首页> 外文期刊>Diagnostic microbiology and infectious disease >Detection of human enterovirus and human parechovirus (HPeV) genotypes from clinical stool samples: polymerase chain reaction and direct molecular typing, culture characteristics, and serotyping.
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Detection of human enterovirus and human parechovirus (HPeV) genotypes from clinical stool samples: polymerase chain reaction and direct molecular typing, culture characteristics, and serotyping.

机译:从临床粪便样本中检测人类肠道病毒和人类副病毒(HPeV)基因型:聚合酶链反应和直接分子分型,培养特性和血清分型。

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摘要

Molecular (polymerase chain reaction [PCR]) methods are increasingly used to detect and type human enteroviruses (HEVs) and parechoviruses (HPeV). Here, we assessed their value in comparison to virus culture and serotyping for detection and typing of HEV and HPeV in stool samples from hospitalized patients. By use of real-time PCR, 221/1174 patients (18.8%) were found positive for HEV/HPeV. By cell culture, a virus could be isolated from 107 of the HEV/HPeV PCR-positive samples. Culture efficiency was correlated to the Ct value, (geno)type, and cell lines used. Of the HEV/HPeV PCR-positive samples, 47% could be genotyped by VP1 genotyping and 25% by serotyping. In conclusion, PCR detection of HEV/HPeV from stool is more sensitive than virus culture, particularly for coxsackieviruses A and HPeVs. However, the genotyping method used here could identify only 47% of the HEV/HPeV strains. Further optimization and validation of direct genotyping are needed, and clinical relevance of HEV/HPeV detection in stool needs to be determined.
机译:分子(聚合酶链反应[PCR])方法越来越多地用于检测和鉴定人类肠道病毒(HEV)和副病毒(HPeV)。在这里,我们评估了它们与病毒培养和血清分型相比的价值,用于检测住院患者粪便样本中的HEV和HPeV并进行分型。通过实时PCR,发现221/1174名患者(18.8%)的HEV / HPeV阳性。通过细胞培养,可以从107份HEV / HPeV PCR阳性样品中分离出病毒。培养效率与Ct值,(基因)类型和所用细胞系相关。在HEV / HPeV PCR阳性样本中,可以通过VP1基因分型进行基因分型,而通过血清分型可以进行25%的分型。总之,粪便中HEV / HPeV的PCR检测比病毒培养更敏感,尤其是对于柯萨奇病毒A和HPeV。但是,此处使用的基因分型方法只能识别47%的HEV / HPeV菌株。需要进一步的优化和直接基因分型的验证,并且需要确定粪便中HEV / HPeV检测的临床相关性。

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