Development of a Quantitative One-Step RT-PCR Method for the Detection of Sabin 2 Virus Contamination in a Novel Oral Poliovirus Vaccine Type 2

Hasmik Manukyan; Erman Tritama; Rahnuma Wahid; Azeem Ansari; John Konz; Konstantin Chumakov; Majid Laassri

doi:10.3390/vaccines9070688

Vaccines (Jun 2021)

Development of a Quantitative One-Step RT-PCR Method for the Detection of Sabin 2 Virus Contamination in a Novel Oral Poliovirus Vaccine Type 2

Hasmik Manukyan,
Erman Tritama,
Rahnuma Wahid,
Azeem Ansari,
John Konz,
Konstantin Chumakov,
Majid Laassri

Affiliations

Hasmik Manukyan: Division of Viral Products, Center for Biologics Evaluation and Research, US Food and Drug Administration, Silver Spring, MD 20993, USA
Erman Tritama: Research and Development Division, PT. Bio Farma, Bandung 40161, Indonesia
Rahnuma Wahid: Center for Vaccine Innovation and Access, PATH, Seattle, WA 98121, USA
Azeem Ansari: Center for Vaccine Innovation and Access, PATH, Seattle, WA 98121, USA
John Konz: Center for Vaccine Innovation and Access, PATH, Seattle, WA 98121, USA
Konstantin Chumakov: Division of Viral Products, Center for Biologics Evaluation and Research, US Food and Drug Administration, Silver Spring, MD 20993, USA
Majid Laassri: Division of Viral Products, Center for Biologics Evaluation and Research, US Food and Drug Administration, Silver Spring, MD 20993, USA

DOI: https://doi.org/10.3390/vaccines9070688
Journal volume & issue: Vol. 9, no. 7
p. 688

Abstract

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To control circulating vaccine-derived type 2 poliovirus outbreaks, a more genetically stable novel Oral Poliovirus Vaccine type 2 (nOPV2) was developed by targeted modifications of Sabin 2 genome. Since the use of OPV2 made of Sabin 2 strain has been stopped, it is important to exclude the possibility that batches of nOPV2 are contaminated with Sabin 2 virus. Here, we report the development of a simple quantitative one-step reverse-transcription polymerase chain reaction assay for the detection and quantitation of Sabin 2 virus in the presence of overwhelming amounts of nOPV2 strain. The method is specific and linear within 8 log10 range even in the presence of relevant amounts of nOPV2 virus. It is sensitive, with a lower limit of detection of 0.2 CCID50/mL (an equivalent of 198 genome copies per mL), and generates reproducible results. This assay can be used for quality control and lot release of the nOPV2.

Published in Vaccines

ISSN: 2076-393X (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Medicine
Website: http://www.mdpi.com/journal/vaccines

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