INTRODUCTION

Pressures such as climate change, pollution and urbanisation mean that biodiversity research is becoming increasingly important if we are to manage ecosystem functioning and services such as soil fertility, clean water and waste processing (Naeem et al. 1994; Slotow & Hamer 2000; Crouch & Smith 2011; Hamer 2010). However, global change drivers and their synergistic effects (Millennium Ecosystem Assessment 2005) might cause extinctions of species not even known to science (Essl et al. 2013; Costello et al. 2013). One aspect that has often been overlooked is the significant contribution of soil fauna to soil health, below ground diversity, and more broadly to ecosystem functioning (Wardle 2002, Wardle et al. 2004, Louw et al. 2014).

South Africa contains one of the most diverse temperate faunas in the world (Steenkamp & Smith 2006), and has a strong history of biodiversity research (Crouch & Smith 2011). Despite this, knowledge of the soil fauna of South Africa is scattered and the fauna poorly understood (Janion-Scheepers et al. in prep.). Most research has focused on taxonomically well-known groups such as ants (Parr et al. 2005, Botes et al. 2006, Braschler et al. 2012), beetles (Davis 1997, Davis et al. 1999, Botes et al. 2007) and spiders (Dippenaar-Schoeman & Craemer 2000), with only a few recent efforts on groups such as Collembola (Janion et al. 2011, 2015), mites (Ermilov & Hugo-Coetzee 2012) and nematodes (Borgonie et al. 2011, Knoetze et al. 2006). Lack of current research is certainly driven by the logistics of sampling soil fauna. Sampling is often difficult and time consuming. Moreover, the lack of standardisation in sampling protocols has hampered comparisons of diversity between soil fauna studies.

The important role of earthworms as soil processors and ecosystem engineers has been widely demonstrated (Edwards & Bohlen 1996; Lavelle et al 2006), and the role they play in soil fertility and health was even recognised by Darwin (1881). The activities of earthworms in the soil are vital for a healthy, fully functional system (Butt & Grigoropoulou 2010). These activities can substantially change the physical and chemical characteristics of the soil environment either directly or indirectly, with consequences for the entire soil food web, nutrient distribution and even vertebrate and understory plant communities (Edwards & Bohlen 1996). However, many ecological studies group all earthworms together, despite important functional differences between taxa reflecting a great diversity and wide range of adaptations to environmental conditions (Coleman et al. 2004). If the role of earthworms in ecosystems is to be quantified, a precise and accurate estimation of their diversity, abundance and biomass is needed (Valckx et al. 2011).

Earthworm sampling methods can be broadly divided into active, ethological (behavioural) and passive collection methods (Bartlett et al. 2010; Valckx et al. 2011). The main method of active sampling is by digging up a portion of soil (ideally of known volume) and sorting through the soil by hand to collect all earthworms and cocoons. Alternatively, earthworms can be expelled from the soil due to their behavioural response to certain stimuli by a range of chemical expellants or vermifuges (Coleman et al. 2004). It is also common to use both digging and hand sorting as well as chemical expellants (Baretta et al. 2007). Finally, indirect methods involve looking for signs of earthworms or waiting until they emerge on the surface (e.g. dispersal of some species after heavy rains).

Different chemical expellants or irritants can expel earthworms from the soil. Commonly used expellants are formaldehyde (Raw 1959; ISO 11268-3, 1999; Eichinger et al. 2007), commercial hot mustard (Gunn 1992; East & Knight 1998; Chan & Munro 2001; Lawrence & Bowers 2002; Eisenhauer et al. 2008), allyl isothiocyanate (AITC) (Zarborski 2003), household detergents such as washing-up liquid (East & Knight 1998) and potassium permanganate (Evans & Guild 1947, Reinecke & Ryke 1972). Other ethological methods used are the octet or electrical method (Čoja et al. 2008), heat extraction (Čoja et al. 2008), mechanical vibration and the use of pitfall traps (Callaham et al. 2003). Not all of these methods are DNA compatible and certain collection techniques can limit downstream molecular projects. When sampling earthworms formalin is often used as an expellant. However, it is not possible to recover high-quality DNA from tissue that has been exposed to formalin (Moelans et al. 2011), and as such the use of formalin is discouraged when tissues are to be used in molecular studies. Several authors have suggested that mustard be used as an alternative to formalin as an expellant (Gunn 1992; East & Knight 1998; Chan & Munro 2001; Lawrence & Bowers 2002; Eisenhauer et al. 2008; Pelosi et al. 2009; Valckx et al. 2011). Gunn (1992) found that the use of mustard was more successful than formalin, while Lawrence and Bowers (2002) found that mustard was environmentally friendly and a more efficient alternative to formalin across soil and habitat types. The use of mustard powder or prepared mustard presents some problems for standardising earthworm sampling, as the composition of the mustard, how it is applied, and the local soil conditions can vary (Zarborski 2003).

The International Organisation of Standardisation (ISO) set a standard for the sampling of soil invertebrates to address the need to standardise the sampling of terrestrial soil invertebrates (ISO 23611-1, 2006). In part 1 of the ISO document a standard is set for the hand sorting and formalin extraction of earthworms (ISO 23611-1, 2006). The isolation and hand sorting of earthworms in a soil sample of a certain area (0.25 m²) or volume (25 × 25 × 20 cm) is suggested. This method is unfortunately a very laborious procedure and is difficult when the soil has high clay content or if there is a dense root mat present, and when physical disturbance of the study site is not acceptable, meaning digging is not an option (Bouche & Garner 1984; Gunn 1992; Eisenhauer et al. 2007).

Although digging is the most reliable method, a true and complete account of earthworm abundance will require a range of sampling techniques (Lawrence & Bowers 2002), as the relative efficiency of different sampling methods can vary with site characteristics, season and earthworm species (Callaham & Hendrix 1997). Indeed, most studies encourage the use of more than one sampling method (Coleman et al. 2004). By using a combination of active, behavioural, and passive techniques (e.g. digging, formalin extraction, and cast surveys), the accuracy of estimates of earthworm populations can be significantly increased (Bouche & Gardner 1984).

Ecologists and conservationists rely on taxonomists for information regarding species identifications (Chang et al. 2009). Earthworm identification is, however, not straightforward. The use of morphological characters is time consuming, labour intensive and requires trained specialists (Bartlett et al. 2010). A high level of cryptic diversity occurs (Rougerie et al. 2009), and the identification of juveniles and cocoons to species level cannot be made by traditional taxonomic means alone.

Earthworm research in South Africa has been conducted since the nineteenth century (Beddard 1895). As of 2010, there were 282 described earthworm species indigenous to South Africa belonging to three families: Microchaetidae, Tritogeniidae and Acanthodrilidae (specifically to the sub-family Acanthodrilinae) (Plisko 2010). However, large areas of South Africa remain to be surveyed, and most of the groups that have been well sampled require taxonomic revision.

The reference and research collection of earthworms housed in the KwaZulu-Natal Museum (Pietermaritzburg, KwaZulu-Natal) has 138 types (Plisko 2006, 2007, 2008). All types and most specimens were fixed in formalin and so they currently cannot be used in molecular studies. In terms of introduced fauna, 50 species had been recorded by Plisko (2010) but the number has been corrected by Plisko & Nxele (2015) to 44 due to some of the species possibly being indigenous. Many of these species are widespread and abundant, with introduced species dominating disturbed agricultural sites (Ljungström 1972; Visser & Reinecke 1977; Plisko 2000; Dlamini et al. 2001; Haynes et al. 2003; Plisko 2010). While the extent to which introduced earthworms have colonised natural sites is poorly known, results from Dlinza Forest Nature Reserve in Eshowe and from a recent survey of Queen Elizabeth Park, in Pietermaritzburg, highlighted that even at less disturbed sites introduced taxa can be more common than native taxa (Plisko 2000; Nxele 2012). It remains to be seen whether introduced earthworms are having important economic or ecological impacts in South Africa, but introduced earthworms have had major detrimental effects in several locations around the world (Hendrix et al. 2008), particularly in areas where earthworms were not previously present (e.g. islands, or areas post-glaciation).

The aim of this paper is to review the literature on techniques commonly used for earthworm sampling, conduct some preliminary sampling with the two most widely used methods that are compatible with genetic techniques, provide guidelines and recommendations for sampling, and highlight future research focus areas.

MATERIAL AND METHODS

Pilot sampling

Earthworms were sampled using digging and hand sorting at four sites in KwaZulu-Natal, South Africa, during January and February 2012 (i.e. immediately following summer rains when the collection of earthworms is most effective (Plisko 2002a; Fig.1; Table 1). Two of the sites were in natural vegetation in protected areas (a mistbelt forest and a grassland) and two in disturbed areas (National Botanical Gardens—Pietermaritzburg, and a fallow agricultural field). At the agricultural site, sampling was conducted both in ploughed cultivated areas and on contour ridges between the cultivated areas (the latter had kikuyu grass, weeds and tall reeds). At each of the four study sites, 12 sampling plots of 50 cm × 50 cm (after Keith & Schmidt 2013) randomly spaced at intervals not closer than 5 m from each other were selected, and soil to a depth of 20 cm dug out using a metal frame as a guide. The soil was placed onto a plastic sheet and hand sorted for earthworms. Where possible, leaf litter was collected and also searched for earthworms prior to the digging.

Fig. 1.

Earthworm sampling. (A) The most common method is for plots to be dug up, the soil sorted by hand, and earthworms removed. (B) An alternative method is to apply chemical irritants (e.g. mustard solution) to a plot and the earthworms collected once they emerge from the soil. (C) Sorting, cleaning and processing earthworms in the field is a major component of sampling. Decisions as to the size of plot used, how deep the plots are dug, and which chemicals are used in which concentrations, as well as the timing of the sampling, all need to be adjusted depending on the goals of sampling. For large individuals (and anecic species) different sampling methods are needed (see text).

TABLE 1

Localities sampled during the pilot survey.

In addition, 12 more plots of the same size were sampled using a chemical irritant extraction technique. Mustard powder was prepared according to the protocol from ISO 23611-1 (ISO 2006). One hundred grams of dry mustard powder (Colman's) was dissolved in 1 litre of water. In the field, the mixture was diluted with 9 litres of water in 10 litre watering cans, to give a concentration of 10 gL^-1. Leaf litter was removed from each plot and then the mixture poured onto the plot. The earthworms that appeared on top of the soil were collected for about 30 minutes.

Sampled earthworms were washed twice in clean tap water and afterwards narcotised in 20% ethanol. The narcotised earthworms were then weighed (wet mass) to the nearest milligram (mg) using a field balance (Highland portable precision range field balance). Earthworms were then preserved in absolute ethanol, clearly marked with labels and transported to the KZN Museum laboratory for identification. Earthworms were identified to species level using a Wild (Heerbrugg) microscope and descriptions and keys from the published literature (Ljungström 1972; Gates 1972; Plisko 1992; Csuzdi 2010; Blakemore 2011). The collected material was deposited in the KZN Museum.

Sample-based rarefaction curves were plotted and the ACE estimator employed to examine the degree of sampling efficiency and to determine the predicted number of species in each site, using the computer programme EstimateS V9.1.0 (Colwell 2013). All unidentified earthworms (juveniles, damaged adults and other specimens that could not be identified to species level) were removed from the dataset prior to rarefaction and estimation. Sampling was considered adequate if the estimator converged at the highest observed (identified) value (Longino et al. 2002).

RESULTS

Pilot sampling

Of the earthworms collected using the two sampling methods at the four sampling sites, a total of 2 094 earthworms were assigned to 16 species belonging to five families (Table 4). Some earthworms (196) could not be identified as they were unknown juveniles or damaged specimens and were not used in the results. The species accumulation curves (Supplementary material Fig. 2 A–D) indicate that most of the earthworm species at a site were sampled where species richness was relatively low. At sites where earthworm richness was higher, undersampling of species was indicated.

In the grassland of Queen Elizabeth Park a total of 217 earthworms were collected through digging and hand sorting; no earthworms were collected when mustard was used. Only three species (Dichogaster sp., Amynthas corticis (Kinberg, 1867) and Amynthas rodericensis (Grube, 1879)) were found, all introduced to South Africa. Previous studies in this park collected six species in the grassland, including the indigenous Tritogenia howickiana (Michaelsen, 1913) and nine species when including more vegetation types in the park (Nxele 2012). In Cedara, no earthworms were found from the plots that were in the middle of the cultivated field either by digging or mustard, but 85 earthworms from five different species (Octolasion lacteum (Örley, 1881), Amynthas aeruginosus Kinberg, 1867, Amynthas corticis, Amynthas gracilis (Kinberg, 1867) and Amynthas minimus (Horst, 1893)) were collected from plots that were in the grass contour between the fields. All the sampled earthworms were introduced species. In addition, unknown juveniles were also collected, but could not be assigned to any species.

When using the digging and hand sorting method in the Karkloof Forest a total of 766 earthworms and nine species were collected. Eight of these species (Pontoscolex corethrurus (Müller, 1857), Aporrectodea rosea (Savigny, 1826), Dendrobaena octaedra (Savigny, 1826), Dendrobeana sp., Dendrodrilus sp., Amynthas minimus, Amynthas sp., unidentified lumbricid species) were introduced species, and only one indigenous specimen (Tritogenia sp.) was found. When using the mustard method, 485 earthworms were collected from seven species (Pontoscolex corethrurus, Aporrectodea rosea, Dendrobaena octaedra, Dendrobeana sp., Amynthas minimus, Amynthas sp., and unidentified lumbricid species) all of which were also collected using the digging and hand sorting method. When using the digging and hand sorting method in the Botanical gardens a total of 275 earthworms from 11 species were collected. When using the mustard method 266 earthworms from 12 species were collected, including Tritogenia sp (Table 4). The endogeic P. corethrurus was dominant in QEP, the epigeic A. rodericensis was dominant in Cedara, in the Karkloof Forest the endogeic O. lacteum was collected in high numbers using both methods though digging collected almost double the number of individuals than the mustard, and the endogeic A. minimus was dominant in the Botanical Gardens.

TABLE 2

Studies that sampled earthworms in South Africa (1895–2012) combined from the literature collection database in the KwaZulu-Natal Museum and literature review. N/A = no dominant species or number of species and ecological category were mentioned.

(continued)

The earthworms collected by digging and hand sorting weighed on average 0.358 g per worm (n = 294), slightly heavier than the earthworms collected using mustard extraction (average of 0.294 g each, n = 273).

Estimates of the sampling effort are shown in Table 5. Four people completed the pilot study in 10 days with eight working hours in each day. This time included travelling, setting up the field workstation, sampling and travelling with equipment from plot to plot, and packing up and cleaning after each day. As field assistants became more skilled over the course of the study, the time taken to complete a task decreased. When using the digging and hand sorting method it took an average of 40 minutes for one person to sample a plot (50 × 50 × 20 cm) with an average of 44 earthworms per plot. The time taken to collect earthworms with the mustard technique averaged 13 minutes per plot (50 × 50 cm) with an average of 35 earthworms collected per plot. Standardising on 100 earthworms, preserving the earthworms (including washing and narcotising them) and the determination of the biomass took an average of 26 and 42 minutes, respectively. The time taken to identify each earthworm varied greatly depending on (a) the experience of the taxonomist and (b) the identity of the worm. It took three months to complete the classification for all the earthworms in this study, an average of two hours per specimen.

TABLE 3

Sampling methods used in earthworm studies from other countries from the literature collection database in the KwaZulu-Natal Museum.

(continued)

Future directions for earthworm research in South Africa

The key priorities for research identified during the workshop on earthworms are summarised in Box 1. These included foundational biodiversity goals such as preparing an atlas, taxonomic keys, field guides and a DNA barcode library. Other goals included increasing outreach efforts and public interest (e.g. through a roadshow). The latter are considered important in terms of engaging with stakeholders that already have an interest in earthworms as well as providing exposure to taxonomic experts, thereby assisting with the potential enrolment of future taxonomists. There are many urgent needs, but it is clear that these goals must be underpinned by foundational biodiversity survey and description work, which in turn requires capacity building in taxonomy in South Africa.

TABLE 4

Species abundance for each sampled site.

DISCUSSION

A wide variety of techniques are used for the sampling of earthworms in the field (Bouché & Gardner 1984, Druce et al. 2004; Čoja et al. 2008), reflecting in part the different research questions asked, but also because earthworm species have a variety of ecological strategies, patterns of behaviour and habitat preferences (Lee 1985; Blakemore 2002). Epigeic and endogeic species can often be collected by hand; whereas anecic species might require chemical irritants to expel the earthworms from the soil. In our sampling, epigeic earthworms dominated in Cedara and endogeic earthworms dominated in the Botanical Gardens. In addition, earthworm populations are usually spatially aggregated (Valckx et al. 2011). This complicates sampling efforts and attempts to estimate population sizes, particularly as the factors that determine this patchy spatial distribution are not yet sufficiently understood (Valckx et al. 2009). Thus, sampling techniques need to account for the spatial distribution of earthworms in order to get an accurate estimate of species richness and abundance. At the indigenous forest in Karkloof, a greater abundance of earthworms was obtained by digging in comparison to the mustard solution method, whereas almost equal abundances were obtained using the two methods in the transformed habitat of the Botanical Gardens. Despite the existence of international standards (ISO 23611-1 and ISO 11268-3), many studies are not comparable due to the lack of standardisation of sampling protocols. While there has been a substantial and long history of earthworm research in South Africa, for various purposes, most sampling in South Africa has been via digging and hand sorting (Table 2).

In this study we used hand digging with manual sorting and mustard extraction. Only one indigenous earthworm was collected during the whole study (Tritogenia sp.: Table 4). While this might be expected for disturbed areas such as gardens and agricultural areas, it was disconcerting to see a similar pattern in protected areas. This is likely the result of the human activities adjacent to and even in the protected areas. Similarly, Nxele (2012) collected five species of earthworm in grassland in Queen Elizabeth Park by digging 1 m × 1 m quadrats to a depth of 0.5 m: the indigenous Tritogenia howickiana and the non-indigenous Pontoscolex corethrurus, Amynthas gracilis, Amynthas minimus, and Amynthas rodericensis. These results are different from results obtained by Baretta et al. (2007) who also used digging and handsorting plus a chemical expellent, dilute Formol (0.5 %). These authors found four native species and one exotic species when all methods were combined; however the most abundant was the exotic Amynthas corticis. The natural forests have high earthworm diversity because of high food availability and variability (Fragoso et al. 2006). In Karkloof forest, nine species were found and this is the second highest richness of all sampled sites. A native species was collected in this forest, similar to other studies in terms of diversity but completely different in terms of the number of natives found. For example, Huerta et al. (2007) studied the diversity of earthworms in heavily deforested Tabasco in Mexico. They sampled tropical rain forest and plantations of mango (Mangifera indica) and cacao (Cacao theobroma). These authors found 14 native species and five exotics, the tropical rain forest having the greater earthworm diversity.

TABLE 5

Table indicating the average sampling effort and costs per task or activity.*

The method of digging and hand-sorting soil from a 25 × 25 cm quadrat to 20 cm depth seems to be more suitable for sampling epigeic and endogeic earthworm species, probably as a result of their much higher densities in the upper soil layers. As our survey showed, no anecic earthworms were collected with our quadrat size. The size of each plot is a trade-off between collecting individuals and work. Based on available data and experience, we suggest following the ISO standard (i.e. a sample plot size of 50 cm × 50 cm and 20 cm deep) for smaller sized earthworms in South Africa, and digging larger and deeper quadrats for quantitatively sampling larger sized earthworms (i.e. plots of at least 1 m × 1 m × 0.5 m) (Nxele 2012).

Twelve soil samples appeared sufficient to sample most species of non-indigenous earthworms at species-poor sites, but not at species-rich sites as observed in the species accumulative curves (Supplementary material 2). The number of samples per site must be large enough to represent communities at the site adequately, but not so large that they are too time-consuming to process (Stark et al. 2001). From the literature review, the number of samples varied from five or six samples (Chaudhuri & Bhattacharjee 1999; Uys 2006) to 46 samples (Cuendet 1983) depending on the research purpose. Our literature survey indicates that given the high spatial and temporal variability in earthworm communities and variability introduced by different sampling techniques, giving a specific guidance on the sample size is difficult, and will likely be quite context specific.

Additional modifications are required for very large bodied taxa, as they were not collected with our quadrate size in our survey. First, one can dig even larger areas (e.g. approximately 2 m × 2 m × 0.5 m deep for earthworms up to around 100 cm long). Second, sampling of larger earthworms, especially giant earthworms, can be accomplished by searching for fresh casts (indicated by active deposition of fresh mud above ground), in a defined larger area, quickly topping the casts and grabbing the earthworm by the tail end, after which the tail end will anastomose and can immediately be preserved in 95 % ethanol. The species might then be identified using DNA barcoding, and the density per unit area estimated. However, it should be noted that specimens can't be kept for morphological examination with this technique, and as such it is of limited use. Finally, some sampling will need to be opportunistic (e.g. sampling of giant earthworms that cross roads after rains). Owing to the sporadic nature of overland movement, a network of volunteers in various parts of the survey region might be able to track the weather conditions and collect specimens when conditions are right. The specimens would be useful for taxonomic study and a future atlasing project.

Equipment requirements for earthworm sampling techniques and protocols are relatively modest (Supplementary Material 1). However, it takes a lot of time to sample and process samples. Time, resources and expensive equipment are limiting factors to zoological research globally (Bartlett et al. 2010; Butt & Grigoropoulou 2010, Uys et al. 2010). For these reasons the design inventories, sampling methods and planning and monitoring needs to be as effective and efficient as possible (Uys et al. 2010). Two people take 20 minutes to sample a plot of 50 × 50 × 20 cm by digging, and 13 minutes using mustard solution because of the waiting time involved. Mustard may be a useful and quicker method to sample alien earthworm species in leaf litter and topsoil. When using mustard solution, there is less labour involved compared to digging and hand sorting and using mustard solution does not affect the DNA of the specimens, which makes it suitable for molecular analyses. However, the results appear to be variable, and it is hard to control the amount that penetrates into the soil.

Setting a standard for the determination of earthworm biomass would make it possible to compare different datasets, but the biomass of an individual species or of a population as a whole can be used to estimate production and productivity of an ecosystem only when comparing ecosystems of the same or similar structure and species composition. The biomass of earthworm populations varies greatly and in most soils it exceeds the biomass of all other soil-inhabiting invertebrates (Edwards 1994). One practical issue is that the gut contents are a substantial proportion of an earthworm's biomass, and earthworms lose about 10–20 % of their mass during fixation (Lee 1985), thus the point at which individuals are weighed must be made clear.

The major limitation to sampling is the ability to identify all the specimens collected to species level. With few taxonomists trained to identify South African earthworms (South Africa has one retired taxonomist and a full-time junior taxonomist at the KwaZulu- Natal Museum), additional capacity and new methods to facilitate species discovery and description are necessary. Earthworms are well suited to combining DNA-based analysis with morphological taxonomy (Hogg & Hebert 2003; Rougerie et al. 2009; Vernooy et al. 2010), an approach that has been used successfully in other parts of the world (Boyer et al. 2011, Porco et al. 2013). This approach involves training taxonomists in morphological identification, ensuring collections are developed and linked to DNA samples, cataloguing all relevant information and making it accessible.

The need to enlarge South Africa's capacity to answer applied and basic research questions on the roles and impacts of earthworms in the functioning of natural ecosystems was unanimously agreed upon during a workshop on soil organisms at the XVII Congress of the Entomological Society of Southern Africa (July 2011), and separately by the CAPE Invasive Alien Animal Working Group (May 2011) (Louw et al. 2014).

DNA bar-coding and development of user-friendly identification keys are needed to facilitate identification to species level. Given that DNA barcoding has been shown to be extremely useful in the delimitation of difficult to identify species (Pop et al. 2003), the collection of samples in a DNA-compatible way should be included in future sampling protocols. In addition, juvenile specimens can be barcoded to verify their identifications (Richard et al. 2010). The earthworm barcoding library is growing on the Barcode of Life Data System (BOLD), also revealing interesting cryptic diversity (James & Davidson 2012, Porco et al. 2013, Decaëns et al. 2013).

CONCLUSION

We consider that the ISO sampling methodology augmented with more qualitative sampling is suitable for sampling most non-indigenous species of earthworm in South Africa. Sampling of indigenous species apparently requires a larger quadrat size or the use of other methods. Sampling and preservation techniques need to allow DNA-based studies to assist, complement and inform traditional morphology-based taxonomy. However, if we are to understand, conserve and manage earthworms we require more foundational knowledge. This will not happen without capacity-building and substantial resources.