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Cytoplasmic injection of circular plasmids allows targeted expression in mammalian embryos

机译:圆形质粒的细胞质注射可以在哺乳动物胚胎中靶向表达

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摘要

Injection of linearized DNA constructs into the pronuclei of fertilized mammalian eggs is a standard method for producing transgenic embryos and animals. Here, we show that injection of covalently closed circular (ccc) plasmids into the cytoplasm of fertilized bovine and murine eggs is a highly efficient and simple alternative for ectopic expression of foreign DNA in embryos. A broad range of plasmids could be successfully expressed in preimplantation stages, including plasmids and minicircles with a scaffold/matrix attachment region (S/MAR), conventional plasmids, and bacterial artificial chromosomes (BACs). Although the foreign DNA plasmids are mainly maintained as episomal entities during preimplantation development, they accurately behave like nuclear DNA. Onset of transcription of an Oct4 promoter-controlled marker gene coincided with the species-specific time points of major embryonic genome activation, and could be modulated by in vitro DNA-methylation. This approach allows an experimental access to reprogramming events in early mammalian embryos.
机译:将线性化的DNA构建体注射到受精哺乳动物卵的原核中是生产转基因胚胎和动物的标准方法。在这里,我们表明将共价闭合的环状(ccc)质粒注射到受精牛和鼠卵的细胞质中是异源DNA在胚胎中异位表达的高效简单的替代方法。各种各样的质粒可以在植入前阶段成功表达,包括具有支架/基质附着区(S / MAR)的质粒和小环,常规质粒和细菌人工染色体(BAC)。尽管外源DNA质粒在植入前的发育过程中主要维持为游离体,但它们的行为确实像核DNA。 Oct4启动子控制的标记基因转录的发生与主要胚胎基因组激活的物种特异性时间点一致,并且可以通过体外DNA甲基化来调节。这种方法允许实验获得早期哺乳动物胚胎中的重编程事件。

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