Author:
Fagre Anna C.,Lewis Juliette,Miller Megan R.,Mossel Eric C.,Lutwama Julius J.,Nyakarahuka Luke,Nakayiki Teddy,Kityo Robert,Nalikka Betty,Towner Jonathan S.,Amman Brian R.,Sealy Tara K.,Foy Brian,Schountz Tony,Anderson John,Kading Rebekah C.
Abstract
AbstractSerological cross-reactivity among flaviviruses makes determining the prior arbovirus exposure of animals challenging in areas where multiple flavivirus strains are circulating. We hypothesized that prior infection with ZIKV could be confirmed through the presence of subgenomic flavivirus RNA (sfRNA) of the 3′ untranslated region (UTR), which persists in tissues due to XRN-1 stalling during RNA decay. We amplified ZIKV sfRNA but not NS5 from three experimentally-infected Jamaican fruit bats, supporting the hypothesis of sfRNA tissue persistence. Applying this approach to 198 field samples from Uganda, we confirmed presence of ZIKV sfRNA, but not NS5, in four bats representing three species: Eidolon helvum (n = 2), Epomophorus labiatus (n = 1), and Rousettus aegyptiacus (n = 1). Amplified sequence was most closely related to Asian lineage ZIKV. Our results support the use of sfRNA as a means of identifying previous flavivirus infection and describe the first detection of ZIKV RNA in East African bats.
Funder
National Institutes of Health
National Science Foundation
Publisher
Springer Science and Business Media LLC
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