Deep Sequencing of Porcine Reproductive and Respiratory Syndrome Virus ORF7: A Promising Tool for Diagnostics and Epidemiologic Surveillance

Author:

Jakab Szilvia12ORCID,Bali Krisztina12ORCID,Freytag Csongor3,Pataki Anna1,Fehér Enikő12ORCID,Halas Máté4,Jerzsele Ákos25ORCID,Szabó István6ORCID,Szarka Krisztina3ORCID,Bálint Ádám7,Bányai Krisztián125

Affiliation:

1. Veterinary Medical Research Institute, Hungária krt. 21., H-1143 Budapest, Hungary

2. National Laboratory for Infectious Animal Diseases, Antimicrobial Resistance, Veterinary Public Health and Food Chain Safety, Hungária krt. 21., H-1143 Budapest, Hungary

3. Department of Metagenomics, University of Debrecen, H-4032 Debrecen, Hungary

4. Prophyl Ltd., H-7700 Mohács, Hungary

5. Department of Pharmacology and Toxicology, University of Veterinary Medicine, István u 2, H-1078 Budapest, Hungary

6. National PRRS Eradication Committee, Keleti Károly u. 24., H-1024 Budapest, Hungary

7. Veterinary Diagnostic Directorate, National Food Chain Safety Office, H-1143 Budapest, Hungary

Abstract

Porcine reproductive and respiratory syndrome virus (PRRSV) is a major concern worldwide. Control of PRRSV is a challenging task due to various factors, including the viral diversity and variability. In this study, we evaluated an amplicon library preparation protocol targeting the ORF7 region of both PRRSV species, Betaarterivirus suid 1 and Betaarterivirus suid 2. We designed tailed primers for a two-step PCR procedure that generates ORF7-specific amplicon libraries suitable for use on Illumina sequencers. We tested the method with serum samples containing common laboratory strains and with pooled serum samples (n = 15) collected from different pig farms during 2019–2021 in Hungary. Testing spiked serum samples showed that the newly designed method is highly sensitive and detects the viral RNA even at low copy numbers (corresponding to approx. Ct 35). The ORF7 sequences were easily assembled even from clinical samples. Two different sequence variants were identified in five samples, and the Porcilis MLV vaccine strain was identified as the minor variant in four samples. An in-depth analysis of the deep sequencing results revealed numerous polymorphic sites along the ORF7 gene in a total of eight samples, and some sites (positions 12, 165, 219, 225, 315, 345, and 351) were found to be common in several clinical specimens. We conclude that amplicon deep sequencing of a highly conserved region of the PRRSV genome could support both laboratory diagnosis and epidemiologic surveillance of the disease.

Funder

National Laboratory for Infectious Animal Diseases, Antimicrobial Resistance, Veterinary Public Health and Food Chain Safety

National Research, Development and Innovation Fund

Publisher

MDPI AG

Subject

General Veterinary,Animal Science and Zoology

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