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在粪肠球菌中开发用于基因整合和表达的基因组位点。

Development of a genomic site for gene integration and expression in Enterococcus faecalis.

机构信息

Department of Microbiology and Molecular Genetics, The University of Texas Health Science Center at Houston, TX, USA.

出版信息

J Microbiol Methods. 2012 Jul;90(1):1-8. doi: 10.1016/j.mimet.2012.04.011. Epub 2012 Apr 18.

Abstract

Enterococcus faecalis, a gram-positive opportunistic pathogen, has become one of the leading causes of nosocomial infections. Normally a resident of the gastrointestinal tract, extensive use of antibiotics has resulted in the rise of E. faecalis strains that are resistant to multiple antibiotics. This, compounded with the ability to easily exchange antibiotic determinants with other bacteria, has made certain E. faecalis infections difficult to treat medically. The genetic toolbox for the study of E. faecalis has expanded greatly in recent years, but has lacked methodology to stably introduce a gene in single copy in a non-disruptive manner for complementation or expression of non-native genes. In this study, we identified a specific site in the genome of E. faecalis OG1RF that can serve as an expression site for a gene of interest. This site is well conserved in most of the sequenced E. faecalis genomes. A vector has also been developed to integrate genes into this site by allelic exchange. Using this system, we complemented an in-frame deletion in eutV, demonstrating that the mutation does not cause polar effects. We also generated an E. faecalis OG1RF strain that stably expresses the green fluorescent protein and is comparable to the parent strain in terms of in vitro growth and pathogenicity in C. elegans and mice. Another major advantage of this new methodology is the ability to express integrated genes without the need for maintaining antibiotic selection, making this an ideal tool for functional studies of genes in infection models and co-culture systems.

摘要

粪肠球菌是一种革兰氏阳性机会致病菌,已成为医院感染的主要原因之一。正常情况下,粪肠球菌是肠道的常驻菌,但由于广泛使用抗生素,导致对多种抗生素具有耐药性的粪肠球菌菌株大量出现。此外,粪肠球菌还具有与其他细菌轻易交换抗生素决定因子的能力,这使得某些粪肠球菌感染难以通过医学手段进行治疗。近年来,粪肠球菌的遗传工具包有了很大的扩展,但缺乏一种方法,以非破坏性的方式稳定地将单个基因引入非干扰方式,以进行互补或表达非天然基因。在这项研究中,我们在粪肠球菌 OG1RF 的基因组中确定了一个特定的位点,该位点可作为感兴趣基因的表达位点。该位点在大多数测序的粪肠球菌基因组中都得到很好的保守。我们还开发了一种载体,通过等位基因交换将基因整合到该位点。使用该系统,我们对 eutV 的无义突变进行了互补,证明该突变不会导致极性效应。我们还生成了一株稳定表达绿色荧光蛋白的粪肠球菌 OG1RF 菌株,该菌株在体外生长和在秀丽隐杆线虫和小鼠中的致病性方面与亲本菌株相当。这种新方法的另一个主要优点是能够表达整合的基因,而无需维持抗生素选择,这使其成为感染模型和共培养系统中基因功能研究的理想工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d51f/3358487/22ec95a7e13e/nihms371320f1.jpg

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