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Evaluation of Distinct Freezing Methods and Cryoprotectants for Human Amniotic Fluid Stem Cells Cryopreservation

机译:羊水干细胞冷冻保存的不同冷冻方法和冷冻保护剂的评价

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摘要

Amniotic fluid (AF) was described as a potential source of mesenchymal stem cells (MSCs) for biomedicine purposes. Therefore, evaluation of alternative cryoprotectants and freezing protocols capable to maintain the viability and stemness of these cells after cooling is still needed. AF stem cells (AFSCs) were tested for different freezing methods and cryoprotectants. Cell viability, gene expression, surface markers, and plasticity were evaluated after thawing. AFSCs expressed undifferentiated genes Oct4 and Nanog; presented typical markers (CD29, CD44, CD90, and CD105) and were able to differentiate into mesenchymal lineages. All tested cryoprotectants preserved the features of AFSCs however, variations in cell viability were observed. in this concern, dimethyl sulfoxide (Me2SO) showed the best results. the freezing protocols tested did not promote significant changes in the AFSCs viability. Time programmed and nonprogrammed freezing methods could be used for successful AFSCs cryopreservation for 6 months. Although tested cryoprotectants maintained undifferentiated gene expression, typical markers, and plasticity of AFSCs, only Me2SO and glycerol presented workable viability ratios.
机译:羊水(AF)被描述为用于生物医学目的的间充质干细胞(MSCs)的潜在来源。因此,仍然需要评估能够在冷却后保持这些细胞的活力和干性的替代性防冻剂和冷冻方案。测试了AF干细胞(AFSC)的不同冷冻方法和防冻剂。解冻后评估细胞活力,基因表达,表面标记和可塑性。 AFSC表达未分化的基因Oct4和Nanog。提出了典型的标记(CD29,CD44,CD90和CD105),并能够分化为间充质谱系。所有测试的冷冻保护剂都保留了AFSC的功能,但是观察到了细胞活力的变化。在这种情况下,二甲亚砜(Me2SO)表现最好。测试的冷冻方案并未促进AFSC生存能力的显着变化。时间编程和非编程冷冻方法可用于成功进行AFSC冷冻保存6个月。尽管经过测试的防冻剂保持了未分化的基因表达,典型标记和AFSC的可塑性,但只有Me2SO和甘油表现出可行的生存率。

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