Cryopreservation of newly formed human and mouse hybridoma cells.

Allergie und Immunologie Pub Date : 1989-01-01
U Settmacher, S Jahn, R Grunow, M Mehl, R von Baehr
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Abstract

The aim of this study was to develop an optimal technique for cryopreservation of newly formed human and mouse hybridoma cells immediately after fusion. It was shown that human hybridoma cells could be frozen most successfully at a cooling rate of 5 K/min whereas mouse hybridomas at 1 K/min. The percentage of FCS in cryopreservation media (30 or 90%) had no influence on the recovery of both types of hybridomas. For testing the efficiency of freezing, the fusion rate (number of growing and Ig producing hybridomas), the ratio of IgM:IgG-producing initial hybridoma lines and yields of specific wells were analysed. Comparable results were registered when optimally cryopreserved and non-frozen material was studied. Optimization of the cryopreservation of newly formed hybridomas may be of methodological importance, especially when a time-consuming screening for antigenic specificities must be carried out.

新形成的人和小鼠杂交瘤细胞的低温保存。
本研究的目的是开发一种最佳的技术来冷冻保存新形成的人和小鼠杂交瘤细胞融合后立即。实验结果表明,人杂交瘤细胞在5 K/min的冷却速率下冷冻最成功,而小鼠杂交瘤细胞在1 K/min的冷却速率下冷冻最成功。低温保存培养基中FCS的比例(30%或90%)对两种类型杂交瘤的恢复没有影响。分析了冷冻效率、融合率(生长和产Ig杂交瘤的数量)、初始杂交瘤株与产Ig杂交瘤株的比例和特定井的产量。当研究最佳冷冻保存和非冷冻材料时,记录了类似的结果。优化新形成的杂交瘤的冷冻保存可能具有方法学上的重要性,特别是当必须进行耗时的抗原特异性筛选时。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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