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建立一种实时 PCR 方法用于乙型副伤寒沙门菌 Java 变种的血清分型。

Development of a real-time PCR method for the genoserotyping of Salmonella Paratyphi B variant Java.

机构信息

Sciensano, Infectious Diseases in Humans, Bacterial Diseases, Rue Engeland 642, 1180, Brussels, Belgium.

Department of Information Technology, IDLab, imec, Ghent University, 9052, Ghent, Belgium.

出版信息

Appl Microbiol Biotechnol. 2019 Jun;103(12):4987-4996. doi: 10.1007/s00253-019-09854-4. Epub 2019 May 6.

Abstract

Discriminating between D-tartrate fermenting and non-fermenting strains of Salmonella enterica subsp. enterica serotype Paratyphi B is of major importance as these two variants have different pathogenic profiles. While D-tartrate non-fermenting S. Paratyphi B isolates are the causative agent of typhoid-like fever, D-tartrate fermenting isolates (also called variant Java) of the same serotype trigger the less dangerous gastroenteritis. The determination of S. Paratyphi B variants requires a time-consuming process and complex biochemical tests. Therefore, a quadruplex real-time PCR method, based on the allelic discrimination of molecular markers selected from the scientific literature and from whole genome sequencing data produced in-house, was developed in this study, to be applied to Salmonella isolates. This method was validated with the analysis of 178 S. Paratyphi B (D-tartrate fermenting and non-fermenting) and other serotypes reaching an accuracy, compared with the classical methods, of 98% for serotyping by slide agglutination and 100% for replacement of the biochemical test. The developed real-time PCR permits to save time and to obtain an accurate identification of a S. Paratyphi B serotype and its D-tartrate fermenting profile, which is needed in routine laboratories for fast and efficient diagnostics.

摘要

区分肠炎沙门氏菌亚种肠炎血清型副伤寒 B 的 D-酒石酸盐发酵和非发酵菌株非常重要,因为这两种变体具有不同的致病谱。虽然 D-酒石酸盐非发酵 S. Paratyphi B 分离株是伤寒样发热的病原体,但同一血清型的 D-酒石酸盐发酵分离株(也称为变体 Java)引发的是危险性较低的肠胃炎。副伤寒 B 变体的确定需要一个耗时的过程和复杂的生化测试。因此,本研究开发了一种基于从文献中选择的分子标记的等位基因区分的四重实时 PCR 方法,并结合内部产生的全基因组测序数据,应用于沙门氏菌分离株。该方法通过分析 178 株副伤寒 B(D-酒石酸盐发酵和非发酵)和其他血清型进行了验证,与经典方法相比,玻片凝集血清分型的准确性为 98%,生化试验替代的准确性为 100%。开发的实时 PCR 可节省时间,并对副伤寒 B 血清型及其 D-酒石酸盐发酵谱进行准确鉴定,这是常规实验室快速高效诊断所必需的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6ffe/6536469/29618badb223/253_2019_9854_Fig1_HTML.jpg

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