利用 Cas9 靶向和红色重组技术设计噬菌体工程。

IF 4.3 3区 材料科学 Q1 ENGINEERING, ELECTRICAL & ELECTRONIC ACS Applied Electronic Materials Pub Date : 2024-01-01 Epub Date: 2024-02-01 DOI:10.1007/s12275-024-00107-2
Shin-Yae Choi, Danitza Xiomara Romero-Calle, Han-Gyu Cho, Hee-Won Bae, You-Hee Cho
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引用次数: 0

摘要

噬菌体(噬菌体)是天然抗生素和生物纳米粒子,近年来合成生物学工具的进步极大地促进了它们的应用。设计者噬菌体是通过基因组工程创造出的合成噬菌体,可以增加天然噬菌体的优点或减少其缺点。在这里,我们报告了一种直接的基因组工程方法的开发情况,这种方法可以在一种模式细菌病原体--铜绿假单胞菌--中有效地获得工程噬菌体。这是通过消除基于化脓性链球菌 Cas9(SpCas9)的野生型噬菌体,并促进基于大肠杆菌λ(λRed)红色重组系统的重组生成来实现的。通过基于 miniTn7 的染色体整合 SpCas9 基因和诱导启动子下的λRed 基因,产生了铜绿微囊藻菌株 PAO1 的生产者(PD)细胞。为了验证重组产生的效率,我们从温带噬菌体 MP29 中产生了荧光噬菌体。我们通过电穿孔将带有选择性靶向野生型 gp35 基因的单导 RNA(sgRNA)基因的质粒和用超级文件夹绿色荧光蛋白(sfGFP)标记 Gp35 的编辑模板导入 PD 细胞。我们发现,靶向效率受 sgRNA 位置和数量的影响。荧光噬菌体颗粒能从表达双 sgRNA 分子的 PD 细胞培养物中有效回收。该方案可用于在铜绿假单胞菌中制造设计噬菌体,既可用于应用,也可用于研究。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Use of Cas9 Targeting and Red Recombination for Designer Phage Engineering.

Bacteriophages (phages) are natural antibiotics and biological nanoparticles, whose application is significantly boosted by recent advances of synthetic biology tools. Designer phages are synthetic phages created by genome engineering in a way to increase the benefits or decrease the drawbacks of natural phages. Here we report the development of a straightforward genome engineering method to efficiently obtain engineered phages in a model bacterial pathogen, Pseudomonas aeruginosa. This was achieved by eliminating the wild type phages based on the Streptococcus pyogenes Cas9 (SpCas9) and facilitating the recombinant generation based on the Red recombination system of the coliphage λ (λRed). The producer (PD) cells of P. aeruginosa strain PAO1 was created by miniTn7-based chromosomal integration of the genes for SpCas9 and λRed under an inducible promoter. To validate the efficiency of the recombinant generation, we created the fluorescent phages from a temperate phage MP29. A plasmid bearing the single guide RNA (sgRNA) gene for selectively targeting the wild type gp35 gene and the editing template for tagging the Gp35 with superfolder green fluorescent protein (sfGFP) was introduced into the PD cells by electroporation. We found that the targeting efficiency was affected by the position and number of sgRNA. The fluorescent phage particles were efficiently recovered from the culture of the PD cells expressing dual sgRNA molecules. This protocol can be used to create designer phages in P. aeruginosa for both application and research purposes.

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CiteScore
7.20
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4.30%
发文量
567
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