No ontogenetic shift in the realised trophic niche but in Batesian mimicry in an ant-eating spider

In predators an ontogenetic trophic shift includes change from small to large prey of several different taxa. In myrmecophagous predators that are also mimics of ants, the ontogenetic trophic shift should be accompanied by a parallel mimetic change. Our aim was to test whether ant-eating jumping spider, Mexcala elegans, is myrmecomorphic throughout their ontogenetic development, and whether there is an ontogenetic shift in realised trophic niche and their mimetic models. We performed field observations on the association of Mexcala with ant species and investigated the natural prey of the ontogenetic classes by means of molecular methods. Then we measured the mimetic similarity of ontogenetic morphs to putative mimetic models. We found Mexcala is an inaccurate mimic of ants both in the juvenile and adult stages. During ontogenesis it shifts mimetic models. The mimetic similarity was rather superficial, so an average bird predator should distinguish spiders from ants based on colouration. The realised trophic niche was narrow, composed mainly of ants of different species. There was no significant difference in the prey composition between ontogenetic stages. Females were more stenophagous than juveniles. We conclude that Mexcala is an ant-eating specialist that reduces its prey spectrum and shifts ant models during ontogenesis.

no ontogenetic shift in the realised trophic niche but in Batesian mimicry in an ant-eating spider S. pekár 1* , L. petráková Dušátková 1 & c. R. Haddad 2 In predators an ontogenetic trophic shift includes change from small to large prey of several different taxa. in myrmecophagous predators that are also mimics of ants, the ontogenetic trophic shift should be accompanied by a parallel mimetic change. our aim was to test whether ant-eating jumping spider, Mexcala elegans, is myrmecomorphic throughout their ontogenetic development, and whether there is an ontogenetic shift in realised trophic niche and their mimetic models. We performed field observations on the association of Mexcala with ant species and investigated the natural prey of the ontogenetic classes by means of molecular methods. then we measured the mimetic similarity of ontogenetic morphs to putative mimetic models. We found Mexcala is an inaccurate mimic of ants both in the juvenile and adult stages. During ontogenesis it shifts mimetic models. the mimetic similarity was rather superficial, so an average bird predator should distinguish spiders from ants based on colouration. The realised trophic niche was narrow, composed mainly of ants of different species. There was no significant difference in the prey composition between ontogenetic stages. Females were more stenophagous than juveniles. We conclude that Mexcala is an ant-eating specialist that reduces its prey spectrum and shifts ant models during ontogenesis.
True predators capture a high number of prey items during their lifetime 1 . They typically take prey that is smaller than themselves 2 , due to a decline in capture success with relative prey/predator size 3 . As predators grow in size during ontogenesis they are able to accomplish an ontogenetic shift in prey preference by selecting prey of a larger size. This is well known for spiders, the most diversified group of terrestrial true predators, where the size of prey correlates well with the size of growing spiders 4 .
In specialised predators, trophic adaptations are often highly specialised 5 , increasing the capture efficiency of their preferred prey. In rare cases, a specialised capture strategy combined with very effective venom enables even tiny juveniles of specialised predators to catch the same prey type as adult spiders 6 . However, even specialised predators typically accomplish an ontogenetic shift in prey preference within the range of their preferred prey. Two mechanisms of prey shifting have been observed, which depend on the developmental characteristics of their prey. Specialists feeding on prey with a gradual (hemimetabolous) development (e.g., termites), switch between developmental stages of the exclusive prey, from small to large individuals 7 . Specialists preying on holometabolous insects shift between differently sized imagoes of distinct prey types [8][9][10][11] , or if imagoes of prey are polymorphic, then they shift from small to larger forms of the same prey species 12 .
A very few trophic specialists use their prey species also for a defence. This is the case in predators feeding on ants, which are also their Batesian mimics (i.e. myrmecomorphy). For example, Aphantochilus 13 or Zodarion spiders 14 both imitate and feed on the model ant species. If the predator is at the same time a Batesian mimic of its prey, then the ontogenetic trophic shift should be accompanied by a parallel ontogenetic Batesian mimetic shift. Myrmecomorphic species either imitate ant species only during certain ontogenetic stages 15 or imitate different ant species during ontogenesis, i.e. transformational mimicry [16][17][18] . In the latter case, the mimic imitates ant models that co-occur and coexist spatially in the same microhabitat as all of the predator's ontogenetic stages. Alternatively, the predator's early ontogenetic stages are not or are only poorly myrmecomorphic. This is the case in juveniles of both Aphantochilus and Zodarion spiders, whose early instars captured the same ant species as adult individuals, although their mimetic similarity to their prey is rather poor 13 .
Here we focused on a spider that is specialised to catch ants presumably during its entire life cycle. Mexcala elegans Peckham & Peckham (shortened to Mexcala onwards) is a diurnally active salticid spider that appears to feed particularly on its model ant species of the genus Camponotus 19 . However, in the laboratory, adult individuals of this spider species subdued a range of ant species and other prey types 20 . The prey and defensive habits of juvenile individuals of Mexcala remain unknown. Mexcala shows an ontogenetic dimorphism in colouration 19 . Specifically, early instars have metallic blue-green colouration, whereas older instars have silver-grey colouration, in some cases accompanied by two pairs of yellow-orange spots on the abdomen. The colouration may have important implication on its foraging and defensive strategy.
Our aim here was to investigate whether M. elegans spiders are Batesian mimics of ants throughout their ontogenetic development and whether there is ontogenetic shift both in Batesian mimicry (i.e. transformational mimicry) and prey preference. For this purpose, we performed field observations on the association of M. elegans with putative model species, measured the mimetic similarity of major ontogenetic classes to mimetic models, and investigated the natural prey of these classes by means of molecular gut-content analysis, which is a powerful tool able to identify prey obtained via cryptic feeding 21 . We predicted that if the spider is myrmecomorphic at each ontogenetic stage then it would preferably catch its mimetic model because of similarities in body size and close spatial occurrence.

Results
Association with ants. Different  phenotypic similarity. Among all the ant species co-occurring with Mexcala spiders, only three ant species had a similar colouration: C. cinctellus ants, which were black with golden or silver-shining gaster; Cataulacus ants, which were uniformly black; and Polyrhachis schistacea (Gerstäcker) ants (shortened to Polyrhachis onwards), which were silver-shining grey. These were selected as the putative mimetic models in further analyses.
The first two PCA axes of body size measures explained 96.4% of variation (Fig. 1A, Table S1). The sizes of adults and large juveniles of Mexcala were most similar to the control (Stenaelurillus), while that of small juveniles was similar to Cataulacus ants.
The first two PCA axes of body contour explained 73.3% of variation (Figs. 1B, S1C,D). The contours of all Mexcala stages were closer to the control than to the ants. All stages were similarly distant from the ant models.
The first two PCA axes of colouration explained 86.2% of variation (Figs. 1C, S1A,B). The colouration of males, females and large juveniles was similar to Polyrhachis, while the colouration of small juveniles was clearly different and similar to C. cinctellus and Cataulacus. Colouration of all stages was different from the control.
The first two PCA axes of movement explained 67.6% of variation ( Fig. 1D, Table S2). The spiders moved in a zig-zag manner with raised forelegs. The movement of all Mexcala stages overlapped to a large degree, and was also similar to both all ant models and the control.
The first two axes of overall PCA explained 56.6% of variation (Fig. 2). Adult males, females and large juveniles were similar to C. cinctellus and Polyrhachis, while small juveniles were similar to Cataulacus. There was a significant difference in the distance of mimics from their models (ANOVA, P < 0.0001): small juveniles, large juveniles and adult males were significantly closer to their models than adult females. colour discrimination by predators. For adult male and female Mexcala, the average colour contrast of the anterior and posterior body regions were far above the threshold of 3 when compared to the control and Camponotus, but less than 3 when compared to Polyrhachis (Fig. 3A). For juvenile mimics the average perceptual distances from C. cinctellus, Catalulacus and the control were above 3 (Fig. 3B). Thus, adult Mexcala were hardly indistinguishable from Polyrhachis, while juveniles were clearly distinguishable from ant models and the control.
Realised trophic niche. We found 56 MOTUs using the ant primers (Table S3). Due to rather short length of the amplified DNA fragment, we were only able to identify prey to the genus level. We identified ten ant genera: Camponotus , and one MOTU that belonged to the Dipteran family Cecidomyiidae (5,450 seq.). One MOTU was similar to two different genera, Odontomachus and Anochetus (12,634 seq.). Using the general invertebrate primers, we distinguished eight MOTUs. Five of them belonged to prey, while three MOTUs belonged to the predator species. The prey was detected using those primers in one female individual and consisted of ants (Camponotus, Formicidae), Diptera (Cecidomyiidae) and Lepidoptera (unidentified). Overall, the breadth of the trophic niche of all stages on an order prey level was narrow, B A = 0.04.
Comparison of the frequency of capture of ants with their frequency of occurrence for all spiders combined we found a significant difference (Chi-square test, χ 3 2 = 18.2, P = 0004): Mexcala captured more frequently Camponotus and Atopomyrmex ants than available, but less frequently Catalacus and Crematogaster which was not found in the gut.
Camponotus was the most frequent prey, captured by more than 80% of ontogenetic stages. We revealed at least three different Camponotus species in the spiders' guts based on a simple neighbour-joining tree reconstruction (Fig. S2). However, there might have been more Camponotus species, as we found no variability in the sequenced COI fragment between several Camponotus species that were collected as potential prey at the study www.nature.com/scientificreports www.nature.com/scientificreports/  www.nature.com/scientificreports www.nature.com/scientificreports/ site. Thus, Camponotus MOTU 1 was found in 92.5% of the studied spiders, in all ontogenetic stages. This species was placed close to C. natalensis (Smith), C. cinctellus and C. rufoglaucus (Jerdon). Camponotus MOTU 17 was placed close to C. grandidieri Forel and C. postoculatus, and was found in a few juveniles and subadult females. Camponotus MOTU 31 was most similar to C. arminius Forel and was only found in two spider individuals.
While some ant genera (Atopomyrmex, Plagiolepis, Monomorium, Tetramorium and Cataulacus) were slightly more frequently found in the guts of juveniles than in adult and subadult individuals, comparison of the relative frequencies revealed that there was no significant difference between stages/sexes (GEE-b, χ 2 30 < 0.1, P = 1.0). Spiders fed on a variety of ant species with a similar composition. Specifically, the diet was mainly comprised of Camponotus (74.4%, N = 38), followed by Plagiolepis (28.2%), Tetramorium (15.4%), Myrmicaria (12.8%), and others (Fig. 4A). Yet, there was a significant difference between sex/stages in the proportion of individuals that tested positive for ant sequence (GEE-b, χ 2 3 = 19.4, P = 0.0002): small juveniles had the highest proportion (23.8%), followed by large juveniles (17.0%), males (15.2%), and females (9.1%). The number of prey species identified from the gut was significantly different among sex/stages (GLM-p, F 3,35 = 5.5, P = 0.003, Fig. 4B): females had the smallest number (on average 1 prey type/specimen), while small juveniles had the largest number (≥2 prey types/specimen). The relationship between the size of the spider and the average size of its ant prey was not significant (GEE, χ 2 1 = 1.9, P = 0.17).

Discussion
Our results show that Mexcala spiders are inaccurate mimics of ants. Their body contour is not antlike, but the gait is slightly similar to ants, and the body size and the colouration makes them similar to ants. Adults of Mexcala are not imitating one but two species of ants, Camponotus cintellus and Polyrhachis schistacea. Although we have not observed Polyrhachis ants to occur directly on the trunks of Vachellia xanthophloea trees together with Mexcala spiders, we found them on the foliage of neighbouring bushes and low-growing Cissus rotundifolia creepers, where Mexcala also occurs. Small juveniles of Mexcala were most similar to Cataulacus intrudens. This shows that Mexcala shifts from one ant model to another during ontogenetic development, but that this is not coupled with an improvement in mimetic similarity. Similar transformational mimicry has been reported for www.nature.com/scientificreports www.nature.com/scientificreports/ other myrmecomorphic species 15 . As all ant models co-occur, we failed to find an association of certain ontogenetic stages with only specific ant models.
In adult females, there is another colour form that is, however, rare. The colouration of this rare form is black with two pairs of orange spots on the abdomen. The most probable mimetic model of this form is nymphs of an alydid heteropteran (Pekár, unpublished), which occur directly on the trunks of Vachellia xanthophloea trees. These bugs were also rare, so a future study is needed to disclose the similarity and find whether the alydid bugs are noxious models.
One of the plausible hypotheses explaining the evolution and existence of inaccurate mimicry is the multimodel hypothesis 22 . In this case, inaccurate mimics imitate more than one model superficially but none accurately, and this provides the mimic with an advantage to occur on a larger spatial scale than when imitating a single model. Such mimic(s) might be engaged in a mimetic complex that includes both accurate and inaccurate mimics, possessing variety of defence levels. Recently, we discovered such a complex composed mainly of ants, but also spiders, wasps and hemipterans in Australia 23 . Indeed, it has been reported that at Ndumo there are number of ants (Polyrhachis, Camponotus), spiders (Merenius, Apochinomma, Myrmarachne, Corinnomma, Kima, Castianeira), katydid nymphs (Eurycorypha) and heteropterans (Myrmoplasta) with a similar shining-grey colouration 19,[24][25][26] . They all may form a mimetic complex 25 . While ants and heteropterans presumably represent Mullerian mimics because they are defended by physical (Polyrhachis) and chemical (Camponotus, heteropterans) weapons, spiders and katydids are most likely Batesian mimics, as they are harmless 23 .
We have not confirmed the hypothesis of Mexcala being a Batesian mimic of ants experimentally using predators. The most likely predators of these spiders are wasps, mantises, birds and other spiders (Pekár, unpublished). We compared the colouration (chromatic component) of mimics and putative models using a bird visual system. This revealed that the similarity of both adult and juvenile Mexcala individuals to ants is on the verge of the discrimination threshold. So, an average bird should be able to distinguish them from ants. However, we have no evidence for the discrimination by other predators, such as spiders and wasps, which possess lower visual acuity than birds 27 . Mexcala spiders, both adult and juvenile, occurred on the tree trunks syntopically with several ant species, having same temporal activity (Pekár, pers. observation). The ants were far more abundant than the spiders, as most of them were foraging in columns. So, even though a bird predator would be able to discriminate them from ants, the spiders may be lost in the crowd of foraging ants and their chance of being captured is reduced. This is perhaps enforced by a lack of aggression on the spiders by foraging ants, enabling the spiders to move relatively freely without being detected or attacked (Haddad, pers. observation).
Mexcala may use aggressive mimicry, as it mainly captures ants, which is the case in a few other myrmecophagous spiders 14,28 . The superficial colouration and gait may enable spiders to approach ants without inducing an aggressive response by ants from a distance; this could also increase the chance of prey capture.
The realised trophic niche of Mexcala was quite narrow, supporting the former view that it is myrmecophagous. The fundamental niche was wider, as the spiders were able to catch other insect prey with a high frequency in the laboratory (namely Collembola, Isoptera, Auchenorhyncha) than those found in this study 20 . Aside from ants, Diptera and Lepidoptera sequences were only found in the guts of a few field-collected juveniles in this study, indicating that ants remain the preferred prey despite the presence of alternative food sources. As the general invertebrate primers preferentially amplify those two invertebrate orders 29,30 , we cannot exclude the possibility that Mexcala also fed on other prey types in the field. Although we screened the gut content of only 40 Mexcala individuals, obtained data clearly show that it is specialised on ants. Indeed, ants were the most common prey on the trunks (Pekár, pers. observation).
Surprisingly, the species richness of prey found in the gut of spiders was much higher in juveniles than in adults. We expected a reverse pattern, as females aim to maximise prey capture for necessary investments in production and deposition of eggs, and are therefore expected to catch a variety of ants. However, our results indicate that females instead specialise on certain prey, particularly, C. cinctellus. This prey type is large compared to other syntopically occurring ant species, and is probably the most profitable, though at the same time it might be more dangerous than smaller ants. Yet, once spiders possess specialised adaptations for effective capture of prey the costs related to prey capture should be negligible. Males, might kleptoparasitise on female's and juvenile's prey thus their prey richness was in-between those of females and juveniles 31 .
Specialised predators are characterised by a variety of prey capture adaptations 5 . Behavioural adaptations include a specific capture behaviour used against ants, which is based on a frontal approach and capture behind the head. By doing this, the spider eliminates counterattack from the prey. Metabolic adaptation, i.e. the ability to process a selected food type, has not been studied yet in this species, although venomic adaptation has. Mexcala has very potent venom that is more efficient on ants than on termites when compared to a closely related salticid species 32 . Its venom likely possesses specific toxins effective especially on ants 33 .
We expected to find differences in the realised trophic niche among developmental stages. Such difference has been observed in another myrmecophagous predator 12 and is expected to eliminate intraspecific competition. In Zodarion jozefienae Bosmans spiders, which only feed on a highly polymorphic ant species, juveniles catch smaller morphs, adult females exploit large morphs, and adult males are kleptoparasites on their prey 31 . Such niche segregation is accomplished by the fact that males have reduced venom glands. Absence of trophic differences in Mexcala suggests that all developmental stages are adapted to exploit a variety of ant species.
We did not find support for a trophic shift in prey size. Small spiderlings were expected to prey on small body-sized ants, such as Crematogaster or Tetramorium, while adult specimens were expected to feed mainly on larger ants, such as Camponotus or Atopomyrmex. This was supported by the direct observations in the field 20 . However, molecular methods, which have the capacity to reveal cryptic feeding, did not support these observations. The dominant ant prey consumed by all stages was Camponotus. Although five genera, which were found as prey in fewer than 20% of the studied individuals, were more frequently found in juveniles than in adults, this difference was not substantial. This shows that even small juveniles are able to exploit quite large ants. Indeed, one (2020) 10:1250 | https://doi.org/10.1038/s41598-020-58281-3 www.nature.com/scientificreports www.nature.com/scientificreports/ of authors (CRH) witnessed in the field capture of large ants by juveniles. There is gathering evidence that specialised spiders in general possess the ability to catch prey larger than themselves both in juvenile and adult stage 34,35 . For example, even small instars of ant-eating Zodarion spiders are able to catch giant ants 6 .
In the realised trophic niche of Mexcala we found three prey genera of ants that could not be identified correctly -two of them do not occur in South Africa and the third one matched two genera with an identical percentage similarity. In the first two cases, we cannot exclude a possibility of contamination -the sequences have been found in almost all sequenced individuals, and the sequences formed a single MOTU. However, in each PCR set up, several negative controls were included to reveal potential sources of contamination. We never detected any positive band in the negative controls using gel electrophoresis. However, no negative control sample was sequenced together with the pooled predator samples, and thus very weak contamination could not be detected. Another possible explanation is that the sequences belonged to some inconspicuous species with a cryptic way of life that could be overlooked during sampling the potential prey.
We conclude that Mexcala is a specialised myrmecophagous predator that is able to exploit a range of ant species (and sizes) over the course of its ontogenetic development. We failed to find trophic shift in this species. Mexcala is an inaccurate myrmecomorphic species that shifts ant mimetic models during ontogenesis. Thus in myrmecophagous predators ontogenetic trophic shift might not be correlated with shift in ant-mimicry due to sympatric co-occurrence of several ant species.

Methods
Association with mimetic models. Preliminary observations revealed that M. elegans spiders forage during the morning, mainly on the trunks of trees but occasionally also on low foliage or the ground. So, in the field we selected 50 Vachellia xanthophloea trees at Nyamiti Pan in the Ndumo Game Reserve, South Africa, in December and March. In the morning (between 8 am and 12 am) of five sunny days we performed a visual search (in total 80 hours) and recorded the frequency of ontogenetic stages (adults, large and small juveniles) of Mexcala and the presence of putative ant models on the tree trunks. As putative ant models we selected such species which were (1) of similar size as Mexcala instars, (2) foraging upon trunk surface, and (3) more abundant than Mexcala. There were six such ant species: C. cinctellus (Gerstäcker), C. postoculatus Forel, Cataulacus intrudens, Crematogaster castanea, Atopomyrmex mocquerysi, and Crematogaster sp. Five persons were surveying each trunk for approximately 15 min. Each trunk was surveyed only once per day.
The occurrence of different stages of Mexcala were related to the occurrence of six most abundant ant species by means of generalised estimating equations with Poisson distribution (GEE-p) from the geepack 36 within R 37 . GEE is an extension of GLM for correlated data 38 and was used in order to take into account joined occurrence of different stages of Mexcala on the same tree (i.e. nested observations). The linear predictor included the tree as a grouping variable, presence of six ants as binary explanatory variables, and stage as a factor. The working correlation structure was exchangeable. phenotypic similarity. We quantified the movement pattern, morphology (body size, body contour), and colouration of small juveniles (N = 6), large juveniles (N = 7), adult males (N = 6) and adult females (N = 5) of Mexcala; C. cinctellus (N = 10), Polyrhachis schistacea (N = 10) and C. intrudens ants (N = 9); and Stenaelurillus guttiger (Simon) spiders as a control (N = 10). Juvenile stages of Mexcala were split into two size categories, small (total body size: 2.4-4.0 mm) and large (4.6-5.8 mm), adults into males (5.3-7.1 mm) and females (6.6-7.5 mm). The small category presumably included the 2 nd and the 3 rd instars, while the large category included the 4 th and 5 th instars (Pekár, pers. observation).
We recorded the movement patterns of mimics and models using a video camera (Canon Legria HF R606). First, we placed an individual into a white plastic container (14 × 22 × 5 cm). To prevent their escape, we applied a thin layer of butter on the walls. We recorded the continuous movement of each individual for 1-2 minutes.
The video recordings of the movements were then processed using Ethovision XT software (version 11, Noldus Information Technology) to quantify the movement pattern. We estimated 11 parameters: the average and maximum velocity (cm/s); average and total meander (degree/cm) (i.e. amount of turning per unit distance); proportion of movement (%) (i.e. cumulative duration of moving) and no-movement (%); mean of relative turn angle (degree); mean of relative angular velocity (degree/s); total distance moved (cm); mean of body mobility (%); and average acceleration (cm/s 2 ).
Then we killed all mimics and models by exposing them to ethyl acetate for few minutes. Freshly killed specimens were then mounted on blue sticky tape in a natural position. The blue colouration was used to allow the software (see below) to extract the image mask more easily.
We took three pictures of every individual from the dorsal view using an Olympus X12 stereomicroscope with an Olympus SC50 camera; these pictures were then combined into one image using Stream Motion software (version 1.9.4, Olympus). We illuminated specimens from the lateral sides using two fluorescent bulbs (13-W daylight ReptiGlo 2.0 UVB) with a similar light spectrum to natural light.
We then analysed the images using custom-made image analysis software 39 to obtain data on body sizes and contours. When assessing the body contour, we straightened the binary mask of each specimen according to the body axis, measured the length of the body axis, placed 40 evenly distributed points along the body axis relative to each specimen's body length, and measured the distance from each of these points to the body edge (excluding the legs). The software also estimated the index of circularity as another measure of body contour. Body size included the average thickness of each of three leg segments (femur, tibia, metatarsus) and the total body length. The colouration was estimated as a reflectance of the anterior and posterior body regions (see below).
First, all variables describing movement, size, contour and colouration were subjected to separate principal component analyses (PCAs). We used PCA in order to reduce the variation in multivariate space to two orthogonal dimensions. PCA was suitable as the measurements were continuous and assumed to come from the normal Scientific RepoRtS | (2020) 10:1250 | https://doi.org/10.1038/s41598-020-58281-3 www.nature.com/scientificreports www.nature.com/scientificreports/ distribution. Within each analysis input variables were standardised. Then we extracted scores for the first two axes of the four trait groups, which explained the large majority of variation, and subjected them to the final PCA. In this analysis, all variables were standardised. From the final PCA we extracted scores along the first two axes and computed Euclidean distances between mimics and their models. These were then compared among sex/ stages with a permutation ANOVA from the lmPerm package 40 within R. colour discrimination by birds. In order to find whether potential predators could discriminate mimics from models based on their colouration we measured the reflectance of spiders and ants using an Ocean Optics USB4000 spectrometer connected to an Ocean Optics PX-2 pulsed Xenon light source, which emits light in the range of 220-750 nm. The reflectance values were relative to a white standard (PTFE optical diffuser reflecting >98% along the entire wavelength range, Ocean Optics WS-1). A black standard was obtained by blocking the light resource. The optic fibre was 400 nm in diameter and was 1 cm above the subject positioned at a 60° angle. We took two measurements of each spider and ant individual, one of its anterior (head + thorax or prosoma) and one of the posterior (gaster or abdomen) (Fig. S1A,B). The measurements were then smoothed and negative values were removed using functions from the pavo package 41 within R.
We tested whether the differences in colouration between mimics and models would be detectable by a bird predator. Since all mimetic species were collected on the bark of trees, we used the reflectance of the trunk as background. For the illumination spectrum, we used the blue sky setting because the trunks were on the forest margin exposed to direct sun light. A perception of the "average bird" predator from the vismodel function was selected for modelling because the spiders can potentially fall prey to many bird species as is the case of other salticid species 42 . For each individual spectrum, we calculated excitation values for the four photoreceptors using the vismodel function from the pavo package. Then, we estimated the perceptual distances (colour contrast) for chromatic component between mimetic spiders (small juveniles, large juveniles, adult males, adult females) and model ants using the coldist function. According to Vorobyev et al. 43 birds can discriminate colour above a perceptual distance of >1 JND.
Realised trophic niche. Besides observation of prey captured in the field, we identified the consumed prey by means of gut-content analysis. In total, 12 adult females, 12 adult males, eight large juveniles and eight small juveniles were used for gut analysis. The numbers are not high because the spiders were quite are. DNA was isolated from the legs of Mexcala and bodies of all potential prey collected at the study site (Table S4) using the DNeasy Blood & Tissue Kit (Qiagen), according to the manufacturer's protocol for small tissue volumes. The cytochrome c oxidase gene was amplified using LCO1490 and HCO2198 primers 44 and sequenced on an ABI Prism 3130 Genetic Analyzer (Applied Biosystems). Sequences are deposited in the GenBank database (accession numbers: MH673867, MK591886-MK591933). The COI sequences served as a reference for the prey assignment and for the primer design.
Prey DNA was isolated from spider opisthosomas, which were crushed and incubated overnight with Proteinase K at 56 °C, then the same protocol as mentioned above was used. Two different primer sets were used to amplify the prey DNA: the ant specific primers (ZodFormF: 5′-TTTATTAATRAWGGAGYAGGAACAGG and ZodFormR: 5′-CCTAARATTGAAGATATWCCTGCAAT 45 ), and general invertebrate primers (ZBJArtF1c: 5′-AGATATTGGAACWTTATATTTTATTTTTGG-3′ and ZBJArtR2c: 5′-WACTAATCAAT TWCCAAATCCTCC 46 ). A specific blocking oligo with a C3 spacer modification at the 3′end, which helped to reduce the predator's DNA amplification, was used together with the general invertebrate primers. The PCR reaction mixture consisted of 10.6 μL of Multiplex PCR Master Mix, 1.8 μL of Q-Solution, 2.8 μL of RNase-free water, 0.5 μL of 10 μM forward and 0.5 μL of reverse primers, 1 μL of 100 μM blocking oligo, and 7 μL of DNA. In each PCR performance, a negative control was included. The PCR conditions were as follows: initial denaturation at 95 °C for 15 min; 42 cycles of 94 °C for 30 s, annealing temperature (48 °C when using universal primers, 50 °C when using ant primers) for 90 s, 72 °C for 90 s, and a final extension at 72 °C for 10 minutes. The PCR primers were tagged with MID identifiers (10 bases long) and each sample was PCR amplified using primers with a unique combination of MIDs on the forward and on the reverse primer. This allowed us to assign all DNA reads to each individual predator. PCR products were detected by electrophoresis in 2% GoodView-stained agarose gels and purified using QIAquick PCR Purification Kit (Qiagen). Enrichment (emPCR) and sequencing on the Ion Torrent platform with an Ion 318 chip and 400-base read length chemistry was provided by the Centre de Recerca en Agrigenòmica (Bellaterra, Spain) 34 .
The sequencing output was processed using the Galaxy platform (https://usegalaxy.org/), BioEdit 7.2.5 47 , fastx-toolkit and the EMBOSS packages 48 . The data were filtered for quality with a Phred Q score value 20. The reads were split according to their MID combinations, resulting in files corresponding to predator individuals. MIDs were removed and too short and too long reads were excluded. The reads were collapsed and rare haplotypes (containing <2 identical reads) were removed. Sequences were translated to amino acids according to the invertebrate mitochondrial genetic code, and those containing stop codons were excluded, as they represented nonsensical sequences. Sequences with insertions and deletions causing reading frameshifts were also removed. The remaining sequences were clustered into MOTUs (= molecular operational taxonomic units) using swarm 49 with a 4-bp cut-off (corresponding to 3% of the sequence divergence). The MOTUs that contained fewer than 10 sequences (corresponding to 0.001% of the total valid reads) were removed as potentially erroneous reads.
Each MOTU was compared to the GenBank database (https://blast.ncbi.nlm.nih.gov/Blast.cgi) using megablast, to the BOLD database (https://www.boldsystems.org/), and to the sequences obtained from the potential prey. As we were not able to reliably identify all MOTUs, we constructed simple neighbour-joining phylogenetic trees using MEGA6 50 with all MOTUs found and the potential prey and predator sequences. The distances between the MOTUs and reference sequences allowed us to better assign ambiguous MOTUs to a taxonomic level. (2020) 10:1250 | https://doi.org/10.1038/s41598-020-58281-3 www.nature.com/scientificreports www.nature.com/scientificreports/ We transformed the number of reads for each individual spider to qualitative data (using presence/absence coding). These data were then subjected to GEE with binomial errors (GEE-b) to compare the frequency of capture of different prey species among the ontogenetic stages. GEE was used due to nested design of several prey types within a single individual. Exchangeable correlation structure was used. To compare the species richness in the gut we used GLM with Poisson errors (GLM-p) 51 . Overdispersion was resolved by using quasipoisson setting. To test whether the body size of spiders is related to the size of captured ants we used average total body size values for each ant species, as the species show a low level of size polymorphism (Pekár, pers. observation). We used GEE with normal errors to test this hypothesis in order to account for the nested observations: several prey types within each individual. The working correlation structure was exchangeable. The standardized Levin's index (B A ) of niche breadth 52 was used to calculate the fundamental trophic niche breadth.