Abstracts:The glycoprotein lubricin is the primary boundary lubricant of articular cartilage. Its boundary lubricating abilities arise from two key structural features: i) a dense mucin-like domain consisting of hydrophilic oligosaccharides and ii) an end terminus that anchors the molecule to articulating surfaces. When bound, lubricin molecules attract and trap water near a surface, reducing friction and facilitating glide. Synthetic analogues were previously created to mimic lubricin using thiol-terminated polyacrylic acid-graft-polyethylene glycol (pAA-g-PEG) brush copolymers. The PEG moiety was designed to mimic the mucin-like domain of lubricin and the thiol-terminus was designed to anchor the molecules to cartilage surfaces, mimicking the binding domain. In this study, these synthetic lubricin-mimetics were bound to gold-coated surfaces to characterize the relationship between the polymers' molecular architecture and their lubricating capacity. A library of nine copolymer brushes was synthesized using different sizes of pAA and PEG. Larger molecular weight polymers created smoother, more densely covered surfaces (p<0.05). Additionally, the hydrodynamic sizes of the polymers in solution were correlated with their lubricating abilities (p<0.05). Friction coefficients of cartilage against polymer-treated gold surfaces were lower than cartilage against untreated surfaces (Δμeq =−0.065±0.050 to −0.093±0.045, p<0.05).

Abstracts:Abrasions are invariably present in crash events and are partly characterized by the quantity of skin tissue removed from the superficial skin layers through friction contacts. This paper reports work towards predicting tissue loss in crash events quantitatively in order to correlate simulations with real life clinical injury. Towards this, an experimental setup that mimics the crash environment in terms of loading and motion scenarios was developed. Recording of forces at the contact zone was accomplished by a two-channel load cell in conjunction with data acquisition system. A range of normal loads, sliding velocities and surface textures were used to abrade porcine skin specimens. The severity of abrasion to the skin following each abrasive test was estimated by the amount of tissue transferred to the abrading surface by protein mass measurement.

Abstracts:Mechano-biochemical wear encompasses the tribological interplay between biological and mechanical mechanisms responsible for cartilage wear and degradation. The aim of this study was to develop and start validating a novel tribological testing system, which better resembles the natural joint environment through incorporating a live cartilage-on-cartilage articulating interface, joint specific kinematics, and the application of controlled mechanical stimuli for the measurement of biological responses in order to study the mechano-biochemical wear of cartilage. The study entailed two parts. In Part 1, the novel testing rig was used to compare two bearing systems: (a) cartilage articulating against cartilage (CoC) and (b) metal articulating against cartilage (MoC). The clinically relevant MoC, which is also a common tribological interface for evaluating cartilage wear, should produce more wear to agree with clinical observations. In Part II, the novel testing system was used to determine how wear is affected by tissue viability in live and dead CoC articulations. For both parts, bovine cartilage explants were harvested and tribologically tested for three consecutive days. Wear was defined as release of glycosaminoglycans into the media and as evaluation of the tissue structure. For Part I, we found that the live CoC articulation did not cause damage to the cartilage, to the extent of being comparable to the free swelling controls, whereas the MoC articulation caused decreased cell viability, extracellular matrix disruption, and increased wear when compared to CoC, and consistent with clinical data. These results provided confidence that this novel testing system will be adequate to screen new biomaterials for articulation against cartilage, such as in hemiarthroplasty. For Part II, the live and dead cartilage articulation yielded similar wear as determined by the release of proteoglycans and aggrecan fragments, suggesting that keeping the cartilage alive may not be essential for short term wear tests. However, the biosynthesis of glycosaminoglycans was significantly higher due to live CoC articulation than due to the corresponding live free swelling controls, indicating that articulation stimulated cell activity. Moving forward, the cell response to mechanical stimuli and the underlying mechano-biochemical wear mechanisms need to be further studied for a complete picture of tissue degradation.