöglichen.
Um über die Mobilfunk-Untersuchungen hinaus die hämatopoetischen Stammzellen besser charakterisieren zu können, sowie die Sensitivität von Blutzellen mit unterschiedlichem Differenzierungsstatus zu analysieren, wurden sie anderen Zellen des blutbildenden Systems (undifferenzierte und differenzierte HL-60-Zellen und TK6-Zellen) gegenübergestellt. Eine Behandlung der verschiedenen Zelltypen mit mutagenen Substanzen zeigte, dass sich die hämatopoetischen Stammzellen in den meisten der untersuchten Endpunkte von den Zelllinien unterschieden. Deutliche Abweichungen zeigten sich beim oxidativen Stress, der DNA-Reparatur und der Histonacetylierung; kein Unterschied konnte dagegen bei den DNA-Schäden beobachtet werden. Eine erste Interpretation der erhaltenen Ergebnisse ist auf der Grundlage der unterschiedlichen Eigenschaften von Zellen mit abweichendem Differenzierungsstatus möglich. Um jedoch eine eindeutige Aussage treffen zu können, müssten noch weitere Untersuchungen durchgeführt werden.