Community eDNA metabarcoding as a detection tool for documenting freshwater mussel (Unionidae) species assemblages

Stephanie A. Coghlan; Charise A. Currier; Joanna Freeland; Todd J. Morris; Chris C. Wilson

doi:10.1002/edn3.239

Environmental DNA (Nov 2021)

Community eDNA metabarcoding as a detection tool for documenting freshwater mussel (Unionidae) species assemblages

Stephanie A. Coghlan,
Charise A. Currier,
Joanna Freeland,
Todd J. Morris,
Chris C. Wilson

Affiliations

Stephanie A. Coghlan: Ontario Ministry of Natural Resources and Forestry Peterborough ON Canada
Charise A. Currier: Great Lakes Laboratory for Fisheries and Aquatic Sciences, Fisheries and Oceans Canada Burlington ON Canada
Joanna Freeland: Department of Biology Trent University Peterborough ON Canada
Todd J. Morris: Great Lakes Laboratory for Fisheries and Aquatic Sciences, Fisheries and Oceans Canada Burlington ON Canada
Chris C. Wilson: Ontario Ministry of Natural Resources and Forestry Peterborough ON Canada

DOI: https://doi.org/10.1002/edn3.239
Journal volume & issue: Vol. 3, no. 6
pp. 1172 – 1191

Abstract

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Abstract Documenting species occurrences and habitat occupancy of unionid mussels can often be challenging. Environmental DNA (eDNA) has been shown to be a reliable tool for detecting unionids with comparable or greater sensitivity than conventional sampling and has the added advantages of not disturbing individuals or occupied habitats. However, single‐species eDNA assays are limited to targeting individual species of interest and are functionally blind to the presence of other species. Community eDNA assays have the potential to characterize local species assemblages simultaneously but are currently less extensively developed and implemented than single‐species eDNA testing. We tested the effectiveness of community eDNA markers to identify unionid species assemblages, using two overlapping conserved primers that target the maternal mitochondrial 16S rDNA region. Both primer sets were optimized using three mock communities and successfully amplified 62.5%–81.6% of species with largely consistent results between the primer sets. Following optimization, eDNA from water samples from 24 reference sites with known mussel communities was amplified and sequenced to quantify species richness and diversity within and among sites. Metabarcoding results from the monitoring sites largely mirrored those from the mock communities, with >80% of species detections identified by both assays. The results were broadly consistent with species data from quadrat‐based manual field surveys, although both community eDNA and conventional sampling detected some species that the other method did not. These results demonstrate that community eDNA assays using conserved primers and next‐generation sequencing have the potential to simultaneously target eDNA from multiple unionid species and provide a powerful tool for complementing or augmenting conventional field surveys to characterize and monitor unionid species assemblages.

Published in Environmental DNA

ISSN: 2637-4943 (Online)
Publisher: Wiley
Country of publisher: United Kingdom
LCC subjects: Geography. Anthropology. Recreation: Environmental sciences; Science: Microbiology: Microbial ecology
Website: https://onlinelibrary.wiley.com/journal/26374943

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