Drop it all: extraction-free detection of targeted marine species through optimized direct droplet digital PCR

Michelle Scriver; Ulla von Ammon; Cody Youngbull; Xavier Pochon; Jo-Ann L. Stanton; Neil J. Gemmell; Anastasija Zaiko

doi:10.7717/peerj.16969

PeerJ (Feb 2024)

Drop it all: extraction-free detection of targeted marine species through optimized direct droplet digital PCR

Michelle Scriver,
Ulla von Ammon,
Cody Youngbull,
Xavier Pochon,
Jo-Ann L. Stanton,
Neil J. Gemmell,
Anastasija Zaiko

Affiliations

Michelle Scriver: Biosecurity Group, Cawthron Institute, Nelson, New Zealand
Ulla von Ammon: Biosecurity Group, Cawthron Institute, Nelson, New Zealand
Cody Youngbull: Nucleic Sensing Systems, LCC, Saint Paul, Minnesota, United States
Xavier Pochon: Biosecurity Group, Cawthron Institute, Nelson, New Zealand
Jo-Ann L. Stanton: Department of Anatomy, School of Biomedical Sciences, University of Otago, Dunedin, New Zealand
Neil J. Gemmell: Department of Anatomy, School of Biomedical Sciences, University of Otago, Dunedin, New Zealand
Anastasija Zaiko: Biosecurity Group, Cawthron Institute, Nelson, New Zealand

DOI: https://doi.org/10.7717/peerj.16969
Journal volume & issue: Vol. 12
p. e16969

Abstract

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Molecular biomonitoring programs increasingly use environmental DNA (eDNA) for detecting targeted species such as marine non-indigenous species (NIS) or endangered species. However, the current molecular detection workflow is cumbersome and time-demanding, and thereby can hinder management efforts and restrict the “opportunity window” for rapid management responses. Here, we describe a direct droplet digital PCR (direct-ddPCR) approach to detect species-specific free-floating extra-cellular eDNA (free-eDNA) signals, i.e., detection of species-specific eDNA without the need for filtration or DNA extraction, with seawater samples. This first proof-of-concept aquarium study was conducted with three distinct marine species: the Mediterranean fanworm Sabella spallanzanii, the ascidian clubbed tunicate Styela clava, and the brown bryozoan Bugula neritina to evaluate the detectability of free-eDNA in seawater. The detectability of targeted free-eDNA was assessed by directly analysing aquarium marine water samples using an optimized species-specific ddPCR assay. The results demonstrated the consistent detection of S. spallanzanii and B. neritina free-eDNA when these organisms were present in high abundance. Once organisms were removed, the free-eDNA signal exponentially declined, noting that free-eDNA persisted between 24–72 h. Results indicate that organism biomass, specimen characteristics (e.g., stress and viability), and species-specific biological differences may influence free-eDNA detectability. This study represents the first step in assessing the feasibility of direct-ddPCR technology for the detection of marine species. Our results provide information that could aid in the development of new technology, such as a field development of ddPCR systems, which could allow for automated continuous monitoring of targeted marine species, enabling point-of-need detection and rapid management responses.

Published in PeerJ

ISSN: 2167-8359 (Online)
Publisher: PeerJ Inc.
Country of publisher: United States
LCC subjects: Medicine; Science: Biology (General)
Website: https://peerj.com/

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