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海藻糖作为二甲基亚砜溶液添加剂对冰形成、细胞活力及代谢的影响。

Effect of trehalose as an additive to dimethyl sulfoxide solutions on ice formation, cellular viability, and metabolism.

作者信息

Solocinski Jason, Osgood Quinn, Wang Mian, Connolly Aaron, Menze Michael A, Chakraborty Nilay

机构信息

Department of Mechanical Engineering, University of Michigan-Dearborn, 4901 Evergreen Road, Dearborn, MI 48128, United States.

Department of Biology, University of Louisville, Louisville, KY 40292, United States.

出版信息

Cryobiology. 2017 Apr;75:134-143. doi: 10.1016/j.cryobiol.2017.01.001. Epub 2017 Jan 4.

Abstract

Cryopreservation is the only established method for long-term preservation of cells and cellular material. This technique involves preservation of cells and cellular components in the presence of cryoprotective agents (CPAs) at liquid nitrogen temperatures (-196 °C). The organic solvent dimethyl sulfoxide (MeSO) is one of the most commonly utilized CPAs and has been used with various levels of success depending on the type of cells. In recent years, to improve cryogenic outcomes, the non-reducing disaccharide trehalose has been used as an additive to MeSO-based freezing solutions. Trehalose is a naturally occurring non-toxic compound found in bacteria, fungi, plants, and invertebrates which has been shown to provide cellular protection during water-limited states. The mechanism by which trehalose improves cryopreservation outcomes remains not fully understood. Raman microspectroscopy is a powerful tool to provide valuable insight into the nature of interactions among water, trehalose, and MeSO during cryopreservation. We found that the addition of trehalose to MeSO based CPA solutions dramatically reduces the area per ice crystals while increasing the number of ice crystals formed when cooled to -40 or -80 °C. Differences in ice-formation patterns were found to have a direct impact on cellular viability. Despite the osmotic stress caused by addition of 100 mM trehalose, improvement in cellular viability was observed. However, the substantial increase in osmotic pressure caused by trehalose concentrations above 100 mM may offset the beneficial effects of changing the morphology of the ice crystals achieved by addition of this sugar.

摘要

低温保存是细胞和细胞材料长期保存的唯一既定方法。该技术涉及在冷冻保护剂(CPA)存在的情况下,于液氮温度(-196°C)下保存细胞和细胞成分。有机溶剂二甲基亚砜(MeSO)是最常用的CPA之一,根据细胞类型的不同,其使用效果也各有差异。近年来,为了改善低温保存效果,非还原性二糖海藻糖已被用作基于MeSO的冷冻溶液的添加剂。海藻糖是一种天然存在的无毒化合物,存在于细菌、真菌、植物和无脊椎动物中,已被证明在水分受限状态下能提供细胞保护作用。海藻糖改善低温保存效果的机制仍未完全明确。拉曼光谱显微镜是一种强大的工具,可深入了解低温保存过程中水、海藻糖和MeSO之间相互作用的本质。我们发现,在基于MeSO的CPA溶液中添加海藻糖,能显著减小冰晶的面积,但在冷却至-40或-80°C时会增加冰晶的数量。发现冰晶形成模式的差异对细胞活力有直接影响。尽管添加100 mM海藻糖会引起渗透压应激,但仍观察到细胞活力有所改善。然而,海藻糖浓度高于100 mM时渗透压的大幅增加可能会抵消添加这种糖所带来的改变冰晶形态的有益效果。

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