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Chondrogenic differentiation of human mesenchymal stem cells and articular cartilage reconstruction
(2008)
Articular cartilage defects are still one of the major challenges in orthopedic and trauma surgery. Today, autologous chondrocyte transplantation (ACT), as a cell-based therapy, is an established procedure. However, one major limitation of this technique is the loss of the chondrogenic phenotype during expansion. Human mesenchymal stem cells (hMSCs) have an extensive proliferation potential and the capacity to differentiate into chondrocytes when maintained under specific conditions. They are therefore considered as candidate cells for tissue engineering approaches of functional cartilage tissue substitutes. First in this study, hMSCs were embedded in a collagen type I hydrogel to evaluate the cartilaginous construct in vitro. HMSC collagen hydrogels cultivated in different culture media showed always a marked contraction, most pronounced in chondrogenic differentiation medium supplemented with TGF-ß1. After stimulation with chondrogenic factors (dexamethasone and TGF-ß1) hMSCs were able to undergo chondrogenesis when embedded in the collagen type I hydrogel, as evaluated by the temporal induction of cartilage-specific gene expression. Furthermore, the cells showed a chondrocyte-like appearance and were homogeneously distributed within a proteoglycan- and collagen type II-rich extracellular matrix, except a small area in the center of the constructs. In this study, chondrogenic differentiation could not be realized with every hMSC preparation. With the improvement of the culture conditions, e.g. the use of a different FBS lot in the gel fabrication process, a higher amount of cartilage-specific matrix deposition could be achieved. Nevertheless, the large variations in the differentiation capacity display the high donor-to-donor variability influencing the development of a cartilaginous construct. Taken together, the results demonstrate that the collagen type I hydrogel is a suitable carrier matrix for hMSC-based cartilage regeneration therapies which present a promising future alternative to ACT. Second, to further improve the quality of tissue-engineered cartilaginous constructs, mechanical stimulation in specific bioreactor systems are often employed. In this study, the effects of mechanical loading on hMSC differentiation have been examined. HMSC collagen hydrogels were cultured in a defined chondrogenic differentiation medium without TGF-ß1 and subjected to a combined mechanical stimulation protocol, consisting of perfusion and cyclic uniaxial compression. Bioreactor cultivation neither affected overall cell viability nor the cell number in collagen hydrogels. Compared with non-loaded controls, mechanical loading promoted the gene expression of COMP and biglycan and induced an up-regulation of matrix metalloproteinase 3. These results circumstantiate that hMSCs are sensitive to mechanical forces, but their differentiation to chondrocytes could not be induced. Further studies are needed to identify the specific metabolic pathways which are altered by mechanical stimulation. Third, for the development of new cell-based therapies for articular cartilage repair, a reliable cell monitoring technique is required to track the cells in vivo non-invasively and repeatedly. This study aimed at analyzing systematically the performance and biological impact of a simple and efficient labeling protocol for hMSCs. Very small superparamagnetic iron oxide particles (VSOPs) were used as magnetic resonance (MR) contrast agent. Iron uptake was confirmed histologically with prussian blue staining and quantified by mass spectrometry. Compared with unlabeled cells, VSOP-labeling did neither influence significantly the viability nor the proliferation potential of hMSCs. Furthermore, iron incorporation did not affect the differentiation capacity of hMSCs. The efficiency of the labeling protocol was assessed with high resolution MR imaging at 11.7 Tesla. VSOP-labeled hMSCs were visualized in a collagen type I hydrogel indicated by distinct hypointense spots in the MR images, resulting from an iron specific loss of signal intensity. This was confirmed by prussian blue staining. In summary, this labeling technique has great potential to visualize hMSCs and track their migration after transplantation for articular cartilage repair with MR imaging.
No abstract available
Für die Rekonstruktion von Gelenkknorpeldefekten des Kniegelenkes in Folge eines Traumas oder einer Osteochondrosis dissecans (OD) stehen verschiedene operative Verfahren zur Verfügung. Die Autologe Chondrozytentransplantation (ACT) hat sich als zuverlässiges Rekonstruktionsverfahren erwiesen. In der vorliegenden Arbeit wurde eine prospektive Fallseriestudie für eine neue Form der ACT mit einem Kollagen I Hydrogel (CaReS-Technologie) durchgeführt. Die Vorteile der Technologie liegen zum Einen darin, dass sich die Zellen homogen im Gel verteilen und zum Anderen, dass die Zellen unmittelbar nach dem Herauslösen aus dem Gelenkknorpel in das Gel eingebracht werden und dadurch eine geringere Dedifferenzierung der Chondrozyten stattfindet. Von März 2003 bis Ende 2006 wurden 29 Patienten in die Studie eingeschlossen. Die Ein- und Ausschlusskriterien erfüllten die Kriterien der Arbeitsgruppe ACT und Tissue Engineering der Deutschen Gesellschaft für Orthopädie und Unfallchirurgie. Die Eingangs- und Nachuntersuchungsbögen wurden an die IKDC Form 2000 angelehnt. Insgesamt zeigte sich ein signifikanter Anstieg des IKDC Scores im mittleren follow-up von 30,7 Monaten von 47,3 auf 74,9 bei den 29 Patienten. Bei Aufschlüsselung der Patienten bzgl. Diagnose, Defektgröße, Lokalisation und Defektanzahl zeigte sich bei den Behandlungsgruppen OD, Trauma/degenerativ, > 4 cm2, mediale Femurkondyle und Einzeldefekte eine signifikante Zunahme des IKDC Scores im zeitlichen Verlauf. Der postoperative Schmerz zeigte einhergehend mit dem Anstieg des IKDC Scores eine signifikante Abnahme der Schmerzintensität in den Behandlungsgruppen OD, Trauma/degenerativ, > 4 cm2, mediale Femurkondyle und Einzeldefekte. Nachgewiesen wurde ebenfalls ein Anstieg des SF36 Scores, der den gegenwärtigen Gesundheitszustand sowohl körperlich als auch psychisch beurteilt. Zusammen mit einer globalen Patientenzufriedenheit von 80% und einem IKDC Funktionsstatus von I und II bei 77% der Patienten spiegeln die gewonnenen Daten die Ergebnisse der klassischen ACT bzw. anderer matrixgekoppelten Verfahren wieder. Die CaReS-Technologie stellt somit ein gleichwertiges Verfahren zu den bisher auf dem Markt befindlichen Techniken der ACT dar.