Huang You-Zhang, Shen Jian-Liang, Gong Li-Zhong, Zheng Pei-Hao, Liu Yi, Yin Wen-Jie, Cen Jian, Wang Ning, Zhao De-Feng
Department of Hematology, Navy General Hospital of Chinese PLA, Beijing, 100048, China.
Zhongguo Shi Yan Xue Ye Xue Za Zhi. 2010 Feb;18(1):224-9.
The aim of this study was to investigate the best method to preserve human bone marrow cells and the effectiveness of long term cryopreservation at -80 degrees C. The human bone marrow cells in 20 samples were firstly frozen by a programmed freezer or -80 degrees C refrigerator, and then were preserved in liquid nitrogen with DMSO-AuP (10% dimethylsulfonamide, 10% autologous plasma) or DMSO-HES-HuA (5% dimethylsulfonamide, 6% hydroxyethyl starch, 4% human serum albumin) as cryoprotectant for 21 to 25 years. They were thawed in 38 degrees C. The cell sample frozen in -80 degrees C refrigerator was frozen at a low frozen speed of 1 degrees C/min which was the same as the programmed freezer before -30 degrees C. Before detection the bone marrow cells were taken from liquid nitrogen and were thawed in 38 degrees C, then the suspension of bone marrow cells was prepared for detection. The cell morphology and recovery rate of erythrocytes, nucleocytes and platelets; the recovery rate of hematopoietic stem progenitors cells, as well as mesenchymal stem cells were determined. The results showed that the protective effectiveness of DMSO-HES-HuA was better than DMSO-AuP. The mature erythrocytes were destroyed lightly [(3.5 +/- 1.5)% versus (12.6 +/- 4.8)%], the hemolysis rate was lower [(3.3 +/- 1.6)% versus (23.1 +/- 5.1)%]. Osmotic fragility of erythrocytes in the former was not changed, but was dropped in the latter. The recovery rates of red cell, platelet, granulocyte-macrophage colony forming units and long term culture-initiating cells were higher in the former than that in the latter [(96.1 +/- 1.8)%, (70.0 +/- 9.5)%, (49.2 +/- 10.9)%, (54.2 +/- 13.8)% versus (76.3 +/- 5.6)%, (52.7 +/- 8.1)%, (43.5 +/- 12.3)%, (47.2 +/- 13.6)% respectively]. With each kind of cryoprotectant or frozen method, the frozen MSC could keep the original growth properties. With the same cryoprotectant and different frozen method, the cryopreservative effectiveness was not different. The influence of the cryoprotectant prescriptions and the frozen methods on the cryopreservative effectiveness was little. It is concluded that the human bone marrow cells with DMSO-AuP or DMSO-HES-HuA as cryoprotectant, frozen by a programmed freezer or -80 degrees C refrigerator, could be then preserved in liquid nitrogen for long time. When the preserving time was as long as 21 to 25 years, the morphology, the recovery rate and the activity of various kinds of cells were still good. The method of freezing by -80 degrees C refrigerator with 5% DMSO-6% HES-4% HuA and preserving in liquid nitrogen would be convenient, cheap and easily-manipulated for preservation of the human bone marrow cells.
本研究的目的是探讨保存人骨髓细胞的最佳方法以及在 -80℃长期冷冻保存的效果。20份样本中的人骨髓细胞首先通过程序降温仪或 -80℃冰箱进行冷冻,然后以二甲基亚砜 - 自体血浆(DMSO - AuP,10%二甲基亚砜,10%自体血浆)或二甲基亚砜 - 羟乙基淀粉 - 人血清白蛋白(DMSO - HES - HuA,5%二甲基亚砜,6%羟乙基淀粉,4%人血清白蛋白)作为 cryoprotectant 在液氮中保存21至25年。它们在38℃解冻。在 -80℃冰箱中冷冻的细胞样本以1℃/分钟的低冷冻速度冷冻,该速度在 -30℃之前与程序降温仪相同。在检测前,将骨髓细胞从液氮中取出并在38℃解冻,然后制备骨髓细胞悬液用于检测。测定细胞形态以及红细胞、有核细胞和血小板的回收率;造血干祖细胞以及间充质干细胞的回收率。结果表明,DMSO - HES - HuA 的保护效果优于 DMSO - AuP。成熟红细胞受损较轻[(3.5±1.5)%对(12.6±4.8)%],溶血率较低[(3.3±1.6)%对(23.1±5.1)%]。前者红细胞的渗透脆性未改变,而后者降低。前者红细胞、血小板、粒 - 巨噬细胞集落形成单位和长期培养起始细胞的回收率高于后者[分别为(96.1±1.8)%,(70.0±9.5)%,(49.2±10.9)%,(54.2±13.8)%对(76.3±5.6)%,(52.7±8.1)%,(43.5±12.3)%,(47.2±13.6)%]。使用每种 cryoprotectant 或冷冻方法,冷冻的间充质干细胞都能保持原有的生长特性。使用相同的 cryoprotectant 和不同的冷冻方法,冷冻保存效果无差异。cryoprotectant 配方和冷冻方法对冷冻保存效果的影响较小。结论是,以 DMSO - AuP 或 DMSO - HES - HuA 作为 cryoprotectant,通过程序降温仪或 -80℃冰箱冷冻的人骨髓细胞,随后可在液氮中长期保存。当保存时间长达21至25年时,各种细胞的形态、回收率和活性仍然良好。采用含5%DMSO - 6%HES - 4%HuA 的 -80℃冰箱冷冻并在液氮中保存的方法,对于保存人骨髓细胞将是方便、廉价且易于操作的。
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