Sturgeons in large rivers: detecting the near-extinct needles in a haystack via eDNA metabarcoding from water samples

For the purposes of the present study, we selected a total of 47 sites covering the entire Danube catchment. The 29 sampling sites along the Danube itself were selected to provide a reasonably comparable distance between sites (average: 99.2 km, Sx: 26.0 km, range: 38–149 km). By adopting sampling site distances of this scale, we could effectively minimize the potential influence of eDNA transported from the site immediately upstream (Pont et al. 2018). Furthermore, we ensured that no sampling sites were located closely downstream of the confluence of a major tributary. During the same period, we collected samples from 18 tributaries at distances of between 1 and 55 km upstream from their confluence with the Danube. Sites were sampled between June 29 and July 19, 2019, with the exception being a single site near Vienna (sampled August 6, 2019). Owing to no or low DNA amplification from samples at the Inn River site, this site was re-sampled in May 2020, and for site “Hainburg”, samples collected in July 2017 were used. Further information regarding the sampling sites (sampling date, location along the Danube, coordinates, discharge and physico-chemical water paramters) is presented in Table S1. Sampling was conducted under conditions of approximately mean discharge. At each site, 2 surface samples (less than 50 cm depth) were collected using a peristaltic pump, either by wading or from a boat moving from shore to shore to facilitate an integrated sampling of the river cross-section. The water was filtered (VigiDNA 0.45-μm crossflow filtration capsule; SPYGEN), using sterile disposable tubing. Having completed filtration, the water in the capsule was drained and the capsule was filled with 80 mL of preservation buffer CL1 (SPYGEN) to prevent eDNA degradation. The mean filtration time per sample and the mean volume of water filtered were 22.34 min (3 to 40 min) and 28.73 L (3 to 40 L), respectively, depending on the clogging rate of the filtration capsule.

The procedure used for the eDNA metabarcoding workflow (extraction, amplification using “teleo” primers, high-throughput sequencing, and bioinformatic analysis) followed the protocol described by Pont et al. (2018). “Teleo” primers (Sequence 5′–3′: forward: ACACCGCCCGTCACTCT; reverse: CTTCCGGTACACTTACCATG) amplify a short fragment (roughly 60 bp) at the end of the 12S rRNA region (Valentini et al. 2016). The extracted eDNA was PCR amplified, with 12 replicate reactions being performed for each sample. A corresponding 12 libraries were prepared using the Fasteris MetaFast protocol and 12 paired-end sequencings (2 × 125 bp) were carried out in a Miseq sequencer (Illumina) at Fasteris facilities, using a Miseq Kit v3 (Illumina) following the manufacturer's instructions. To monitor for potential contaminants, 11 negative extraction controls and seven negative PCR controls (ultrapure water) were amplified with 12 replicates and sequenced in parallel with the aforementioned samples. Sequence reads were analyzed using programs implemented in the OBITools package (Boyer et al. 2016). The forward and reverse reads were assembled using the ILLUMINAPAIREDEND program, based on a minimum score of 40 and retrieving only joined sequences. Subsequently, we assigned the reads to each sample using NGSFILTER software and a separate data set was created for each sample by splitting the original data set into several files using OBISPLIT. Thereafter, we analyzed each sample individually prior to merging the taxon list for the final ecological analysis. Strictly identical sequences were clustered together using OBIUNIQ. Sequences shorter than 20 bp, or with fewer than 10 (or labeled “internal” by the OBICLEAN program) occurrences were excluded. The taxonomic assignment of molecular operational taxonomical units was performed using the ECOTAG program, based on a local “Sturgeon” reference database (see later), the “Danubian” database, obtained from (Pont et al. 2022), the database obtained from Valentini et al. (2016), and the sequences extracted from the release 142 (standard sequences) of the ENA database (http://​www.​ebi.​ac.​uk/​ena). Given the incorrect assignment of a few sequences to the sample due to tag-jumps (Schnell et al. 2015), all sequences with a frequency of occurrence < 0.001 per sequence and per library were discarded. The data thus obtained were curated for Index-Hopping (MacConaill et al. 2018) with a threshold empirically determined for each sequencing batch using experimental blanks (i.e., combinations of tags not present in the libraries) for a given sequencing batch between libraries. Relative species abundance refers to relative number of standardized reads of all fish species as described in Pont et al. (2018). Total number of reads, % positive PCR and number of reads for Acipenser ruthenus are given in Table S2. A total of 60 taxa known to occur in the Danube River Basin were detected. 48 taxa were assigned at the species level, while 12 taxa assigned at a higher taxonomic level corresponded to a potential of 26 known Danubian species, resulting in a maximum number of 74 species detected. A full list of all species per site is available in Fig. 1 in Pont et al. (2021); and in Suppl. Figure 1 in Pont et al. (2022). This value was comparable to the total number of 71 species captured in the TEF survey conducted during the same period (Bammer et al. 2021).

All reference specimens (Acipenser stellatus, Acipenser gueldenstaedtii, Acipenser ruthenus, Acipenser nudiventris, Huso huso, Acipenser baerii, and Acipenser transmontanus) were provided by the Institute of Hydrobiology and Aquatic Ecosystem Management, University of Natural Resources and Life Sciences, Vienna, either from wild catches or from a hatchery. Total DNA was extracted from 10 mg of muscle tissue, following the protocol described in Valentini et al. (2016). The extracted DNA was amplified using the eDNA metabarcoding protocol with “teleo” primers and was sequenced using a Miseq sequencer at Fasteris facilities. The sequences thus obtained were analyzed using the ObiTools package following the same protocol used for eDNA samples, excluding the taxonomical assignation step. The most abundant sequence was retrieved for reference database construction.

At a hatchery station on the Danube Island in Vienna (https://​life-sterlet.​boku.​ac.​at/​index.​php/​the-project.​html), 3 A. baerii (total biomass 180 g), 3 A. gueldenstaedtii (180 g), 2 A. nudiventris (210 g), 30 A. ruthenus (7500 g), and 2 H. huso (140 g) specimens have been housed in a circular tank (volume = 0.9 m³, water flow through 0.5 L/s) as a part of a conservation breeding program. Using water samples collected from the tank, we evaluated our sampling protocols and the reliability of the developed assay. A single 28-L water sample was collected as described above with a 20-min filtration time. eDNA metabarcoding analysis was performed using the aforementioned procedure.