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用于高效电穿孔的感受态完整酵母细胞的冷冻保存。

Cryopreservation of competent intact yeast cells for efficient electroporation.

作者信息

Suga M, Isobe M, Hatakeyama T

机构信息

Department of Materials and Biosystem Engineering, Toyama University, 3190 Gofuku Toyama-City, Toyama 930-8555, Japan.

出版信息

Yeast. 2000 Jul;16(10):889-96. doi: 10.1002/1097-0061(200007)16:10<889::AID-YEA582>3.0.CO;2-R.

DOI:10.1002/1097-0061(200007)16:10<889::AID-YEA582>3.0.CO;2-R
PMID:10870100
Abstract

We have developed a simple method for cryopreserving Schizosaccharomyces pombe and Saccharomyces cerevisiae competent intact cells that permits high transformation efficiency and long-term storage for electroporation. Transformation efficiency is significantly decreased if intact cells are frozen in common permeating cryoprotectants such as glycerol or dimethyl sulphoxide. On the other hand, we found that a high transformation efficiency could be maintained if the cells were frozen in a non-permeating cryoprotectant such as sorbitol. The optimum concentration of sorbitol was found in a hypertonic solution of around 2 M. It was also very important to use S. pombe cells grown in minimal medium and S. cerevisiae cells grown in nutrient medium in the exponential growth phase. A slow freezing rate of 10 degrees C/min and a rapid thawing rate of 200 degrees C/min resulted in the highest transformation efficiency. We also found it necessary to wash the thawed cells with 1.0 M of non-electrolyte sorbitol, since the intracellular electrolytes had leaked as a result of cryoinjury. The frozen competent cells stored at -80 degrees C could be used for more than 9 months without any loss of transformation efficiency. This cryopreservation method for electroporation is simple and useful for routine transformations of intact cells. Frozen competent cells offer the advantages of long-term storage with high efficiency and freedom from the preparation of fresh competent cells for each transformation.

摘要

我们开发了一种简单的方法来冷冻保存粟酒裂殖酵母和酿酒酵母感受态完整细胞,该方法可实现高效转化并能长期储存用于电穿孔。如果将完整细胞冷冻在常见的渗透性冷冻保护剂(如甘油或二甲基亚砜)中,转化效率会显著降低。另一方面,我们发现如果将细胞冷冻在非渗透性冷冻保护剂(如山梨醇)中,则可以维持较高的转化效率。山梨醇的最佳浓度在约2 M的高渗溶液中。使用在基本培养基中生长的粟酒裂殖酵母细胞和在营养培养基中指数生长期的酿酒酵母细胞也非常重要。10℃/分钟的缓慢冷冻速率和200℃/分钟的快速解冻速率可实现最高的转化效率。我们还发现有必要用1.0 M的非电解质山梨醇洗涤解冻后的细胞,因为细胞内电解质因冷冻损伤而泄漏。储存在-80℃的冷冻感受态细胞可使用9个月以上而转化效率无任何损失。这种用于电穿孔的冷冻保存方法简单,对完整细胞的常规转化很有用。冷冻感受态细胞具有高效长期储存的优点,且无需每次转化都制备新鲜的感受态细胞。

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