TY - JOUR A1 - Niedermair, Tanja A1 - Lukas, Christoph A1 - Li, Shushan A1 - Stöckl, Sabine A1 - Craiovan, Benjamin A1 - Brochhausen, Christoph A1 - Federlin, Marianne A1 - Herrmann, Marietta A1 - Grässel, Susanne T1 - Influence of Extracellular Vesicles Isolated From Osteoblasts of Patients With Cox-Arthrosis and/or Osteoporosis on Metabolism and Osteogenic Differentiation of BMSCs JF - Frontiers in Bioengineering and Biotechnology N2 - Background: Studies with extracellular vesicles (EVs), including exosomes, isolated from mesenchymal stem cells (MSC) indicate benefits for the treatment of musculoskeletal pathologies as osteoarthritis (OA) and osteoporosis (OP). However, little is known about intercellular effects of EVs derived from pathologically altered cells that might influence the outcome by counteracting effects from “healthy” MSC derived EVs. We hypothesize, that EVs isolated from osteoblasts of patients with hip OA (coxarthrosis/CA), osteoporosis (OP), or a combination of both (CA/OP) might negatively affect metabolism and osteogenic differentiation of bone-marrow derived (B)MSCs. Methods: Osteoblasts, isolated from bone explants of CA, OP, and CA/OP patients, were compared regarding growth, viability, and osteogenic differentiation capacity. Structural features of bone explants were analyzed via μCT. EVs were isolated from supernatant of naïve BMSCs and CA, OP, and CA/OP osteoblasts (osteogenic culture for 35 days). BMSC cultures were stimulated with EVs and subsequently, cell metabolism, osteogenic marker gene expression, and osteogenic differentiation were analyzed. Results: Trabecular bone structure was different between the three groups with lowest number and highest separation in the CA/OP group. Viability and Alizarin red staining increased over culture time in CA/OP osteoblasts whereas growth of osteoblasts was comparable. Alizarin red staining was by trend higher in CA compared to OP osteoblasts after 35 days and ALP activity was higher after 28 and 35 days. Stimulation of BMSC cultures with CA, OP, and CA/OP EVs did not affect proliferation but increased caspase 3/7-activity compared to unstimulated BMSCs. BMSC viability was reduced after stimulation with CA and CA/OP EVs compared to unstimulated BMSCs or stimulation with OP EVs. ALP gene expression and activity were reduced in BMSCs after stimulation with CA, OP, and CA/OP EVs. Stimulation of BMSCs with CA EVs reduced Alizarin Red staining by trend. Conclusion: Stimulation of BMSCs with EVs isolated from CA, OP, and CA/OP osteoblasts had mostly catabolic effects on cell metabolism and osteogenic differentiation irrespective of donor pathology and reflect the impact of tissue microenvironment on cell metabolism. These catabolic effects are important for understanding differences in effects of EVs on target tissues/cells when harnessing them as therapeutic drugs. KW - extracellular vesicles KW - mesenchymal stem cells KW - osteoblasts KW - osteoarthritis KW - osteoporosis KW - EVs KW - osteogenic differentiation Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-219902 SN - 2296-4185 VL - 8 ER - TY - JOUR A1 - Rath, Subha N. A1 - Brandl, Andreas A1 - Hiller, Daniel A1 - Hoppe, Alexander A1 - Gbureck, Uwe A1 - Horch, Raymund E. A1 - Boccaccini, Aldo R. A1 - Kneser, Ulrich T1 - Bioactive Copper-Doped Glass Scaffolds Can Stimulate Endothelial Cells in Co-Culture in Combination with Mesenchymal Stem Cells JF - PLOS ONE N2 - Bioactive glass (BG) scaffolds are being investigated for bone tissue engineering applications because of their osteoconductive and angiogenic nature. However, to increase the in vivo performance of the scaffold, including enhancing the angiogenetic growth into the scaffolds, some researchers use different modifications of the scaffold including addition of inorganic ionic components to the basic BG composition. In this study, we investigated the in vitro biocompatibility and bioactivity of Cu2+-doped BG derived scaffolds in either BMSC (bone-marrow derived mesenchymal stem cells)-only culture or co-culture of BMSC and human dermal microvascular endothelial cells (HDMEC). In BMSC-only culture, cells were seeded either directly on the scaffolds (3D or direct culture) or were exposed to ionic dissolution products of the BG scaffolds, kept in permeable cell culture inserts (2D or indirect culture). Though we did not observe any direct osteoinduction of BMSCs by alkaline phosphatase (ALP) assay or by PCR, there was increased vascular endothelial growth factor (VEGF) expression, observed by PCR and ELISA assays. Additionally, the scaffolds showed no toxicity to BMSCs and there were healthy live cells found throughout the scaffold. To analyze further the reasons behind the increased VEGF expression and to exploit the benefits of the finding, we used the indirect method with HDMECs in culture plastic and Cu2+-doped BG scaffolds with or without BMSCs in cell culture inserts. There was clear observation of increased endothelial markers by both FACS analysis and acetylated LDL (acLDL) uptake assay. Only in presence of Cu2+-doped BG scaffolds with BMSCs, a high VEGF secretion was demonstrated by ELISA; and typical tubular structures were observed in culture plastics. We conclude that Cu2+-doped BG scaffolds release Cu2+, which in turn act on BMSCs to secrete VEGF. This result is of significance for the application of BG scaffolds in bone tissue engineering approaches. KW - arteriovenous loop KW - calcium-phosphate KW - iron release KW - bone KW - angiogenesis KW - expression KW - differentation KW - proliferation KW - osteoblasts KW - growth Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-114339 SN - 1932-6203 VL - 9 IS - 12 ER - TY - JOUR A1 - Boschert, Verena A1 - van Dinther, Maarten A1 - Weidauer, Stella A1 - van Pee, Katharina A1 - Muth, Eva-Maria A1 - ten Dijke, Peter A1 - Mueller, Thomas D. T1 - Mutational Analysis of Sclerostin Shows Importance of the Flexible Loop and the Cystine-Knot for Wnt-Signaling Inhibition JF - PLoS ONE N2 - The cystine-knot containing protein Sclerostin is an important negative regulator of bone growth and therefore represents a promising therapeutic target. It exerts its biological task by inhibiting the Wnt (wingless and int1) signaling pathway, which participates in bone formation by promoting the differentiation of mesenchymal stem cells to osteoblasts. The core structure of Sclerostin consists of three loops with the first and third loop (Finger 1 and Finger 2) forming a structured \(\beta\)-sheet and the second loop being unstructured and highly flexible. Biochemical data showed that the flexible loop is important for binding of Sclerostin to Wnt co-receptors of the low-density lipoprotein related-protein family (LRP), by interacting with the Wnt co-receptors LRP5 or -6 it inhibits Wnt signaling. To further examine the structural requirements for Wnt inhibition, we performed an extensive mutational study within all three loops of the Sclerostin core domain involving single and multiple mutations as well as truncation of important regions. By this approach we could confirm the importance of the second loop and especially of amino acids Asn92 and Ile94 for binding to LRP6. Based on a Sclerostin variant found in a Turkish family suffering from Sclerosteosis we generated a Sclerostin mutant with cysteines 84 and 142 exchanged thereby removing the third disulfide bond of the cystine-knot. This mutant binds to LRP6 with reduced binding affinity and also exhibits a strongly reduced inhibitory activity against Wnt1 thereby showing that also elements outside the flexible loop are important for inhibition of Wnt by Sclerostin. Additionally, we examined the effect of the mutations on the inhibition of two different Wnt proteins, Wnt3a and Wnt1. We could detect clear differences in the inhibition of these proteins, suggesting that the mechanism by which Sclerostin antagonizes Wnt1 and Wnt3a is fundamentally different. KW - Wnt signaling cascade KW - binding analysis KW - osteoblasts KW - sequence motif analysis KW - biological locomotion KW - signal inhibition KW - cell binding assay KW - luciferase Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129862 VL - 8 IS - 11 ER - TY - THES A1 - Schilling, Tatjana T1 - Transdifferentiation of Human Mesenchymal Stem Cells T1 - Transdifferenzierung humaner Mesenchymaler Stammzellen N2 - With ageing, the loss of bone mass correlates with the expansion of adipose tissue in human bone marrow thus facilitating bone-related diseases like osteopenia and osteoporosis. The molecular mechanisms underlying these events are still largely unknown. Reduced osteogenesis and concurrently enhanced adipogenesis might not only occur due to the impairment of conventional osteogenic differentiation originating from mesenchymal stem cells (MSCs). Additionally, transdifferentiation of (pre-)osteoblasts into adipocytes could contribute to the fatty conversion. Therefore, the aim of the present study was to prove the existence of transdifferentiation between the adipogenic and osteogenic lineage and to elucidate molecular mechanisms underlying this phenomenon. At first, a cell culture system of primary human MSCs was established that allowed for differentiation into the adipogenic and osteogenic lineage and proved that the MSC-derived adipocytes and pre-osteoblasts were capable of transdifferentiation (reprogramming) from one into the other lineage. Thereby, lineage-specific markers were completely reversed after reprogramming of pre-osteoblasts into adipocytes. The osteogenic transdifferentiation of adipocytes was slightly less efficient since osteogenic markers were present but the adipogenic ones partly persisted. Hence, plasticity also reached into the differentiation pathways of both lineages and the better performance of adipogenic reprogramming further supported the assumption of its occurrence in vivo. The subsequent examination of gene expression changes by microarray analyses that compared transdifferentiated cells with conventionally differentiated ones revealed high numbers of reproducibly regulated genes shortly after initiation of adipogenic and osteogenic reprogramming. Thereof, many genes were correlated with metabolism, transcription, and signal transduction as FGF, IGF, and Wnt signalling, but only few of the established adipogenesis- and none of the osteogenesis-associated marker genes were detected within 24 h after initiation of transdifferentiation. To find possible key control factors of transdifferentiation amongst the huge amount of regulated genes, a novel bioinformatic scoring scheme was developed that ranked genes due to their potential relevance for reprogramming. Besides the reproducibility and level of their regulation, also the possible reciprocity between the adipogenic and osteogenic transdifferentiation pathway was taken into account. Fibroblast growth factor 1 (FGF1) that ranked as one of the leading candidates to govern reprogramming was proven to inhibit adipogenic differentiation as well as adipogenic transdifferentiation in our cell culture system. Further examination of the FGF signalling pathway and other highly ranked genes could help to better understand the age-related fatty degeneration at the molecular level and therefore provide target molecules for therapeutic modulation of the plasticity of both lineages in order to inhibit adipogenic degeneration and to enhance osteogenesis. N2 - Der Verlust an Knochenmasse im Alter ist mit der Ausbreitung von Fettgewebe im menschlichen Knochenmark assoziiert und fördert daher auch knochenspezifische Erkrankungen wie Osteopenie und Osteoporose. Die diesen Ereignissen zu Grunde liegenden Mechanismen sind immer noch weitgehend unbekannt. Die abnehmende Osteogenese und die gleichzeitig zunehmende Adipogenese treten wahrscheinlich nicht nur wegen der Beeinträchtigung der konventionellen osteogenen Differenzierung von mesenchymalen Stammzellen (MSZ) auf. Zusätzlich könnte auch die Transdifferenzierung (Reprogrammierung) von Osteoblasten(vorläufern) zu Adipozyten zur fettigen Umwandlung beitragen. Das Ziel der vorliegenden Studie war es daher, die Existenz der Transdifferenzierung zwischen dem adipogenen und osteogenen Differenzierungsweg nachzuweisen und die molekularen Mechanismen aufzuklären, die diesem Phänomen zu Grunde liegen. Zunächst wurde ein Zellkultursystem primärer mesenchymaler Stammzellen etabliert, in dem eine Differenzierung zu Adipozyten und Osteoblasten durchgeführt werden konnte, und nachgewiesen, dass aus MSZ erhaltene Adipozyten und Osteoblastenvorläufer von einer zur anderen Zelllinie transdifferenziert (reprogrammiert) werden können. Dabei wurden die zelllinienspezifischen Marker nach der Reprogrammierung von Osteoblastenvorläufern zu Adipozyten vollständig umgekehrt. Die osteogene Transdifferenzierung von Adipozyten war etwas weniger effizient, da die osteogenen Marker zwar vorhanden waren, aber auch die adipogenen Marker weiterhin auftraten. Die Plastizität erstreckte sich also auch auf die Differenzierungswege der beiden Zellpopulationen, wobei das bessere Ergebnis bezüglich der adipogenen Reprogrammierung die Annahme ihres Auftretens in vivo weiter unterstützte. Die nachfolgende Untersuchung von Genexpressionsänderungen mittels Mikroarray-Analysen, die transdifferenzierte mit konventionell differenzierten Zellen verglichen, führte kurz nach Initiation der adipogenen und osteogenen Transdifferenzierung zum Auffinden zahlreicher, reproduzierbar regulierter Gene. Viele dieser Gene standen mit Metabolismus, Transkription und Signaltransduktion wie dem FGF-, IGF- und Wnt-Signalweg in Zusammenhang, es wurden allerdings nur einige Adipogenese- und keinerlei Osteogenese-assoziierte Markergene innerhalb 24 h nach Initiation der Transdifferenzierung detektiert. Um unter der großen Zahl an regulierten Genen mögliche Schlüsselkontrollfaktoren der Transdifferenzierung zu finden, wurde ein neuartiges, bioinformatisches Punktesystem entwickelt, das Gene entsprechend ihrer potenziellen Relevanz für die Reprogrammierung auflistete. Dabei wurde neben der Reproduzierbarkeit und dem Ausmaß ihrer Regulation auch eine mögliche Reziprozität der Regulation zwischen dem adipogenen und osteogenen Transdifferenzierungsweg berücksichtigt. Es konnte nachgewiesen werden, dass der Fibroblastenwachstumsfaktor 1 (FGF1), der als einer der Hauptkandidaten für die Steuerung der Reprogrammierung eingeordnet worden war, in unserem Zellkultursystem sowohl die adipogene Differenzierung als auch die adipogene Transdifferenzierung hemmt. Die weitere Untersuchung des FGF-Signalwegs und anderer, hoch gelisteter Gene könnte zum besseren Verständnis der altersbezogenen fettigen Degeneration auf molekularer Ebene beitragen und daher Zielmoleküle liefern, die eine therapeutische Beeinflussung der Plastizität zwischen beiden Zelllinien zur Verhinderung der fettigen Degeneration und zur Förderung der Osteogenese erlauben. KW - Zelldifferenzierung KW - Metaplasie KW - Mesenchymale Stammzellen KW - Transdifferenzierung KW - Osteoblasten KW - Adipozyten KW - Mesenchymal Stem Cells KW - transdifferentiation KW - osteoblasts KW - adipocytes Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-24299 ER - TY - THES A1 - Glückermann, Susanne Karola T1 - Zytotoxizitätsprüfung verschiedener Silbertitanlegierungen auf Titanbasis mittels humaner Osteoblasten T1 - Cytotoxicity of silver-titanium-alloy on titan grade 2 with human osteoblasts N2 - In der vorliegenden Arbeit wurde die Zytotoxizität verschiedener Schichten bestehend aus Silber-Titanlegierungen auf Titanbasis mittels der humanen Osteoblastenzelllinie hFOB 1.19 geprüft. Es sollte der Einfluß des Silberanteils in der Beschichtung auf die Zellen getestet werden. Es wurde die Wirkung auf die Proliferations- und Differenzierungsleistung der Zellen mit standardisierten Untersuchungsmethoden getestet. Des weiteren wurde die Aktivität der alkalischen Phosphatase und die Biomassebestimmung vorgenommen.Als Kontrolluntersuchung wurde der gleiche Versuch mit der bronchialen Epithelzelllinie HBE 16 durchgeführt. Die Zellkultivierung erfolgte über einen 14-tägigen Zeitraum. Als Referenzoberfläche wurde konventionelles Zellkultur-Polystyrol verwendet. Die Zellvitalität wurde mit Hilfe des WST-1-Tests, der Differenzierungstatus anhand der Aktivität der alkalischen Phosphatase und der Proteingehalt mittels der Proteinbestimmung nach Bradford erfaßt. Es zeigten sich bei allen Messungen starke Schwankungen der Zellzahl, Zellvitalität, der spezifischen Aktivität der alkalischen Phosphatase und des Proteingehalts auf den Oberflächen. Eine Proportionalität zwischen den verschiedenen Silberkonzentrationen und den Proliferationszahlen war nicht zu beobachten. Mit dem Wissen über die hervorragende Biokompatibilität von Titan und der nachgewiesenen bakteriostatischen Wirkung von Silber ist dies ein hervorragender Werkstoff , welcher schädliche Bakterien um das Implantat herum eliminiert und trotzdem ein ungehindertes Einwachsen des Implantats in den Knochen erlaubt. KW - Silber-Titan-Legierung KW - Osteoblasten KW - Zytotoxizitätsprüfung KW - bronchiale Epithelzellen HBE 16 KW - PVD-Verfahren KW - silver-titanium-alloy KW - osteoblasts KW - cytotoxicity KW - human respiratory epithelial cells Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-11021 ER -