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一项关于小鼠胚胎冷冻保存的比较研究,包括对一种热电冷冻装置的检测。

A comparative study of mouse embryo freeze-preservation including the examination of a thermoelectric freezing device.

作者信息

Schiewe M C, Schmidt P M, Wildt D E

出版信息

Cryobiology. 1987 Jun;24(3):238-46. doi: 10.1016/0011-2240(87)90026-5.

Abstract

In Study 1 over 2000 4- to 8-cell mouse embryos were randomly pooled and assigned to 1 of 12 treatment groups. A 2 X 2 X 3 factorial design was used to analyze two types of cryoprotectant/post-thaw (PT) dilutions (dimethyl sulfoxide [Me2SO]/stepwise dilution versus glycerol/sucrose dilution), two storage containers (glass ampoules versus plastic straws), and three cooling treatments. Two commercial, controlled-rate freezing machines were examined, employing either nitrogen gas (Planer) or thermoelectric (Glacier) cooling. Embryos were cooled slowly (0.5 degrees C/min) to -35 or -80 degrees C and then cooled rapidly by transfer into liquid nitrogen (LN2). Thawed embryos were cultured for 24 hr after which developmental stage, post-thaw survival (PTS), embryo degeneration rate (EDR), quality grade (QG), and fluorescein diacetate viability grade (VG) were assessed. Overall, PTS and EDR were similar (P greater than 0.05) among the three freezing unit/plunge temperature treatments. Cumulative results of container and cryoprotectant/PT dilution treatments consistently demonstrated greater PTS, QG, and VG ratings and lower EDR values when embryos were frozen in ampoules using glycerol/sucrose dilution. Embryos treated with Me2SO/stepwise dilution were particularly sensitive to freezing damage when stored in plastic straws and plunged into LN2 at -35 degrees C. Study 2 was directed at determining whether Study 1 methods for diluting Me2SO-protected embryos markedly affected PTS rates. Post-thaw culture percentages were no different (P greater than 0.05) for four- to eight-cell Me2SO-treated embryos frozen in ampoules (using the forced-LN2 device), thawed, and diluted either conventionally in reduced concentrations of Me2SO or in the sucrose treatment normally accorded glycerolated embryos.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在研究1中,超过2000个4至8细胞期的小鼠胚胎被随机汇集,并分配到12个处理组中的1组。采用2×2×3析因设计来分析两种冷冻保护剂/解冻后(PT)稀释液(二甲基亚砜[Me2SO]/逐步稀释与甘油/蔗糖稀释)、两种储存容器(玻璃安瓿与塑料细管)以及三种冷却处理。检查了两台商用的程序降温冷冻机,分别采用氮气(Planer)或热电(Glacier)冷却。胚胎先以0.5℃/分钟的速度缓慢冷却至-35℃或-80℃,然后迅速转移至液氮(LN2)中进行快速冷却。解冻后的胚胎培养24小时,之后评估发育阶段、解冻后存活率(PTS)、胚胎退化率(EDR)、质量等级(QG)以及荧光素二乙酸活力等级(VG)。总体而言,在三种冷冻装置/投入温度处理中,PTS和EDR相似(P大于0.05)。当胚胎使用甘油/蔗糖稀释液在安瓿中冷冻时,容器和冷冻保护剂/PT稀释液处理的累积结果始终显示出更高的PTS、QG和VG评级以及更低的EDR值。当使用Me2SO/逐步稀释液处理的胚胎储存在塑料细管中并在-35℃投入LN2时,对冷冻损伤特别敏感。研究2旨在确定研究1中稀释Me2SO保护胚胎的方法是否显著影响PTS率。对于在安瓿中冷冻(使用强制LN2装置)、解冻并以常规方式用降低浓度的Me2SO或通常用于甘油化胚胎的蔗糖处理进行稀释的4至8细胞期经Me2SO处理的胚胎,解冻后培养百分比没有差异(P大于0.05)。(摘要截选至250词)

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