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Recombinant Dendroides canadensis antifreeze proteins as potential ingredients in cryopreservation solutions
Authors:Dina O Halwani  Kelvin GM Brockbank  John G Duman  Lia H Campbell
Institution:1. Cell & Tissue Systems, Inc., N. Charleston, SC 29406, USA;2. Institute for Bioengineering and Bioscience, Georgia Institute of Technology, Atlanta, GA 30332, USA;3. Department of Regenerative Medicine and Cell Biology, Medical University of South Carolina, Charleston, SC 29425, USA;4. Department of Biological Sciences, University of Notre Dame, Notre Dame, IN 46556, USA
Abstract:Expanding cryopreservation methods to include a wider range of cell types, such as those sensitive to freezing, is needed for maintaining the viability of cell-based regenerative medicine products. Conventional cryopreservation protocols, which include use of cryoprotectants such as dimethylsulfoxide (Me2SO), have not prevented ice-induced damage to cell and tissue matrices during freezing. A family of antifreeze proteins (AFPs) produced in the larvae of the beetle, Dendroides canadensis allow this insect to survive subzero temperatures as low as −26 °C. This study is an assessment of the effect of the four hemolymph D. canadensis AFPs (DAFPs) on the supercooling (nucleating) temperature, ice structure patterns and viability of the A10 cell line derived from the thoracic aorta of embryonic rat. Cryoprotectant solution cocktails containing combinations of DAFPs in concentrations ranging from 0 to 3 mg/mL in Unisol base mixed with 1 M Me2SO were first evaluated by cryomicroscopy. Combining multiple DAFPs demonstrated significant supercooling point depressing activity (∼9 °C) when compared to single DAFPs and/or conventional 1 M Me2SO control solutions. Concentrations of DAFPs as low as 1 μg/mL were sufficient to trigger this effect. In addition, significantly improved A10 smooth muscle cell viability was observed in cryopreservation experiments with low DAFP-6 and DAFP-2 concentrations in combination with Me2SO. No significant improvement in viability was observed with either DAFP-1 or DAFP-4. Low and effective DAFP concentrations are advantageous because they minimize concerns regarding cell cytotoxicity and manufacturing cost. These findings support the potential of incorporating DAFPs in solutions used to cryopreserve cells and tissues.
Keywords:Antifreeze proteins  Cryoprotectants  Recrystallization  Dendroides canadensis  Supercooling  Thermal hysteresis  Cryopreservation  Subzero storage  Ice-free cryopreservation  Cryomicroscopy
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