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In vitro selection of tRNAs for efficient four-base decoding to incorporate non-natural amino acids into proteins in an Escherichia coli cell-free translation system

机译:tRNA的体外选择,可进行有效的四碱基解码,以将非天然氨基酸整合到大肠杆菌无细胞翻译系统中的蛋白质中

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摘要

Position-specific incorporation of non-natural amino acids into proteins is a useful technique in protein engineering. In this study, we established a novel selection system to obtain tRNAs that show high decoding activity, from a tRNA library in a cell-free translation system to improve the efficiency of incorporation of non-natural amino acids into proteins. In this system, a puromycin–tRNA conjugate, in which the 3'-terminal A unit was replaced by puromycin, was used. The puromycin–tRNA conjugate was fused to a C-terminus of streptavidin through the puromycin moiety in the ribosome. The streptavidin–puromycin–tRNA fusion molecule was collected and brought to the next round after amplification of the tRNA sequence. We applied this system to select efficient frameshift suppressor tRNAs from a tRNA library with a randomly mutated anticodon loop derived from yeast . After three rounds of the selection, we obtained novel frameshift suppressor tRNAs which had high decoding activity and good orthogonality against endogenous aminoacyl-tRNA synthetases. These results demonstrate that the in vitro selection system developed here is useful to obtain highly active tRNAs for the incorporation of non-natural amino acid from a tRNA library.
机译:非天然氨基酸到蛋白质的位置特异性掺入是蛋白质工程中的有用技术。在这项研究中,我们建立了一个新的选择系统,以从无细胞翻译系统中的tRNA文库中获得具有高解码活性的tRNA,以提高将非天然氨基酸掺入蛋白质的效率。在该系统中,使用了嘌呤霉素-tRNA偶联物,其中3'-末端A单元被嘌呤霉素替代。嘌呤霉素-tRNA偶联物通过核糖体中的嘌呤霉素部分与链霉亲和素的C末端融合。收集抗生蛋白链菌素-嘌呤霉素-tRNA融合分子,并在扩增tRNA序列后将其带入下一轮。我们应用这个系统从一个tRNA库中选择了一个有效的移码抑制tRNA,带有一个随机突变的来自酵母菌的反密码子环。经过三轮选择,我们获得了新型的移码抑制器tRNA,它们具有高解码活性和对内源性氨酰基-tRNA合成酶的良好正交性。这些结果表明,此处开发的体外选择系统可用于从tRNA文库获得用于掺入非天然氨基酸的高活性tRNA。

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