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基因的全合成

Total synthesis of a gene.

作者信息

Khorana H G

出版信息

Science. 1979 Feb 16;203(4381):614-25. doi: 10.1126/science.366749.

Abstract

The method developed for the total synthesis of a given DNA containing biologically specific sequences consists of the following. The DNA in the double-stranded form is carefully divided into short single-stranded segments with suitable overlaps in the complementary strands. All the segments are chemically synthesized starting with protected nucleosides and mononucleotides. The 5'-OH ends of the appropriate oligonucleotides are then phosphorylated with the use of [y-32P]ATP and polynucleotide kinase. A few to several neighboring oligonucleotides are then allowed to form bihelical complexes in aqueous solution, and the latter are joined end to end by polynucleotide ligase to form covalently linked duplexes. Subsequent heat-to-tail joining of the short duplexes leads to the total DNA. The methods are described for the construction of a biologically functional suppressor transfer RNA gene. The total work involved (i) the synthesis of a 126-nucleotide-long bihelical DNA corresponding to a known precursor to the tyrosine suppressor transfer RNA, (ii) the sequencing of the promoter region and the distal region adjoining the C-C-A end, which contained a signal for the processing of the RNA transcript, (iii) total synthesis of the 207 base-pair-long DNA, which included the control elements, as well as the Eco R1 restriction endonuclease specific sequences at the two ends, and (iv) full characterization by transcription in vitro and amber suppressor activity in vivo of the synthetic gene.

摘要

为全合成具有生物特异性序列的特定DNA所开发的方法如下。双链形式的DNA被小心地分割成短的单链片段,互补链之间有合适的重叠部分。所有片段均从受保护的核苷和单核苷酸开始进行化学合成。然后使用[γ-32P]ATP和多核苷酸激酶将合适的寡核苷酸的5'-OH末端磷酸化。接着让几个到几个相邻的寡核苷酸在水溶液中形成双螺旋复合物,然后通过多核苷酸连接酶将后者首尾相连,形成共价连接的双链体。随后将短双链体进行从头到尾的连接,从而得到完整的DNA。文中描述了构建具有生物功能的抑制性转移RNA基因的方法。整个工作包括:(i)合成一段126个核苷酸长的双螺旋DNA,其对应于酪氨酸抑制性转移RNA的已知前体;(ii)对启动子区域以及与C-C-A末端相邻的远端区域进行测序,该区域包含RNA转录本加工的信号;(iii)全合成一段207个碱基对长的DNA,其包括控制元件以及两端的Eco R1限制性内切酶特异性序列;(iv)通过体外转录和体内琥珀抑制活性对合成基因进行全面表征。

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