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快速冷冻和解冻的小鼠胚胎的存活情况。

Survival of mouse embryos frozen and thawed rapidly.

作者信息

Kasai M, Niwa K, Iritani A

出版信息

J Reprod Fertil. 1980 May;59(1):51-6. doi: 10.1530/jrf.0.0590051.

Abstract

Mouse morulae were frozen rapidly to -196 degrees C in the presence of 1.0-2.5 M-DMSO by a 3-step procedure; the samples were seeded at -4 to -8 degrees C, held at -20 degrees C in an ethanol bath for 10 min, suspended over liquid nitrogen at approximately -100 degrees C for 10 min and then plunged directly into liquid nitrogen at -196 degrees C. The cooling rate between -20 and -75 degrees C was approximately 17 degrees C/min. In all concentrations of DMSO significantly higher proportions of embryos developed to fully expanded blastocysts after 48 h in culture after rapid thawing (360 degrees C/min) than after slow thawing (25 degrees C/min). The highest survival rates were obtained for the embryos frozen rapidly in the presence of 1.5 and 2.0 M-DMSO (36 and 53% respectively). Various methods for removal of DMSO (2.0 M) were tested with the 3-step freezing and rapid thawing procedures. The best results for development to fully expanded blastocysts were obtained with PBS + 2.0 M DMSO + 0.5 M-sucrose (2 min) followed by PBS + 0.5 M-sucrose (2 min) at room temperature (82%) and with stepwise dilution in PBS at 30 degrees C (70%). When 26 embryos developed to blastocysts in culture after rapid freezing and thawing were transferred into 2 recipients, 11 newborn young (42%) were obtained.

摘要

小鼠桑椹胚通过三步程序在1.0 - 2.5M二甲基亚砜(DMSO)存在的情况下迅速冷冻至-196℃;样品在-4至-8℃接种,在乙醇浴中于-20℃保持10分钟,在约-100℃悬浮于液氮上方10分钟,然后直接投入-196℃的液氮中。-20至-75℃之间的冷却速率约为17℃/分钟。在所有DMSO浓度下,快速解冻(360℃/分钟)后培养48小时发育为完全扩张囊胚的胚胎比例显著高于缓慢解冻(25℃/分钟)后的比例。在1.5M和2.0M DMSO存在下快速冷冻的胚胎获得了最高的存活率(分别为36%和53%)。采用三步冷冻和快速解冻程序测试了去除DMSO(2.0M)的各种方法。在室温下用PBS + 2.0M DMSO + 0.5M蔗糖(2分钟),然后用PBS + 0.5M蔗糖(2分钟)处理,发育为完全扩张囊胚的效果最佳(82%),在30℃下在PBS中逐步稀释的效果也较好(70%)。当26个经快速冷冻和解冻后在培养中发育为囊胚的胚胎移植到2只受体动物体内时,获得了11只新生幼崽(42%)。

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