Abstract

Serology is a core component of the surveillance and management of viral zoonoses. Virus neutralization tests are a gold standard serological diagnostic, but requirements for large volumes of serum and high biosafety containment can limit widespread use. Here, focusing on Rabies lyssavirus, a globally important zoonosis, we developed a pseudotype micro-neutralization rapid fluorescent focus inhibition test (pmRFFIT) that overcomes these limitations. Specifically, we adapted an existing micro-neutralization test to use a green fluorescent protein-tagged murine leukaemia virus pseudotype in lieu of pathogenic rabies virus, reducing the need for specialized reagents for antigen detection and enabling use in low-containment laboratories. We further used statistical models to generate rapid, quantitative predictions of the probability and titre of rabies virus-neutralizing antibodies from microscopic imaging of neutralization outcomes. Using 47 serum samples from domestic dogs with neutralizing antibody titres estimated using the fluorescent antibody virus neutralization test (FAVN), pmRFFIT showed moderate sensitivity (78.79%) and high specificity (84.62%). Despite small conflicts, titre predictions were correlated across tests repeated on different dates both for dog samples (r=0.93) and in a second data set of sera from wild common vampire bats (r=0.72, N=41), indicating repeatability. Our test uses a starting volume of 3.5 µl of serum, estimates titres from a single dilution of serum rather than requiring multiple dilutions and end point titration, and may be adapted to target neutralizing antibodies against alternative lyssavirus species. The pmRFFIT enables high-throughput detection of rabies virus-neutralizing antibodies in low-biocontainment settings and is suited to studies in wild or captive animals where large serum volumes cannot be obtained.

Highlights

  • The last few decades have seen a surge in newly emerging human viruses that originate from wildlife (Cunningham, Daszak, & Wood, 2017; Daszak, Cunningham, & Hyatt, 2000; Goodin, Jonsson, Allen, &Owen, 2018)

  • To understand the variability of the pseudotype micro-neutralization rapid fluorescent focus inhibition test (pmRFFIT), replicate standard rabies immune globulin (SRIG) titer concentration curves were produced on 6 different dates between 30/05/2019 and 27/06/2019

  • The number of infected cells declined at higher SRIG titers in all replicates; the shape of the antibody decay curve varied across test dates (Figure 2)

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Summary

Introduction

The last few decades have seen a surge in newly emerging human viruses that originate from wildlife (Cunningham, Daszak, & Wood, 2017; Daszak, Cunningham, & Hyatt, 2000; Goodin, Jonsson, Allen, &Owen, 2018). Serological tests for studies of wildlife should be amenable to the small volumes of serum that often characterize collections from small-bodied hosts

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