变异克雷伯氏菌中基于 CRISPR-Cas 的原生可编程多重基因抑制

IF 2 4区 生物学 Q3 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Zhifeng Mo, Siying Lin, Ting Li, Guohui Yu, Yunhao Sun, Jianuan Zhou, Zeling Xu
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引用次数: 0

摘要

变异克雷伯氏菌是一种革兰氏阴性细菌,经常从各种自然环境中分离出来。它是一种无处不在的机会性病原体,可引起植物、动物和人类的各种感染。它还具有巨大的生物技术潜力。然而,由于缺乏有效的遗传工具,人们对 K. variicola 的致病机理和有益活动的分子基础仍然知之甚少。在本研究中,我们发现并鉴定了最近分离出的 K. variicola 菌株 KV-1 中的原生 I-E 型 CRISPR-Cas 系统。由于转座元件使Cas3核酸酶失活,该系统不能切割目标DNA序列,但保留了crRNA引导的Cascade与目标DNA序列结合的活性。我们设计了一种携带微型CRISPR以编码crRNA的靶向质粒,并将其导入到KV-1菌株中,成功地将原生的I-E型CRISPR-Cas系统重新利用,从而高效、特异地抑制了靶基因的表达。此外,通过创建一个迷你 CRISPR 来编码多个 crRNA,只需提供一个靶向质粒就能实现多重基因抑制。这项工作提供了第一个基于CRISPR-Cas的可编程多重基因抑制K. variicola的原生工具,这将有助于研究K. variicola的致病机制,并通过代谢工程生产有价值的生物产品。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Native CRISPR-Cas-based programmable multiplex gene repression in Klebsiella variicola

Native CRISPR-Cas-based programmable multiplex gene repression in Klebsiella variicola

Klebsiella variicola is a Gram-negative bacterium that is frequently isolated from a wide variety of natural niches. It is a ubiquitous opportunistic pathogen that can cause diverse infections in plants, animals, and humans. It also has significant biotechnological potential. However, due to the lack of efficient genetic tools, the molecular basis contributing to the pathogenesis and beneficial activities of K. variicola remains poorly understood. In this study, we found and characterized a native type I-E CRISPR-Cas system in a recently isolated K. variicola strain KV-1. The system cannot cleave target DNA sequences due to the inactivation of the Cas3 nuclease by a transposable element but retains the activity of the crRNA-guided Cascade binding to the target DNA sequence. A targeting plasmid carrying a mini-CRISPR to encode a crRNA was designed and introduced into the KV-1 strain, which successfully repurposed the native type I-E CRISPR-Cas system to inhibit the expression of the target gene efficiently and specifically. Moreover, by creating a mini-CRISPR to encode multiple crRNAs, multiplex gene repression was achieved by providing a single targeting plasmid. This work provides the first native CRISPR-Cas-based tool for programmable multiplex gene repression in K. variicola, which will facilitate studying the pathogenic mechanism of K. variicola and enable metabolic engineering to produce valuable bioproducts.

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来源期刊
Biotechnology Letters
Biotechnology Letters 工程技术-生物工程与应用微生物
CiteScore
5.90
自引率
3.70%
发文量
108
审稿时长
1.2 months
期刊介绍: Biotechnology Letters is the world’s leading rapid-publication primary journal dedicated to biotechnology as a whole – that is to topics relating to actual or potential applications of biological reactions affected by microbial, plant or animal cells and biocatalysts derived from them. All relevant aspects of molecular biology, genetics and cell biochemistry, of process and reactor design, of pre- and post-treatment steps, and of manufacturing or service operations are therefore included. Contributions from industrial and academic laboratories are equally welcome. We also welcome contributions covering biotechnological aspects of regenerative medicine and biomaterials and also cancer biotechnology. Criteria for the acceptance of papers relate to our aim of publishing useful and informative results that will be of value to other workers in related fields. The emphasis is very much on novelty and immediacy in order to justify rapid publication of authors’ results. It should be noted, however, that we do not normally publish papers (but this is not absolute) that deal with unidentified consortia of microorganisms (e.g. as in activated sludge) as these results may not be easily reproducible in other laboratories. Papers describing the isolation and identification of microorganisms are not regarded as appropriate but such information can be appended as supporting information to a paper. Papers dealing with simple process development are usually considered to lack sufficient novelty or interest to warrant publication.
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