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De novo design and synthesis of a 30-cistron translation-factor module

机译:De Novo设计和合成30 Cistron Transport系数模块

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摘要

Two of the many goals of synthetic biology are synthesizing large biochemical systems and simplifying their assembly. While several genes have been assembled together by modular idempotent cloning, it is unclear if such simplified strategies scale to very large constructs for expression and purification of whole pathways. Here we synthesize from oligodeoxyribonucleotides a completely de-novo-designed, 58-kb multigene DNA. This BioBrick plasmid insert encodes 30 of the 31 translation factors of the PURE translation system, each His-tagged and in separate transcription cistrons. Dividing the insert between three high-copy expression plasmids enables the bulk purification of the aminoacyl-tRNA synthetases and translation factors necessary for affordable, scalable reconstitution of an in vitro transcription and translation system, PURE 3.0.
机译:合成生物学的两个目标中的两个是合成大型生化系统并简化其组装。 虽然通过模块化幂克隆已经组装了几种基因,但如果这种简化的策略规模尚不清楚,以表达和纯化整个途径的非常大的构建体。 在这里,我们从寡脱氧氧核糖核苷酸合成完全脱诺夫设计的58kb多烯DNA。 这种Biobrick质粒插入纯翻译系统的平移因子中的30个,每个他标记的和单独的转录等级。 将插入划分在三种高拷贝表达质粒之间,使氨基酰基-TRNA合成酶的体积纯化能够实惠,可扩展的体外转录和翻译系统所需的翻译因子,纯3.0。

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  • 来源
    《Nucleic Acids Research》 |2017年第18期|共11页
  • 作者单位

    Uppsala Univ Dept Cell &

    Mol Biol S-75136 Uppsala Sweden;

    Vanderbilt Univ Med Ctr Dept Pharmacol Nashville TN 37232 USA;

    Uppsala Univ Dept Cell &

    Mol Biol S-75136 Uppsala Sweden;

    Uppsala Univ Dept Cell &

    Mol Biol S-75136 Uppsala Sweden;

    Uppsala Univ Dept Cell &

    Mol Biol S-75136 Uppsala Sweden;

    Uppsala Univ Dept Phys &

    Analyt Chem S-75123 Uppsala Sweden;

    Uppsala Univ Dept Phys &

    Analyt Chem S-75123 Uppsala Sweden;

    East China Normal Univ Inst Biol &

    Informat Sci Sch Comp Sci &

    Software Engn Sch Life Sci Shanghai 200062 Peoples R China;

    Uppsala Univ Dept Cell &

    Mol Biol S-75136 Uppsala Sweden;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物化学;
  • 关键词

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