Chen Tsan-Chi, Chen Guang-Wu, Hsiung Chao Agnes, Yang Jyh-Yuan, Shih Shin-Ru, Lai Yiu-Kay, Juang Jyh-Lyh
Division of Molecular and Genomic Medicine, National Health Research Institutes, Zhunan, Miaoli 350, Taiwan.
J Clin Microbiol. 2006 Jun;44(6):2212-9. doi: 10.1128/JCM.02393-05.
Cluster A enteroviruses, including enterovirus 71 (EV71) and coxsackievirus A16 (CA16), are known to cause hand-foot-and-mouth disease (HFMD). Despite the close genetic relationship between these two viruses, EV71 is generally known to be a more perpetuating pathogen involved in severe clinical manifestations and deaths. While the serotyping of enteroviruses is mostly done by conventional immunological methods, many clinical isolates remain unclassifiable due to the limited number of antibodies against enterovirus surface proteins. Array-based assays are able to detect several serotypes with high accuracy. We combined an enterovirus microarray with multiplex reverse transcription-PCR to try to develop a method of sensitively and accurately detecting and differentiating EV71 and CA16. In an effort to design serotype-specific probes for detection of the virus, we first did an elaborate bioinformatic analysis of the sequence database derived from different enterovirus serotypes. We then constructed a microarray using 60-mer degenerate oligonucleotide probes covalently bound to array slides. Using this enterovirus microarray to study 144 clinical specimens from patients infected with HFMD or suspected to have HFMD, we found that it had a diagnostic accuracy of 92.0% for EV71 and 95.8% for CA16. Diagnostic accuracy for other enteroviruses (non-EV71 or -CA16) was 92.0%. All specimens were analyzed in parallel by real-time PCR and subsequently confirmed by neutralization tests. This highly sensitive array-based assay may become a useful alternative in clinical diagnostics of EV71 and CA16.
A组肠道病毒,包括肠道病毒71型(EV71)和柯萨奇病毒A16型(CA16),已知可引起手足口病(HFMD)。尽管这两种病毒在基因上关系密切,但一般认为EV71是一种更具持续性的病原体,可导致严重的临床表现和死亡。虽然肠道病毒的血清分型大多通过传统免疫方法进行,但由于针对肠道病毒表面蛋白的抗体数量有限,许多临床分离株仍无法分类。基于芯片的检测方法能够高精度地检测多种血清型。我们将肠道病毒微阵列与多重逆转录PCR相结合,试图开发一种灵敏、准确地检测和区分EV71和CA16的方法。为了设计用于检测病毒的血清型特异性探针,我们首先对来自不同肠道病毒血清型的序列数据库进行了详细的生物信息学分析。然后,我们构建了一个微阵列,使用与芯片载玻片共价结合的60聚体简并寡核苷酸探针。使用这种肠道病毒微阵列研究了144例手足口病感染患者或疑似患者的临床标本,我们发现它对EV71的诊断准确率为92.0%,对CA16的诊断准确率为95.8%。对其他肠道病毒(非EV71或CA16)的诊断准确率为92.0%。所有标本均通过实时PCR进行平行分析,并随后通过中和试验进行确认。这种基于芯片的高灵敏度检测方法可能成为EV71和CA16临床诊断中一种有用的替代方法。