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Evaluation of a protocol for molecular broad-range diagnosis of culture-negative bacterial infections in clinical routine diagnosis

机译:在临床常规诊断中评估培养阴性细菌感染的分子广谱诊断方案的评估

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摘要

Aim: Introduction of a protocol for broad-range diagnosis of bacterial infections, which remain negative in culture. Methods and Results: The new TaqMan real-time PCR assay amplifies part of the 16S rRNA gene. Species are identified by subsequent sequencing and phylogenetic blast analysis. The analytical sensitivity showed to be 50 fg DNA per PCR. The lowest detectable bacterial cell concentration in blood was 1000 CFU per 200 mu l EDTA-blood. The utility in clinical routine diagnosis was evaluated by testing 136 clinical specimens. Bacterial pathogens were detected in 33 samples (24.3%) either by culture or molecular diagnosis. In 10 culture negative cases, pathogens such as Mycoplasma timone/orale, Ureaplasma parvum/urealyticum, Treponema pallidum, different streptococci and staphylococci were identified by molecular diagnosis only. Conclusions: The introduced broad-range real-time PCR protocol showed to be useful in the clinical routine in cases where bacterial infection was highly anticipated but culture remained negative. However, the obtained data have to be always interpreted with caution and in conjunction with the clinical data, crossing-point values and with the Blast result of both the sample and the controls. Significance and Impact of the Study: This work introduces a new and well-evaluated broad-range real-time PCR protocol for diagnosis of bacterial infections.
机译:目的:介绍一种对细菌感染进行广泛诊断的方案,在培养中仍为阴性。方法和结果:新的TaqMan实时PCR检测扩增了16S rRNA基因的一部分。通过随后的测序和系统发育胚分析来鉴定物种。每次PCR分析灵敏度为50 fg DNA。血液中可检测到的最低细菌细胞浓度是每200 ul EDTA血液1000 CFU。通过测试136个临床标本,评估了在临床常规诊断中的效用。通过培养或分子诊断,在33个样品(24.3%)中检测到细菌病原体。在10例培养阴性的病例中,仅通过分子诊断就可以鉴定出病原体,如:支原体/口头支原体,小支气管炎/解脲支原体,梅毒螺旋体,不同链球菌和葡萄球菌。结论:在高度期望细菌感染但培养阴性的情况下,引入的宽范围实时PCR方案在临床常规中显示出有用的效果。但是,获得的数据必须始终谨慎地解释,并与临床数据,交叉点值以及样品和对照的Blast结果结合使用。研究的意义和影响:这项工作介绍了一种新的且经过充分评估的广范围实时PCR方案,用于诊断细菌感染。

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