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一种用于木醋酸杆菌基因缺失的无痕框内敲除系统。

A clean in-frame knockout system for gene deletion in Acetobacterium woodii.

机构信息

Clostridia Research Group, BBSRC/EPSRC Synthetic Biology Research Centre (SBRC), School of Life Sciences, Biodiscovery Institute, The University of Nottingham, Nottingham NG7 2RD, UK.

The Novo Nordisk Foundation Center for Biosustainability, Technical University of Denmark, Kongens Lyngby, Denmark.

出版信息

J Biotechnol. 2022 Jul 20;353:9-18. doi: 10.1016/j.jbiotec.2022.05.013. Epub 2022 May 31.

Abstract

Acetogenic bacteria produce acetate following the fixation of CO via the Wood-Ljungdahl pathway. As such, they represent excellent process organisms for the production of novel chemicals and fuels from this waste greenhouse gas. Acetobacterium woodii is the model acetogen and numerous studies have been conducted investigating its biochemistry, gas consumption and use as a production chassis. However, there are a dearth of available tools for A. woodii gene modification which limits the research options available for genetic studies. Here, the previously proposed Clostridia Roadmap is implemented in A. woodii leading to the derivation of a knockout system for the generation of clean, in-frame deletions. The replicon of the Gram-positive plasmid pCD6 that originated in Clostridioides difficile was identified as being replication-defective in A. woodii, a property that was exploited to construct a pseudo-suicide knockout plasmid which was used to generate an auxotrophic, pyrE mutant. This allowed the subsequent use of a heterologous pyrE gene (from Clostridium acetobutylicum) as a counter selection marker and the deletion of a number of genes by allelic exchange. Specific mutants generated were affected in growth on glucose, fructose and ethanol as a consequence of deletion of fruA, pstG and adhE, respectively.

摘要

产乙酸菌通过 Wood-Ljungdahl 途径固定 CO 后生成乙酸。因此,它们是利用这种温室气体废物生产新型化学品和燃料的理想过程生物。伍德氏醋酸杆菌是模式产乙酸菌,已有大量研究对其进行了生物化学、气体消耗和作为生产底盘的研究。然而,可用于 A. woodii 基因修饰的工具却很少,这限制了遗传研究的可用研究选择。在这里,先前提出的梭菌路线图在 A. woodii 中实施,导致产生用于生成清洁、框内缺失的敲除系统。最初源自艰难梭菌的革兰氏阳性质粒 pCD6 的复制子被鉴定为在 A. woodii 中复制缺陷,这一特性被利用来构建假自杀敲除质粒,用于生成营养缺陷型 pyrE 突变体。这允许随后使用异源 pyrE 基因(来自丙酮丁醇梭菌)作为反向选择标记,并通过等位基因交换删除多个基因。由于 fruA、pstG 和 adhE 的缺失,分别生成的特定突变体在葡萄糖、果糖和乙醇上的生长受到影响。

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