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首页> 外文期刊>BMC Microbiology >In vivo bioluminescence imaging of the spatial and temporal colonization of lactobacillus plantarum 423 and enterococcus mundtii ST4SA in the intestinal tract of mice
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In vivo bioluminescence imaging of the spatial and temporal colonization of lactobacillus plantarum 423 and enterococcus mundtii ST4SA in the intestinal tract of mice

机译:体内乳酸菌植物乳杆菌423和蒙氏肠球菌ST4SA在小鼠肠道中的时空定植

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摘要

Lactic acid bacteria (LAB) are major inhabitants and part of the normal microflora of the gastrointestinal tract (GIT) of humans and animals. Despite substantial evidence supporting the beneficial properties of LAB, only a few studies have addressed the migration and colonization of probiotic bacteria in the GIT. The reason for this is mostly due to the limitations, or lack of, efficient reporter systems. Here we describe the development and application of a non-invasive in vivo bioluminescence reporter system to study, in real-time, the spatial and temporal persistence of Lactobacillus plantarum 423 and Enterococcus mundtii ST4SA in the intestinal tract of mice. This study reports on the application of the firefly luciferase gene (ffluc) from Photinus pyralis to develop luciferase-expressing L. plantarum 423 and E. mundtii ST4SA, using a Lactococcus lactis NICE system on a high copy number plasmid (pNZ8048) and strong constitutive lactate dehydrogenase gene promoters (Pldh and STldh). The reporter system was used for in vivo and ex vivo monitoring of both probiotic LAB strains in the GIT of mice after single and multiple oral administrations. Enterococcus mundtii ST4SA reached the large intestine 45 min after gavage, while L. plantarum 423 reached the cecum/colon after 90 min. Both strains predominantly colonized the cecum and colon after five consecutive daily administrations. Enterococcus mundtii ST4SA persisted in faeces at higher numbers and for more days compared to L. plantarum 423. Our findings demonstrate the efficiency of a high-copy number vector, constitutive promoters and bioluminescence imaging to study the colonization and persistence of L. plantarum 423 and E. mundtii ST4SA in the murine GIT. The system allowed us to differentiate between intestinal transit times of the two strains in the digestive tract. This is the first report of bioluminescence imaging of a luciferase-expressing E. mundtii strain to study colonization dynamics in the murine model. The bioluminescence system developed in this study may be used to study the in vivo colonization dynamics of other probiotic LAB.
机译:乳酸菌(LAB)是主要的居民,是人类和动物胃肠道(GIT)正常菌群的一部分。尽管有大量证据支持LAB的有益特性,但仅有少数研究解决了益生菌在GIT中的迁移和定植。其原因主要是由于有效的报告程序系统的局限性或缺乏。在这里,我们描述了一种无创的体内生物发光报告系统的开发和应用,以实时研究小鼠肠道中的植物乳杆菌423和芒氏肠球菌ST4SA的时空持久性。这项研究报道了利用Pactinus pyralis的萤火虫萤光素酶基因(ffluc)在高拷贝数质粒(pNZ8048)和高组成型上使用乳酸乳球菌NICE系统开发表达萤光素酶的植物乳杆菌423和芒氏大肠杆菌ST4SA。乳酸脱氢酶基因启动子(Pldh和STldh)。在单次和多次口服给药后,将报道系统用于小鼠GIT中益生菌LAB菌株的体内和离体监测。芒氏肠球菌ST4SA在管饲后45分钟到达大肠,而植物乳杆菌423在90分钟后到达盲肠/结肠。连续五次每日给药后,两种菌株都主要在盲肠和结肠中定殖。与植物乳杆菌423相比,芒球菌ST4SA在粪便中的数量更高且持续时间更长。我们的发现表明,高拷贝数载体,组成型启动子和生物发光成像技术能够有效地研究植物乳杆菌423和200的定殖和持久性。鼠GIT中的E. mundtii ST4SA。该系统使我们能够区分两种菌株在消化道中的肠道运输时间。这是表达萤光素酶的芒氏大肠杆菌菌株进行生物发光成像以研究鼠模型中定植动力学的第一份报告。本研究开发的生物发光系统可用于研究其他益生菌LAB的体内定植动力学。

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