Developmental Competence of Somatic Cell Nuclear Transfer Embryos and Interspecies ICSI Zygotes From Bovine Small Antral Follicles

胚泡 生物 男科 体细胞核移植 合子 胚胎 体外成熟 卵母细胞 窦卵泡 体细胞 胚胎发生 细胞生物学 遗传学 卵巢 基因 医学
作者
Pham‐Truong Duy,Bui Le Quynh Nhu,Pham Quoc Dinh,Cao H. Nam,Lam Do Truc Phuong,Dao Quang Tri,Pham Minh Chien,Nhat‐Thinh Nguyen,Nguyen Van Thuan,Hong‐Thuy Bui
出处
期刊:Reproduction in Domestic Animals [Wiley]
卷期号:59 (10)
标识
DOI:10.1111/rda.14726
摘要

ABSTRACT Assisted reproductive technologies (ART) play a crucial role in conserving threatened wildlife species such as Bos gaurus . ART requires a large number of mature oocytes, and small antral follicles (SAFs) in the ovary are often used to obtain abundant sources of bovine oocytes. However, oocytes from SAFs often experience difficulty completing maturation and obtaining high quality and quantity of blastocyst formation compared to fully grown oocytes. This study aimed to increase the number of high‐quality mature oocytes and improve their potential for ART applications in cloned and interspecies intracytoplasmic sperm injection (ICSI) embryos by utilising L‐ascorbic acid (LAA) in pre in vitro maturation (pre‐IVM) culture. First, oocytes isolated from SAFs were cultured with the duration of pre‐IVM 0, 6, 8, 10 h and different concentrations of LAA to determine good conditions for oocyte maturation. Then, mature oocytes were assessed for their developmental competence through parthenogenesis, cloned and interspecies ICSI embryos. The results showed that 8‐h pre‐IVM with 50 μg/mL LAA improved the maturation rate and developmental competence of parthenogenetic and clone embryos, especially, improving the high blastocyst quality by increasing cell number and expression of histone acetylation at lysine 9 (H3K9ac). In addition, the culture process improved the nuclear reprogramming of somatic cells after nuclear transfer into mature oocytes, resulting in an increased hatching rate of cloned embryos. It also enhanced the activation and the pronuclear formation rate of Gaurus‐Taurus zygotes. Overall, the established pre‐IVM culture method enhanced the meiotic and developmental competence of embryos. This procedure opened hope for the preservation of endangered species and other applications.
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