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早期合子是牛体细胞核移植的合适受体,并能产生克隆后代。

Early zygotes are suitable recipients for bovine somatic nuclear transfer and result in cloned offspring.

作者信息

Schurmann Anita, Wells David N, Oback Björn

机构信息

AgResearch Ltd, Ruakura Research Centre, Reproductive Technologies, East Street, Hamilton, New Zealand.

出版信息

Reproduction. 2006 Dec;132(6):839-48. doi: 10.1530/REP-06-0054.

Abstract

Cloning by somatic cell nuclear transfer (SCNT) subverts sperm-mediated fertilization that normally leads to physiological activation of the oocyte. Therefore, artificial activation is required and it is presently unclear what developmental consequences this has. In this study, we aimed to improve cattle cloning efficiency by utilizing a more physiological method of activating SCNT reconstructs. We carried out in vitro fertilization (IVF) of zona-intact bovine oocytes before SCNT. We removed the zona pellucida 4 h after insemination, stained the fertilized eggs with Hoechst 33342 and mechanically removed both male and female chromatin. The enucleated pre-activated cytoplasts were fused with male adult ear skin fibroblasts ("IVF-NT" group). Chemically activated SCNT embryos, produced according to our standard operating procedure for zona-free SCNT, served as controls. After 7 days, in vitro development to blastocysts of morphological grade 1-3 or grade 1-2 was very similar in both groups (39 vs 40% and 20 vs 21% respectively). However, post-implantation development was improved after sperm-mediated activation. Across four replicate runs, pregnancy establishment at day 35 was significantly higher for IVF-NT than for control SCNT embryos (30/49 = 61 vs 17/41 = 42% respectively; P < 0.05). Development into calves at term or weaning was also higher in the IVF-NT group compared with control SCNT (9/49 = 18 vs 3/41 = 7% and 6/49 = 12 vs 3/41 = 7%; P = 0.11 and 0.34 respectively).

摘要

通过体细胞核移植(SCNT)进行克隆颠覆了正常情况下导致卵母细胞生理激活的精子介导的受精过程。因此,需要进行人工激活,而目前尚不清楚这会产生什么发育后果。在本研究中,我们旨在通过采用更符合生理的方法激活SCNT重构胚胎来提高牛的克隆效率。我们在进行SCNT之前,对完整透明带的牛卵母细胞进行体外受精(IVF)。授精4小时后去除透明带,用Hoechst 33342对受精卵进行染色,并机械去除雄原核和雌原核。将去核的预激活细胞质体与雄性成年耳皮肤成纤维细胞融合(“IVF-NT”组)。按照我们无透明带SCNT的标准操作程序生产的化学激活SCNT胚胎作为对照。7天后,两组中形态学等级为1-3级或1-2级的囊胚的体外发育情况非常相似(分别为39%对40%和20%对21%)。然而,精子介导的激活后植入后发育得到改善。在四次重复实验中,IVF-NT组在第35天的妊娠建立率显著高于对照SCNT胚胎(分别为30/49 = 61%对17/41 = 42%;P < 0.05)。与对照SCNT相比,IVF-NT组足月发育成犊牛或断奶的比例也更高(分别为9/49 = 18%对3/41 = 7%和6/49 = 12%对3/41 = 7%;P分别为0.

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