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一种改良的培养方法显著提高了小鼠体细胞核移植胚胎的发育。

A modified culture method significantly improves the development of mouse somatic cell nuclear transfer embryos.

作者信息

Dai Xiangpeng, Hao Jie, Zhou Qi

机构信息

State Key Laboratory of Reproductive Biology, Institute of Zoology, Chinese Academy of Sciences, Beijing, PR China.

出版信息

Reproduction. 2009 Aug;138(2):301-8. doi: 10.1530/REP-09-0069. Epub 2009 Jun 3.

Abstract

Many strategies have been established to improve the efficiency of somatic cell nuclear transfer (SCNT), but relatively few focused on improving culture conditions. The effect of different culture media on preimplantation development of mouse nuclear transfer embryos was investigated. A modified sequential media method, named D media (M16/KSOM and CZB-EG/KSOM), was successfully established that significantly improves SCNT embryo development. Our result demonstrated that while lacking any adverse effect on in vivo fertilized embryos, the D media dramatically improves the blastocyst development of SCNT embryos compared with other commonly used media, including KSOM, M16, CZB, and alphaMEM. Specifically, the rate of blastocyst formation was 62.3% for D1 (M16/KSOM) versus 10-30% for the other media. An analysis of media components indicated that removing EDTA and glutamine from the media can be beneficial for early SCNT embryo development. Our results suggest that in vitro culture environment plays an important role in somatic cell reprogramming, and D media represent the most efficient culture method reported to date to support mouse SCNT early embryo development in vitro.

摘要

人们已经建立了许多策略来提高体细胞核移植(SCNT)的效率,但相对较少关注改善培养条件。本研究调查了不同培养基对小鼠核移植胚胎着床前发育的影响。成功建立了一种改良的序贯培养基方法,称为D培养基(M16/KSOM和CZB-EG/KSOM),该方法显著改善了SCNT胚胎的发育。我们的结果表明,D培养基虽然对体内受精胚胎没有任何不利影响,但与其他常用培养基(包括KSOM、M16、CZB和αMEM)相比,它显著提高了SCNT胚胎的囊胚发育率。具体而言,D1(M16/KSOM)培养基的囊胚形成率为62.3%,而其他培养基的囊胚形成率为10%-30%。对培养基成分的分析表明,从培养基中去除EDTA和谷氨酰胺可能有利于SCNT早期胚胎的发育。我们的结果表明,体外培养环境在体细胞重编程中起着重要作用,并表明D培养基是迄今为止报道的支持小鼠SCNT早期胚胎体外发育的最有效培养方法。

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