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Extreme rapid warming yields high functional survivals of vitrified 8-cell mouse embryos even when suspended in a half-strength vitrification solution and cooled at moderate rates to −196°C

机译:即使悬浮在半强度玻璃化溶液中并以中等速率冷却至-196°C极度快速的加热仍能获得玻璃化的8细胞小鼠胚胎的高功能存活率

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摘要

To cryopreserve cells, it is essential to avoid intracellular ice formation during cooling and warming. One way to do so is to subject them to procedures that convert cell water into a non-crystalline glass. Current belief is that to achieve this vitrification, cells must be suspended in very high concentrations of glass-inducing solutes (i.e., ≥ 6 molal) and cooled at very high rates (i.e., >> 1,000°C/min). We report here that both these beliefs are incorrect with respect to the vitrification of 8-cell mouse embryos. In this study, precompaction 8-cell embryos were vitrified in several dilutions of EAFS10/10 using various cooling rates and warming rates. Survival was based on morphology, osmotic functionality, and on the ability to develop to expanded blastocysts. With a warming rate of 117,500°C/min, the percentages of embryos vitrified in 1×, 0.75×, and 0.5× EAFS that developed to blastocysts were 93%, 92%, and 86%, respectively. And the percentages of morphological survivors that developed to expanded blastocysts were 100%, 92%, and 97%, respectively. Even when the solute concentration of the EAFS was reduced to 33% of normal, we obtained 40% functional survival of these 8-cell embryos.
机译:要冷冻保存细胞,必须在冷却和加热过程中避免细胞内冰的形成。一种方法是使它们经受将细胞水转化为非晶玻璃的程序。当前认为,要实现这种玻璃化,必须将细胞悬浮在非常高浓度的玻璃诱导溶质(即≥6 molal)中,并以非常高的速率(即 1,000°C / min)冷却。我们在这里报告这两种信念相对于8细胞小鼠胚胎的玻璃化是不正确的。在这项研究中,使用不同的冷却速率和加热速率,在EAFS10 / 10的几种稀释液中对预紧致8细胞胚胎进行了玻璃化。存活的依据是形态学,渗透功能以及发育为扩大的胚泡的能力。以117,500°C / min的升温速度,在1倍,0.75倍和0.5倍EAFS中玻璃化的胚胎发育为胚泡的百分比分别为93%,92%和86%。发育成囊胚的形态幸存者的百分比分别为100%,92%和97%。即使当EAFS的溶质浓度降低到正常水平的33%时,我们也获得了这些8细胞胚胎40%的功能存活率。

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