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受体卵母细胞细胞周期阶段对核移植牛胚胎中DNA合成、核膜破裂、染色体组成及发育的影响。

Influence of recipient oocyte cell cycle stage on DNA synthesis, nuclear envelope breakdown, chromosome constitution, and development in nuclear transplant bovine embryos.

作者信息

Barnes F L, Collas P, Powell R, King W A, Westhusin M, Shepherd D

机构信息

Genmark, Inc., Salt Lake City, Utah 84108.

出版信息

Mol Reprod Dev. 1993 Sep;36(1):33-41. doi: 10.1002/mrd.1080360106.

DOI:10.1002/mrd.1080360106
PMID:8398128
Abstract

Nuclear transplantations into metaphase II (MII) and S phase oocyte cytoplasm were performed to investigate the influence of recipient cell cycle stage on nuclear function and development of bovine nuclear transplant (NT) embryos. Rate of inactivation of histone H1 kinase and duration of DNA synthesis in activated oocytes were determined. The proportion of S phase blastomeres in in vivo produced day 5.5 bovine embryos was measured. DNA synthesis was also assessed in NT embryos after transfer into MII and S phase cytoplasm. MII NT embryos were produced by fusing a blastomere into a MII oocyte; the fusion pulse served to activate the oocyte. S NT embryos were produced by fusing a blastomere into an early S phase oocyte electrically activated 4 h prior to fusion. Nuclear envelope structure, chromosome constitution, and extent of development were examined in MII and S NT embryos. Histone H1 kinase activity dropped to baseline within 2 h of electrical activation. A second electrical pulse did not alter H1 kinase activity when delivered 4 h after the first pulse. The frequency of S phase blastomeres in day 5.5 bovine embryos ranged from 79% to 100%, depending on the duration of culture in 3H-thymidine. Nuclear transplantation into MII cytoplasm resulted in a transient drop in DNA synthesis over 3.5 h. DNA synthesis resumed at 4.5 h post activation (hpa), concomittantly with initiation of DNA replication in activated oocytes. In contrast, DNA synthesis was not interrupted after transfer into S phase cytoplasm. DNA synthesis persisted until 13.5 hpa, as in activated oocytes.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

进行细胞核移植到中期II(MII)和S期卵母细胞胞质中,以研究受体细胞周期阶段对牛细胞核移植(NT)胚胎的核功能和发育的影响。测定了活化卵母细胞中组蛋白H1激酶的失活率和DNA合成持续时间。测量了体内产生的第5.5天牛胚胎中S期卵裂球的比例。还评估了NT胚胎移植到MII和S期胞质后的DNA合成情况。MII NT胚胎通过将一个卵裂球融合到一个MII卵母细胞中产生;融合脉冲用于激活卵母细胞。S NT胚胎通过将一个卵裂球融合到融合前4小时电激活的早期S期卵母细胞中产生。检查了MII和S NT胚胎的核膜结构、染色体组成和发育程度。电激活后2小时内,组蛋白H1激酶活性降至基线。在第一个脉冲后4小时给予第二个电脉冲不会改变H1激酶活性。第5.5天牛胚胎中S期卵裂球的频率在79%至100%之间,这取决于在3H-胸腺嘧啶中培养的持续时间。细胞核移植到MII胞质中导致DNA合成在3.5小时内短暂下降。DNA合成在激活后4.5小时(hpa)恢复,与活化卵母细胞中DNA复制的开始同时发生。相比之下,移植到S期胞质后DNA合成没有中断。DNA合成持续到激活后13.5小时,如同在活化卵母细胞中一样。(摘要截断于250字)

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