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Effect of slow freezing on morphology and developmental competence of buffalo (Bubalus bubalis) immature oocytes

机译:慢速冷冻对水牛(Bubalus bubalis)未成熟卵母细胞形态和发育能力的影响

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The present study was conducted to evaluate the effects of three cryoprotectants, dimethyl sulphoxide (DMSO), ethylene glycol (EG) and 1,2-propanediol (PROH), each used at two concentrations (1.0 and 1.5M) on the morphology, maturation rate and developmental capacity of usable quality immature buffalo oocytes subjected to slow freezing. The addition of the cryoprotectant before freezing and its dilution after thawing were carried out in a two- (for 1.0M) or three-step manner (for 1.5M). The incidence of damage was found to be significantly higher (P <0.05) with the lower concentration of 1.0M, compared to that with 1.5M for all the three cryoprotectants examined. The proportion of immature oocytes recovered in a morphologically normal state was significantly higher (P <0.05) for DMSO than those for EG or PROH at both 1.0 and 1.5M concentrations. Among the six combinations evaluated, that of DMSO at 1.5M concentration was found to be superior to others. Irrespective of the type or concentration of the cryoprotectant, partial or complete loss of the cumulus mass was the most prevalent damage. Following in vitro maturation, the nuclear maturation rate was significantly higher (P <0.05) for DMSO than those for EG or PROH at both 1.0 and 1.5M concentrations. When the in vitro matured oocytes were subjected to in vitro fertilization after slow freezing, using 1.5M DMSO as cryoprotectant, 4.5% and 0.6% of them were able to develop to morulae and blastocysts, respectively, on Day 9 post insemination, compared to 19.2% and 10.6%, respectively, for the controls. In conclusion, DMSO was more effective than EG or PROH for the slow freezing of immature buffalo oocytes and blastocysts could be produced from immature buffalo oocytes subjected to slow freezing in 1.5M DMSO.
机译:进行本研究以评估三种冷冻保护剂,即二甲亚砜(DMSO),乙二醇(EG)和1,2-丙二醇(PROH),分别以两种浓度(1.0和1.5M)使用对形态,成熟度的影响速冻后可用质量的未成熟水牛卵母细胞的生长速率和发育能力。冷冻前的冷冻保护剂的添加和解冻后的稀释以两步法(1.0M)或三步法(1.5M)进行。发现在三种浓度的防冻剂中,浓度分别为1.0M和1.5M时,损伤的发生率显着更高(P <0.05),而浓度为1.5M的损伤发生率则更高。在1.0M和1.5M浓度下,DMSO的形态正常状态下恢复的未成熟卵母细胞的比例显着高于EG或PROH(P <0.05)。在评估的六种组合中,发现浓度为1.5M的DMSO优于其他组合。不论冷冻保护剂的类型或浓度如何,积云部分或全部损失是最普遍的损害。在体外成熟后,在1.0和1.5M浓度下,DMSO的核成熟率均显着高于EG或PROH的核成熟率(P <0.05)。当将体外成熟的卵母细胞缓慢冷冻后进行体外受精时,使用1.5M DMSO作为冷冻保护剂,在受精后第9天,分别有4.5%和0.6%能够发育为桑ula和胚泡,而19.2对照分别为%和10.6%。总之,对于未成熟的水牛卵母细胞缓慢冷冻,DMSO比EG或PROH更有效,在1.5M DMSO中经过缓慢冷冻的未成熟水牛卵母细胞可以产生胚泡。

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