Chemical inactivation of foot-and-mouth disease virus in bovine tongue epithelium for safe transport and downstream processing

Petrus Jansen van Vuren; Nagendrakumar Balasubramanian Singanallur; Hanna Keck; Michael Eschbaumer; Wilna Vosloo

doi:10.1016/j.jviromet.2022.114539

Chemical inactivation of foot-and-mouth disease virus in bovine tongue epithelium for safe transport and downstream processing

J Virol Methods. 2022 Jul:305:114539. doi: 10.1016/j.jviromet.2022.114539. Epub 2022 May 4.

Authors

Petrus Jansen van Vuren¹, Nagendrakumar Balasubramanian Singanallur¹, Hanna Keck², Michael Eschbaumer², Wilna Vosloo³

Affiliations

¹ Australian Centre for Disease Preparedness, CSIRO Health and Biosecurity, 5 Portarlington rd, Geelong, VIC, Australia.
² National Reference Laboratory for FMD, Institute of Diagnostic Virology, Friedrich-Loeffler-Institut, Suedufer 10, 17493 Greifswald-Insel Riems, Germany.
³ Australian Centre for Disease Preparedness, CSIRO Health and Biosecurity, 5 Portarlington rd, Geelong, VIC, Australia. Electronic address: wilna.vosloo@csiro.au.

PMID: 35523370
DOI: 10.1016/j.jviromet.2022.114539

Abstract

Epithelial tissue or vesicular fluid from an unruptured or recently ruptured vesicle is the sample of choice for confirmatory laboratory diagnosis of foot-and-mouth disease (FMD). However, in 'FMD-free' countries the transport and downstream processing of such samples from potentially infected animals present a biosafety risk, particularly during heightened surveillance, potentially involving decentralised testing in laboratories without adequate biocontainment facilities. In such circumstances, rapid inactivation of virus, if present, prior to transport becomes a necessity, while still maintaining the integrity of diagnostic analytes. Tongue epithelium collected from cattle infected with FMD virus (FMDV) of serotype O (O/ALG/3/2014 - Lineage O/ME-SA/Ind-2001d) or A (A/IRN/22/2015 - Lineage A/ASIA/G-VII) was incubated in the PAXGene Tissue System Fixative (pH 4) and Stabiliser (pH 6.5) components respectively, in McIlvaine's citrate-phosphate buffer (pH 2.6) or in phosphate-buffered saline (PBS, pH 7.4) at room temperature for 2, 6, 24 or 48 h. Following incubation, tissues were homogenised and tested by virus isolation and titration using LFBK_αVβ6 cells. The integrity of FMD viral RNA was assessed by RT-qPCR (3D^pol coding region), Sanger sequencing of the VP1 region and transfection of LFBK_αVβ6 cells to recover infectious virus. Viable virus could be recovered from samples incubated in PBS for at least 48 h. The PAXgene Tissue System Stabiliser component yielded variable results dependent on virus serotype, requiring at least 6 h of incubation to inactivate A/IRN/22/2015 in most samples, whereas the Fixative component required up to 2 h in some samples. McIlvaine's citrate-phosphate buffer rapidly inactivated both viruses within 2 h of incubation. There was no demonstrable degradation of FMD viral RNA resulting from incubation in any of the buffers for up to 48 h, as assessed by RT-qPCR, and 24 h by sequencing and transfection to recover infectious virus. McIlvaine's citrate-phosphate buffer (pH 2.6) is easy to prepare, inexpensive and inactivates serotype A and O FMDV in epithelial tissue within 2 h, while maintaining RNA integrity for downstream diagnostic processes and virus characterisation.

Keywords: Foot-and-mouth disease virus; Inactivation; Sample transport; Tongue epithelium.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cattle
Citrates
Epithelium
Fixatives
Foot-and-Mouth Disease Virus* / genetics
Foot-and-Mouth Disease*
Phosphates
RNA, Viral / genetics
Serogroup
Tongue

Substances

Citrates
Fixatives
Phosphates
RNA, Viral