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Viability of ligaments after freezing: An experimental study in a rabbit model

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AbstractOur purpose in this study was to assess ligament fibroblast viability after freezing by quantifying the subsequent ability of fibroblasts to synthesize collagen in vitro. Both medial collateral ligament (MCL) complexes from 40 adolescent rabbits were studied. Collagen production was determined by in vitro incubation of ligaments in 3H‐proline (a collagen precursor) and subsequent analysis of 3H‐hydroxyproline (a marker of newly synthesized collagen). Autoradiographs determined the distributions of ligament cell activity. All right MCL complexes served as fresh controls, providing a baseline of collagen production. Each left MCL was assigned to an experimental group and was either incubated fresh (10 animals); “killed” by drying, multiple freeze thawing, or cycloheximide (six animals); or slowly frozen at −70°C without cryoprotection (24 animals). Collagen production of rapidly thawed ligaments was studied by proline incubation at 1 day, 9 days, or 6 weeks after freezing and was compared with that of contralateral fresh controls. Results demonstrate that some cells in the substance of these rabbit ligaments retained the ability to synthesize collagen in vitro after being frozen for up to 6 weeks. Mean collagen production of frozen ligaments was decreased, but tests of mean and median values as well as ratios were statistically similar to fresh contralateral ligaments in all animals. This postfreezing ligament cell survival and collagen production after −70°C storage may have implications for ligament transplantation.
Title: Viability of ligaments after freezing: An experimental study in a rabbit model
Description:
AbstractOur purpose in this study was to assess ligament fibroblast viability after freezing by quantifying the subsequent ability of fibroblasts to synthesize collagen in vitro.
Both medial collateral ligament (MCL) complexes from 40 adolescent rabbits were studied.
Collagen production was determined by in vitro incubation of ligaments in 3H‐proline (a collagen precursor) and subsequent analysis of 3H‐hydroxyproline (a marker of newly synthesized collagen).
Autoradiographs determined the distributions of ligament cell activity.
All right MCL complexes served as fresh controls, providing a baseline of collagen production.
Each left MCL was assigned to an experimental group and was either incubated fresh (10 animals); “killed” by drying, multiple freeze thawing, or cycloheximide (six animals); or slowly frozen at −70°C without cryoprotection (24 animals).
Collagen production of rapidly thawed ligaments was studied by proline incubation at 1 day, 9 days, or 6 weeks after freezing and was compared with that of contralateral fresh controls.
Results demonstrate that some cells in the substance of these rabbit ligaments retained the ability to synthesize collagen in vitro after being frozen for up to 6 weeks.
Mean collagen production of frozen ligaments was decreased, but tests of mean and median values as well as ratios were statistically similar to fresh contralateral ligaments in all animals.
This postfreezing ligament cell survival and collagen production after −70°C storage may have implications for ligament transplantation.

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