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犊牛卵母细胞的玻璃化冷冻:成熟阶段和成熟前处理对卵母细胞核及细胞骨架成分及其后续发育的影响。

Vitrification of calf oocytes: effects of maturation stage and prematuration treatment on the nuclear and cytoskeletal components of oocytes and their subsequent development.

作者信息

Albarracín José Luis, Morató Roser, Izquierdo Dolors, Mogas Teresa

机构信息

Departament de Medicina i Cirurgia Animals, Facultat de Veterinària, Universitat Autònoma de Barcelona, 08193 Bellaterra, Spain.

出版信息

Mol Reprod Dev. 2005 Oct;72(2):239-49. doi: 10.1002/mrd.20326.

Abstract

This study was designed to establish the effects of the meiotic stage of bovine oocytes and of a prematuration treatment with roscovitine (ROS) on their resistance to cryopreservation. Oocytes from prepubertal calves at the stages of germinal vesicle breakdown (GVBD) or at metaphase II (MII) were vitrified by the open pulled straw (OPS) method. In another experiment, oocytes were kept under meiotic arrest with 50 microM ROS for 24 hr and vitrified at the GVBD stage. After warming, some oocyte samples were fixed, stained using specific fluorescent probes and examined under a confocal microscope. The remaining oocytes were fertilized, and cleavage and blastocyst rates recorded. Significantly lower cleavage rates were obtained for the vitrified GVBD and MII oocytes (9.9% and 12.6%, respectively) compared to control oocytes (73.9%). Significantly worse results in terms of cleavage rates were obtained when GVBD calf oocytes were exposed to cryoprotectants (CPAs: ethylene glycol plus dimethyl sulfoxide, DMSO) (13.1%) or vitrified (1.6%) after a prematuration treatment with ROS, when compared to untreated control oocytes (68.7%) or ROS-control oocytes (56.6%). None of the vitrification procedures yielded blastocysts, irrespective of the initial meiotic stage or previous prematuration treatment. Compared to the control oocytes, significantly fewer oocytes exhibited normal spindle configuration after being exposed to CPAs or after vitrification of either GVBD or MII calf oocytes. These results indicate that the vitrification protocol has a deleterious effect on the meiotic spindle organization of calf oocytes cryopreserved at both the GVBD and MII stage, which impairs the capacity for further development of the embryos derived from these vitrified oocytes. Prematuration treatment with ROS has no beneficial effect on the outcome of vitrification by the OPS method.

摘要

本研究旨在确定牛卵母细胞的减数分裂阶段以及用罗哌卡因(ROS)进行的早熟处理对其冷冻保存抗性的影响。来自青春期前小牛处于生发泡破裂(GVBD)阶段或中期II(MII)的卵母细胞通过开放式拉管(OPS)方法进行玻璃化。在另一项实验中,卵母细胞用50微摩尔ROS减数分裂阻滞24小时,并在GVBD阶段进行玻璃化。解冻后,一些卵母细胞样本被固定,使用特定荧光探针染色,并在共聚焦显微镜下检查。其余卵母细胞受精,并记录分裂和囊胚率。与对照卵母细胞(73.9%)相比,玻璃化的GVBD和MII卵母细胞的分裂率显著降低(分别为9.9%和12.6%)。当GVBD小牛卵母细胞在用ROS进行早熟处理后暴露于冷冻保护剂(CPA:乙二醇加二甲基亚砜,DMSO)(13.1%)或玻璃化(1.6%)时,与未处理的对照卵母细胞(68.7%)或ROS对照卵母细胞(56.6%)相比,在分裂率方面得到的结果明显更差。无论初始减数分裂阶段或先前的早熟处理如何,所有玻璃化程序均未产生囊胚。与对照卵母细胞相比,暴露于CPA后或GVBD或MII小牛卵母细胞玻璃化后,显示正常纺锤体构型的卵母细胞明显减少。这些结果表明,玻璃化方案对在GVBD和MII阶段冷冻保存的小牛卵母细胞的减数分裂纺锤体组织具有有害影响,这损害了源自这些玻璃化卵母细胞的胚胎的进一步发育能力。用ROS进行早熟处理对OPS方法玻璃化的结果没有有益影响。

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