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基于大肠杆菌的无细胞表达系统中感染性噬菌体的合成。

Synthesis of Infectious Bacteriophages in an E. coli-based Cell-free Expression System.

作者信息

Rustad Mark, Eastlund Allen, Marshall Ryan, Jardine Paul, Noireaux Vincent

机构信息

School of Physics and Astronomy, University of Minnesota.

Department of Diagnostic and Biological Sciences and Institute for Molecular Virology, University of Minnesota.

出版信息

J Vis Exp. 2017 Aug 17(126):56144. doi: 10.3791/56144.

Abstract

A new generation of cell-free transcription-translation (TXTL) systems, engineered to have a greater versatility and modularity, provide novel capabilities to perform basic and applied sciences in test tube reactions. Over the past decade, cell-free TXTL has become a powerful technique for a broad range of novel multidisciplinary research areas related to quantitative and synthetic biology. The new TXTL platforms are particularly useful to construct and interrogate biochemical systems through the execution of synthetic or natural gene circuits. In vitro TXTL has proven convenient to rapidly prototype regulatory elements and biological networks as well as to recapitulate molecular self-assembly mechanisms found in living systems. In this article, we describe how infectious bacteriophages, such as MS2 (RNA), ΦΧ174 (ssDNA), and T7 (dsDNA), are entirely synthesized from their genome in one-pot reactions using an all Escherichia coli, cell-free TXTL system. Synthesis of the three coliphages is quantified using the plaque assay. We show how the yield of synthesized phage depends on the biochemical settings of the reactions. Molecular crowding, emulated through a controlled concentration of PEG 8000, affects the amount of synthesized phages by orders of magnitudes. We also describe how to amplify the phages and how to purify their genomes. The set of protocols and results presented in this work should be of interest to multidisciplinary researchers involved in cell-free synthetic biology and bioengineering.

摘要

新一代无细胞转录-翻译(TXTL)系统经过设计,具有更高的通用性和模块化,为在试管反应中开展基础科学和应用科学研究提供了新的能力。在过去十年中,无细胞TXTL已成为一种强大的技术,可用于广泛的与定量生物学和合成生物学相关的新型多学科研究领域。新的TXTL平台对于通过执行合成或天然基因回路来构建和研究生化系统特别有用。体外TXTL已被证明便于快速构建调控元件和生物网络的原型,以及重现活系统中发现的分子自组装机制。在本文中,我们描述了如何使用全大肠杆菌无细胞TXTL系统在一锅反应中从其基因组完全合成感染性噬菌体,如MS2(RNA)、ΦΧ174(单链DNA)和T7(双链DNA)。使用噬菌斑测定法定量三种大肠杆菌噬菌体的合成。我们展示了合成噬菌体的产量如何取决于反应的生化条件。通过控制聚乙二醇8000的浓度模拟的分子拥挤效应,会使合成噬菌体的数量发生几个数量级的变化。我们还描述了如何扩增噬菌体以及如何纯化其基因组。这项工作中展示的一系列实验方案和结果应该会引起参与无细胞合成生物学和生物工程的多学科研究人员的兴趣。

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