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人类单核细胞的玻璃化冷冻

Vitrification of human monocytes.

作者信息

Takahashi T, Hirsh A, Erbe E F, Bross J B, Steere R L, Williams R J

出版信息

Cryobiology. 1986 Apr;23(2):103-15. doi: 10.1016/0011-2240(86)90001-5.

DOI:10.1016/0011-2240(86)90001-5
PMID:3698640
Abstract

Human monocytes purified from peripheral blood by counterflow centrifugal elutriation were cryopreserved in a vitreous state at 1 atm pressure. The vitrification solution was Hanks' balanced salt solution (HBSS) containing (w/v) 20.5% Me2SO, 15.5% acetamide, 10% propylene glycol, and 6% polyethylene glycol. Fifteen milliliters of this solution was added dropwise to 1 ml of a concentrated monocyte suspension at 0 degrees C. Of this, 0.8 ml was drawn into silicone tubing and rapidly cooled to liquid nitrogen temperature, stored for various periods, and rapidly warmed in an ice bath. The vitrification solution was removed by slow addition of HBSS containing 20% fetal calf serum. The numerical cell recovery was about 92% and most of these retained normal phagocytic and chemotactic ability. Differential scanning calorimeter records of the solution show a glass transition at -115 degrees C during cooling and warming, but no evidence of ice formation during cooling. Devitrification occurs at about -70 degrees C during warming at rates as rapid as 80 degrees C/min. The amount of devitrification is dependent upon the warming rate. Freeze-fracture freeze-etch electron microscope observations revealed no ice either intra- or extracellularly in samples rapidly cooled to liquid nitrogen temperatures except for small amounts in some cellular organelles. However, if these cell suspensions were warmed rapidly to -70 degrees C and then held for 5 min, allowing devitrification to occur, the preparation contained significant amounts of both intra- and extracellular ice. Biological data showed that this devitrification was associated with severe loss of cell function.

摘要

通过逆流离心淘析从外周血中纯化的人单核细胞在1个大气压下以玻璃态进行冷冻保存。玻璃化溶液是含有(重量/体积)20.5%二甲基亚砜、15.5%乙酰胺、10%丙二醇和6%聚乙二醇的汉克斯平衡盐溶液(HBSS)。将15毫升该溶液在0℃下逐滴加入到1毫升浓缩单核细胞悬液中。取其中0.8毫升吸入硅胶管,迅速冷却至液氮温度,保存不同时间,然后在冰浴中迅速复温。通过缓慢加入含有20%胎牛血清的HBSS去除玻璃化溶液。细胞数量回收率约为92%,其中大多数保留了正常的吞噬和趋化能力。该溶液的差示扫描量热仪记录显示,在冷却和复温过程中,玻璃化转变温度为-115℃,但冷却过程中没有结冰迹象。在以高达80℃/分钟的速度复温过程中,约-70℃时发生脱玻璃化。脱玻璃化的量取决于复温速度。冷冻断裂冷冻蚀刻电子显微镜观察显示,快速冷却至液氮温度的样品中,细胞内和细胞外均未发现冰,除了一些细胞器中有少量冰。然而,如果将这些细胞悬液迅速复温至-70℃,然后保持5分钟,使脱玻璃化发生,则制剂中含有大量的细胞内和细胞外冰。生物学数据表明,这种脱玻璃化与细胞功能的严重丧失有关。

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