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功能性信使核糖核酸通过克隆的互补脱氧核糖核酸的SP6体外转录产生。

Functional messenger RNAs are produced by SP6 in vitro transcription of cloned cDNAs.

作者信息

Krieg P A, Melton D A

出版信息

Nucleic Acids Res. 1984 Sep 25;12(18):7057-70. doi: 10.1093/nar/12.18.7057.

Abstract

We describe a method for the synthesis of microgram quantities of eucaryotic messenger RNAs. Injection into the cytoplasm of frog oocytes and addition to wheat germ extracts show that these synthetic RNAs function efficiently as messenger RNAs. We confirm that a 5' cap on the mRNA is essential for translation in injected oocytes and show that most of the 3' flanking region, including the poly A tail, can be deleted without the abolition of protein synthesis. The method of mRNA synthesis involves in vitro transcription of cDNAs which have been cloned into SP6 vectors (described in the accompanying paper). This method enables one to produce large amounts of mRNA and consequently protein from any cDNA clone.

摘要

我们描述了一种合成微克量真核生物信使RNA的方法。将其注射到蛙卵母细胞的细胞质中以及添加到麦胚提取物中表明,这些合成RNA作为信使RNA能高效发挥作用。我们证实,mRNA上的5'帽对于注射的卵母细胞中的翻译至关重要,并且表明3'侧翼区域的大部分,包括聚腺苷酸尾,可以被删除而不影响蛋白质合成。mRNA合成方法涉及对已克隆到SP6载体中的cDNA进行体外转录(随附论文中有描述)。这种方法能够从任何cDNA克隆大量生产mRNA并进而生产蛋白质。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7544/320142/780bab626bfc/nar00336-0145-a.jpg

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