Optimized DNA isolation from marine sponges for natural sampler DNA metabarcoding

Author:

Harper Lynsey R.12ORCID,Neave Erika F.13,Sellers Graham S.4,Cunnington Alice V.1,Arias María Belén3,Craggs Jamie3,MacDonald Barry5,Riesgo Ana36,Mariani Stefano1ORCID

Affiliation:

1. School of Biological and Environmental Sciences Liverpool John Moores University Liverpool UK

2. NatureMetrics Ltd Surrey Research Park Guildford UK

3. Department of Life Sciences The Natural History Museum London UK

4. Department of Biological and Marine Sciences University of Hull Kingston upon Hull UK

5. Fisheries and Oceans Canada Dartmouth Nova Scotia Canada

6. Department of Biodiversity and Evolutionary Biology Museo Nacional de Ciencias Naturales (CSIC) Madrid Spain

Abstract

AbstractMarine sponges have recently been recognized as natural samplers of environmental DNA (eDNA) due to their effective water filtration and their ubiquitous, sessile, and regenerative nature. However, laboratory workflows for metabarcoding of sponge tissue have not been optimized to ensure that these natural samplers achieve their full potential for community survey. We used a phased approach to investigate the influence of DNA isolation procedures on the biodiversity information recovered from sponges. In Phase 1, we compared three treatments of residual ethanol preservative in sponge tissue alongside five DNA extraction protocols. The results of Phase 1 informed which ethanol treatment and DNA extraction protocol should be used in Phase 2, where we assessed the effect of starting tissue mass on extraction success and whether homogenization of sponge tissue is required. Phase 1 results indicated that ethanol preservative may contain unique and/or additional biodiversity information to that present in sponge tissue, but blotting tissue dry generally recovered more taxa and generated more sequence reads from the wild sponge species. Tissue extraction protocols performed best in terms of DNA concentration, taxon richness, and proportional read counts, but the non‐commercial tissue protocol was selected for Phase 2 due to cost‐efficiency and greater recovery of target taxa. In Phase 2 overall, we found that homogenization may not be required for sponge tissue and more starting material does not necessarily improve taxon detection. These results combined provide an optimized DNA isolation procedure for sponges to enhance marine biodiversity assessment using natural sampler DNA metabarcoding.

Funder

Consejo Superior de Investigaciones Científicas

Ministerio de Ciencia e Innovación

Natural Environment Research Council

Publisher

Wiley

Subject

Genetics,Ecology,Ecology, Evolution, Behavior and Systematics

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