Performance of a Taqman Assay for Improved Detection and Quantification of Human Rhinovirus Viral Load

نویسندگان

  • Kim Tien Ng
  • Jack Bee Chook
  • Xiang Yong Oong
  • Yoke Fun Chan
  • Kok Gan Chan
  • Nik Sherina Hanafi
  • Yong Kek Pang
  • Adeeba Kamarulzaman
  • Kok Keng Tee
چکیده

Human rhinovirus (HRV) is the major aetiology of respiratory tract infections. HRV viral load assays are available but limitations that affect accurate quantification exist. We developed a one-step Taqman assay using oligonucleotides designed based on a comprehensive list of global HRV sequences. The new oligonucleotides targeting the 5'-UTR region showed high PCR efficiency (E = 99.6%, R2 = 0.996), with quantifiable viral load as low as 2 viral copies/μl. Assay evaluation using an External Quality Assessment (EQA) panel yielded a detection rate of 90%. When tested on 315 human enterovirus-positive specimens comprising at least 84 genetically distinct HRV types/serotypes (determined by the VP4/VP2 gene phylogenetic analysis), the assay detected all HRV species and types, as well as other non-polio enteroviruses. A commercial quantification kit, which failed to detect any of the EQA specimens, produced a detection rate of 13.3% (42/315) among the clinical specimens. Using the improved assay, we showed that HRV sheds in the upper respiratory tract for more than a week following acute infection. We also showed that HRV-C had a significantly higher viral load at 2-7 days after the onset of symptoms (p = 0.001). The availability of such assay is important to facilitate disease management, antiviral development, and infection control.

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عنوان ژورنال:

دوره 6  شماره 

صفحات  -

تاریخ انتشار 2016