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无冷冻保护剂的哺乳动物细胞超快速冷冻保存。

Cryoprotectant-free cryopreservation of mammalian cells by superflash freezing.

机构信息

Department of Mechanical Engineering and Robotics, Faculty of Textile Science and Technology, Shinshu University, 3-15-1, Tokida, Ueda, Nagano 386-8567, Japan;

Department of Mechanical Engineering and Robotics, Faculty of Textile Science and Technology, Shinshu University, 3-15-1, Tokida, Ueda, Nagano 386-8567, Japan.

出版信息

Proc Natl Acad Sci U S A. 2019 Apr 16;116(16):7738-7743. doi: 10.1073/pnas.1808645116. Epub 2019 Apr 1.

Abstract

Cryopreservation is widely used to maintain backups of cells as it enables the semipermanent storage of cells. During the freezing process, ice crystals that are generated inside and outside the cells can lethally damage the cells. All conventional cryopreservation methods use at least one cryoprotective agent (CPA) to render water inside and outside the cells vitreous or nanocrystallized (near-vitrification) without forming damaging ice crystals. However, CPAs should ideally be avoided due to their cytotoxicity and potential side effects on the cellular state. Herein, we demonstrate the CPA-free cryopreservation of mammalian cells by ultrarapid cooling using inkjet cell printing, which we named superflash freezing (SFF). The SFF cooling rate, which was estimated by a heat-transfer stimulation, is sufficient to nearly vitrify the cells. The experimental results of Raman spectroscopy measurements, and observations with an ultrahigh-speed video camera support the near-vitrification of the droplets under these conditions. Initially, the practical utility of SFF was demonstrated on mouse fibroblast 3T3 cells, and the results were comparable to conventional CPA-assisted methods. Then, the general viability of this method was confirmed on mouse myoblast C2C12 cells and rat primary mesenchymal stem cells. In their entirety, the thus-obtained results unequivocally demonstrate that CPA-free cell cryopreservation is possible by SFF. Such a CPA-free cryopreservation method should be ideally suited for most cells and circumvent the problems typically associated with the addition of CPAs.

摘要

冷冻保存被广泛用于细胞备份,因为它可以实现细胞的半永久存储。在冷冻过程中,细胞内外形成的冰晶会对细胞造成致命的伤害。所有传统的冷冻保存方法都至少使用一种冷冻保护剂 (CPA) 使细胞内外的水玻璃化或纳米结晶(接近玻璃化),而不会形成破坏性的冰晶。然而,由于 CPAs 的细胞毒性和对细胞状态的潜在副作用,理想情况下应避免使用它们。在这里,我们通过喷墨细胞打印(我们称之为超快速冷冻 (SFF))展示了哺乳动物细胞无 CPA 冷冻保存。通过热传递模拟估计的 SFF 冷却速率足以使细胞几乎玻璃化。拉曼光谱测量的实验结果和超高速摄像机的观察结果支持在这些条件下液滴的近玻璃化。最初,SFF 的实际用途在小鼠成纤维细胞 3T3 细胞上得到了验证,结果与传统的 CPA 辅助方法相当。然后,在小鼠成肌细胞 C2C12 细胞和大鼠原代间充质干细胞上证实了这种方法的普遍生存能力。总之,这些结果明确证明了通过 SFF 可以实现无 CPA 的细胞冷冻保存。这种无 CPA 的细胞冷冻保存方法应该非常适合大多数细胞,并避免与添加 CPAs 相关的问题。

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Nat Methods. 2014 Apr 29;11(5):483-8. doi: 10.1038/nmeth.2932.
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Unexpected low-dose toxicity of the universal solvent DMSO.意想不到的通用溶剂 DMSO 的低剂量毒性。
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