Introduction
Anguillicoloides crassus (Kuwahara et al., Reference Kuwahara and Itagaki1999) is a nematode parasite of the Anguilla japonica that also infects other Anguilla species, including the European eel Anguilla anguilla (Lefebvre et al., Reference Lefebvre, Wielgoss, Nagasawa and Moravec2012). Anguillicoloides crassus originates from East Asia, having been introduced into Europe in the early 1980s as a result of the trade in live Japanese eels, A. japonica (Temminck & Schlegel, 1847) (Laetsch et al., Reference Laetsch, Heitlinger, Taraschewski, Nadler and Blaxter2012; Weclawski et al., Reference Weclawski, Heitlinger, Baust, Klar, Petney, Han and Taraschewski2013). Anguillicoloides crassus is now well established in the Western Hemisphere and can be found in almost all European rivers and lakes, where it can tolerate salinities up to 12 ppt (Aguilar et al., Reference Aguilar, Álvarez, Leiro and Sanmartín2005; Becerra-Jurado et al., Reference Becerra-Jurado, Cruikshanks, O'Leary, Kelly, Poole and Gargan2014). While A. crassus was unlikely to have been the primary cause of the A. anguilla recruitment collapse since the 1980s, in conjunction with low recruitment, infections of the parasite may have contributed to declining adult stocks (Henderson et al., Reference Henderson, Plenty, Newton and Bird2012) and to the quality of emigrating silver eels, thereby potentially impacting on effective spawner biomass and the ability of the stock to recover (Kirk, Reference Kirk2003).
Anguillicoloides crassus reproduces sexually in the swim bladder of the eels. The eggs hatch in the female worm inside the swim bladder and L2 larvae migrate to the intestinal tract via the pneumatic duct to be excreted with the feces (Didžiulis, Reference Didžiulis2013). As part of its life cycle, A. crassus is then trophically transmitted to various intermediate hosts including several zooplankton species (especially copepods of the orders Cyclopoidea and Calanoidea) as well as planktivorous fish such as the 3-spined sticklebacks, Gasterosteus aculeatus (Linnaeus, 1758) (Kuwahara and Itagaki, Reference Kuwahara and Itagaki1999). In the intermediate host, the parasite develops into the infectious phase L4 larvae, which, once ingested, parasitize the eel as the final host. The parasite migrates from the gut system perforating the connective tissue and muscles reaching the swim bladder (Heitlinger et al., Reference Heitlinger, Laetsch, Weclawski, Han and Taraschewski2009). The number of parasites found in the swim bladder can vary from <10 to >70 individuals per eel (Jousseaume et al., Reference Jousseaume, Roussel, Beaulaton, Bardonnet, Faliex, Amilhat and Launey2021). The presence of the parasite has been shown to detrimentally affect many features of eel physiology and life history (Newbold et al., Reference Newbold, Hockley, Williams, Cable, Reading, Auchterlonie and Kemp2015). Adult nematodes feed on blood supplied to the swim bladder wall and can result in increased eel mortality as a consequence of damage caused to the organ (Schneebauer et al., Reference Schneebauer, Dirks and Pelster2017). The swim bladder wall becomes thicker, opaque and less elastic due to the perforation caused by the parasite feeding habit with an impact on buoyancy control (Weclawski et al., Reference Weclawski, Heitlinger, Baust, Klar, Petney, Han and Taraschewski2013; Barry et al., Reference Barry, Mcleish, Dodd, Turnbull, Boylan and Adams2014; Newbold et al., Reference Newbold, Hockley, Williams, Cable, Reading, Auchterlonie and Kemp2015). Anguillicoloides crassus infection is also thought to alter the physiological mechanisms involved in silvering – the process by which freshwater sub-adults adapt to life in the ocean. In this respect, infected eels have also been found to silver faster as a result of an over-production of cortisol, which seems to have a stimulatory effect on GTH2 synthesis (Muñoz et al., Reference Muñoz, Peñalver, Ruiz de Ybañez and Garcia2015; Di Biase et al., Reference Di Biase, Lokman, Govoni, Casalini, Emmanuele, Parmeggiani and Mordenti2017). Moreover, cortisol is the key hormone produced during fasting, typical of the silvering phase stage (Fazio et al., Reference Fazio, Sasal, Mouahid, Lecomte-Finiger and Moné2012). During the silvering phase, a normal increase of erythropoiesis occurs, but the parasite, due to their blood feeding behaviour, increase erythropoiesis in infected eels prior their silvering (Churcher et al., Reference Churcher, Pujolar, Milan, Huertas, Hubbard, Bargelloni and Canário2015). The presence of the parasite may impact on the eel's migration speed in rivers (Newbold et al., Reference Newbold, Hockley, Williams, Cable, Reading, Auchterlonie and Kemp2015) and in the ocean as the energy demand increases (Pelster, Reference Pelster2015), due to the reduction of the swim bladder elasticity. The presence of the parasite appears not to affect the speed and migratory behaviour during the first phase of the migration in shallow water (Simon et al., Reference Simon, Westerberg, Righton, Sjöberg and Dorow2018). However, where deep diving is required in the ocean, damage to the integrity of the swim bladder is believed to seriously impact on an infected eel's chances of survival (Lefebvre et al., Reference Lefebvre, Wielgoss, Nagasawa and Moravec2012; Righton et al., Reference Righton, Westerberg, Feunteun, Økland, Gargan, Amilhat and Aarestrup2016).
Currently accurate detection of the parasite can only be achieved via post-mortem dissection and thus requires the eel to be dissected. However, several non-lethal techniques are under development (Frisch et al., Reference Frisch, Davie, Schwarz and Turnbull2016). Anal redness can be used as an indicator for the presence or absence of the parasite, but this approach lacks both specificity and objectivity (Crean et al., Reference Crean, Dick, Evans, Elwood and Rosell2003). A radio diagnostic method has been developed to detect inflammation caused by the nematode's feeding habits (Beregi et al., Reference Beregi, Molnár, Békési and Székely1998). The method uses X-ray to scan the pneumatic duct and can detect swim bladder damage and parasite presence. The quality of the images has a large margin of error so the accuracy of detection can be low and swim bladder alterations can be caused by other factors (Beregi et al., Reference Beregi, Molnár, Békési and Székely1998). Frisch et al. (Reference Frisch, Davie, Schwarz and Turnbull2016) made improvements to the method developed by Beregi et al. (Reference Beregi, Molnár, Békési and Székely1998). Using compound radiography, they were able to detect small alterations to the thickness of the swim bladder wall and to inflations of the lumen. However, to perform a full body scan using this method, the animal is also to be euthanized. Recently, attempts have been made to develop a molecular test for A. crassus infection based in nuclear microsatellite markers (Jousseaume et al., Reference Jousseaume, Roussel, Beaulaton, Bardonnet, Faliex, Amilhat and Launey2021); however, reported sensitivity and specificity was below 71%, and the test, which involves fine-scale size discrimination of microsatellite locus sizes between target and off-target nematode species, is not easily transferred to field conditions. Finally, it is not clear from this molecular study whether feces could be sampled non-lethally (Jousseaume et al., Reference Jousseaume, Roussel, Beaulaton, Bardonnet, Faliex, Amilhat and Launey2021).
To support the assessment of eel stocks and ultimately fisheries management in the context of A. crassus, sensitive, specific and rapid non-lethal and in situ methods for pathogen detection are urgently required. Screening of translocated eel populations could, for example, limit the spread of the pathogen. Furthermore, non-lethal screening of silver eels alongside satellite tagging studies could reveal the impact of infection on the migratory and breeding success. Several non-lethal and/or molecular methods have been proposed to detect parasites in various fish species related to the food health safety chain and conservation management (Cavallero et al., Reference Cavallero, Bruno, Arletti, Caffara, Fioravanti, Costa and D'Amelio2017; Levsen et al., Reference Levsen, Svanevik, Cipriani, Mattiucci, Gay, Hastie and Pierce2018). A non-lethal qPCR-based eDNA approach has also been optimized to detect the cestode Schistocephalus solidus in samples taken by needle from the intra-peritoneal cavity of a fish (Berger and Aubin-Horth, Reference Berger and Aubin-Horth2018).
In the current study, we developed an alternate, rapid, non-lethal and portable, in situ PCR-based approach to detect A. crassus in the European eel using parasite DNA traces in fecal material. We tested the specificity and sensitivity of 2 different DNA extraction methods, the former lab-based extraction protocol, the latter more suited to the field. Using necropsy data, we were also able to explore any link between host condition and parasite infection load.
Materials and methods
Sample collection
The study was conducted at 2 different locations in the UK and Ireland. In the Burrishoole catchment, Ireland 53°55ʹ27.6ʺN 9°34ʹ27.0ʺW, yellow eels (feeding stage) were collected from Lough Feeagh (freshwater) and Furnace (tidal brackish water) using unbaited fyke nets deployed overnight in chains of 10 nets set at different lake depths in summer 2017, 2018 and 2019. Eels undergoing silvering were collected in autumn 2019 using permanent downstream river Wolf-type traps. The study was carried out under a Health Products Regulatory Authority (HPRA) license number AE19130-P096. In Lough Neagh, UK-Northern Ireland 54°36ʹ05.5ʺN 6°24ʹ55.5ʺW, yellow eels were collected with baited long lines fished overnight in the lake in summer 2018. Between capture and the procedures, eels were kept in holding tanks at the Marine Institute of the Burrishoole catchment. Under mild anaesthesia, colonic irrigation with 2 mL 0.09% sterile saline solution was performed to collect fecal material using a 5 mL syringe and a modified (needle removed) Terumo Surflo Winged Infusion Set (Fig. 1). Each colonic irrigation procedure lasted <30 s. The eels were then euthanized with an overdose of MS-222 (10 min in a 100 mg L−1 Tricaine methane sulfonate solution, FishVet Group (FVG) Ireland) followed by a cervical separation of the spinal cord. A total number of 131 eels were sampled and weight and length were recorded to the nearest 0.1 cm and gram (Supplementary Material 1). A drop of the collected wash material was placed on 1 cm2 of Whatman qualitative filter paper No. 1 and air dried for 5 min at room temperature. The air-dried paper was used to perform instant in situ DNA extraction or preserved at −80° C. The remaining wash was stored in 100% ethanol (1 wash: 9 ETOH) at −20°C. Subsequently, all eels were dissected, swim bladder inspected and the number of A. crassus present counted. Anguillicoloides crassus were collected and stored in 100% ethanol before being stored at −20° C. An eel was considered infected if at least one parasite, regardless of its lifecycle stage, was found in the swim bladder.
DNA collection and extraction methods development
DNA extraction
A total of 131 eels were sampled and fecal material was collected from all. DNA was extracted from fecal wash of 104 eels using the Qiagen stool. The Whatman extraction protocol was used in situ for eels sampled in 2019 (N = 55). To enable direct comparison between the 2 protocols, DNA was extracted from 28 eels caught in 2019 (14 in Lough Furnace and 14 in Lough Feeagh) using both Qiagen and Whatman extraction methods for each eel. DNA concentrations for Qiagen extractions are included in Supplementary Table 3.
Laboratory genomic DNA extraction
DNA from 200 μL of stored fecal material was centrifuged for 5 min at 12 000 rpm to concentrate the pellet. For each sample, 180 μL of supernatant was removed and the remaining material was extracted with a slight modification to the suggested protocol of the QIAamp Stool Kit (Qiagen, Hilden, Germania). ATL tissue lysis buffer volume was increased to 350 μL, proteinase K up to 20 μL, AL lysis buffer up to 300 μL and ethanol 100% up to 400 μL.
In situ genomic DNA extraction
A small sample of the filter paper (where fecal material had been previously deposited) of 1 mm diameter was removed by a punch from the Whatman qualitative filter paper No. 1 and DNA was extracted using adjusted extraction protocol of DNA from Whatman™ FTA™ cards (Santos et al., Reference Santos, Sasal, Verneau and Lenfant2006) (Fig. 1) (Supplementary Material 1).
Primer design, PCR conditions and species specificity
A pair of specific customized primers were designed using all 467 cytochrome c oxidase subunit 1 (COI) gene sequences available for A. crassus (NCBI). All sequences were aligned to build a consensus sequence using BioEdit version 7.0.5.3 (Hall, Reference Hall2017). The obtained consensus sequence was used to identify a conserved region within A. crassus suitable for primer design (Table 1). The designed primer pair was assayed for cross-reactivity in silico against common fish nematode parasites Camallanus sp. (NCBI Accession: EU598889), Contracaecum sp. (NCBI Accession: FJ866816) and Capillaria sp (NCBI Accession: AJ288168) (Pouder et al., Reference Pouder, Curtis and Yanong2009). The total length of the expected amplicon is 187 bp. The same PCR conditions and mastermix were used to test the efficiency and specificity of the primer using a miniPCR DNA Discovery System. The PCR Mastermix was made with 10 μL of Q5® High-Fidelity DNA Polymerase, 1 μL of FWD primer (10 nm), 1 μL of RV primer (10 nm), 0.5 μL MgCl2 (0.5 m), 6.5 μL of RNA and DNA-free water and 1 μL of extracted DNA. The total volume of the PCR reaction was 20 μL per sample. The cycle used for the PCR started with 5 min at 95°C, followed by 35 cycles of 95°C for 30 s, 60°C for 30 s and 72°C for 30 s and a last step of 10 min at 72°C. In total, 5 μL of PCR products was visualized on a 2% agarose gel using SYBR safe staining (Invitrogen). Each sample was amplified in technical triplicate alongside negative controls (ddH20) and a positive control of either 20 ng μL−1 DNA (Qiagen extraction) or A. crassus tissue crushed onto Whatman FTA card. Species specificity of the primer set was confirmed using a series of parasites collected in the same study system, various non-nematode parasites (Anisakis sp.) and other animal taxa, including the European eel, to assay cross-reactivity (Lepeophtheirus salmonis, A. anguilla, Neoparamoeba perurans, Scomber scombrus, Diphyllobothrium sp., Schistocephalus sp., Dentitruncus truttae). For each organism, 1 μL of DNA was used. To identify amplicons as A. crassus, a subset of positive amplifications were Sanger-sequenced at MRC PPU DNA Sequencing and Services, Dundee, UK.
Sensitivity, specificity, PPV and NPV
Several parameters were calculated to assay the validity of the test. Here sensitivity is defined as the ability of the test to correctly classify an individual as infected (i.e. a true positive). The ability of a test to correctly classify an individual as non-infected (i.e. a true negative) is called the test's specificity. The positive predictive value (PPV) is the percentage of eels with a positive test which are actually infected on dissection and the negative predictive value (NPV) is the percentage of eels with a negative test which do not have the parasite on dissection. PPV and NPV are directly related to the prevalence of the disease in the population (Stojanović et al., Reference Stojanović, Apostolović, Stojanović, Milošević, Toplaović, Lakušić and Golubović2014) (Table 2).
Animals that are infected and test positive are considered true positive (TP). Animals that are infected and test negative are described as false negative (FN). Animals that have no visible parasites, but test positive are false positive (FP), and those that have no visible parasites but test negative are true negative (TN).
NPV, negative predictive value; PPV, positive predictive value.
Biological validation of eel infection status
Eggs count in fecal wash
Nematode larvated and unlarvated eggs and L2 larvae were counted with a modified McMaster Salt Flotation Technique. In total, 200 μg of fecal material was diluted in 1.5 mL of distilled water. After mechanical homogenization, the suspension was poured through a 250-micron aperture sieve and the filtrate collected. After thorough mixing, the solution was transferred to a centrifuge tube and spun for 5 min at 2500 rpm. The supernatant was discarded and the remaining fecal pellet covered and homogenized with 300 μL of saturated sodium chloride solution, mixed by inverting slowly 6 times. Then, using a Pasteur pipette, the mixture was transferred to a McMaster slide. Each chamber holds 0.15 mL beneath the gridded area. The preparation is then examined using the 25× objective of a stereoscopic microscope, and the number of eggs present in the grids of both chambers was counted to give an estimate of the numbers of eggs per gram of fecal material.
Anguillicoloides crassus count in swim bladder necropsy
All dissected eels were checked for A. crassus, and where present, they were counted. The swim bladder was extracted whole from the animal and stored at 4°C until the procedure was completed for all the specimens. The swim bladder was then opened and nematodes were counted and classified to adults and larval stages. A Mann–Whitney test was performed in R studio between years of infection to test if there was significant change in the parasitic load.
Results
Rapid test in situ
The in situ non-lethal test was performed on 55 eels collected in 2019. Individuals were anally catheterized to enable colonic irrigation with a soft silicon tube without causing internal lesions. The amount of saline solution used (between 0.5 and 2 mL) varied in approximate proportion to the size of the tested animals. The procedure was deployed to minimize the invasiveness of the collection of the fecal material. In situ DNA extraction took 20 min for 16 samples, PCR reaction was undertaken over a period of 2 h and electrophoresis with gel visualization took a further 17 min. Thus, the test can be performed for 16 individuals in approximately 3 h (Fig. 1).
Comparison of different DNA extraction methods
The DNA Whatman paper extraction method provides a rapid and more reliable assessment of infection compared to the method based on the Qiagen Stool and Blood kit. Both specificity (P < 0.006) and sensitivity (P < 0.003) were shown to be significantly higher using the Whatman protocol (Fig. 2, Table 3). The resulting improvement of using the Whatman test in specificity was 46%, in sensitivity 45%, in PPV 30% and in NPV 41% (Fig. 2). Additionally, the time for DNA extraction from 1 sample using the Whatman paper as compared to a Qiagen extraction was reduced from c.80 to c.20 min.
For 2019 the same samples were tested with both methods. 2018n considers samples collected in Lough Neagh and 2019s silver eels collected in the Burrishoole catchment.
Parasite count in swim bladder and eggs count in fecal material
Fecal material from all 131 samples was tested to detect the presence of eggs and/or L2 larvae using the McMaster floatation protocol. All 131 collected swim bladders were then screened under the microscope and number of nematode eggs reported (Supplementary Material 1). No eggs or larvae were detected in any samples. Number of nematodes in the swim bladder showed an increasing trend in infection across the 3 sampling years and a significant increase in the silver eels collected in 2019 (Fig. 3).
Discussion
Our study represents the first attempt to develop a sensitive, non-lethal and, importantly, in situ method to establish A. crassus infection in A. anguilla via the detection of parasite DNA in fecal material. High values for NPV (87%) and PPV (95%) suggest the test may have a useful role in both veterinary and fisheries management contexts. We found inter-annual differences in the prevalence of infected eels in the 3 years we sampled in the Burrishoole catchment with the total number of infected animals significantly higher in 2019.
Sensitivity is a key consideration for any molecular test. Mitochondrial genes are the major target genes in PCR-based detection systems because they are highly conserved and present in multiple copies (Paoletti et al., Reference Paoletti, Mattiucci, Colantoni, Levsen, Gay and Nascetti2018). High target copy number may explain the high sensitivity of the test we deployed. The mitochondrial gene COI has been widely used to detect the presence of nematode parasites in commercially important fish species (Santos et al., Reference Santos, Sasal, Verneau and Lenfant2006; Herrero et al., Reference Herrero, Vieites and Espiñeira2011; Godínez-González et al., Reference Godínez-González, Roca-Geronès, Cancino-Faure, Montoliu and Fisa2017; Paoletti et al., Reference Paoletti, Mattiucci, Colantoni, Levsen, Gay and Nascetti2018). The use of microsatellites is also a well-established method for parasite detection (Vieira et al., Reference Vieira, Santini, Diniz and de Munhoz2016), although these nuclear markers can suffer from lower sensitivity than their mitochondrial counterparts, which may contribute to their poorer performance in detecting A. crassus in eels (Jousseaume et al., Reference Jousseaume, Roussel, Beaulaton, Bardonnet, Faliex, Amilhat and Launey2021).
Some improvement in detecting sensitivity and specificity was achieved here by adopting a more ‘crude’ nucleic acid extraction approach using a Whatman paper. Nucleic acid extraction is increasingly recognized as a major rate limiting step in molecular diagnostics; however, paper-based options offer several advantages in terms of speed and cost (Zou et al., Reference Zou, Mason, Wang, Wee, Turni, Blackall and Botella2017), as seems to be the case in our study. Nonetheless, our final protocol did show both false positives and false negatives, albeit at a low rate. False negatives likely relate to issues with template purification and PCR amplification, or potentially the reduced biomass of younger worms (Barry et al., Reference Barry, Mcleish, Dodd, Turnbull, Boylan and Adams2014). Similarly juvenile, un-mated worms are likely to shed less genetic material in the form of larvae. False positives could indicate the presence of early infections, not yet detectable via necropsy – and further investigation of such cases is warranted. It is not clear whether the DNA we are detecting originates from embryonated eggs, cellular material or free DNA shed from the worms. Our inability to microscopically detect the presence of A. crassus larvae or eggs in fecal material suggests that the DNA or cellular fragments from worms are the likely source. However, our use of ethanol as a fixative for storing samples could have played a role in our low success in detecting eggs or larvae (Crawley et al., Reference Crawley, Chapman, Lummaa and Lynsdale2016).
The test we present relies on a simple PCR, not qPCR. Nonetheless, validation against ‘real’ infection levels assayed via necropsy reveals excellent specificity and sensitivity. Point-of-care qPCR for viral pathogens can now deliver a result in <20 min (Melchers et al., Reference Melchers, Kuijpers, Sickler and Rahamat-Langendoen2017). Similarly, several mobile qPCR instruments have been brought to the market and have been successfully deployed to deliver veterinary diagnoses in remote locations on actionable timescales for cattle (Hole and Nfon, Reference Hole and Nfon2019). However, the cost of such approaches may be prohibitive in respect to their application to the detection of pathogens fish. Our experimental set-up, which fits in a carry-on suitcase and can be performed in the field powered with a portable battery, shows that standard PCR, using low-cost reagents and equipment, may be just as portable, and informative epidemiologically, as ‘higher-end’ devices, although benchmarking against a portable qPCR device could be a focus of future study.
Stocking, as part of eel population enhancement, is likely a major contributor to A. crassus dispersal, as are translocations associated with the trade in live eels (Laetsch et al., Reference Laetsch, Heitlinger, Taraschewski, Nadler and Blaxter2012; Weclawski et al., Reference Weclawski, Heitlinger, Baust, Klar, Petney, Han and Taraschewski2013). Screening of such individuals and early detection with a non-lethal method could be a powerful tool to avoid the spread of the parasite. However, there remains a need to clarify whether our approach has enough sensitivity to detect infection in glass eels and elvers. Anguillicoloides crassus is known to infect the elvers or European eels (Haenen et al., Reference Haenen, Grisez, De Charleroy, Belpaire and Ollevier1989) and natural infection has been detected in late-stage glass eels as well as elvers of the American eel Anguilla rostrata (Hein et al., Reference Hein, de Buron, Roumillat, Post, Hazel and Arnott2016). Both juvenile stages are a major component of stocking biomass. Advances in sample pooling designs and detection algorithms during the recent coronavirus epidemic can achieve individual-level identification using a 7-fold lower number of tests than the number of individuals (Shental et al., Reference Shental, Levy, Wuvshet, Skorniakov, Shalem, Ottolenghi and Hertz2020). Such algorithms could also be adapted to screen large cohorts of eels, but regulation and legislation may be required before industry agrees to bear the associated cost.
The increase in parasite load we noted from 2017 to 2019 follows a trend that is also found all over Europe, where the parasite is established and is fast colonizing all the freshwater basins (Aguilar et al., Reference Aguilar, Álvarez, Leiro and Sanmartín2005; Schabuss et al., Reference Schabuss, Kennedy, Konecny, Grillitsch, Schiemer and Herzig2005; Wielgoss et al., Reference Wielgoss, Taraschewski, Meyer and Wirth2008; Selim and El-ashram, Reference Selim and El-ashram2012). Anguillicoloides crassus has a very recent history in the Burrishoole catchment. First detection occurred in 2010 in a yellow eel in brackish water and in 2016 for the first time in a silver eel from freshwater (R. Poole, personal communication). In contrast to the rising burdens across much of Europe, in some lakes where the parasite had been detected since first discovery, there is stabilization and even a slight decline in nematode abundance and intensities (Wielgoss et al., Reference Wielgoss, Taraschewski, Meyer and Wirth2008). There is a possibility of an increased resistance towards the parasites in the long term (Schabuss et al., Reference Schabuss, Kennedy, Konecny, Grillitsch, Schiemer and Herzig2005). Although some evidence of increasing tolerance of A. anguilla to parasite infection, the overall impact of the parasite on the eel's mortality has been severe and is likely a contributor to the European population's steep decline impeding a recovery (Molnar et al., Reference Molnar, England and Martinod1993; Kirk, Reference Kirk2003; Schabuss et al., Reference Schabuss, Kennedy, Konecny, Grillitsch, Schiemer and Herzig2005). Treatment of infected eels with anti-helminthic has not been trialled, and a single vaccination study aimed at reducing the development of adult from irradiated L3 larvae was unsuccessful and revealed the antibody response is not a key element in the resistance of A. anguilla against A. crassus (Knopf and Lucius, Reference Knopf and Lucius2008). Infection control via physically blocking transmission, which requires extensive diagnostic testing, therefore represents the only feasible route to reducing population-wide parasite burden.
In this study, we developed potentially useful tool that can be deployed for specific parasite screening for the European eel. Cost per sample is low and the time to run a test comprising 16 samples is under 3 h. Our test offers managers the opportunity to engage in infection control by assessing the disease status of adult eels before allowing transfers between river systems, although further work is required to establish whether it can survey juveniles. Nonetheless, the rapid test represents an important contribution to the conservation and management of this critically endangered species.
Supplementary material
The supplementary material for this article can be found at https://doi.org/10.1017/S0031182021002146.
Data
All data generated or analysed during this study are included in this published article. The dataset supporting the conclusions of this article is available in the Supplementary material section. Supplementary Table 1 reports all the data collected, Supplementary Table 2 the DNA extraction protocol and Supplementary Table 3 the DNA concentration of the fecal material extracted with the Qiagen method.
Acknowledgements
We would like to express our sincere gratitude to Dr Derek Evans who provided the samples from Lough Neagh, to Sara Gandy for the support in statistical analysis and to all the members of the Marine Institute in Newport, Ireland, for the immense help during sampling.
Author contributions
M.D.N. collected the data, analysed and wrote the manuscript draft. R.P. and J.K. helped with data collection and analysis. C.W. supported the data collection and experimental set up. C.A. and P.M. supervised the data collection and analysis. M.L. supervised the overall project, data analysis and writing of the manuscript. All authors read and approved the final manuscript.
Financial support
This research was supported in part by a research grant from the BBSRC (grant number BB/P001203/1), by Science Foundation Ireland, the Marine Institute, Ireland (Beyond 2020 program) and the Department for the Economy, Northern Ireland, under the Investigators Program grant number SFI/15/IA/3028.
Conflict of interest
None.
Ethical standards
The study was carried out under a Health Products Regulatory Authority (HPRA) license number AE19130-P096.