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打破限制壁垒并将CRISPRi作为一种基因沉默工具应用于…… (原文此处不完整)

Breaking the Restriction Barriers and Applying CRISPRi as a Gene Silencing Tool in .

作者信息

Ganguly Joyshree, Martin-Pascual Maria, Montiel González Diego, Bulut Alkan, Vermeulen Bram, Tjalma Ivo, Vidaki Athina, van Kranenburg Richard

机构信息

Corbion, 4206 AC Gorinchem, The Netherlands.

Laboratory of Microbiology, Wageningen University and Research, 6708 WE Wageningen, The Netherlands.

出版信息

Microorganisms. 2022 Mar 24;10(4):698. doi: 10.3390/microorganisms10040698.

Abstract

is a thermophilic bacterium capable of producing succinate from lignocellulosic-derived sugars and has the potential to be exploited as a platform organism. However, exploitation of has been limited partly due to the genetic inaccessibility and lack of genome engineering tools. In this study, we established the genetic accessibility for DSM 5809. By overcoming restriction barriers, transformation efficiencies of 10 CFU/µg plasmid DNA were achieved. To this end, the plasmid DNA was methylated in vivo when transformed into an engineered HST04 strain expressing three native methylation systems of the thermophile. This protocol was used to introduce a ThermodCas9-based CRISPRi tool targeting the gene encoding malic enzyme in , demonstrating the principle of gene silencing. This resulted in 75% downregulation of its expression and had an impact on the strain's fermentation profile. Although the details of the functioning of the restriction modification systems require further study, in vivo methylation can already be applied to improve transformation efficiency of Making use of the ThermodCas9-based CRISPRi, this is the first example demonstrating that genetic engineering in is feasible and establishing the way for metabolic engineering of this bacterium.

摘要

是一种能够从木质纤维素衍生糖中生产琥珀酸的嗜热细菌,有潜力被开发为一种平台生物。然而,对其的开发受到一定限制,部分原因是基因难以操作且缺乏基因组工程工具。在本研究中,我们建立了DSM 5809的基因可操作性。通过克服限制障碍,实现了10 CFU/μg质粒DNA的转化效率。为此,当将质粒DNA转化到表达嗜热菌三种天然甲基化系统的工程化HST04菌株中时,质粒DNA在体内被甲基化。该方案用于引入靶向编码苹果酸酶基因的基于ThermodCas9的CRISPRi工具,证明了基因沉默的原理。这导致其表达下调75%,并对菌株的发酵谱产生影响。尽管限制修饰系统的具体作用细节需要进一步研究,但体内甲基化已可用于提高的转化效率。利用基于ThermodCas9的CRISPRi,这是第一个证明在中进行基因工程是可行的例子,并为该细菌的代谢工程奠定了基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8430/9044749/17305f60afff/microorganisms-10-00698-g001.jpg

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