Novel Tools for Lassa Virus Surveillance in Peri-domestic Rodents

Author:

Smither Allison R.,Koninga James,Kanneh Franklyn B.,Foday Momoh,Boisen Matthew L.,Bond Nell G.,Momoh Mambu,Demby Sandi John,Kanneh Lansana,Alhasan Foday,Mustapha Kanneh Ibrahim,Yillah Mohamed S.,Grant Donald S.,Bush Duane J.,Nelson Diana K. S.,Cruz Kaitlin M.,Klitting Raphaëlle,Pauthner Matthias,Andersen Kristian G.,Shaffer Jeffrey G.,Cross Robert W.,Schieffelin John S.,Garry Robert F.ORCID

Abstract

AbstractBackgroundLassa fever (LF) is a rodent-borne disease endemic to West Africa. In the absence of licensed therapeutics or vaccines, rodent exclusion from living spaces remains the primary method of preventing LF. Zoonotic surveillance of Lassa virus (LASV), the etiologic agent of LF, can assess the burden of LASV in a region and guide public health measures against LF.MethodsIn this study, we adapted commercially available LASV human diagnostics to assess the prevalence of LASV in peri-domestic rodents in Eastern Sierra Leone. Small mammal trapping was conducted in Kenema district, Sierra Leone between November 2018-July 2019. LASV antigen was detected using a commercially available LASV NP antigen rapid diagnostic test. LASV IgG antibodies against LASV nucleoprotein (NP) and glycoprotein (GP) were tested by adapting a commercially available semi-quantitative enzyme linked immunosorbent assay (ELISA) for detection of mouse-related and rat-related species IgG.FindingsOf the 373 tested specimens, 74 (20%) tested positive for LASV antigen. 40 (11%) specimens tested positive for LASV NP IgG, while an additional 12 (3%) specimens only tested positive for LASV GP IgG. Simultaneous antigen presence and IgG antibody presence was linked inMastomys sp. specimens (p< 0.01), but notRattus sp. specimens (p= 1). Despite the link between antigen presence and IgG antibody presence inMastomys sp., the strength of antigen response did not correlate with the strength of IgG response to either GP IgG or NP IgG.InterpretationThe tools developed in this study can aid in the generation of valuable public health data for rapid field assessment of LASV burden during outbreak investigations and general LASV surveillance.FundingFunding for this work was supported by the National Institute of Allergy and Infectious Diseases National Institute of Health, Department of Health and Human Services under the following grants: International Collaboration in Infectious Disease Research on Lassa fever and Ebola - ICIDR - U19 AI115589, Consortium for Viral Systems Biology - CViSB - 5U19AI135995, West African Emerging Infectious Disease Research Center - WARN-ID - U01AI151812, West African Center for Emerging Infectious Diseases: U01AI151801.

Publisher

Cold Spring Harbor Laboratory

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