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Molecular Programming with a Transcription and Translation Cell-Free Toolbox: From Elementary Gene Circuits to Phage Synthesis.

机译:使用转录和翻译无细胞工具箱进行分子编程:从基本基因电路到噬菌体合成。

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摘要

Cell-free synthetic/systems biology is an emerging field connecting biology, chemistry, physics, and engineering to understand biological systems and expand their capabilities. In vitro approaches compared to in vivo allow much better control of parameters and give much more freedom to program and study biological systems. Among the in vitro approaches, a transcription and translation (TX-TL) cell-free gene expression system mimicking a natural biological system offers the closest context to an intact cell. The conventional cell-free system as a playground to perform an experiment, however, has a couple of serious problems such as an insufficient sink system and the lack of transcriptional diversity. In this dissertation, I report the preparation of a custom-made E. coli cell-free system for the purpose of quantitative synthetic/systems biology, demonstrate synthetic gene circuits with cell-free toolbox, and show cell-free synthesis of a functional entity from genome-sized DNA. The custom-made cell-free system expresses genes with only endogenous TX-TL machinery and the sink systems for two biomolecules, mRNA and protein, can be applied in it. Moreover, mathematical models of gene expression including sink systems in this cell-free system are described. As a concept of cell-free toolbox, this cell-free system also makes it possible to use a variety of transcriptional activation and repression units to construct elementary circuit motifs. Furthermore, a bacteriophage as complex as T7 phage is synthesized from its genome-sized DNA with this cell-free system. This cell-free synthesis in a single test tube includes the central dogma of molecular biology including transcription, translation, and DNA replication as an internal process, and self-assembly and DNA packaging as a post-gene-expression process.
机译:无细胞合成/系统生物学是连接生物学,化学,物理学和工程学的新兴领域,以了解生物系统并扩展其功能。与体内方法相比,体外方法可以更好地控制参数,并为编程和研究生物系统提供更大的自由度。在体外方法中,模仿天然生物系统的无转录和翻译(TX-TL)无细胞基因表达系统提供了与完整细胞最接近的环境。然而,传统的无细胞系统作为进行实验的游乐场,存在一些严重的问题,例如接收器系统不足和转录多样性不足。在这篇论文中,我报告了为定量合成/系统生物学目的而定制的大肠杆菌无细胞系统的制备,展示了具有无细胞工具箱的合成基因电路,并展示了功能实体的无细胞合成来自基因组大小的DNA。定制的无细胞系统仅使用内源TX-TL机器表达基因,并且可以应用两个生物分子(mRNA和蛋白质)的宿系统。此外,描述了该无细胞系统中基因表达的数学模型,包括宿系统。作为无细胞工具箱的概念,这种无细胞系统还可以使用各种转录激活和抑制单位来构建基本的电路基序。此外,利用该无细胞系统,从其基因组大小的DNA合成了与T7噬菌体一样复杂的噬菌体。在单个试管中进行的这种无细胞合成包括分子生物学的核心教条,包括转录,翻译和DNA复制(作为内部过程)以及自组装和DNA包装(作为后基因表达过程)。

著录项

  • 作者

    Shin, Jonghyeon G.Y.N.;

  • 作者单位

    University of Minnesota.;

  • 授予单位 University of Minnesota.;
  • 学科 Biophysics General.;Biology Molecular.;Chemistry Biochemistry.
  • 学位 Ph.D.
  • 年度 2012
  • 页码 117 p.
  • 总页数 117
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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