
Embryogenic calli of pedunculate oak (Quercus robur L.) were cryopreserved using direct immersion in liquid nitrogen. The pretreatment consisted of culture on a solid medium with increasing sucrose concentrations (0.25 M for 1 day, 0.5 M for 1 day, 0.75 M for 2 days, and 1.0 M for 3 days), followed by air desiccation of embryogenic calli to 17.3 percent (fresh weight basis). This method of cryoprotection was compared to a liquid cryoprotection treatment using high concentrations of sucrose solutions, followed by glycerol solutions. Regrowth of frozen tissue pretreated on a solid medium was significantly higher than those pretreated in the liquid solutions.
Cryopreservation, Quercus, Sucrose, Cryoprotective Agents, Seeds, Desiccation, Cells, Cultured, Cell Line, Culture Media
Cryopreservation, Quercus, Sucrose, Cryoprotective Agents, Seeds, Desiccation, Cells, Cultured, Cell Line, Culture Media
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