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小鼠卵母细胞顶体反应增强及单精子透明带下授精

Enhancement of acrosome reaction and subzonal insemination of a single spermatozoon in mouse eggs.

作者信息

Palermo G, Van Steirteghem A

机构信息

Centre for Reproductive Medicine, Brussels Free University, Belgium.

出版信息

Mol Reprod Dev. 1991 Dec;30(4):339-45. doi: 10.1002/mrd.1080300408.

Abstract

The acrosome reaction in mouse spermatozoa was induced by various means. These were 1) varying incubation time in T6 medium, 2) incubation in T6 medium with added A23187, 3) incubation in T6 medium with added dbcGMP and imidazole, 4) exposure to an electric field, and 5) a combination of incubation in a medium with dbcGMP and imidazole and electroporation. The mean percentages of acrosome-free spermatozoa obtained by these various methods and assessed on the basis of both Bryan's stain and immunolocalization by FITC-labeled monoclonal antibodies increased by steps from 36% to 67%, 73%, 86%, and 92%. Individual spermatozoa from the various treatments were afterwards microinjected under the zona pellucida of a mouse oocyte. The fertilization rate for eggs microinjected with a spermatozoon treated with A23187, dbcGMP, and imidazole, by electroporation and by a combination of the last two methods also increased by steps from 17% to 34%, 36%, and 70%, respectively. Ninety-five percent of the fertilized oocytes reached the early blastocyst stage, thirty-eight percent of these blastocysts implanted in pseudopregnant mice, and twenty-eight percent developed to term. These results indicated the varying degrees of success of different ways of inducing acrosomal loss in spermatozoa and their subsequent success rates in fertilization and further in vitro and in vivo development.

摘要

通过多种方法诱导小鼠精子发生顶体反应。这些方法包括:1)在T6培养基中改变孵育时间;2)在添加了A23187的T6培养基中孵育;3)在添加了二丁酰环磷腺苷(dbcGMP)和咪唑的T6培养基中孵育;4)暴露于电场;5)在含有dbcGMP和咪唑的培养基中孵育并结合电穿孔。通过这些不同方法获得的无顶体精子的平均百分比,基于布莱恩染色和异硫氰酸荧光素(FITC)标记的单克隆抗体免疫定位进行评估,从36%逐步增加到67%、73%、86%和92%。随后,将来自不同处理的单个精子显微注射到小鼠卵母细胞的透明带下。用A23187、dbcGMP和咪唑处理的精子,通过电穿孔以及最后两种方法结合处理后进行显微注射的卵子,其受精率也分别从17%逐步增加到34%、36%和70%。95%的受精卵发育到早期囊胚阶段,其中38%的囊胚在假孕小鼠体内着床,28%发育至足月。这些结果表明,诱导精子顶体丢失的不同方法取得了不同程度的成功,以及它们随后在受精以及进一步体外和体内发育中的成功率。

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