
doi: 10.2144/05386st01
pmid: 16018548
A significant obstacle to using human embryonic stem cells (hESCs) arises from extremely poor survival associated with freezing, typically in the range of 1%. This report describes a slow controlled-rate freezing technique commonly used for mammalian embryo cryopreservation. Using a combination of surviving colony number and colony diameter; survival was determined relative to untreated hESCs. Using a dimethyl sulfoxide (DMSO) cryoprotectant and either a homemade controlled-rate freezing device or a commercial freezing device, survival rates of 20%-80% were obtained. To achieve the highest levels of survival, the critical factors were an ice crystal seed (at -7 degrees to -10 degrees C), a freeze rate between 0.3 degrees and 1.8 degrees C/min, and a rapid thaw rate using room temperature water. Slow controlled-rate cooling allows a rapid, simple, and reproducible means of cryopreserving hESCs.
Cryopreservation, QH301-705.5, Cell Survival, Stem Cells, Embryo, Mammalian, Cytoprotection, Karyotyping, Freezing, Humans, Dimethyl Sulfoxide, Biology (General)
Cryopreservation, QH301-705.5, Cell Survival, Stem Cells, Embryo, Mammalian, Cytoprotection, Karyotyping, Freezing, Humans, Dimethyl Sulfoxide, Biology (General)
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