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使用改良(密封)开放式拉制细管法对兔胚胎进行非平衡冷冻保存。

Nonequilibrium cryopreservation of rabbit embryos using a modified (sealed) open pulled straw procedure.

作者信息

López-Béjar M, López-Gatius F

机构信息

Department of Animal Health and Anatomy, Autonomous University of Barcelona, Bellaterra, Spain.

出版信息

Theriogenology. 2002 Nov;58(8):1541-52. doi: 10.1016/s0093-691x(02)01045-2.

Abstract

The study was designed to evaluate the efficiency of a modified (sealed) open pulled straw (mOPS) method for cryopreserving rabbit embryos by vitrification or rapid freezing. An additional objective was to determine whether the mOPS method could cause the vitrification of a cryoprotectant solution generally used in rapid freezing procedures. Two consecutive experiments of in vitro and in vivo viability were performed. In Experiment 1, the in vitro viability of rabbit embryos at the morula, compacted morula, early blastocyst and blastocyst stages was assessed after exposure to a mixture of 25% glycerol and 25% ethylene glycol (25GLY:25EG: vitrification solution) or 4.5 M (approximately 25% EG) ethylene glycol and 0.25 M sucrose (25EG:SUC: rapid freezing solution). Embryos were loaded into standard straws or mOPS and plunged directly into liquid nitrogen. The mOPS consisted of standard straws that were heat-pulled, leaving a wide opening for the cotton plug and a narrow one for loading embryos by capillarity. The embryos were aspirated into the mOPS in a column positioned between two columns of cryoprotectant solution separated by air bubbles. The mOPS were then sealed with polyvinyl-alcohol (PVA) sealing powder. The vitrification 25GLY:25EG solution became vitrified both in standard straws and mOPS, whereas the rapid freezing 25EG:SUC solution crystallized in standard straws, but vitrified in mOPS. The total number of embryos cryopreserved was 1695. Embryos cryopreserved after exposure to each solution in mOPS showed higher rates (88.2%) of survival immediately after thawing and removal of the cryoprotectant than those cryopreserved in 0.25 ml standard straws (78.8%; P < 0.0001). After culture, the developmental stage of the cryopreserved embryos significantly affected the rates of development to the expanded blastocyst stage. Regardless of the cryoprotectant used, lower rates of in vitro development were obtained when the embryos were cryopreserved at the morula stage, and higher rates achieved using embryos at blastocyst stages. Based on the results of Experiment 1, the second experiment was performed on blastocysts using the mOPS method. Experiment 2 was designed to evaluate the in vivo viability of cryopreserved rabbit blastocysts loaded into mOPS after exposure to 25GLY:25EG or 25EG:SUC. Embryos cryopreserved in mOPS and 25GLY:25EG solution gave rise to rates of live offspring (51.7%) not significantly different to those achieved using fresh embryos (58.5%). In conclusion, the modified (sealed) OPS method allows vitrification of the cryoprotectant solution at a lower concentration of cryoprotectants than that generally used in vitrification procedures. Rabbit blastocysts cryopreserved using a 25GLY:25EG solution in mOPS showed a similar rate of in vivo development after thawing to that shown by fresh embryos.

摘要

本研究旨在评估改良(密封)开放式拉细麦管(mOPS)法通过玻璃化或快速冷冻保存兔胚胎的效率。另一个目标是确定mOPS法是否会导致快速冷冻程序中常用的冷冻保护剂溶液发生玻璃化。进行了连续两个关于体外和体内活力的实验。在实验1中,将兔桑椹胚、致密桑椹胚、早期囊胚和囊胚阶段的胚胎暴露于25%甘油和25%乙二醇的混合物(25GLY:25EG:玻璃化溶液)或4.5 M(约25%EG)乙二醇和0.25 M蔗糖(25EG:SUC:快速冷冻溶液)后,评估其体外活力。将胚胎装入标准麦管或mOPS中,然后直接投入液氮。mOPS由经过热拉的标准麦管组成,棉塞处开口宽,通过毛细作用装载胚胎处开口窄。将胚胎吸入位于由气泡隔开的两列冷冻保护剂溶液之间的一列mOPS中。然后用聚乙烯醇(PVA)密封粉密封mOPS。玻璃化25GLY:25EG溶液在标准麦管和mOPS中均发生玻璃化,而快速冷冻25EG:SUC溶液在标准麦管中结晶,但在mOPS中玻璃化。冷冻保存的胚胎总数为1695个。与在0.25 ml标准麦管中冷冻保存的胚胎(78.8%;P < 0.0001)相比,在mOPS中暴露于每种溶液后冷冻保存的胚胎在解冻并去除冷冻保护剂后立即显示出更高的存活率(88.2%)。培养后,冷冻保存胚胎的发育阶段显著影响发育至扩张囊胚阶段的比率。无论使用何种冷冻保护剂,当胚胎在桑椹胚阶段冷冻保存时,体外发育率较低,而使用囊胚阶段的胚胎则获得更高比率。基于实验1的结果,对囊胚进行了使用mOPS法的第二个实验。实验2旨在评估暴露于25GLY:25EG或25EG:SUC后装入mOPS的冷冻保存兔囊胚的体内活力。在mOPS和25GLY:25EG溶液中冷冻保存的胚胎产生的活仔率(51.7%)与使用新鲜胚胎获得的活仔率(58.5%)无显著差异。总之,改良(密封)OPS法允许在比玻璃化程序中通常使用的冷冻保护剂浓度更低的情况下使冷冻保护剂溶液玻璃化。在mOPS中使用25GLY:25EG溶液冷冻保存的兔囊胚解冻后的体内发育率与新鲜胚胎相似。

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