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OC15: CHONDROCYTE SURVIVAL IN ARTICULAR CARTILAGE EXPLANTS - THE INFLUENCE OF SUBCHONDRAL BONE



Abstract

Articular cartilage is attached to subchondral bone but little is known regarding bone-cartilage interactions important for chondrocyte survival. In this study, bovine articular cartilage has been evaluated in vitro to determine if the presence of subchondral bone influences chondrocyte survival. We hypothesised that

  1. Excision of subchondral bone from articular cartilage would increase in situ chondrocyte death in explant culture and,

  2. Chondrocyte death could be abrogated by co-culturing articular cartilage with the excised subchondral bone.

Articular cartilage explants (n=132) harvested from the metacarpophalangeal joints of three-year old cows (N=12) were placed into three groups:

  1. subchondral bone excised from articular cartilage (Group A)

  2. sub-chondral bone left attached to articular cartilage (Group B)

  3. subchondral bone excised, but co-cultured with articular cartilage (Group C).

Explants were cultured in serum-free media over 7 days with or without media changes to assess the effect of potential soluble mediators. Using confocal laser scanning microscopy to image in situ chondrocytes, fluorescent probes to determine cell viability and biochemical assays to detect alterations in the culture media, differences in the chondrocyte responses (cell density, spatial distribution, percentage cell death) and culture medium composition between Groups A, B and C were quantified over time (2.5 hours versus 7 days).

There was no significant change in cell density for Groups A, B and C over 7 days (t-test, p> 0.05). With excision of subchondral bone from articular cartilage (Group A), there was a marked increase in chondrocyte death over 7 days primarily within the superficial zone involving an extensive area of the articular surface (p< 0.05). There was no significant increase in chondrocyte death over the same time period for Groups B and C (p> 0.05). Corresponding increases in the protein content of the culture media for Groups B and C but not for Group A, suggested that the release of soluble factors from subchondral bone may have influenced chondrocyte survival in the superficial zone.

Subchondral bone interacts with articular cartilage in vitro and promotes chondrocyte survival in the superficial zone. These data support the concept of a functional bone-cartilage system in vivo.

Correspondence should be addressed to Dr Roger Bayston, Division of Orthopaedic and Accident Surgery, Queen’s Medical Centre, Nottingham, NG7 2UH, England.