Agriotes obscurus larvae used in the 2005 study were collected by hand-sifting soil taken from pastureland in 2005 at the Pacific Agri-Food Research Centre (PARC) in Agassiz, BC. Collected larvae represented all instars, but were considered as belonging to one population since they were collected within 100 m of each other. Limonius canus larvae used in the 2005 study were collected using flour baits placed in a fallowed field at an organic farm in Kelowna, BC, in June 2005, while L. canus larvae used in the 2006 study were collected similarly from the same location in June 2006. Virtually all collected larvae were late instar (i.e. > 15 mm long) and were considered as belonging to one population since they were collected within 50 m of each other. All wireworms were stored at 4°C in 40 L Rubbermaid (Rubbermaid, Atlanta, GA) tubs filled with sandy-clay loam soil collected at PARC, until needed. To reduce variability, only late-instar feeding wireworms were used in the bioassays. Feeding wireworms were obtained by placing potato slices in the storage tubs. Wireworms assembled at the potato baits were then isolated in soil without food following methods described by van Herk and Vernon (2007a), and were used in bioassays within 3 d.

Wireworms were exposed to germinated wheat seeds in soil-filled circular bioassays as described by van Herk and Vernon (2007a). Using circular bioassays ensures that wireworms moving along the edge of the arena (a common pre-orienting behaviour) remain within 13 cm from the seeds and do not become trapped in corners. Bioassay arenas consisted of three separate 30 cm x 30 cm sections of transparent, 4 mm thick Plexiglas® connected by small carriage bolts. A 26 cm diam hole machined into the centre section created a circular chamber that could be filled with soil to a depth of 4 mm. A transparent plastic grid overlaying both the top and bottom sections divided the chamber into 113 equally-sized cells that were grouped into eight concentric rings and four quadrants. Rings and cells were numbered from the centre outwards, with ring 1 consisting of a single cell (cell 1) touching all four quadrants; other cells were restricted to individual quadrants. Five wheat seeds (cv. AC Superb) were placed in cell 1 after the bioassay chamber had carefully been filled with an even 4 mm layer of screened, sandy-clay loam soil. Soil used was adjusted to contain 20% moisture by weight. Wheat seeds were pre-germinated for 44-48 h at 25 ± 1°C on moist paper towels, ensuring approximately 15 mm shoot length prior to bioassays. Seedlings were placed in ring 1; seedling shoots extended partly into ring 2 (cells 2-5).

After the seeds were placed, the top section of the bioassay was put into place and fastened. Arenas were positioned horizontally on a raised wooden frame to make observations possible through both the top and bottom sections. Seedlings were allowed to grow in the soil in the assembled bioassay for 30 min to establish CO₂ gradients (Doane et al. 1975), after which wireworms (one per arena) were introduced head first into the bioassay chamber through a 5 mm hole in the top centre of either cell 89, 96, 103 or 110 (the centre cells of ring 8 in quadrants I, II, III and IV, respectively). The wireworm introduction hole was sealed with pressure-sensitive tape (VWR International Ltd., Delta, BC) throughout the seed incubation and wireworm observation periods, and opened only for wireworm insertion (< 1 min).

Wireworm position in the bioassay, contact and/or repellence behaviour towards the seed, and health (if abnormal) were recorded every 5 min for 3 h in 2005 and for 5 h in 2006. Wireworms were considered to have come into contact with the seeds when they were within rings 1 or 2 of the bioassay (van Herk and Vernon 2007a). The duration of contact was estimated by multiplying the number of observed contact events by 5 min, i.e. the interval between observations. For the 2006 study, wireworms were observed long enough to assess two or more contact periods and to measure the duration between these contact periods (hereafter referred to as ’inter-contact’ periods). All observations were conducted at room temperature (21 ± 1°C) under low intensity red light (0.75 µE s^‑1 m^‑2, measured with a Li-188B integrating quantum radiometer/photometer; Li-Cor, Lincoln, NB).

Post-exposure wireworm health was assessed immediately after bioassays using methods and criteria developed by Vernon et al. (2008). Wireworms that could move out of an 8 cm diam circle drawn on 12.5 cm filter paper in Petri dish arenas within 2 min were designated as ’alive’. Wireworms that were incapable of directed movement but were capable of body movements obvious to the naked eye were designated as ’writhing’. Wireworms that made no visible body movements with or without prodding were inspected under a dissecting microscope to determine if they exhibited leg and/or mouthpart movements. These wireworms were designated as ’appendage movement’. Wireworms exhibiting no spontaneous or elicited writhing or leg/mouthpart movements were temporarily classified as ’probably dead’, but were not recorded as ’dead’ until they showed signs of decomposition (Vernon et al. 2008). Wireworms were stored individually into 150 mL plastic containers (Fisher Scientific, Whitby, ON) with screened soil (as described above) for 70 d after exposure (DAE) in the 2005 studies, and for 126 DAE in 2006. Wireworm health was assessed 1 and 7 DAE, and weekly thereafter. For the 2006 study, wireworm health was also assessed 3 DAE. Mortality was compared among treatments at 56 DAE in the 2005 studies and at 70 DAE in the 2006 study, after which time no further mortality was observed.

Wheat seeds used in the 2005 studies were treated with Vitavax Dual (containing 50 g lindane and 54 g carbathiin) at 124 g a.i. 100 kg^‑1 seed, Gaucho 480FL (imidacloprid) at 15 g a.i. 100 kg^‑1 seed, Admire 240FS (imidacloprid) at 10 and 30 g a.i. 100 kg^‑1 seed, Poncho 600F (clothianidin) at 25 g a.i. 100 kg^‑1 seed, Tefluthrin 20CS (tefluthrin) at 10 g a.i. 100 kg^‑1 seed, Cruiser 350FS (thiamethoxam) at 10 and 30 g a.i. 100 kg^‑1 seed, and a combination of Cruiser 350FS and Tefluthrin 20CS (both at 10 g a.i. 100 kg^‑1 seed) (Table 1). Wheat seeds treated with Poncho and Gaucho were treated by Gustafson Inc. (now Bayer CropScience Canada, Toronto, ON), and were also treated with the fungicide Raxil MD (1.5 g a.i. tebuconazole and 2.0 g a.i. metalaxyl 100 kg^‑1 seed). Seeds treated with Vitavax Dual, Tefluthrin and/or Cruiser were treated by Syngenta Crop Protection Canada Inc. (Guelph, ON) and, except for Vitavax Dual, were also treated with the fungicide Dividend XLRTA (containing 3.21% difenoconazole and 0.27% mefenoxam) at 13 g a.i. 100 kg^‑1 seed. These insecticide/fungicide combinations reflect treatments under evaluation for wireworm control by Bayer and Syngenta. Admire 240FS was applied to untreated seeds by the authors. In addition, untreated wheat seeds and seeds treated with Raxil MD and Dividend XLRTA alone were tested as control treatments. Due to limited wireworm availability, not all treatments were tested on both wireworm species in 2005 (Table 1).

Wheat seeds used in the 2006 study were treated by Syngenta Crop Protection Canada Inc. with Vitavax Dual at 124 g a.i. 100 kg^‑1 seed, Tefluthrin 20CS, Cruiser 350FS, or both Tefluthrin 20CS and Cruiser 350FS. Tefluthrin 20CS and Cruiser 350FS were tested individually at 5, 10, 15, 20 and 30 g a.i. 100 kg^‑1 seed to determine if the concentration of either chemical affected wireworm behaviour. The combined Tefluthrin 20CS and Cruiser 350FS treatments were tested at 5, 10, 15 and 20 g a.i. 100 kg^‑1 seed of each insecticide to determine if using both chemicals on the seeds had an enhanced effect on wireworm behaviour and health. Seeds treated with Tefluthrin and/or Cruiser were also treated with the fungicide Dividend XLRTA at 13 g a.i. 100 kg^‑1 seed.

Between 20 and 30 A. obscurus larvae were exposed to each treatment in 2005. Due to a shortage of L. canus in 2005, only 10 wireworms were exposed to the Raxil and Dividend treatments. Depending on the availability of feeding wireworms, 20 to 60 L. canus larvae were exposed to each treatment in the 2006 study. Each treatment was conducted over several weeks, with several, randomly-chosen treatments assayed per day. Ten to twenty wireworms were observed concurrently on each observation day. As wireworms have long larval periods (approximately 6 mo per instar), can be maintained in storage for extensive periods (> 2 yr), and were handled similarly in all bioassays (i.e. similar storage conditions, selection and handling, bioassay preparation, observation methods), observation date was not considered to have an impact on wireworm behaviour.

These insecticides were chosen for study as they are currently being evaluated for wireworm management (see above) and as some (e.g. Poncho, Gaucho) appear to provide stand protection in wheat without reducing wireworm populations (R.S. Vernon, unpublished data). Of these insecticides, clothianidin (Poncho), thiamethoxam (Cruiser) and tefluthrin (Force 3.0G) are currently registered in Canada for wireworm management in corn; Vitavax Dual was also included as it has historically been used for wireworm management and is considered repellent to wireworms (Long and Lilly 1958; Toba et al. 1988).

The proportion of wireworms that came into contact with the seeds, or were moribund or dead at the end of the observation or health assessment periods, was compared among treatments with Chi-square analyses (Proc FREQ, SAS 9.1; SAS Institute Inc. 2002) followed by Ryan’s test (α = 0.05) to separate treatments (Ryan 1960). Mean contact and inter-contact durations were compared among treatments with ANOVA (Proc GLM, SAS 9.1) followed by the Ryan-Einot-Gabriel-Welsch multiple range test (α = 0.05) (Ramsey 1978); normality of data was assessed with Proc UNIVARIATE (SAS 9.1) and by plotting of data points and residuals. For selected treatments, comparisons between the two wireworm species exposed to the same insecticide in 2005, and between L. canus exposed to the same insecticide in 2005 and 2006, were made with t-tests (Proc TTEST, SAS 9.1) (α = 0.05). Comparisons between the duration of the first and second contact periods were made for the same subset of wireworms with a paired sample t-test. Among-treatment comparisons of the duration of three consecutive contact periods were made for a subset of treatments from the 2006 study that contained tefluthrin (i.e. treatments in which > 10 wireworms made three contacts) with a repeated measures ANOVA (Proc GLM). Comparisons between the two inter-contact periods were made with paired sample t-tests for these treatments.

For all three studies (A. obscurus in 2005, L. canus in 2005, and L. canus in 2006), a high percentage (> 80%) of wireworms introduced into bioassay arenas came into contact with the seeds during the observation period (Tables 1 and 2), suggesting that insecticide treatments did not prevent wireworm movement towards, or contact with, the seeds. However, in each study, first contact duration differed significantly among treatments (F_11,227 = 9.77, P < 0.0001, Table 1; F_5,87 = 8.61, P < 0.0001, Table 1; F_16,478 = 22.64, P < 0.0001, Table 2), as the insecticides affected normal wireworm behaviour. In the 2006 L. canus study, poorer seed germination in untreated seeds and, to a lesser extent, in the Cruiser 20 g a.i. treatment also affected first contact duration. Seedlings in these two treatments had shorter roots (approx. 5-10 mm, instead of 15 mm in the other treatments), likely because seeds were mistakenly given less moisture during pre-germination (Cruiser 20 g) or were not treated with a fungicide (untreated seeds). All seeds used in the 2006 study came from the same lot and were treated at the same time, and the poorer germination seen in the above treatments does not suggest poorer germination in the field, though the absence of fungicide in the untreated seeds may cause a slight delay in emergence. However, poorer seed germination will affect seedling CO₂ production, which may affect wireworm contact with the seeds since CO₂ stimulates feeding in wireworms (Doane et al. 1975).

Some wireworms that had moved away from the seeds after the first contact subsequently re-contacted the seeds. In the 2005 studies, most A. obscurus (95%) and L. canus (80%) came into contact with seeds treated with Tefluthrin (alone) more than once. However, there was no significant difference between the duration of the first and second contacts [A. obscurus: 15.0 (SEM = 2.0), 15.3 (2.5) min, respectively; t = 0.10, P = 0.92; L. canus: 20.3 (3.5), 13.8 (3.5) min, respectively; t = 1.21, P = 0.24]. Similarly, most (85%) A. obscurus re-contacted seeds treated with the Tefluthrin and Cruiser combination treatment, but there was no significant difference between the duration of the first and second contacts [14.7 (2.3), 15.6 (2.4) min, respectively; t = 0.31, P = 0.76]. Not enough repeated contacts were observed in the other treatments to permit analysis (data not shown).

The longer observation periods in the 2006 study made it possible to observe repeated contacts with seeds in all treatments (Table 2). Duration of the second contact differed significantly among treatments (F_16,329 = 6.91, P < 0.0001), with contact with Dividend-treated seeds being significantly longer than with all other treatments, including untreated seeds (Table 2). As with the first contact, duration of the second contact was shortest in Tefluthrin treatments, and no significant difference in second contact duration was observed among Tefluthrin (plus Cruiser) treatments (Table 2).

Within-treatment comparisons between mean first and second contact durations (Table 2) indicated no significant difference (P > 0.05) when wireworms were exposed to Dividend or untreated seeds, or to treatments containing Tefluthrin, except for the Tefluthrin and Cruiser combination treatment at 20 g a.i. in which second contact duration was significantly shorter than the first (t = 3.01, P = 0.005). Second contact duration was briefer than the first in the Vitavax Dual (t = 3.67, P = 0.0004), Cruiser at 5 g a.i. (t = 2.91, P = 0.01), 10 g a.i. (t = 3.58, P = 0.0007), 15 g a.i. (t = 5.51, P < 0.0001), 20 g a.i. (t = 2.31, P = 0.02) and 30 g a.i. (t = 2.38, P = 0.02) treatments, suggesting that these insecticides had an effect on L. canus contact behaviour.

To further explore this sublethal effect, first and second contact durations were compared within treatments for only those larvae that came into contact twice (data for the first contact period not shown for this subgroup). This comparison revealed no significant difference (P > 0.05) when wireworms were first exposed to Dividend, Vitavax Dual or Cruiser at 5, 10 and 30 g a.i. However, second contact was significantly shorter than first contact when wireworms were exposed to Cruiser at 15 g a.i. [first contact = 141.9 (15.6) min, second contact = 37.7 (13.1); t = 3.60, P = 0.001] and 20 g a.i. [first contact = 90.0 (14.1), second contact = 63.0 (12.0); t = 2.46, P = 0.02], indicating that a single exposure to Cruiser could affect subsequent behaviour.

The effect of repeated contacts with Tefluthrin was assessed by within-treatment comparisons of the mean duration of the first, second and third contacts for L. canus larvae that made three or more contacts with seeds in the 2006 study (Table 3). This comparison indicated no significant difference (P > 0.05) in contact duration among treatments. Similarly, comparisons among different treatments for all first, all second and all third contact durations indicated no significant difference among treatments (P > 0.05). However, in all treatments (except Tefluthrin at 10 g a.i.), the second inter-contact interval was considerably longer than the first inter-contact interval (Table 3). While these differences were not statistically significant (P > 0.05), it may indicate that repeated contact with Tefluthrin had an effect on wireworm behaviour. Previous work has shown that even very brief (1 min) contact with Tefluthrin-treated seeds will induce temporary morbidity in L. canus (van Herk and Vernon 2007b).

Due to the repellence elicited by Tefluthrin, total contact duration in L. canus in the 2006 study differed significantly among treatments (F_16,478 = 32.56, P < 0.0001; Table 2). Contact in the Tefluthrin treatments was consistently shorter than in all other treatments, and the total contact duration in Cruiser (alone) treatments decreased as concentration increased, suggesting that when exposed to Cruiser, wireworm deterrence from contact increases with the concentration (Table 2).

Similarly, despite repeated contacts with seeds containing Tefluthrin (1-5 contacts), the total contact duration of A. obscurus remained lowest among these treatments over the 180-min observation period (F_11,227 = 8.56, P < 0.0001; Table 1), and it was significantly lower than in the control, Cruiser at 10 g a.i., Gaucho and Vitavax Dual treatments. In 2005, total contact duration of L. canus over the observation period differed significantly among treatments (F_5,87 = 14.18, P < 0.0001; Table 1), with total contact duration in the Tefluthrin and Poncho treatments being significantly shorter than in the control treatments (Table 1).

There were significant differences among treatments in the proportion of larvae of A. obscurus, L. canus in 2005 and L. canus in 2006 that were moribund at the end of the observation period (χ² = 119.7, df = 11, P < 0.0001, Table 1; χ² = 32.87, df = 5, P < 0.0001, Table 1; χ² = 128.81, df = 15, P < 0.0001, Table 2). There were significant differences among treatments in the proportion of dead larvae at 56 DAE in A. obscurus (χ² = 42.72, df = 11, P < 0.0001), but not in the 2005 L. canus study (χ² = 8.65, df = 5, P = 0.12). There were also significant differences in the proportion of L. canus wireworms dead at 70 DAE (χ² = 157.04, df = 15, P < 0.0001) in 2006.

The results presented here indicate that contact with insecticide-treated seeds in the soil may cause morbidity in wireworms without causing subsequent mortality and that, consequently, long-term post-contact wireworm health checks are important for assessing an insecticide’s efficacy. These results also indicate that wireworms will move towards seeds treated with insecticides but will often move away after contact. As an insect’s internal state (e.g. concentration of nutrients or immune peptides in hemolymph) affects its behaviour (Miller and Strickler 1984; Pompilio et al. 2006; Riddell and Mallon 2006), it is probable that the onset of morbidity is the stimulus that elicits repellence in wireworms. Wireworms that moved away from insecticide-treated seeds often showed signs of morbidity later on, even if contact was very brief (i.e. in the tefluthrin treatments). Insecticides that cause a rapid induction of morbidity (e.g. tefluthrin) may not be effective for wireworm population control, as wireworms may be repelled before they can absorb toxic doses. While wireworms that are repelled may return for subsequent contact(s), repeated induction of morbidity by some insecticides (e.g. Tefluthrin) increases their ability to recover from morbidity (van Herk and Vernon 2007b). Furthermore, wireworms that become moribund after coming into contact with seeds treated with Poncho, Gaucho, Admire or Vitavax Dual may do so before ingesting enough insecticide to die. Since recovery from morbidity induced by these chemicals may continue for months (van Herk et al. 2008a; Vernon et al. 2008), wireworms returning to the same insecticide-treated plants that induced morbidity initially may not be affected once the plants are established (i.e. wheat and corn). Finally, while an insecticide that elicits repellence may permit crop establishment and provide stand protection, it may be ineffective for wireworm management, particularly if the crop matures in the soil (e.g. potatoes) and if wireworms return after the chemical’s repellent effects have dissipated.

The rapid orientation and high proportion of wireworms that came into contact with wheat seeds in these studies confirm that, contrary to what Chaton et al. (2008) suggested, wireworm host finding is non-random. Like many subterranean insect larvae, wireworms follow CO₂ gradients to find their hosts in the soil (Doane et al. 1975; Guerenstein and Hildebrand 2008) and are able to detect the presence of a single germinating wheat seed in the soil from a 20 cm distance (Doane and Klinger 1978; Westcott et al. 1980). These characteristics have been used to develop effective bioassays for studying wireworm behaviour (e.g. Doane et al. 1975; Horton and Landolt 2002; van Herk and Vernon 2007a).

The results presented here also confirm that observing wireworm position and behaviour every 5 min is sufficient to assess contact and feeding behaviour (van Herk and Vernon 2007a), and they indicate that different insecticides elicit different behaviours in wireworms. However, as these observations were conducted under laboratory conditions over limited observation periods, the results presented here may not accurately reflect what occurs in the field. Increasing the number of seeds in the bioassay or the duration of observation periods will likely increase wireworm mortality in treatments in which wireworms became moribund in situ or continued to come into repeated contact with treated seeds.