An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications

BACKGROUND: Lake Sinai Viruses (LSV) are common RNA viruses of honey bees (Apis mellifera) that frequently reach high abundance but are not linked to overt disease. LSVs are genetically heterogeneous and collectively widespread, but despite frequent detection in surveys, the ecological and geographi...

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Autores principales: Iwanowicz, Deborah D., Wu-Smart, Judy Y., Olgun, Tugce, Smart, Autumn H., Otto, Clint R.V., Lopez, Dawn, Evans, Jay D., Cornman, Robert
Formato: Online Artículo Texto
Lenguaje:English
Publicado: PeerJ Inc. 2020
Materias:
Agricultural Science
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7370930/
https://www.ncbi.nlm.nih.gov/pubmed/32742773
http://dx.doi.org/10.7717/peerj.9424
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author Iwanowicz, Deborah D.
Wu-Smart, Judy Y.
Olgun, Tugce
Smart, Autumn H.
Otto, Clint R.V.
Lopez, Dawn
Evans, Jay D.
Cornman, Robert
author_facet Iwanowicz, Deborah D.
Wu-Smart, Judy Y.
Olgun, Tugce
Smart, Autumn H.
Otto, Clint R.V.
Lopez, Dawn
Evans, Jay D.
Cornman, Robert
author_sort Iwanowicz, Deborah D.
collection PubMed
description BACKGROUND: Lake Sinai Viruses (LSV) are common RNA viruses of honey bees (Apis mellifera) that frequently reach high abundance but are not linked to overt disease. LSVs are genetically heterogeneous and collectively widespread, but despite frequent detection in surveys, the ecological and geographic factors structuring their distribution in A. mellifera are not understood. Even less is known about their distribution in other species. Better understanding of LSV prevalence and ecology have been hampered by high sequence diversity within the LSV clade. METHODS: Here we report a new polymerase chain reaction (PCR) assay that is compatible with currently known lineages with minimal primer degeneracy, producing an expected 365 bp amplicon suitable for end-point PCR and metagenetic sequencing. Using the Illumina MiSeq platform, we performed pilot metagenetic assessments of three sample sets, each representing a distinct variable that might structure LSV diversity (geography, tissue, and species). RESULTS: The first sample set in our pilot assessment compared cDNA pools from managed A. mellifera hives in California (n = 8) and Maryland (n = 6) that had previously been evaluated for LSV2, confirming that the primers co-amplify divergent lineages in real-world samples. The second sample set included cDNA pools derived from different tissues (thorax vs. abdomen, n = 24 paired samples), collected from managed A. mellifera hives in North Dakota. End-point detection of LSV frequently differed between the two tissue types; LSV metagenetic composition was similar in one pair of sequenced samples but divergent in a second pair. Overall, LSV1 and intermediate lineages were common in these samples whereas variants clustering with LSV2 were rare. The third sample set included cDNA from individual pollinator specimens collected from diverse landscapes in the vicinity of Lincoln, Nebraska. We detected LSV in the bee Halictus ligatus (four of 63 specimens tested, 6.3%) at a similar rate as A. mellifera (nine of 115 specimens, 7.8%), but only one H. ligatus sequencing library yielded sufficient data for compositional analysis. Sequenced samples often contained multiple divergent LSV lineages, including individual specimens. While these studies were exploratory rather than statistically powerful tests of hypotheses, they illustrate the utility of high-throughput sequencing for understanding LSV transmission within and among species.
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spelling pubmed-73709302020-07-31 An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications Iwanowicz, Deborah D. Wu-Smart, Judy Y. Olgun, Tugce Smart, Autumn H. Otto, Clint R.V. Lopez, Dawn Evans, Jay D. Cornman, Robert PeerJ Agricultural Science BACKGROUND: Lake Sinai Viruses (LSV) are common RNA viruses of honey bees (Apis mellifera) that frequently reach high abundance but are not linked to overt disease. LSVs are genetically heterogeneous and collectively widespread, but despite frequent detection in surveys, the ecological and geographic factors structuring their distribution in A. mellifera are not understood. Even less is known about their distribution in other species. Better understanding of LSV prevalence and ecology have been hampered by high sequence diversity within the LSV clade. METHODS: Here we report a new polymerase chain reaction (PCR) assay that is compatible with currently known lineages with minimal primer degeneracy, producing an expected 365 bp amplicon suitable for end-point PCR and metagenetic sequencing. Using the Illumina MiSeq platform, we performed pilot metagenetic assessments of three sample sets, each representing a distinct variable that might structure LSV diversity (geography, tissue, and species). RESULTS: The first sample set in our pilot assessment compared cDNA pools from managed A. mellifera hives in California (n = 8) and Maryland (n = 6) that had previously been evaluated for LSV2, confirming that the primers co-amplify divergent lineages in real-world samples. The second sample set included cDNA pools derived from different tissues (thorax vs. abdomen, n = 24 paired samples), collected from managed A. mellifera hives in North Dakota. End-point detection of LSV frequently differed between the two tissue types; LSV metagenetic composition was similar in one pair of sequenced samples but divergent in a second pair. Overall, LSV1 and intermediate lineages were common in these samples whereas variants clustering with LSV2 were rare. The third sample set included cDNA from individual pollinator specimens collected from diverse landscapes in the vicinity of Lincoln, Nebraska. We detected LSV in the bee Halictus ligatus (four of 63 specimens tested, 6.3%) at a similar rate as A. mellifera (nine of 115 specimens, 7.8%), but only one H. ligatus sequencing library yielded sufficient data for compositional analysis. Sequenced samples often contained multiple divergent LSV lineages, including individual specimens. While these studies were exploratory rather than statistically powerful tests of hypotheses, they illustrate the utility of high-throughput sequencing for understanding LSV transmission within and among species. PeerJ Inc. 2020-07-17 /pmc/articles/PMC7370930/ /pubmed/32742773 http://dx.doi.org/10.7717/peerj.9424 Text en ©2020 Iwanowicz et al. https://creativecommons.org/publicdomain/zero/1.0/ This is an open access article, free of all copyright, made available under the Creative Commons Public Domain Dedication (https://creativecommons.org/publicdomain/zero/1.0/) . This work may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose.
spellingShingle Agricultural Science
Iwanowicz, Deborah D.
Wu-Smart, Judy Y.
Olgun, Tugce
Smart, Autumn H.
Otto, Clint R.V.
Lopez, Dawn
Evans, Jay D.
Cornman, Robert
An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title_full An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title_fullStr An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title_full_unstemmed An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title_short An updated genetic marker for detection of Lake Sinai Virus and metagenetic applications
title_sort updated genetic marker for detection of lake sinai virus and metagenetic applications
topic Agricultural Science
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7370930/
https://www.ncbi.nlm.nih.gov/pubmed/32742773
http://dx.doi.org/10.7717/peerj.9424
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