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Natural variation in host-finding behaviour of gastropod parasitic nematodes (Phasmarhabditis spp.) exposed to host-associated cues

Published online by Cambridge University Press:  24 February 2021

J. Cutler  and
R. Rae Open the ORCID record for R. Rae [Opens in a new window]
J. Cutler
Affiliation:
School of Biological and Environmental Sciences, Liverpool John Moores University, Byrom Street, LiverpoolL33AF, UK
R. Rae*
Affiliation:
School of Biological and Environmental Sciences, Liverpool John Moores University, Byrom Street, LiverpoolL33AF, UK
*
Author for correspondence: R. Rae, E-mail: r.g.rae@ljmu.ac.uk
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Abstract

The gastropod parasitic nematode Phasmarhabditis hermaphrodita has been formulated into a successful biological control agent (Nemaslug®, strain DMG0001) used to kill slugs on farms and gardens. When applied to soil, P. hermaphrodita uses slug mucus and faeces to find potential hosts. However, there is little information on what cues other species of Phasmarhabditis (P. neopapillosa and P. californica) use to find hosts and whether there is natural variation in their ability to chemotax to host cues. Therefore, using chemotaxis assays, we exposed nine wild isolates of P. hermaphrodita, five isolates of P. neopapillosa and three isolates of P. californica to mucus from the pestiferous slug host Deroceras invadens, as well as 1% and 5% hyaluronic acid – a component of slug mucus that is highly attractive to these nematodes. We found P. hermaphrodita (DMG0010) and P. californica (DMG0018) responded significantly more to D. invadens mucus and 1% hyaluronic acid than other strains. Also, P. hermaphrodita (DMG0007), P. neopapillosa (DMG0015) and P. californica (DMG0017) were superior at locating 5% hyaluronic acid compared to other isolates of the same genera. Ultimately, there is natural variation in chemoattraction in Phasmarhabditis nematodes, with some strains responding significantly better to host cues than others.

Keywords

ChemotaxisPhasmarhabditis hermaphroditaDeroceras invadensnatural variationCaenorhabditis elegansbehaviour
Type
Research Paper
Information
Journal of Helminthology , Volume 95 , 2021 , e10
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution, and reproduction in any medium, provided the original work is properly cited.
Copyright
Copyright © The Author(s), 2021. Published by Cambridge University Press

Introduction

Parasitic nematodes use many diverse cues exuded from hosts to ensure successful infection (Lee, Reference Lee and Lee2002). For example, Howardula aoronymphium parasitizes the mushroom fly (Drosophila fallen) and is attracted to mushroom-derived odorants such as 3-octanone and 1-octen-3-one (Cevallos et al., Reference Cevallos, Okubo, Perlman and Hallem2017). The mammalian parasite Heligmosomoides polygyrus is attracted to mouse faeces and compounds such as geranyl acetone and 2-butanone and averted from carbon dioxide (Ruiz et al., Reference Ruiz, Castelletto, Gang and Hallem2017). Entomopathogenic nematodes (Steinernema carpocapsae and Heterorhabditis bacteriophora), which are lethal pathogens of insects, are attracted to different host-derived compounds. For example, Hallem et al. (Reference Hallem, Dillman, Hong, Zhang, Yano, DeMarco and Sternberg2011) found S. carpocapsae was attracted to propanoic acid and hexanal, 2,3-butanedione (as well as others), yet H. bacteriophora was only attracted to 1-propanol. The relationships between olfaction of parasitic nematodes and hosts are poorly understood (Cevallos et al., Reference Cevallos, Okubo, Perlman and Hallem2017); hence, we are attempting to develop a model nematode (Rae, Reference Rae2017) to elucidate the molecular nature of host location by parasites. The model we propose is the slug and snail parasite Phasmarhabditis hermaphrodita, which has been successfully formulated into a biological control agent (Nemaslug®) to kill pestiferous gastropods on farms and gardens (Rae et al., Reference Rae, Verdun, Grewal, Robertson and Wilson2007). Nematodes are mixed with water and sprayed on to soil where they locate and kill slugs in 4–21 days (Wilson et al., Reference Wilson, Glen and George1993; Tan & Grewal, Reference Tan and Grewal2001). The host cues P. hermaphrodita uses to find gastropods have been studied in detail. In agar-based chemotaxis assays, the nematodes positively chemotax towards slug and snail mucus and faeces (Rae et al., Reference Rae, Robertson and Wilson2006, Reference Rae, Robertson and Wilson2009; Hapca et al., Reference Hapca, Budha, Crawford and Young2007a, Reference Hapca, Crawford, Rae, Wilson and Youngb; Andrus et al., Reference Andrus, Ingle, Coleman and Rae2018; Andrus & Rae, Reference Andrus and Rae2019a). They have also been shown to be attracted to alive and dead slugs in soil-based experiments (MacMillan et al., Reference MacMillan, Haukeland, Rae, Young, Crawford, Hapca and Wilson2009; Nermut’ et al., Reference Nermut’, Půža and Mráček2012). Mucus from some slug species is more attractive to P. hermaphrodita than others. More specifically, Rae et al. (Reference Rae, Robertson and Wilson2009) showed that P. hermaphrodita was strongly attracted to mucus from slugs such as Arion subfuscus, but less attracted to Limax marginatus and the snail Cepaea hortensis (for reasons unknown). Small & Bradford (Reference Small and Bradford2008) recorded a selection of behaviours when P. hermaphrodita came in contact with mucus from six gastropod species, including forward crawling, head thrusting and head waving, but observed few differences between species. In order to investigate the specific components of slug mucus that the nematodes are attracted to, Andrus et al. (Reference Andrus, Ingle, Coleman and Rae2018) showed that Phasmarhabditis nematodes were strongly attracted to hyaluronic acid – a common component of slug mucus, in a dose-dependent manner.

The majority of chemotaxis experiments using P. hermaphrodita have concentrated on studying one strain, designated ‘DMG0001’ by Hooper et al. (Reference Hooper, Wilson, Rowe and Glen1999), which has been used in commercial production by BASF Agricultural Specialities since 1994 and sold as Nemaslug®. There is little information about whether there is natural variation in chemoattraction of not just wild strains of P. hermaphrodita but any of the 12 other species in the Phasmarhabditis genus (P. bohemica, P. circassica, P. clausilliae, P. meridionalis, P. apuliae, P. bonaquaense, P. californica, P. safricana, P. huizhouensis, P. neopapillosa, P. papillosa and P. tawfiki) (Tandingan De Ley et al., Reference Tandingan De Ley, McDonnell, Paine, De Ley, Abd-Elgawad, Askary and Coupland2017; Ivanova et al., Reference Ivanova, Geraskina and Spiridonov2020). One study (Andrus & Rae, Reference Andrus and Rae2019a) reported natural variation in the chemoattraction of P. hermaphrodita, P. californica and P. neopapillosa to certain slug species. For example, P. hermaphrodita isolates differed in their preference of slug species but P. neopapillosa preferred Arion sp. However, there is little information about whether these species differ in their response to mucus from a single slug species or other attractants like hyaluronic acid.

From sampling and dissecting slugs from the UK, we have isolated numerous strains of P. hermaphrodita, P. californica and P. neopapillosa, which are in culture at Liverpool John Moores University (LJMU) (for further information, see Andrus & Rae, Reference Andrus and Rae2019b). To understand whether there is natural variation in the ability of these nematodes to chemotax to slug mucus and associated cues, we exposed nine isolates of P. hermaphrodita (including the commercial strain DMG0001), five isolates of P. neopapillosa and three isolates of P. californica to mucus from the pestiferous slug Deroceras invadens (Hutchinson et al., Reference Hutchinson, Reise and Robinson2014), which is a common host for these nematodes (Andrus & Rae, Reference Andrus and Rae2019b), as well as two concentrations of hyaluronic acid (1% and 5%). Ultimately, this will unravel whether behavioural mechanisms responsible for host chemoattraction in the Phasmarhabditis genus are under selective pressure.

Materials and methods

Source of invertebrates

Phasmarhabditis hermaphrodita (strains DMG0002, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (strains DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (strains DMG0017, DMG0018 and DMG0019) were isolated from slugs from a small survey conducted in 2014 around the UK, and were positively identified using molecular biology (see Andrus & Rae, Reference Andrus and Rae2019b). They have been kept in culture in LJMU fed on dead Limax flavus on White traps (White, Reference White1927; Andrus & Rae, Reference Andrus and Rae2019b). For the experiments, each nematode isolate was grown on fresh White traps for 21 days until they were at the dauer stage and stored in tissue culture flasks until use. The commercial strain of P. hermaphrodita (DMG0001) was purchased from BASF Agricultural Specialities, Littlehampton, UK and stored at 10°C until use. Deroceras invadens were collected from Sefton Park in Liverpool and stored in non-airtight plastic boxes lined with moist paper at 15°C until use.

Chemotaxis assay

A chemotaxis assay was used to assess the ability of Phasmarhabditis nematodes to locate slug mucus and hyaluronic acid (Rae et al., Reference Rae, Robertson and Wilson2006, Reference Rae, Robertson and Wilson2009; Andrus et al., Reference Andrus, Ingle, Coleman and Rae2018). Briefly, 10 cm Petri dishes were half filled with 1.2% technical agar and left to solidify. A 1 cm2 piece of Whatman number 1 filter paper was placed 0.5 cm from the edge of the Petri dish and 10 μl of distilled water was added and acted as the control. Another piece of filter paper (same size) was placed equidistant from the control after being used to swab 0.01 g of mucus from adult D. invadens (or 10 μl of 1% or 5% hyaluronic acid was added). Approximately 50 dauer larvae of each Phasmarhabditis isolate were added to the middle of each Petri dish. They were then sealed with Parafilm® and stored at 20°C overnight. The following morning, the numbers of nematodes that had graduated to the control or treated piece of filter paper were quantified (as well as those that remained in the middle). For each isolate of Phasmarhabditis, three Petri dishes were used to test the response to D. invadens mucus or hyaluronic acid (1% or 5%) and each experiment was repeated three times (nine dishes per isolate).

Statistical analysis

The numbers of Phasmarhabditis nematodes found in the mucus or hyaluronic acid (1% or 5%) versus water was analysed using a Student's t test. To understand which Phasmarhabditis strain responded strongest to mucus or hyaluronic acid (1% or 5%), the numbers of nematodes found in each treatment from each species was compared using a one-way analysis of variance with Tukey's post-hoc test.

Results

Natural variation in the ability of Phasmarhabditis nematodes to chemotax to D. invadens mucus

There were significantly more P. hermaphrodita (DMG0001, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (DMG0017, DMG0018 and DMG0019) found in the D. invadens mucus compared to the water control (fig. 1) (P < 0.05). However, this was not the case for P. hermaphrodita (DMG0002), as there was no significant difference in the number of nematodes found on each side (fig. 1) (P > 0.05).

Fig. 1. The mean number of Phasmarhabditis hermaphrodita (DMG0001, DMG0002, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (DMG0017, DMG0018 and DMG0019) found in filter paper with water (control) (white bars), in the middle of the agar plate (black bars) or in filter paper with 0.01 g Deroceras invadens mucus (grey bars). Significant differences between the number of nematodes found in the mucus or water are denoted with * for P < 0.05 and ** for P < 0.001. Different letters denote a significant difference at P < 0.05 between the strains of each Phasmarhabditis species found in mucus. Bars represent ± one standard error.

Of all the P. hermaphrodita isolates tested, isolate DMG0010 chemotaxed significantly more to D. invadens mucus compared to P. hermaphrodita (DMG0001, DMG0002, DMG0003, DMG0005, DMG0008, DMG0009 and DMG0011) (P < 0.05) (fig. 1).

There was no difference in the numbers of P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) that were found in the D. invadens mucus (P > 0.05) (fig. 1).

Significantly more P. californica (DMG0018) were found in the D. invadens mucus than P. californica (DMG0019) (P > 0.05) (fig. 1), but no difference was found between P. californica (DMG0017) (P < 0.05).

Natural variation in the ability of Phasmarhabditis nematodes to chemotax to 1% hyaluronic acid

Phasmarhabditis hermaphrodita (DMG0001, DMG0002, DMG0007, DMG0008, DMG0009 and DMG0011) responded positively to 1% hyaluronic acid, with significantly more nematodes found in the treated filter paper compared to the control (P < 0.05) (fig. 2a). However, there was no difference between the numbers of P. hermaphrodita (DMG0010, DMG0003 and DMG0005) in the 1% hyaluronic acid compared to the water control (P > 0.05) (fig. 2a). Although there was no significant difference between the numbers of P. hermaphrodita (DMG0010) in the mucus and water, this strain reacted more to the 1% hyaluronic acid than P. hermaphrodita (DMG0002, DMG0003 and DMG0008) (P < 0.05) (fig. 2a).

Fig. 2. The mean number of Phasmarhabditis hermaphrodita (DMG0001, DMG0002, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (DMG0017, DMG0018 and DMG0019) found in filter paper with water (control) (white bars), in the middle of the agar plate (black bars) or in 1% (A) or 5% (B) hyaluronic acid (grey bars). Significant differences between the number of nematodes found in hyaluronic acid or water are denoted with * for P < 0.05 and ** for P < 0.001. Different letters denote a significant difference at P < 0.05 between the strains of each Phasmarhabditis species found in hyaluronic acid. Bars represent ± one standard error.

Significantly more P. neopapillosa (DMG0012, DMG0013 and DMG0015) were found in the 1% hyaluronic acid compared to the control (P < 0.05) (fig. 2a); however, there was no significant difference between the numbers of P. neopapillosa (DMG0014 and DMG0016) in the hyaluronic acid or water control (P > 0.05) (fig. 2a). Of the P. neopapillosa strains tested, significantly more P. neopapillosa (DMG012) were found in the 1% hyaluronic acid than P. neopapillosa (DMG0016) (P < 0.05) (fig. 2a). There was no difference between the numbers of P. neopapillosa (DMG0013, DMG0014 and DMG0015) found in 1% hyaluronic acid (P > 0.05) (fig. 2a).

Only P. californica (DMG0018) significantly chemotaxed to 1% hyaluronic acid compared to water (P < 0.05) (fig. 2a). There was no difference between the numbers of P. californica (DMG0017 and DMG0019) found on each side (P > 0.05) (fig. 2a). There was no difference in the numbers of P. californica (DMG0017, DMG0018 and DMG0019) found in the 1% hyaluronic acid (P > 0.05) (fig. 2a).

Natural variation in the ability of Phasmarhabditis nematodes to chemotax to 5% hyaluronic acid

When exposed to 5% hyaluronic acid, all isolates of all Phasmarhabditis species tested were found significantly more in the hyaluronic acid compared to the water control (P < 0.05) (fig. 2b).

Significantly more P. hermaphrodita (DMG0007) were found in 5% hyaluronic acid compared to P. hermaphrodita (DMG0002, DMG0003, DMG0008 and DMG0011) (P < 0.05) (fig. 2b). Also, there were significantly more P. hermaphrodita (DMG0009) found in the 5% hyaluronic acid than P. hermaphrodita (DMG0002 and DMG0011) (P < 0.05) (fig. 2b).

From the P. neopapillosa isolates tested, strain DMG0015 was found significantly more in the 5% hyaluronic acid compared to the others (DMG0012, DMG0013, DMG0014 and DMG0016) (P < 0.05) (fig. 2b).

This was also the case with the P. californica isolates tested, where one strain (DMG0017) was found significantly more in the 5% hyaluronic acid compared to the others (DMG0018 and DMG0019) (P < 0.01) (fig. 2b).

Discussion

When exposed to mucus from D. invadens, P. hermaphrodita (DMG010) and P. californica (DMG0018) were found significantly more in D. invadens mucus than the other strains tested, suggesting that they are perhaps better at finding hosts. There was also natural variation in chemotaxis observed when we repeated the experiments with hyaluronic acid (1% and 5%), which is a common attractant for other parasites such as the trematode Acanthostomum brauni and the protozoan Plasmodium falciparum (Haas & Ostrowskide de Núñez, Reference Haas and Ostrowskide de Núñez1988; Beeson et al., Reference Beeson, Rogerson, Cooke, Reeder, Chai, Lawson, Molyneux and Brown2000). At 1% hyaluronic acid, significantly more P. hermaphrodita (DMG0010), P. neopapillosa (DMG0012) and P. californica (DMG0018) were found in the attractant than the other strains of the same genus. When given the choice of 5% hyaluronic acid or water, P. hermaphrodita (DMG0007), P. neopapillosa (DMG0015) and P. californica (DMG0017) were found significantly more in the attractant than other strains of the same genus. Natural variation in chemoattraction has been shown in parasitic and genetic model nematodes. For example, Laznik & Trdan (Reference Laznik and Trdan2013) demonstrated differences in attraction to damaged maize-derived β-caryophyllene by H. bacteriophora strain D54 and S. carpocapsae B49, but Steinernema kraussei C46 only showed weak attraction and Steinernema feltiae (two strains) exhibited no attraction. Strains of Caenorhabditis elegans differ in their evasion response when exposed to the pathogen Bacillus thuringiensis (Schulenburg & Müller, Reference Schulenburg and Müller2004). Also, Hong et al. (Reference Hong, Witte and Sommer2008) reported natural variation in chemotaxis of 19 strains of the scarab-beetle-associated nematode Pristionchus pacificus exposed to insect pheromones E-11-tetradecenyl acetate (EDTA) and Z-7-tetradece-2-one (ZTDO). Similarly, McGaughran et al. (Reference McGaughran, Morgan and Sommer2013) reported significant variation in the chemoattraction of 21 P. pacificus strains to organic compounds, beetle washes and live beetles from several island locations.

The strain of P. hermaphrodita (DMG0001) used in the production of Nemaslug® has been commercially produced since 1994, fed on a diet of the bacterium Moraxella osloensis (Rae et al., Reference Rae, Verdun, Grewal, Robertson and Wilson2007). This strain is lethal to pestiferous gastropods such as D. invadens (Williams & Rae, Reference Williams and Rae2015), yet in our experiments it did not respond as well as some wild isolates to slug mucus. This is contrary to previous research (Rae et al., Reference Rae, Robertson and Wilson2009) that used the same assay with the same strain and slug species and found that approximately 40% of the nematodes graduated towards the mucus. Perhaps after over ten years of being grown in industrial fermenters the chemotactic response of P. hermaphrodita has diminished or perhaps the population of D. invadens used in our study (collected from Liverpool) were more attractive than those from Aberdeen (for some unknown reason). Nevertheless, by taking our approach and testing chemotaxis behaviour, strains with superior host-finding behaviour could be collected and developed as biological control agents.

The relationships between olfaction of parasitic nematodes and hosts warrants further attention (Cevallos et al., Reference Cevallos, Okubo, Perlman and Hallem2017). We propose to address this using our model nematode P. hermaphrodita. Although understudied in terms of genetics and genomics, it has a plethora of attributes that make it an excellent model for olfaction of parasitic nematodes. First, it can be isolated easily, facilitating analysis of natural variation at the inter- and intra-species level. Second, it is a facultative parasite yet can be kept in culture on agar plates or under ‘semi-natural’ conditions fed rotting slug (Andrus & Rae, Reference Andrus and Rae2019b). Third, there are multiple studies, inspired by chemoattraction work by C. elegans (e.g. Bargmann et al., Reference Bargmann, Hartwieg and Horvitz1993), examining the olfactory response of P. hermaphrodita (and closely related Phasmarhabditis species) towards slug mucus (Rae et al., Reference Rae, Robertson and Wilson2006, Reference Rae, Robertson and Wilson2009; Hapca et al., Reference Hapca, Budha, Crawford and Young2007a, Reference Hapca, Crawford, Rae, Wilson and Youngb; Andrus & Rae, Reference Andrus and Rae2019a) and snail mucus (Andrus et al., Reference Andrus, Ingle, Coleman and Rae2018) using agar plates and in more realistic soil conditions (Nermut’ et al., Reference Nermut’, Půža and Mráček2012; MacMillan et al., Reference MacMillan, Haukeland, Rae, Young, Crawford, Hapca and Wilson2009). Specific components of slug mucus – for example, hyaluronic acid – have been shown to be strong attractants to these nematodes (Andrus et al., Reference Andrus, Ingle, Coleman and Rae2018; this study), which will allow in-depth analysis of how this compound can affect olfaction at a neurobiological and genomic level. Interestingly, there are similarities in the genetic mechanisms C. elegans and P. pacificus use to find food and hosts, respectively, as they both rely on the protein kinase EGL-4 (Hong et al., Reference Hong, Witte and Sommer2008; Kroetz et al., Reference Kroetz, Srinivasan, Yaghoobian, Sternberg and Hong2012). Chemoattraction in P. hermaphrodita towards snail mucus was enhanced by exogenous exposure to cyclic guanosine monophosphate, which activates EGL-4 (Andrus et al., Reference Andrus, Ingle, Coleman and Rae2018). Therefore, we believe P. hermaphrodita (and other Phasmarhabditis nematodes) could be used as a parasitic comparison to closely related non-parasitic species such as C. elegans and P. pacificus to examine the evolution of parasitic behaviours at the molecular and neurobiological level.

Acknowledgements

We are grateful to Tom Goddard, Jack Shepherd, Craig Wilding and Will Swaney for their discussions.

Financial support

This research was funded by BASF Agricultural Specialities.

Conflicts of interest

None.

References

Andrus, P and Rae, R (2019a) Natural variation in chemoattraction of Phasmarhabditis hermaphrodita, Phasmarhabditis neopapillosa and Phasmarhabditis californica exposed to slug mucus. Nematology 21, 479488.CrossRefGoogle Scholar
Andrus, P and Rae, R (2019b) Development of Phasmarhabditis hermaphrodita (and members of the Phasmarhabditis genus) as new genetic model nematodes to study the genetic basis of parasitism. Journal of Helminthology 2, 113.Google Scholar
Andrus, P, Ingle, O, Coleman, T and Rae, R (2018) Gastropod parasitic nematodes (Phasmarhabditis sp.) are attracted to hyaluronic acid in snail mucus by cGMP signalling. Journal of Helminthology 94, e9.CrossRefGoogle ScholarPubMed
Bargmann, CI, Hartwieg, E and Horvitz, HR (1993) Odorant-selective genes and neurons mediate olfaction in C. elegans. Cell 74, 515527.CrossRefGoogle ScholarPubMed
Beeson, JG, Rogerson, SJ, Cooke, BM, Reeder, JC, Chai, W, Lawson, AM, Molyneux, ME and Brown, GV (2000) Adhesion of Plasmodium falciparum-infected erythrocytes to hyaluronic acid in placental malaria. Nature Medicine 6, 8690.CrossRefGoogle ScholarPubMed
Cevallos, JA, Okubo, RP, Perlman, SJ and Hallem, EA (2017) Olfactory preferences of the parasitic nematode Howardula aoronymphium and its insect host Drosophila falleni. Journal of Chemical Ecology 43, 362373.CrossRefGoogle ScholarPubMed
Haas, W and Ostrowskide de Núñez, M (1988) Chemical signals of fish skin for the attachment response of Acanthostomum brauni cercariae. Parasitological Research 74, 552557.CrossRefGoogle ScholarPubMed
Hallem, EA, Dillman, AR, Hong, AV, Zhang, Y, Yano, JM, DeMarco, SF and Sternberg, PW (2011) A sensory code for host seeking in parasitic nematodes. Current Biology 21, 377383.CrossRefGoogle ScholarPubMed
Hapca, S, Budha, P, Crawford, J and Young, I (2007a) Movement of Phasmarhabditis hermaphrodita nematode in heterogeneous structure. Nematology 95, 731738.Google Scholar
Hapca, S, Crawford, J, Rae, R, Wilson, M and Young, I (2007b) Movement of the parasitic nematode Phasmarhabditis hermaphrodita in the presence of the slug Deroceras reticulatum. Biological Control 41, 223229.CrossRefGoogle Scholar
Hong, RL, Witte, H and Sommer, RJ (2008) Natural variation in Pristionchus pacificus insect pheromone attraction involves the protein kinase EGL-4. Proceedings of the National Academy of Sciences of the United States of America 105, 77797784.CrossRefGoogle ScholarPubMed
Hooper, DJ, Wilson, MJ, Rowe, JA and Glen, DM (1999) Some observations on the morphology and protein profiles of the slug parasitic nematodes Phasmarhabditis hermaphrodita and P. neopapillosa (Nematoda: Rhabditidae). Nematology 1, 173182.CrossRefGoogle Scholar
Hutchinson, J, Reise, H and Robinson, D (2014) A biography of an invasive terrestrial slug: the spread, distribution and habitat of Deroceras invadens. NeoBiota 23, 1764.CrossRefGoogle Scholar
Ivanova, ES, Geraskina, AP and Spiridonov, SE (2020) Two new species of Phasmarhabditis Andrássy, 1976 (Nematoda: Rhabditiae) associated with land snails in Northwest Caucasus, Russian Federation: description and molecular affiliation. Nematology 22, 179197.CrossRefGoogle Scholar
Kroetz, SM, Srinivasan, J, Yaghoobian, J, Sternberg, PW and Hong, RL (2012) The cGMP signalling pathway affects feeding behaviour in the necromenic nematode Pristionchus pacificus. PLoS One 7, e34464.CrossRefGoogle ScholarPubMed
Laznik, Ž and Trdan, S (2013) An investigation on the chemotactic responses of different entomopathogenic nematode strains to mechanically damaged maize root volatile compounds. Experimental Parasitology 134, 349355.CrossRefGoogle ScholarPubMed
Lee, D (2002) Behaviour. pp. 369388 in Lee, D (Ed) The biology of nematodes. Boca Raton, CRC Press.CrossRefGoogle Scholar
MacMillan, K, Haukeland, S, Rae, RG, Young, IM, Crawford, JW, Hapca, S and Wilson, MJ (2009) Dispersal patterns and behaviour of the nematode Phasmarhabditis hermaphrodita in mineral soils and organic media. Soil Biology and Biochemistry 41, 14831490.CrossRefGoogle Scholar
McGaughran, A, Morgan, K and Sommer, RJ (2013) Natural variation in chemosensation: lessons from an island nematode. Ecology and Evolution 3, 52095224.CrossRefGoogle ScholarPubMed
Nermut’, J, Půža, V and Mráček, Z (2012) The response of Phasmarhabditis hermaphrodita (Nematoda: Rhabditidae) and Steinernema feltiae (Nematoda: Steinernematidae) to different host-associated cues. Biological Control 61, 201206.CrossRefGoogle Scholar
Rae, R (2017) Phasmarhabditis hermaphrodita – a new model to study the genetic evolution of parasitism. Nematology 19, 375387.CrossRefGoogle Scholar
Rae, RG, Robertson, JF and Wilson, MJ (2006) The chemotactic response of Phasmarhabditis hermaphrodita (Nematoda: Rhabditidae) to cues of Deroceras reticulatum (Mollusca: Gastropoda). Nematology 8, 197200.Google Scholar
Rae, R, Verdun, C, Grewal, PS, Robertson, JF and Wilson, MJ (2007) Biological control of terrestrial molluscs using Phasmarhabditis hermaphrodita-progress and prospects. Pest Management Science 63, 11531164.CrossRefGoogle ScholarPubMed
Rae, RG, Robertson, JF and Wilson, MJ (2009) Chemoattraction and host preference of the gastropod parasitic nematode Phasmarhabditis hermaphrodita. Journal of Parasitology 95, 517526.CrossRefGoogle ScholarPubMed
Ruiz, F, Castelletto, ML, Gang, SS and Hallem, EA (2017) Experience-dependent olfactory behaviors of the parasitic nematode Heligmosomoides polygyrus. PLoS Pathogens 13, e1006709.CrossRefGoogle ScholarPubMed
Schulenburg, H and Müller, S (2004) Natural variation in the response of Caenorhabditis elegans towards Bacillus thuringiensis. Parasitology 128, 433443.CrossRefGoogle ScholarPubMed
Small, R and Bradford, C (2008) Behavioural responses of Phasmarhabditis hermaphrodita (Nematoda: Rhabditida) to mucus from potential hosts. Nematology 10, 591598.CrossRefGoogle Scholar
Tan, L and Grewal, PS (2001) Infection behaviour of the rhabditid nematode Phasmarhabditis hermaphrodita to the grey garden slug Deroceras reticulatum. Journal of Parasitology 87, 13491354.CrossRefGoogle ScholarPubMed
Tandingan De Ley, I, McDonnell, R, Paine, TD and De Ley, P (2017) Phasmarhabditis: the slug and snail parasitic nematodes in North America. pp. 560578 in Abd-Elgawad, MMM, Askary, TH and Coupland, JC (Eds) Biocontrol agents: entomopathogenic and slug parasitic nematodes. Wallingford, CABI.Google Scholar
White, GF (1927) A method for obtaining infective nematode larvae from cultures. Science 66, 302303.CrossRefGoogle ScholarPubMed
Williams, AJ and Rae, R (2015) Susceptibility of the Giant African snail (Achatina fulica) exposed to the gastropod parasitic nematode Phasmarhabditis hermaphrodita. Nematology 127, 122126.Google ScholarPubMed
Wilson, MJ, Glen, DM and George, SK (1993) The rhabditid nematode Phasmarhabditis hermaphrodita as a potential biological control agent for slugs. Biocontrol Science and Technology 3, 503511.CrossRefGoogle Scholar
Figure 0

Fig. 1. The mean number of Phasmarhabditis hermaphrodita (DMG0001, DMG0002, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (DMG0017, DMG0018 and DMG0019) found in filter paper with water (control) (white bars), in the middle of the agar plate (black bars) or in filter paper with 0.01 g Deroceras invadens mucus (grey bars). Significant differences between the number of nematodes found in the mucus or water are denoted with * for P < 0.05 and ** for P < 0.001. Different letters denote a significant difference at P < 0.05 between the strains of each Phasmarhabditis species found in mucus. Bars represent ± one standard error.

Figure 1

Fig. 2. The mean number of Phasmarhabditis hermaphrodita (DMG0001, DMG0002, DMG0003, DMG0005, DMG0007, DMG0008, DMG0009, DMG0010 and DMG0011), P. neopapillosa (DMG0012, DMG0013, DMG0014, DMG0015 and DMG0016) and P. californica (DMG0017, DMG0018 and DMG0019) found in filter paper with water (control) (white bars), in the middle of the agar plate (black bars) or in 1% (A) or 5% (B) hyaluronic acid (grey bars). Significant differences between the number of nematodes found in hyaluronic acid or water are denoted with * for P < 0.05 and ** for P < 0.001. Different letters denote a significant difference at P < 0.05 between the strains of each Phasmarhabditis species found in hyaluronic acid. Bars represent ± one standard error.