Department of Pharmacy and Biotechnology.
J Clin Microbiol. 2013 Nov;51(11):3753-9. doi: 10.1128/JCM.01970-13. Epub 2013 Sep 4.
Three genotypes have been identified within the parvovirus B19 species (B19V), and such genetic diversity may have significant implications for the development of molecular detection assays. In the present study, B19V genetic variability has been examined on a subset of genomic sequences available in the NCBI nucleotide database, and a quantitative PCR (qPCR) assay able to detect, differentiate, and quantify all viral variants has been established. The designed primers and probes have been used for the development of alternative detection formats, based on a combined use of intercalating dye and genotype-specific hydrolysis probes. The qPCR assay analytical performances have been determined on the 1st WHO International Reference Panel for Parvovirus B19 Genotypes. The developed qPCR protocols allow for the detection of genotypes 1 to 3 with equal accuracy, and with a limit of detection (LOD) of 200 IU/ml. A comparison of routine performance was carried out with respect to a previously established assay specifically validated on B19V genotype 1. For 130 clinical samples analyzed, 126 showed concordant results (31 positive and 97 negative), while 4 showed discordant results. Overall, the genotype-specific qPCR assay showed a sensitivity of 93.94% and a specificity of 97.94%, with an agreement rate of 96.92%. The proposed qPCR assay and the alternative protocols developed, each with robust performance, may allow choice with respect to operational systems and diagnostic requirements and might contribute to provide a more reliable diagnostic service and epidemiological surveillance of B19 virus.
已在细小病毒 B19 种内鉴定出 3 种基因型(B19V),这种遗传多样性可能对分子检测方法的发展具有重要意义。本研究在 NCBI 核苷酸数据库中可用的基因组序列子集中检查了 B19V 的遗传变异性,并建立了能够检测、区分和定量所有病毒变体的定量 PCR(qPCR)检测方法。设计的引物和探针已用于开发替代检测格式,其基于使用嵌入染料和基因型特异性水解探针的组合。qPCR 检测方法的分析性能已在第 1 个世界卫生组织细小病毒 B19 基因型国际参考小组上确定。开发的 qPCR 方案可平等准确地检测基因型 1 至 3,其检测限(LOD)为 200 IU/ml。与专门针对 B19V 基因型 1 进行验证的先前建立的检测方法进行了常规性能比较。对于分析的 130 个临床样本,126 个显示出一致的结果(31 个阳性和 97 个阴性),而 4 个显示出不一致的结果。总体而言,基因型特异性 qPCR 检测方法的灵敏度为 93.94%,特异性为 97.94%,一致性率为 96.92%。所提出的 qPCR 检测方法和开发的替代方案均具有稳健的性能,可能允许根据操作系统和诊断要求进行选择,并有助于提供更可靠的诊断服务和 B19 病毒的流行病学监测。