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Induced Collagen Cross-Links Enhance Cartilage Integration

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Autore
Athens, A. A.; Makris, E. A.; Hu, J. C.
Data
2013
DOI
10.1371/journal.pone.0060719
Soggetto
collagen
protein lysine 6 oxidase
animal cell
animal experiment
animal tissue
article
calf (bovine)
cartilage
cartilage cell
cell density
complex formation
controlled study
drug mechanism
enzyme activity
histology
male
molecular mechanics
muscle rigidity
muscle strength
muscle stress
nonhuman
protein assembly
protein cross linking
protein interaction
protein synthesis
tensile strength
tissue engineering
tissue structure
treatment response
Animals
Cartilage, Articular
Cattle
Guided Tissue Regeneration
Protein-Lysine 6-Oxidase
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Abstract
Articular cartilage does not integrate due primarily to a scarcity of cross-links and viable cells at the interface. The objective of this study was to test the hypothesis that lysyl-oxidase, a metalloenzyme that forms collagen cross-links, would be effective in improving integration between native-to-native, as well as tissue engineered-to-native cartilage surfaces. To examine these hypotheses, engineered cartilage constructs, synthesized via the self-assembling process, as well as native cartilage, were implanted into native cartilage rings and treated with lysyl-oxidase for varying amounts of time. For both groups, lysyl-oxidase application resulted in greater apparent stiffness across the cartilage interface 2-2.2 times greater than control. The construct-to-native lysyl-oxidase group also exhibited a statistically significant increase in the apparent strength, here defined as the highest observed peak stress during tensile testing. Histology indicated a narrowing gap at the cartilage interface in lysyl-oxidase treated groups, though this alone is not sufficient to indicate annealing. However, when the morphological and mechanical data are taken together, the longer the duration of lysyl-oxidase treatment, the more integrated the interface appeared. Though further data are needed to confirm the mechanism of action, the enhancement of integration may be due to lysyl-oxidase-induced pyridinoline cross-links. This study demonstrates that lysyl-oxidase is a potent agent for enhancing integration between both native-to-native and native-to-engineered cartilages. The fact that interfacial strength increased manifold suggests that cross-linking agents should play a significant role in solving the difficult problem of cartilage integration. Future studies must examine dose, dosing regimen, and cellular responses to lysyl-oxidase to optimize its application. © 2013 Athens et al.
URI
http://hdl.handle.net/11615/26042
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  • Δημοσιεύσεις σε περιοδικά, συνέδρια, κεφάλαια βιβλίων κλπ. [19735]

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