High throughput AS LNA qPCR method for the detection of a specific mutation in poliovirus vaccine strains

Lizet Opmeer; Isabella Gazzoli; Mónika Ballmann; Marieke Willemsen; Gerben P Voshol; Magda Grudniewska-Lawton; Menzo Havenga; Christopher Yallop; Ahd Hamidi; Gert Gillissen; Wilfried A M Bakker

doi:10.1016/j.vaccine.2024.01.103

High throughput AS LNA qPCR method for the detection of a specific mutation in poliovirus vaccine strains

Vaccine. 2024 Apr 2;42(9):2475-2484. doi: 10.1016/j.vaccine.2024.01.103. Epub 2024 Mar 19.

Affiliations

¹ Batavia Biosciences B.V., Bioscience Park Leiden, Zernikedreef 16, 2333CL Leiden, The Netherlands.
² GenomeScan B.V., Plesmanlaan 1d, 2333 BZ Leiden, The Netherlands.
³ Batavia Biosciences B.V., Bioscience Park Leiden, Zernikedreef 16, 2333CL Leiden, The Netherlands. Electronic address: w.bakker@bataviabiosciences.com.

Abstract

Sabin Inactivated Poliovirus Vaccine (sIPV) has become one of the preferred vaccination options for the last step in the Poliovirus eradication program. Sequencing of poliovirus samples is needed during the manufacturing of poliovirus vaccines to assure the safety and immunogenicity of these vaccines. Next-generation sequencing analysis is the current costly and time-consuming gold standard for monitoring the manufacturing processes. We developed a low-cost and quick, highly sensitive, and allele-specific locked nucleic acid-probe-based reverse transcription quantitative PCR alternative that can accurately detect mutations in poliovirus vaccine samples during process development, scaling up, and release. Using the frequently in vitro occurring and viral replication-impacting VP1-E₂₉₅K mutation as a showcase, we show that this technology can accurately detect E₂₉₅K mutations in poliovirus 2 samples to similar levels as NGS. The qPCR technology was developed employing a synthetic dsDNA fragment-based standard curve containing mixes of E₂₉₅K-WT (wildtype) and Mut (mutant) synthetic dsDNA fragments ranging from 1 × 10⁷ copies/µL to 1 × 10² copies/µL to achieve a linear correlation with R² > 0.999, and PCR efficiencies of 95-105 %. Individual standard concentration levels achieved accuracies of ≥92 % (average 96 %) and precisions of ≤17 % (average 3.3 %) RSD. Specificity of locked nucleic acid (LNA)-probes was confirmed in the presence and absence of co-mutations in the probe-binding region. Application of the developed assay to Sabin Poliovirus type 2 production run samples, illustrated a linear relationship with an R² of 0.994, and an average accuracy of 97.2 % of the variant (allele)-specific AS LNA qPCR result, compared to NGS. The assay showed good sensitivity for poliovirus samples, containing E₂₉₅K mutation levels between 0 % and 95 % (quantification range). In conclusion, the developed AS LNA qPCR presents a valuable low-cost, and fast tool, suitable for the process development and quality control of polio vaccines.

Keywords: AS LNA qPCR; Mutations; NGS; Quality control; Sabin Poliovirus 2; VP1-E295K; Vaccine; qPCR; sIPV.

MeSH terms

Humans
Mutation
Oligonucleotides*
Poliomyelitis* / prevention & control
Poliovirus Vaccine, Inactivated
Poliovirus Vaccine, Oral / genetics
Poliovirus* / genetics
Quality Control

Substances

Poliovirus Vaccine, Oral
locked nucleic acid
Poliovirus Vaccine, Inactivated
Oligonucleotides