4.5 Article

How many replicates to accurately estimate fish biodiversity using environmental DNA on coral reefs?

Journal

ECOLOGY AND EVOLUTION
Volume 11, Issue 21, Pages 14630-14643

Publisher

WILEY
DOI: 10.1002/ece3.8150

Keywords

biomonitoring; coral reef diversity; environmental DNA; MOTU; sampling variability; tropical marine ecosystems

Funding

  1. Conseil Regional des Pays de la Loire [2020_10792]
  2. H2020 European Research Council [759457]
  3. Schweizerischer Nationalfonds zur Forderung der Wissenschaftlichen Forschung [310030E-164294]
  4. Instituto de Investigaciones Marinas y Costeras [2017011000113]
  5. Swiss National Science Foundation (SNF) [310030E-164294] Funding Source: Swiss National Science Foundation (SNF)

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Quantifying fish species diversity in rich tropical marine environments remains challenging, with eDNA metabarcoding showing promise but limited reliability due to low eDNA concentration. Local diversity may be underestimated with multiple replicates at the same location, while regional diversity often reaches saturation with multiple replicates at variable locations. Variability in diversity estimates may arise from uneven distribution of eDNA, skewed frequency of eDNA traces per MOTU, and processing variability.
Quantifying fish species diversity in rich tropical marine environments remains challenging. Environmental DNA (eDNA) metabarcoding is a promising tool to face this challenge through the filtering, amplification, and sequencing of DNA traces from water samples. However, because eDNA concentration is low in marine environments, the reliability of eDNA to detect species diversity can be limited. Using an eDNA metabarcoding approach to identify fish Molecular Taxonomic Units (MOTUs) with a single 12S marker, we aimed to assess how the number of sampling replicates and filtered water volume affect biodiversity estimates. We used a paired sampling design of 30 L per replicate on 68 reef transects from 8 sites in 3 tropical regions. We quantified local and regional sampling variability by comparing MOTU richness, compositional turnover, and compositional nestedness. We found strong turnover of MOTUs between replicated pairs of samples undertaken in the same location, time, and conditions. Paired samples contained non-overlapping assemblages rather than subsets of one another. As a result, non-saturated localized diversity accumulation curves suggest that even 6 replicates (180 L) in the same location can underestimate local diversity (for an area <1 km). However, sampling regional diversity using similar to 25 replicates in variable locations (often covering 10 s of km) often saturated biodiversity accumulation curves. Our results demonstrate variability of diversity estimates possibly arising from heterogeneous distribution of eDNA in seawater, highly skewed frequencies of eDNA traces per MOTU, in addition to variability in eDNA processing. This high compositional variability has consequences for using eDNA to monitor temporal and spatial biodiversity changes in local assemblages. Avoiding false-negative detections in future biomonitoring efforts requires increasing replicates or sampled water volume to better inform management of marine biodiversity using eDNA.

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