Study sites, sampling, and targeted species

The study was carried out in river and lake habitats in the canton of Zurich in the northeastern part of Switzerland (Fig. 1,  Table S1 (2013348_TableS1.docx)). All study sites are natural water bodies and belong to 2 independent drainages (Glatt River and Limmat River, which drain Lake Greifensee and Lake Zurich, respectively). For the eDNA surveillance method, we collected 2 water samples/site in 1-L sterile octagonal polyethylene terephthalate bottles (VWR International, Radnor, Pennsylvania) by dipping the mouth of the bottle just below the surface of the water near the edge of the water body. We placed water bottles in an ice-filled container during transport and stored them at -20°C until processed. Maximum transport time was 5 h. Immediately after taking water samples, we collected macroinvertebrates with standard kicknet sampling following federal and cantonal guidelines (Stucki 2010, Altermatt 2013;  Appendix S1 (2013348_AppendixS1.docx)). Thereby, we could compare detection of macroinvertebrates using the novel eDNA surveillance method with the traditional kicknet sampling (for a description of the workflows, see Fig. 2). We took 8 independent kicknet samples per site to reflect the different microhabitats at each study site and pooled them to get an accurate and robust presence/absence measure for all macroinvertebrates (Stucki 2010,  Appendix S1 (2013348_AppendixS1.docx)).

We choose a range of 6 species belonging to 3 major classes of invertebrates (Table 1) for which we compared the eDNA surveillance method with the conventional kicknet method. We chose species that live in rivers and lakes and are either rare or belong to indicator groups used for water-quality assessment in the study area (von der Ohe et al. 2007). We chose species that had been detected in the study area by the conventional biodiversity monitoring conducted by the Office of Waste, Water, Energy, and Air (WWEA/AWEL) of the Canton of Zurich over the years 1995–2011 (AWEL 2012) and were known to be part of the regional species pool.

Table 1.

Overview of the study species.

Primer development and tests of sensitivity and specificity

We chose the cytochrome c oxidase subunit I (COI) gene to develop primer pairs for our study species (Thomsen et al. 2011, Mahon et al. 2013). We targeted COI because mitochondrial genes have many more copies per cell than nuclear genes (Mills et al. 2000) and, thus, are more likely to be detected. Furthermore, the COI sequence is generally used and advocated for identification of macroinvertebrate species from aquatic systems (Deiner et al. 2013), and existing sequence data can be used for primer development. We gathered sequence data from GenBank for each of the target species (Benson et al. 2012;  Table S2 (2013348_TableS2.docx)). For each target species, we aligned COI sequences using Sequencher® (version 4.9; Gene Codes, Ann Arbor, Michigan) to observe intraspecific conserved regions. We also aligned sequences of related species to compare intra- and interspecific differences. We selected sequence regions with 180 to 450 base pairs (bp) that showed low intraspecific divergence and high interspecific divergence. We developed primer pairs with amplicon sizes of ∼200 bp, which is a size that has been detected successfully for other species (Jerde et al. 2011, Mahon et al. 2013). We acknowledge that eDNA in water is probably a mixture of cellular and extracellular DNA (Taberlet et al. 2012) and can vary in fragment length once concentrated and extracted. Detection with fragments that are too short (<100 bp for COI) may hinder adequate species identification and probably depends on the genetic region used for identification (Meusnier et al. 2008). Therefore, detection of species based on longer fragments of DNA from a water sample allows more accurate species identification and possibly detection of DNA recently released to the environment because the DNA has not had time to degrade into small fragments (Dejean et al. 2011, Thomsen et al. 2011, Goldberg et al. 2013). Primers were designed with Primer3 (version 0.4.0; Rozen and Skaletsky 1999) software using the selected 180- to 450-bp region and the default parameters of the program. When the selected region did not return primers with default parameters, we designed primers by eye from the alignments ( Table S3 (2013348_TableS3.docx)). We tested the specificity of all designed primers with the software Primer-BLAST with default settings (Ye et al. 2012; see  Table S4 (2013348_TableS4.docx) for results).

Figure 1.

Locations of sampling sites in the northeastern part of Switzerland. All sites were in the drainage systems of the river Glatt and river Limmat and Lake Greifensee and Lake Zurich, respectively. Blue areas represent main water bodies and rivers, whereas red areas represent settlements in the relief map (gray). Numbers correspond to sites listed in  Table S1 (2013348_TableS1.docx).

Figure 2.

Illustrative overview of the workflow of the 2 surveillance methods. A.—Environmental DNA (eDNA) method (from left to right): collection of water, water filtration, DNA extraction, polymerase chain reaction (PCR), visualization of products on a gel, and sequencing, eventually leading to a list of positive or negative detections of target species. B.—Conventional kicknet method: kicknet sampling, sorting, and morphological identification of species, eventually leading to a species list present at a sampling site.

To confirm primer amplification success in the target species, we ran standard PCRs with our designed primers on DNA extracts from 2 individuals of each species and sequenced the amplified products. DNA was extracted from tissue of each species using the DNeasy Blood and Tissue Kit (Qiagen GmbH, Hilden, Germany) following the manufacturer's spin-column protocol. All PCR mixtures contained 1 × buffer (Roche, Basel Switzerland), 0.18 mM dNTP, 1 × BSA, 0.05 U/µL Taq (Roche, Switzerland), 2.0 mM MgCl₂, 0.5 µM of each primer ( Table S3 (2013348_TableS3.docx)), and 1 µL of DNA (1.04– 108 ng/µL) in a total reaction volume of 15 µL. Quantification of DNA concentrations was confirmed with a Qubit® (1.0; Life Technologies, Carlsbad, California) fluorometer following recommended protocols for the broad-range DNA concentration kit (Life Technologies). The manufacturer reported ≤3% variation of repeated sample testing. The PCR thermal-cycling program started with a denaturation step at 95°C for 4 min and was followed by 35 cycles of 95°C for 30 s, 30 s at the individual annealing temperature for each primer pair ( Table S3 (2013348_TableS3.docx)), and 1 min at 72°C. A final extension of 5 min at 72°C was done before the PCR was paused at 10°C until removed. We visualized PCR products using gel electrophoresis and photo-documented gels with ultraviolet light on a 1.4% agarose gel either stained with ethidium bromide or GelRed^™ (Biotium, Hayward, California). Only single-banded, positive amplicons that we could directly sequence were used for further analyses. We cleaned each positive PCR product with Exo I Nuclease (EXO I) and Shrimp Alkaline Phosphatase (SAP) (Thermo Fisher Scientific, Waltham, Maryland) to remove leftover primers and dNTPs from the previous PCR. The master mix consisted of 1.6 U/µL Exo I and 0.15 U/µL SAP in a total volume of 1 µL, which was then added to 7.5 µL of the PCR product. Products were heated to 37°C for 15 min and followed by 15 min at 80°C. We did sequencing in both directions with the BigDye® Terminator (version 3.1) system on 3730 × 1 DNA Analyzer following manufacturers' protocols (Applied Biosystems, Foster City, California). We aligned and edited sequences for each PCR product with Sequencher. To confirm the species identity of the band amplified from extracted DNA from tissues, we aligned sequences to those used for primer design and compared sequences to the nucleotide database on GenBank using default settings in Basic Local Alignment Search Tool (BLAST; Benson et al. 2012). We could not test primer pairs against all closely related species, but we checked whether sequence databases covered COI sequences for all closely related species (i.e., species within same the genus or family) occurring in the regional species pool ( Table S5 (2013348_TableS5.docx)) and, thus, would align when we entered our sequences. This approach (i.e., sequencing all bands) is more time-intensive than inferring species presence from positive PCR amplicons only, but avoids false-positive detection of other (possibly related) species, which may yield positive PCR products of similar length, but with a different COI sequence.

To test the sensitivity of our primers, we tested a dilution series of DNA extracts from 2 species (B. buceratus, C. pseudogracilis). We diluted extracted DNA to confirm primer amplification success for these 2 species to 1 ng/µL. We then did a serial dilution to create a DNA concentration range of 0.1 ng/µL to 10^-8 ng/µL. We used each dilution as template in a PCR for final concentrations ranging from 1.08 × 10^-1 to 1.04 × 10^-8 ng/µL. We ran 3 PCR replicates/ concentration. PCR and sequencing to confirm products were carried out as described above except that 50 cycles instead of 35 were used for PCR amplification because we expected low DNA concentrations. We analyzed detection rate of the individual species with a generalized linear model (GLM), with dilution rate and species identity as predictor variables. The binary response variable described detection success or failure. We used a quasibinomial link function because of over-dispersion in the model (Crawley 2012). We started with a full model including interactions and subsequently simplified the model. We selected the best model with an F-significance test. All statistical analyses were conducted with the program R (version 2.15.3; R Project for Statistical Computing, Vienna, Austria).

Detection of species from eDNA and conventional methods

We filtered 280 to 300 mL of water from each site onto a single 0.7-µm glass fiber filter 4 times (Whatman International Ltd., Maidstone, UK). We processed 4 filters for each sampling site independently. The filter was housed in a filter case (Swinnex, EMD Millipore Co., Billerica, Massachusetts) to which we could attach a disposable 20-mL syringe. We drew water into the syringe and pushed it through the filter in the housing. We repeated this step until the desired filtered volume was reached. Filtration setup was followed as described by Deiner and Altermatt (2014). After filtration, we removed the filter from the filter housing, rolled it with tweezers, and placed it in a 1.5-mL tube. We stored all filters at -20°C until extraction. We treated all equipment used for filtration with 10% household bleach and sterilized with an ultraviolet light treatment for 30 min after handling samples from a site. We extracted DNA from each filter with a modified cell-lysis, phenol chloroform isoamyl procedure followed by ethanol precipitation of environmental DNA captured on filter as described by Deiner and Altermatt (2014).

We tested for the presence of DNA from target species with our designed primers by PCR amplification, product visualization, and sequencing of amplified products with the same protocol as described for primer tests on tissue-extracted DNA, except that we used 50 PCR cycles instead of 35, and we added 2 µL of eDNA template to each reaction. In a few cases, we used the sequence from only the forward or reverse to confirm presence (indicated with an asterisk in  Table S6 (2013348_TableS6.docx)). If a sequenced amplicon could not be confirmed in both directions, but 1 direction met our strict protocol for confirmation, we counted the case as a positive detection and reported the shorter fragment from only 1 direction. We first tested for presence of every species with eDNA derived from extraction of 280 mL water and triplicate PCR. When detection for some species (A. fluviatilis, C. pseudogracilis, and T. waeneri) was not optimal, we subsequently optimized PCR protocols by performing a temperature and MgCl₂-gradient on tissue extracted and on environmental DNA to improve specificity. Second, we repeated PCR on eDNA extracted from a larger volume of water (900 mL; 3 extractions of 300 mL water each were pooled; for details see  Table S1 (2013348_TableS1.docx)) and replicated PCR 5 times for each species at each site. We analyzed this larger total volume (900 mL vs the initial 280 mL) in a 2^nd step after realizing that this 4 × increase in volume would allow us to minimize the risk of false-absence detections (KD, J. C. Walser, EM, and FA, unpublished data). For all subsequent analyses, we pooled positive detections from the 2 volumes of water. Therefore, the presence/absence of species identified from eDNA is based on a total of 1180 mL of water extracted/site (280 + 900 mL).

We defined a species as present at a site when ≥1 PCR replicate from either volume of water showed positive amplification that could be confirmed by sequencing the amplified product. PCR is a highly stochastic process, and PCR replication in present eDNA studies ranges from 3 to 8 (Deiner and Altermatt 2014). For sequencing confirmation of a detected species, we required that the following criteria be met: 1) the generated sequences must align to the GenBank sequences used in primer design, and 2) the generated sequence must match the expected species with a high score (>99% maximum identity and >100% query coverage, except for B. buceratus) when compared against the National Center for Biotechnology Information (NCBI) nucleotide database using default settings in BLAST (Benson et al. 2012). For B. buceratus, only 1 sequence was available on GenBank. This sequence was delivered from a specimen presumably collected in the Czech Republic. Extracted DNA from a specimen collected in our study region matched this sequence with 100% query coverage but with 98% maximum identity. Use of a 2%-dissimilarity threshold allows for intraspecific diversity. This level of dissimilarity can occur in species with geographical isolation (Hebert et al. 2003). However, all water-derived DNA sequences for B. buceratus matched our tissue-derived DNA sequence with ≥99.5% maximum identity.

To identify invertebrates sampled with the kicknet method, we first presorted macroinvertebrates into higher taxonomic groups and then identified them to species level based on morphology with the aid of dichotomous taxonomic keys (Studemann et al. 1992, Waringer and Graf 1997, Glöer and Meier-Brook 1998, Tachet et al. 2000, Eggers and Martens 2001; Table 1). We compared detection rates of the kicknet sample and eDNA surveillance methods based on presence with the kicknet method, presence with the eDNA method, and their overlap. All eDNA presence data used in the comparison ( Table S7 (2013348_TableS7.docx)) were confirmed by sequencing the PCR product ( Table S6 (2013348_TableS6.docx)). The total number of sites used was in accordance to the expected habitat type (n = 10 for species living in lotic habitat only and n = 14 for species living in lentic and lotic habitats).

Laboratory precautions

eDNA is expected to occur at low density. Therefore, we took precautions similar to those used in ancient DNA protocols in all of our laboratory routines to avoid contamination (Fulton 2012). Filtrations, extractions, and prePCR work were done in a DNA-clean laboratory where no post-PCR products and extracted target-species DNA from tissues entered the room. Researchers were required to wear full-body protective gear. Negative filter, extraction, and PCR controls always were run in parallel with the samples and showed no amplifications. Equipment, such as the laminar-flow hood and pipettes were cleaned regularly with 10% household bleach and sterilized with a 30-min ultraviolet-light treatment. In addition, we applied a multitube approach and replicated PCR reactions ≥3 times (and 8 times for all eDNA detections), each with its own negative control (Taberlet et al. 1996).

Primer development and tests of sensitivity and specificity

We were able to amplify the COI region of all 6 species from tissue-derived DNA with our set of primer pairs designed from pre-existing data from GenBank. Furthermore, we confirmed primer amplification success at low target DNA concentrations via specificity tests for 2 species (Fig. 3). Detection rate was significantly affected by the dilution of DNA in DNA-free water and species identity (Table 2, Fig. 3). Detection success was 100% for the 2 tested primer pairs at target DNA concentrations >∼10^-5 ng/µL and dropped to 0% detection success at lower DNA concentrations (based on the GLM prediction) for all primers. The GLM model predicted a sudden decrease of detectability at ∼10^-6 to 10^-8 ng/µL target DNA (Table 2, Fig. 3).

Figure 3.

Correlation of detection rate and concentration of total DNA before polymerase chain reaction (PCR) for Baetis buceratus and Crangonyx pseudogracilis. Detection rate is given as proportion of positive bands across 3 PCR replicates. Lines are predictions of a generalized linear model. The detection rates for DNA concentrations from 10^-1 to 10^-5 ng/µl are all 1.0, but lines were slightly vertically displaced for better visibility.

Our primer pairs were not completely species-specific ( Table S4 (2013348_TableS4.docx)) and amplified some nontarget species. However, most of these nontarget species had geographic distributions that did not overlap our study area. To avoid the occurrence of false-positive detections completely, we subsequently sequenced every positive PCR amplification. We used only records based on a sequencing confirmation. There-by, we are certain that positive PCR amplicons used for our analysis reflect detection of eDNA of our target species.

Table 2.

Generalized linear model (GLM) on the effect of known target DNA concentration and species identity on polymerase chain reaction (PCR) detection success of species-specific environmental DNA (eDNA) in water. Proportion of detection was used as response variable (odds ratio). GLM was done with quasibinomial error distribution and subsequent F-significance testing. df = degrees of freedom.

Method comparison

The 6 study species were found with the conventional kicknet method in 3 to 9 of the 14 sampling localities (Fig. 4). We were able to detect 5 of the 6 study species (A. fluviatilis, A. aquaticus, B. buceratus, C. pseudogracilis, and G. pulex) with the eDNA method in 3 to 9 of the 14 sampling sites ( Table S7 (2013348_TableS7.docx)). We were unable to detect T. waeneri with the eDNA method.

Site occupancy based on positive species detection varied among the 5 species and between the eDNA and kicknet methods (Fig. 4). Asellus aquaticus and B. buceratus could be detected at more sites with the eDNA than the kicknet method. All other species were detected more often with the kicknet than the eDNA method. The % positive equivalency, i.e., the combined positive detection success with the kicknet and eDNA method at the same site, was 56% for A. fluviatilis, 43% for A. aquaticus, 100% for B. buceratus, 43% for C. pseudogracilis, and 71% for G. pulex.

Figure 4.

Proportion of sites occupied based on the environmental DNA (eDNA) and kicknet methods, and equivalency between methods in detecting different macroinvertebrate species. Maximum possible number of sites was 14 for species living in lakes and rivers (Ancylus fluviatilis, Asellus aquaticus, Crangonyx pseudogracilis, and Tinodes waeneri) and 10 for species living in the study area in rivers only (Baetis buceratus and Gammarus pulex). Black bars show the proportion of sites in which a species was detected based on the eDNA method. White bars show proportion of sites in which a species was detected through kicknet sampling. Gray bars denote equivalency in both methods, i.e., positive detections at the same sampling sites by both the eDNA and the kicknet method.

Data Accessibility

The final DNA sequence assembly ( Table S6 (2013348_TableS6.docx)) and eDNA sequences that could not be identified through sequence databases ( Table S8 (2013348_TableS8.docx)) were uploaded as online supplemental material.

Author contributions

EM, KD, and FA designed the study. EM and KD developed and performed the work on macroinvertebrate detection using eDNA. PS performed and analyzed conventional kicknet samples. EM, KD, and FA analyzed data and wrote the paper.