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神经胚形成过程中小鼠胚胎的培养。

Culture of mouse embryos during neurulation.

作者信息

Sadler T W, New D A

出版信息

J Embryol Exp Morphol. 1981 Dec;66:109-16.

PMID:7338707
Abstract

A comparison between static versus rotator culture systems and a variety of media (rat serum, new born calf serum, DMEM and Waymouth's) was made in an attempt to promote in vitro growth of mouse embryos from the beginning of neurulation (headfold stage) to the closure of the neural tube and formation of the limb buds (48 h). The results demonstrate that good development can be achieved for 48 h using a rotator system and that 80% of embryos cultured on rotators show growth and differentiation similar to that obtained for the same time period in vivo. Static cultures are less successful and embryos grown in this system show lower protein content and somite numbers than those maintained on rotators. Undiluted rat serum is superior to all other media tested and supports better growth and development as monitored by total protein and developmental abnormalities.

摘要

为了促进小鼠胚胎从神经胚形成开始(头褶期)到神经管闭合和肢芽形成(48小时)的体外生长,对静态培养系统与旋转培养系统以及多种培养基(大鼠血清、新生小牛血清、DMEM和Waymouth培养基)进行了比较。结果表明,使用旋转培养系统48小时可实现良好的发育,并且在旋转培养器上培养的胚胎中有80%显示出与体内相同时间段所获得的生长和分化相似。静态培养不太成功,在该系统中生长的胚胎与在旋转培养器上培养的胚胎相比,蛋白质含量和体节数量较低。未稀释的大鼠血清优于所有其他测试培养基,并且通过总蛋白和发育异常监测显示其支持更好的生长和发育。

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