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在 L 型细菌中对定制合成噬菌体基因组进行跨属重编程。

Cross-genus rebooting of custom-made, synthetic bacteriophage genomes in L-form bacteria.

机构信息

Institute of Food, Nutrition, and Health, Eidgenoessische Technische Hochschule Zurich, 8092 Zurich, Switzerland

Institute of Food, Nutrition, and Health, Eidgenoessische Technische Hochschule Zurich, 8092 Zurich, Switzerland.

出版信息

Proc Natl Acad Sci U S A. 2018 Jan 16;115(3):567-572. doi: 10.1073/pnas.1714658115. Epub 2018 Jan 3.

Abstract

Engineered bacteriophages provide powerful tools for biotechnology, diagnostics, pathogen control, and therapy. However, current techniques for phage editing are experimentally challenging and limited to few phages and host organisms. Viruses that target Gram-positive bacteria are particularly difficult to modify. Here, we present a platform technology that enables rapid, accurate, and selection-free construction of synthetic, tailor-made phages that infect Gram-positive bacteria. To this end, custom-designed, synthetic phage genomes were assembled in vitro from smaller DNA fragments. We show that replicating, cell wall-deficient L-form bacteria can reboot synthetic phage genomes upon transfection, i.e., produce virus particles from naked, synthetic DNA. Surprisingly, L-form cells not only support rebooting of native and synthetic phage genomes but also enable cross-genus reactivation of and phages from their DNA, thereby broadening the approach to phages that infect other important Gram-positive pathogens. We then used this platform to generate virulent phages by targeted modification of temperate phage genomes and demonstrated their superior killing efficacy. These synthetic, virulent phages were further armed by incorporation of enzybiotics into their genomes as a genetic payload, which allowed targeting of phage-resistant bystander cells. In conclusion, this straightforward and robust synthetic biology approach redefines the possibilities for the development of improved and completely new phage applications, including phage therapy.

摘要

工程噬菌体为生物技术、诊断、病原体控制和治疗提供了强大的工具。然而,目前的噬菌体编辑技术在实验上具有挑战性,并且仅限于少数噬菌体和宿主生物。靶向革兰氏阳性细菌的病毒尤其难以修饰。在这里,我们提出了一种平台技术,能够快速、准确、无需选择地构建感染革兰氏阳性细菌的合成、定制噬菌体。为此,我们在体外从小的 DNA 片段组装定制设计的、合成的噬菌体基因组。我们表明,复制、细胞壁缺陷的 L 型细菌可以在转染后重新启动合成噬菌体基因组,即用裸露的合成 DNA 产生病毒颗粒。令人惊讶的是,L 型细胞不仅支持天然和合成噬菌体基因组的重新启动,而且还能够使和噬菌体从其 DNA 中进行跨属复活,从而将该方法扩展到感染其他重要革兰氏阳性病原体的噬菌体。然后,我们使用该平台通过靶向修饰温和噬菌体基因组来生成毒性噬菌体,并证明了它们优越的杀伤效力。这些合成的、毒性噬菌体进一步通过将酶制剂整合到其基因组中作为遗传有效载荷来武装,这允许针对噬菌体抗性旁观者细胞进行靶向。总之,这种简单而强大的合成生物学方法重新定义了开发改良和全新噬菌体应用的可能性,包括噬菌体治疗。

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本文引用的文献

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Engineering of Bacteriophage T4 Genome Using CRISPR-Cas9.利用CRISPR-Cas9对噬菌体T4基因组进行工程改造
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Adapting Drug Approval Pathways for Bacteriophage-Based Therapeutics.调整基于噬菌体的治疗药物的审批途径。
Front Microbiol. 2016 Aug 3;7:1209. doi: 10.3389/fmicb.2016.01209. eCollection 2016.
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Genetically Engineered Phages: a Review of Advances over the Last Decade.基因工程噬菌体:过去十年进展综述
Microbiol Mol Biol Rev. 2016 Jun 1;80(3):523-43. doi: 10.1128/MMBR.00069-15. Print 2016 Sep.
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Revisiting phage therapy: new applications for old resources.重新审视噬菌体疗法:旧资源的新应用。
Trends Microbiol. 2015 Apr;23(4):185-91. doi: 10.1016/j.tim.2015.01.006. Epub 2015 Feb 21.

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