Abstract
The invasive caprellid amphipod Caprella mutica is one of the most widely dispersed marine non-native species globally. Originating in sub-boreal north-east Asia, it has now been found in both the northern and the southern hemispheres. One potential reason why this species is such a successful invader is its ability to utilise a wide variety of food sources. The contribution of different food sources to the diet of C. mutica was estimated using fatty acids as biomarkers. Caprella mutica was collected from three field sites, including sea cages stocked with Atlantic salmon Salmo salar, shellfish longlines stocked with the blue mussel Mytilus edulis and mooring lines marking the Loch Linnhe Artificial Reef (>2 km from caged finfish aquaculture), where established populations of this species are known to occur. In addition, the fatty acid compositions of C. mutica held in aquaria and either fed the microalga, Dunaliella tertiolecta, or the diatom, Phaeodactylum tricornutum, for a period of 21 days were investigated. The fatty acid composition of the diatom and the microalgal diets was also examined. The results showed that C. mutica contained high levels of polyunsaturated fatty acids, particularly 20:5(n-3); other dominant fatty acids included 18:1(n-9), 22:6(n-3) and 16:0 (in decreasing order based on abundance). Significant differences in the fatty acid profiles between caprellids fed on the microalgae and the diatom diets and between C. mutica collected from the field sites were observed. These results provide evidence that lipid biomarkers can be successfully used to provide evidence of feeding strategy for C. mutica and that the flexibility observed in this strategy may play an important role in its invasion success.
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Introduction
The introduction of non-native species is one of the most pervasive, irreversible and devastating impacts of human activity on natural ecosystems. The frequency and distribution of biological invasions is ever-increasing, and it is important to understand the consequences of these invasions on native ecosystems. One of the effects of the introduction of non-native species can be the displacement of native plants and/or animals as a result of competition for food (Porter and Savignano 1990; Byers 2000). Many successful invasive species exhibit a generalist feeding strategy, consuming a wide variety of diet types (Snyder and Evans 2006; Ribeiro et al. 2007; Rocha and Anjos 2007).
Caprella mutica, a non-native epifaunal amphipod, which originates from sub-boreal areas of north-east Asia, was first identified in the United Kingdom on the west coast of Scotland in 2002 (Willis et al. 2004); however, it is now known to have a global distribution (Ashton et al. 2007b; Cook et al. 2007a). This species typically inhabits artificial structures, including aquaculture infrastructure, marina pontoons and boat hulls at extremely high densities (>300,000 m−2) (Ashton 2006) and can dominate sub-littoral fouling communities at certain times of year (Cook et al. 2006). Yet, little is known about the feeding strategies of this species and the implications that C. mutica may have on the abundance of prey items and potential competitors for food in the water column. Stomach content analysis has shown that C. mutica is predominantly a detritivore (Guerra-Garcia and Tierno de Figueroa 2009). In addition, it is known that C. mutica is capable of filtering particles out of the water column by swaying its body through the water and using its second pair of antennae as a sieve (Nauwelaerts et al. 2007). It is also possible that this species uses a more passive method of particle collection, as other parts of the body of C. mutica contain setae which is frequently observed grooming (Nauwelaerts et al. 2007). It has been suggested that caprellid amphipods which have setae on their second antennae obtain a significant part of their diet through filtering and scraping periphyton, whereas caprellids without setae are mainly predators (Caine 1977). Caprella mutica, however, is known to consume on average 15 Artemia nauplii h−1 in laboratory studies (K. Boos, pers. comm.), which suggests that this species can use a variety of different feeding strategies depending on the abundance of potential prey.
The use of fatty acid biomarkers to investigate food web relationships has been used extensively as a reliable method for determining important dietary information over an extended time span (Graeve et al. 1994a, b), unlike stomach content analysis that are both extremely time consuming and can only give an indication of the most recent ingestion of food (Sano et al. 2003). Previous studies have found that diet type can influence the fatty acid composition of crustaceans (Sargent et al. 1987; Falk-Petersen et al. 2000; Virtue et al. 2000), including the Caprellidae (Guerra-Garcia et al. 2004) and that certain fatty acids (“marker lipids”), or their ratios, can be used to provide a more precise indication of an organism’s diet and hence it’s trophic position. Typical phytoplankton markers are 16:1(n-7), 18:4(n-3) and 18:1(n-7) (Falk-Petersen et al. 2000), 16:1(n-7), C16 PUFA and 20:5(n-3) and a 16:0/16:1(n-7) greater than 1 indicates a dominance of diatoms in the diet (Dunstan et al. 1994; Kharlamenko et al. 1995; Falk-Petersen et al. 2000). Dinoflagellates tend to contain high proportions of 18:4(n-3), 18:5(n-3) and particularly 22:6(n-3) and deficient in 16:1(n-7) (Harrington et al. 1970; Falk-Petersen et al. 2000). The proportion of odd-chained and branched fatty acids and the ratio of 18:1(n-9)/18:1(n-7) fatty acids are also an indicator of bacterial input in the diet (Sargent et al. 1987; Kharlamenko et al. 1995). Carnivorous feeding in marine invertebrates has been associated with 22:6(n-3), 18:1(n-9) and a low ratio 18:1(n-9)/18:1(n-7) (Kharlamenko et al. 1995; Cook et al. 2000). Fatty acids such as 20:1(n-9) and 22:1(n-11) are also thought to be formed by de novo biosynthesis in calanoid copepods (Sargent and Whittle 1981; Kattner and Hagen 1995), and the presence of high amounts of these fatty acids reflects animal dietary input (Falk-Petersen et al. 2000). High proportions of 22:1(n-11) are also found in salmon feed pellets, and this fatty acid has been associated with a fish farm-derived diet (Cook et al. 2000).
In a previous study on the fatty acids of C. mutica collected from ropes for Undaria culture in its native region (Otsuchi Bay, Japan), significant amounts of 20:5(n-3) and 16:1(n-7) and a 16:0/16:1(n-7) ratio of 2.5 (Kawashima et al. 1999) strongly indicate a diatom component to the diet. However, substantial amounts of 18:1(n-9) and relatively high levels of 20:1(n-9) and 22:6(n-3) indicate that this species also had an animal dietary input, including calanoid copepods. Sano et al. (2003) studied the gut contents of C. mutica on drifting seaweed off the coast of northern Japan and confirmed that a high proportion of the diet was composed of ephiphytic pennate diatoms and crustaceans. Caprella mutica has been successfully reared in aquaria on microalgae and the pennate diatoms (Cook et al. 2007b); however, little is known about the diet of this species in non-native environments.
The aims of this study were to determine the diet and the degree of specificity in the feeding strategy of C. mutica in the field using fatty acid biomarkers. Replicate samples were collected from sites where established populations of C. mutica are located on the west coast of Scotland including (1) fish farm cage netting, (2) mussel farm longlines and (3) mooring lines for an experimental artificial reef. The fatty acid profiles were determined for these samples and compared to C. mutica that either fed (1) the microalga, Dunaliella tertiolecta, (2) the pennate diatom, Phaeodactylum tricornutum or (3) no additional feed for 21 days in the laboratory. The fatty acid composition of these diets was also obtained, to increase our understanding of the feeding habits of C. mutica.
Materials and methods
Sample collection
Caprella mutica was collected from three artificial sites in the Lynne of Lorne, west coast of Scotland in June and July 2005, where established populations are known to occur (Ashton 2006). The sites included sea cages stocked with Atlantic salmon Salmo salar (56°27′N, 05°28′W), shellfish longlines stocked with the blue mussel Mytilus edulis (56°32′N, 05°20′W) and mooring lines marking the Loch Linnhe Artificial Reef (56°32′N, 05°27′W; > 2 km from caged finfish aquaculture). Treatment groups are hereafter referred to as ‘Fish’, ‘Mussel’ and ‘Reef’, respectively.
Additional C. mutica was collected from mooring lines (depth 1–5 m) in the Lynne of Lorne (56°33′N, 05°24′W), west coast of Scotland in August 2005 and maintained in aquaria at the Scottish Association for Marine Science. Plastic mesh (1-mm mesh diameter) provided substratum in the aquaria. Replicate groups of 100 C. mutica were held in nine 15-l aquaria for 21 days and fed either (1) the microalga, D. tertiolecta (2) the diatom, P. tricornutum or (3) given no additional feed, apart from organic material (<5 μm) which would have entered the aquaria via the filtered seawater. Experimental treatment groups are hereafter referred to as ‘Algae’, ‘Diatoms’ and ‘NF’, respectively. Cripps and Atkinson (2000) found that diet could significantly influence fatty acid composition in Antarctic krill, Euphausia superba in 16 days, and Cook et al. (2007b) have previously reported that C. mutica could be held in aquaria without food for a period of 18 days with approximately 80% survivorship. The microalga, D. tertiolecta and the diatom, P. tricornutum were supplied by the Culture Collection for Algae and Protozoa (CCAP), Scottish Association for Marine Science (CCAP Collection Code 19/6 B and 1052, respectively). The diatoms were cultured in a semi-continuous culture system (20 l) at 21°C in autoclaved sea water enriched with Walne’s medium and a vitamin solution (Walne 1970). The diatom colonies were added ad libitum every 2 days to each container. Any uneaten food and faecal pellets were removed daily. There were 3 replicates of each treatment. The aquaria were aerated, and the sand-filtered seawater was changed every two days prior to feeding. Temperature and photoperiod were maintained at 13 ± 0.5°C and 14 h light/10 h dark to reflect environmental conditions when C. mutica are at their peak abundance in the field (Ashton 2006).
Post-experimental treatment or upon collection from the field, male individuals were rinsed with distilled water and stored under nitrogen and frozen prior to analysis. Each of the samples of the diatom and the microalga was filtered onto a GF/F filter and were stored as described for the caprellid tissue.
Tissue preparation and fatty acid analysis
Three replicate samples (each including 10 male caprellids; 20–25-mm body length) from each treatment group and three samples of each dietary source were analysed. Whole male caprellids were used in the analysis as Guerra-Garcia et al. (2004) showed sex differentiation using fatty acid signatures. Analysis of the total lipid fatty acid composition was undertaken as differences between phospholipids and triacylglycerols in amphipods are small (Graeve et al. 2001). Total lipid was extracted from the caprellid material and diatom and microalgal diets by the method developed by Folch et al. (1957). The material was placed in glass boiling tubes, homogenised using a pestle and mortar, and 5 ml of chloroform/methanol (2:1 v/v) containing 0.01% of the antioxidant butylated hydroxyl toluene (BHT) was added. A volume of 50–100 μl 19:0 (1.04 mg/ml) was added to the caprellid and microalga samples, and 50 μl of methyl tricosanoate (23:0) (1.02 mg/ml) was added to the diatom samples to act as an internal standard for gas chromatography (GC) quantification. All samples were stored under nitrogen overnight at 4°C. The supernatant was removed by pipette and passed through a glass wool filter into a boiling tube. Then, 2.5 ml of 0.88% KCl was added to the boiling tube. After shaking and separation of the layers, the layer containing the lipid was removed and evaporated to dryness under nitrogen at 30°C. For analysis of fatty acid composition, the total lipid extracts were subjected to acid-catalysed transesterification. To the lipid extract, 1 ml of toluene and 2 ml of 1% sulphuric acid in methanol were added and left sealed under nitrogen at 100°C for 2 h. The esters were extracted using hexane containing 0.01% BHT and purified using thin-layer chromatography. The fatty acid methyl esters (FAME) extracts were spotted onto silica gel 60 plates and developed with hexane/diethyl ether/glacial acetic acid (80:20:2 v/v) and recovered from the adsorbent with chloroform/methanol (2:1 v/v). FAME extracts were dried under nitrogen, and then 100 μl of hexane (containing 0.015 BHT) was added. Samples were then kept frozen under nitrogen until analysis. FAME were analysed with a Perkin Elmer 8320 gas chromatograph (GC) equipped with a spilt column injector (100:1), flame ionisation detector and a Zebron ZB-WAX-fused silica capillary column (30 m × 0.25 mm i.d.) with helium as the carrier gas. The oven temperature was programmed to rise from 160 to 240°C at 4°C/min and then to hold for 10 min. The detector output was coupled to a computerised data system (Varian Star™) for storage and integration of the chromatograms. Individual components were identified by reference to authentic standards (Sigma, Matreya). Non-saponifiable lipids, which contribute to the total lipid content, however, were not measured in this study as previous studies on related organisms had not recorded that these long chain alcohols and sterols were a major factor in the total lipid content (Kawashima et al. 1999; Graeve et al. 1994a, b; Pond et al. 1997). Individual fatty acids were expressed as the percentage by weight of the total fatty acids characterised.
Statistical analysis
Differences in total fatty acid content and each fatty acid between the different treatment groups (Diatoms, Algae, NF, Fish, Mussel and Reef) were tested using a one-factor ANOVA using the statistical package MINITAB 15. Data were tested for normality prior to analysis using the Kolmogorov–Smirnov test. Bartlett’s test was used to test for homogeneity of variances (Zar 1996) and Tukey’s multiple comparison test was used in pair-wise comparisons among treatment groups when significant differences (P < 0.05) were determined. Mean results are reported in the text. Multivariate analysis was carried out on the entire data set using the PRIMER v5 (Plymouth Routines In Multivariate Ecological Research; Clarke and Warwick 1994). The data were left untransformed (Howell et al. 2003; Hughes et al. 2006) and converted into similarity matrices using Euclidean distances as the metric. Similarity patterns in the data were visualised using non-metric multidimensional scaling (nMDS). In these two-dimensional plots, individuals with similar fatty acid signatures are placed closer together than those that are more dissimilar. Crossed analysis of similarity (ANOSIM) was performed to examine differences in fatty acid composition between species and different diet types. The similarity percentages procedure (SIMPER) was used to identify the main fatty acids contributing to the similarity measures obtained (Clarke and Warwick 1994).
Results
Total fatty acid content
A significant difference was found in the total fatty acid content of C. mutica between the different treatment groups (ANOVA; df = 5, F = 15.13, P < 0.001). Caprella mutica collected in the field (‘Fish’, ‘Mussel’ and ‘Reef’) were found to contain a significantly higher quantity of fatty acids compared with C. mutica held in the aquaria and fed on a monoculture of either diatoms, microalgae or NF (Tukey test, P < 0.001) (Fig. 1). Caprella mutica collected from ‘Fish’ also contained higher quantities of total fatty acids compared with samples collected from ‘Reef’ (Tukey Test, P < 0.05) (Fig. 1).
Fatty acid composition
The fatty acid composition of C. mutica was characterised by four major fatty acids, including 20:5(n-3), 18:1(n-9), 22:6(n-3) and 16:0 (in decreasing order based on % of total fatty acids) (Tables 1, 2). These comprised between 61.7 and 73.0% of total fatty acids. The fatty acid composition, however, was significantly different between C. mutica collected from the three field sites (Fig. 2).
In addition to the major fatty acids found in C. mutica, the levels of specific fatty acids, including 16:1(n-7), 18:4(n-3), 20:1(n-9) and 22:1(n-9 + 11), were significantly higher in C. mutica collected from ‘Fish’ compared with ‘Reef’ (P < 0.05). In the case of 22:1(n-9 + 11), this fatty acid in the ‘Fish’ samples was over double (1.2%) the amount observed in samples from the two other field sites (~0.5%). The majority of these fatty acids were also observed in higher levels at ‘Fish’ compared with C. mutica from ‘Mussel’, with the exception of 16:1(n-7) (P < 0.05). Caprella mutica sampled at ‘Fish’ also had a low 16:0/16:1(n-7) ratio (2.8) (Table 2).
Caprella mutica collected from ‘Mussel’ had significantly higher levels of 16:1(n-7) and 18:1(n-7) compared with ‘Fish’ and ‘Reef’ (P < 0.05). 27.3% of the fatty acid composition was 20:5(n-3), which was comparable with the levels of this fatty acid in C. mutica from ‘Reef’, but higher than from ‘Fish’. Significantly lower levels of 20:1(n-9), 22:1(n-9) and 22:6(n-3) were also observed in these C. mutica compared with the other two field sites (P < 0.05). Caprella mutica sampled at ‘Mussel’ had a significantly lower 16:0/16:1(n-7) ratio (2.1) compared with samples from ‘Fish’ and ‘Reef’ (P < 0.05) (Table 2).
Caprella mutica from ‘Reef’ had significantly higher levels of 22:6(n-3) (12.67%) compared with ‘Fish’ and ‘Mussel’ and higher levels of 20:5(n-3) comparable with samples from ‘Mussel’. Significantly lower levels of 16:1(n-7), 18:4(n-3) and 22:1(n-9 + 11) were observed in samples from ‘Reef’ compared with the other two field sites (P < 0.05). Caprella mutica from ‘Reef’ also had a significantly higher 16:0/16:1(n-7) ratio than samples from the other two field sites, but the ratio was still relatively low (3.76) (P < 0.05) (Table 2).
Fatty acid composition for C. mutica collected from the field sites was significantly different compared with C. mutica held in aquaria and fed on known diets (Fig. 2). Caprella mutica in the aquaria had significantly higher levels of 18:1(n-9), 20:4(n-6) and 22:6(n-3) and lower levels of 16:1(n-7), 18:4(n-3), 20:5(n-3) and 22:1(n-9 + 11) compared to C. mutica collected from the field sites (P < 0.05). Within the aquarium-based treatment groups, C. mutica fed on the diatom had significantly higher levels of 16:1(n-7) and a lower 16:0/16:1(n-7) ratio (6.27) than the other two treatment groups reflecting the high quantities of 16:1(n-7) in the diet (44.5%) (P < 0.05). Caprella mutica that fed on the microalgal diet also contained significantly higher levels of 18:3(n-3) compared with the other treatment groups, again reflecting the high levels of this fatty acid in the diet (32.7%) (P < 0.05) (Table 1).
Multivariate analysis of fatty acid signature
Multivariate analysis (ANOSIM) of C. mutica showed significant differences in the fatty acid composition between the field sites and aquarium-based treatments (Table 3). No significant difference was found between the aquarium-based treatments (P > 0.05). A significant difference was observed between all three field sites (Fig. 2). SIMPER analysis indicated the contribution of certain fatty acids to the average dissimilarity between replicate samples at each sampling site. Four fatty acids contributed most to the differences observed between the three field sites: 16:1(n-7), 18:1(n-9), 20:5(n-3) and 22:6(n-3) (Table 4).
Discussion
In this study, we analysed the detailed fatty acid compositions of Caprella mutica in order to determine the diet and the degree of specificity in the feeding strategy of this species which is non-native to the west coast of Scotland. In the analyses, we used specimens collected from three field sites as well as specimens held in aquaria and fed a specific diet for a period of three weeks. A significant difference was observed between the field and the aquarium-based C. mutica, with the latter exhibiting a greater level of particular fatty acids which were found in high abundance in the respective diets over a relatively short time period (21 days). These results provide evidence that lipid biomarkers can be successfully used to provide evidence of feeding strategy for this species.
Stomach content analysis of C. mutica has previously shown that this species consumes a combination of diatoms and crustaceans in its native region (Sano et al. 2003). The fatty acid analysis of C. mutica suggests that this species is adopting a similar omnivorous feeding strategy in the non-native environment, with high levels of 18:1(n-9), 22:6(n-3) and 20:5(n-3), in all the treatment groups indicating the importance of animal-derived material and diatoms in the diet.
Significant differences in the fatty acid composition were observed between the field sites suggesting that C. mutica is able to vary its diet according to available food sources. Elevated levels of 22:1(n-9), a fatty acid that is abundant in both fish feed (Cook et al. 2000) and calanoid copepods (Falk-Petersen et al. 2000), were found in C. mutica collected from the Atlantic salmon sea cage site (‘Fish’) compared with the other field sites (‘Mussel’ and ‘Reef’). Previous work at the same salmon farm found a dominance of the copepods Pseudocalanus spp., Paracalanus spp. and Oithona spp. with densities of ~1000 ind. m−3 (Cook, unpubl.). Oithona spp. and Paracalanus spp. have also been found to dominate plankton samples collected from fish and oyster farm sites in the native region in the Uwa Sea, Japan (Doi et al. 2008). However, the lipid biomarkers were unable to differentiate between fish farm-derived and copepod dietary sources. In addition, high proportions of fatty acids, which indicate the consumption of diatoms, notably 16:1(n-7), a low 16:0/16:1(n-7) ratio, and dinoflagellates 18:4(n-3) were observed in C. mutica at the ‘Fish’ site. Navarro et al. (2008) found increased abundances of phototrophic and heterotrophic plankton in the vicinity of a fish farm on the west coast of Scotland, which may have been an important food source for the caprellids. Again, the biomarkers were unable to determine whether the caprellids were feeding directly on diatoms or on zooplankton which had fed on diatoms. However, stable isotope work by Doi et al. (2008) found that Caprella spp. collected from a fish farm in Japan did consume attached microalgae (~60%).
At the mussel cultivation site, significantly higher levels of 20:5(n-3) were found compared with the fish farm site, together with the lowest 16:0/16:1(n-7) ratio, indicating that diatoms formed a greater component of the diet at this site. Doi et al. (2008) also found that Caprella spp. at an oyster farm had a greater input of attached microalgae and a reduction in phytoplankton in their diet than at a fish farm at a comparable time of year, potentially reflecting the reduced availability of phytoplankton that is typically observed in the vicinity of shellfish cultivation (Asmus and Asmus 1991; Ogilvie et al. 2000).
At the artificial reef site, however, it was apparent that animal material and/or dinoflagellates play a greater role in the diet of C. mutica, with higher levels of 22:6(n-3) (12.67%) compared with the other two field sites. High levels of 20:5(n-3) also indicate that diatoms are an important dietary component at this site. However, lower levels of the lipid biomarkers for phytoplankton input were observed, which may be attributed to the higher flushing rates experienced at this site compared with the other two field sites (Wilding and Sayer 2002, Cook et al. 2006), which may be attributed to the lack of submerged infrastructure that can significantly reduce water flow (Lo et al. 2007). Populations of C. mutica typically expand exponentially during the summer months, reaching a peak in September on the west coast of Scotland (Ashton 2006). The high levels of 22:6(n-3) in the caprellids from the reef site may be attributed to cannibalistic feeding by C. mutica, which has been observed in aquaria when held at high densities (Shucksmith 2007). This result could also be explained by the consumption of other amphipods and isopods, which are known to inhabit sub-littoral fouling communities in this region, such as Jassa spp. and Idotea spp. (Hayward and Ryland 2000, Cook et al. 2006).
In the recipient environment, C. mutica has been found to displace the native caprellids Caprella linearis and Pseudoprotella phasma from substrate (Shucksmith 2007; K. Boos, pers. comm.), potentially competing with these species for similar food types based on the similarity of fatty acid compositions between C. mutica in the present study and the native species (Guerra-Garcia et al. 2004). Sano et al. (2003) also observed through stomach content analysis that C. mutica had similar proportions of pinnate diatoms and crustaceans as other omnivores, such as Caprella spp., Jassa spp., Idotea spp., and thus, may be in direct competition for food resources in recipient environments. These species are typical members of the sub-littoral fouling communities, and further research is required to determine the extent of competition between C. mutica and other ecotrophically similar native fauna.
The aquarium-based C. mutica also appeared to have significantly higher levels of 22:6(n-3) compared to the C. mutica collected from the field sites, suggesting greater carnivory. Cannibalistic behaviour was observed during the course of the experiment and has been recorded in other laboratory-based studies (Shucksmith 2007; K. Boos, pers. comm.). This may also be linked to an inadequate food supply during the course of the experiment with the caprellids conserving this essential fatty acid, but it does highlight the fact that this species is able to switch between feeding strategies depending on food availability, even exhibiting cannibalistic behaviour when food supply is reduced. Caprella spp. have been found in ballast tanks (Carlton 1985) and sea chests (Coutts et al. 2003) in commercial vessels, and its global spread has been attributed to an increase in the frequency and speed of global marine transport (Carlton 2003). The ability of C. mutica to survive in such environments during trans-oceanic voyages, however, can be attributed to the flexibility in its feeding behaviour, in addition to the wide physiological tolerances exhibited by this species (Ashton et al. 2007a). The aquarium-based C. mutica fed on diatoms, however, did have significantly lower levels of 16:1(n-7) compared with the field-based populations. Previous studies on diet-induced changes in the fatty acid composition of urchin larvae (Liu et al. 2007), adult urchins (Hughes et al. 2006) and arctic herbivorous copepods (Graeve et al. 1994b) have all found that feeding experiments less than 24 days are adequate to see significant changes in the fatty acid composition of the target species. This may indicate that the field populations were able to assimilate greater quantities of a preferred diatom species which was more readily consumed compared with the diatom species used in the aquarium experiment rather than this being an artefact of the length of the feeding period.
In conclusion, fatty acid biomarkers have proved extremely useful in revealing differences between site variation in dietary intake, the omnivorous feeding strategy adopted by C. mutica and the flexibility of this species in its ability to assimilate a wide variety of diet types depending on their availability; a trait that can only contribute to the further global spread of this highly successful invasive species.
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Acknowledgments
We thank the staff of the NERC Scientific Dive Facility with all their help. We also thank Karin Boos for her comments on the manuscript. This research was funded by the Esmée Fairbarin Foundation Marine Aliens Programme, Natural Environment Research Council (NERC) OCEANS 2025, the Scottish Funding Council, Highlands and Islands Enterprise and the European Regional Development Fund, under the Addressing Research Capacity (in the Highlands and Islands) project.
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Communicated by U. Sommer.
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Cook, E.J., Shucksmith, R., Orr, H. et al. Fatty acid composition as a dietary indicator of the invasive caprellid, Caprella mutica (Crustacea: Amphipoda). Mar Biol 157, 19–27 (2010). https://doi.org/10.1007/s00227-009-1292-0
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DOI: https://doi.org/10.1007/s00227-009-1292-0