Sensitive and Accurate Quantification of Enterovirus-D68 (EV-D68) Viral Loads Using Droplet Digital PCR (ddPCR)
Cassandra S. Grizer, Zhaozhang Li, Joseph J. Mattapallil

TL;DR
A new ddPCR assay accurately and sensitively quantifies EV-D68 virus in clinical samples and cell cultures.
Contribution
A novel EV-D68-specific ddPCR assay with high specificity and sensitivity for viral load quantification.
Findings
The ddPCR assay quantifies EV-D68 RNA copies in a dynamic range of 6.7 × 10−3 to 1.2 × 104 copies/μL.
The assay is specific to EV-D68 and does not cross-react with other pediatric viruses.
The method successfully quantified EV-D68 in clinical samples from the 2022 outbreak.
Abstract
Enterovirus-D68 (EV-D68) is a reemerging virus that has been associated with numerous outbreaks in children in the past 10 years. Most assays examining viral infection kinetics have relied on the use of quantitative RT-PCR (qRT-PCR) assays as an assay of choice. Though valuable, there are inherent limitations that introduce variability, thereby reducing its value when comparing results across the field. Unlike the qRT-PCR assay that uses a standard curve to determine the copy number of viral RNA, the droplet digital PCR assay (ddPCR) directly quantifies the absolute number of copies within a given sample, which in turn makes the assay highly sensitive and accurate. Here, we have developed an EV-D68-specific ddPCR assay that effectively quantifies EV-D68 RNA copies in both cells and supernatants within a dynamic range of 6.7 × 10−3 copies/μL to 1.2 × 104 copies/μL of the sample. The…
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Taxonomy
TopicsCorporate Governance and Law
