Green lacewings (Neuroptera: Chrysopidae) are commonly associated with a diversity of rickettsial endosymbionts.

BACKGROUND: Bacterial symbionts transmitted from mothers to offspring are found in the majority of arthropods. Numerous studies have illustrated their wide impact on host biology, such as reproduction, behavior, and physiology One of the most common inherited symbionts is Rickettsia spp. (Alphaproteobacteria, Rickettsiales), which are found in about one-quarter of terrestrial arthropods, as well as in other invertebrates. In insect populations, Rickettsia spp. have been reported to cause reproductive modifications and fecundity-enhancing effects. Here, we investigated the incidence and genetic diversity of Rickettsia symbionts in green lacewings (Neuroptera, Chrysopidae), which are best known for their use as biological control agents against crop pests.
RESULTS: We screened 18 species of green lacewings and allies for Rickettsia and found the symbiont in 10 species, infecting 20-100% of sampled individuals. Strain characterization based on multiple bacterial loci revealed an unprecedented diversity of Rickettsia associated with lacewings, suggesting multiple independent acquisitions. Further, the detected Rickettsia lineages are restricted to a specific lineage (i.e., species or genus) of investigated lacewings, and these associations are stable across multiple sampled locations and points in time.
CONCLUSIONS: We conclude that Rickettsia-lacewing symbioses are common and evolutionarily stable. The role of these symbionts remains to be identified, but is potentially important to optimizing their use in biological pest control.

Background

Rickettsia are maternally inherited Alphaproteobacteria that are estimated to be present in one of four terrestrial arthropods [1]. Historically, Rickettsia were best known and studied primarily because of their importance as arthropod-vectored human pathogens, causing diseases such as typhus and various types of spotted fever [2]. Bacteria with genetic similarity to these pathogens have since been discovered in many arthropods and other invertebrates [1, 3], and it has become clear that human pathogens are derived lineages deeply nested within the radiation of most invertebrate-associated Rickettsia [4]. In arthropods, Rickettsia may cause sex-ratio distorting phenotypes, i.e., male-killing [5, 6] or parthenogenesis [7, 8], but has also been associated with positive fitness effects, such as increased fecundity [9, 10] and protection from pathogens [11, 12]. For most hosts, however, the effects of harboring Rickettsia have not been determined.

In a recent large-scale PCR-based survey of Rickettsia, Weinert et al. identified many previously unrecognized arthropod-Rickettsia associations [3]. Among them, one individual ‘green lacewing’ (unidentified Chrysopidae from Mexico) tested positive. Furthermore, in a microscopic screen of tissues from 111 arthropod species more than 90 years ago, Cowdry discovered Rickettsia-like bacteria in one North American green lacewing species (Chrysopa oculata) [13]. Whilst these randomly sampled screens over a large diversity of hosts provide information relating to the global incidence of endosymbionts, they do not inform about the relative importance of a symbiont within a particular taxon. Targeted symbiont screens covering many species within a single taxon have thus been used to identify taxon-specific distribution patterns, and are commonly used as the first step toward deciphering the impact of a symbiont on a taxon’s biology [14, 15]. Based on these previous, isolated findings of Rickettsia in green lacewings, in the present study we sought to determine how frequently these insects carry rickettsial endosymbionts.

Lacewings belong to the Neuroptera, a small (~6000 species [16]) order of holometabolous insects, which also comprises, e.g., antlions (Myrmeleontidae) and owlflies (Ascalaphidae). This group is diverse in ecology and appearance, but is generally characterized by the predaceous lifestyle of larvae and adults of most species. Adults are characterized by two pairs of typically large, extensively veined wings [17]. Green lacewings (Chrysopidae) are probably the best known and studied family of this order, and are common across the globe, with the exception of Antarctica. Two aspects of green lacewing biology have especially attracted research interest in the past. One is the cryptic diversity and courtship songs of green lacewings. Several morphospecies of chrysopids comprise multiple reproductively isolated species, which often can be differentiated based on courtship song characteristics [18-20]. The second is the potential utility of green lacewings as biological control agents in crop environments [21]. Many species are efficient predators of aphids and other pests, and a few are mass-reared because of this quality [22-24].

We here report the first rickettsial symbiont screen of a representative sample of the European chrysopid fauna. We show that Rickettsia is a common symbiont of green lacewings, and that genetically diverse symbiont strains are associated with these insects. In light of the significant impacts of rickettsial and other endosymbionts on insects in general [25, 26], this study provides the first indication of a potentially important aspect of lacewing biology that has been neglected to date.

Methods

Animal collection and DNA extraction

The animals used in this study were collected with hand nets between 2009 and 2014 from a total of 38 locations in Germany (the majority of samples), Austria, France, Great Britain, Hungary, Portugal, and Mongolia. Sampling was focused on green lacewings (Chrysopidae), but also included one species each of brown lacewings (Hemerobiidae) and alderflies (Megaloptera, Sialidae). Where possible, for each species, we collected at least five individuals from multiple populations (i.e., locations). In total, we collected 103 individuals belonging to 18 species. A detailed list of sampled individuals can be found in Additional file 1: Table S1. All animals were either killed and stored in 80% EtOH, or first anaesthetized and killed with ethyl acetate, and later mounted and dried to facilitate determination. For Rickettsia screens, partial or complete abdomens were ground using sterile pestles, and digested using Proteinase K. DNA was then extracted using a chloroform/isoamyl alcohol protocol with subsequent ethanol precipitation, and stored in TE buffer at −20 °C.

Screen for Rickettsia endosymbionts

DNA extracts were quality-checked via PCR by amplifying the mitochondrial cytochrome oxidase subunit I gene (COI), using the primers LCO1490 and HCO2198 [27]. PCR success was assessed visually by electrophoresis, and DNA extraction was repeated for samples in which PCR failed. All samples passing this check were then screened for Rickettsia using four diagnostic primer pairs, each specific for a single Rickettsia locus (16S rRNA, atpA, coxA, gltA, see [3] for primer sequences). All amplified Rickettsia PCR products were Sanger sequenced in both forward and reverse directions by an external service provider (GATC Biotech, Konstanz, Germany). Samples were considered as Rickettsia positive only when unambiguous, high quality Rickettsia sequences from any of the four loci were recovered. All sequences have been submitted to NCBI GenBank (see Additional file 2: Table S2 for accession numbers).

Phylogenetic analyses

To facilitate phylogenetic classification of the Rickettsia strains associated with lacewings, one alignment was created for each of the four sequenced Rickettsia loci, and complemented with sequences from other Rickettsia strains previously characterized by Weinert et al. [3]. The sequences of each locus were aligned with MAFFT version 7.271 [28] using the ‘L-INS-i’ algorithm and concatenated to a supermatrix using FasConCat version 1.0 [29]. The final dataset consisted of 100 Rickettsia strains (32 from lacewings) and 3729 nucleotide positions in total. IQ-TREE version 1.5.3 [30] was then employed to 1) determine the best fitting nucleotide substitution models [31] and partitioning scheme using the ‘greedy’ algorithm [32], 2) perform a maximum likelihood tree search under this partitioning scheme. Clade credibility was assessed using 5000 ‘ultrafast’ bootstrap replicates [33]. Likewise, single gene trees were reconstructed for each of the four Rickettsia loci to identify potential recombination events. One such event was identified (Additional file 3: Figure S1), and the corresponding sample (‘Chrysopa perla CPer7’) removed from subsequent analyses. Finally, a host phylogeny based on mitochondrial COI was reconstructed. Sequences for samples ‘Pseudomalla prasinus DPan’ & ‘Pseudomallada ventralis 14278’ were generated using the COI primers mentioned above; all other sequences were taken from the NCBI nucleotide database. All trees were visualized using the online tool Evolview [34].

Results

In total, 103 individuals belonging to 18 species (Neuroptera: 16 Chrysopidae, 1 Hemerobiidae, Megaloptera :1 Sialidae) were screened, and Rickettsia was detected in 33 individuals from 10 species (Fig. 1). Within host species, Rickettsia prevalence ranged from 20 to 100% (Fig. 1), although these estimates stem mostly from small sample sizes (2–18). We performed a phylogenetic analysis of the detected strains together with previously characterized strains based on an incomplete matrix of four Rickettsia loci (16S rRNA, atpA, coxA, gltA), because not all loci were available for all previously characterized strains, and amplification failed for some of the loci from our strains as well (Additional file 2: Table S2). The tree recovered in our analysis is very similar to previous comprehensive analyses by Weinert et al. [3], and thus in agreement with their proposed classification scheme for Rickettsia species groups. The newly sequenced strains are found in four Rickettsia groups (‘Torix’, ‘Rhizobius’, ‘Bellii’, ‘Transitional’), and seven distinct lineages of rickettsial endosymbionts of lacewings can be differentiated (I–VII in Fig. 2).

Fig. 1

Result of Rickettsia screening in lacewings and allies. Maximum likelihood tree shows phylogenetic relationships of investigated species based on a 657 bp alignment of the mitochondrial cytochrome oxidase subunit 1 gene. For each of the species, a bar chart shows the number of sampled individuals, partitioned in Rickettsia positive individuals (black part of bars) and Rickettsia negative individuals (grey part of bars)

Fig. 2

Maximum likelihood tree of Rickettsia strains based on four loci (3729 bp in total). Bootstrap support is color-coded as illustrate in the legend and based on 5000 replicates. Rickettsia group naming follows [3], as does naming of the strains. Briefly, most names correspond to Rickettsia hosts, and lowest available taxonomic rank is provided. Rickettsial species are named ‘Rickettsia‘ and environmental samples are labeled with ‘(env)’. For collapsed parts of the tree, the number of terminal nodes are parenthesized. Novel sequences are marked with red triangles and each is labeled with host species name, lab ID, and an abbreviation indicating sampling location and sampling date (separated with underscore). See Additional file 1: Table S1 for full information on all samples

All Rickettsia strains isolated from a single lacewing host species were very similar to each other based on the four sequenced loci, irrespective of when and where the individual was collected (Fig. 2). Mapping the presence of seven lineages onto the host phylogeny (Fig. 1) revealed that the presence of Rickettsia is not strongly associated with host phylogeny, i.e., it appears to be phylogenetically random. However, the presence of a particular Rickettsia lineage is not completely independent of host phylogeny. For example, the closely related Chrysoperla carnea, C. lucasina and C. pallida harbor nearly identical Rickettsia strains (Figs. 1 and 2).

Discussion

The incidence of Rickettsia in lacewings reported here (32% of individuals, 44% of species) is considerably higher than that determined from other arthropod taxa via similar PCR screens [35]. It is, however, in line with a recent maximum likelihood estimation of overall Rickettsia incidence in terrestrial arthropods [1]. As other similar PCR based endosymbiont screens, our approach likely missed very low-titer Rickettsia infections and those that are found only in a small proportion of the tested species, and thus, the true Rickettsia incidence in lacewings may be even higher than that reported here. Disregarding the potentially undetected associations, Rickettsia can still be considered a common symbiont in green lacewings. This is true despite the seemingly small number of sampled species, which comprised around half of the German species of the small family Chrysopidae (16/29 species [36]).

Beyond their incidence, lacewings can also be considered as a hotspot for Rickettsia in terms of the genetic diversity of detected strains. With the exception of vectors for pathogenic Rickettsia (e.g., ticks, fleas) [37-39], no other arthropod host lineage shows a comparable diversity of Rickettsia strains. The strains found here belong to seven phylogenetically distinct lineages that are distributed widely across the known Rickettsia diversity (Fig. 2). This implies at least seven independent acquisitions of Rickettsia symbionts in lacewings. One potentially confounding effect for this estimate is homologous recombination. Rickettsia genomes typically harbor a recombination machinery, conjugation genes, and plasmids, all of which could contribute to genetic exchange between Rickettsia strains [40-43]. Within the dataset analyzed here, we found one clear case of recombination; based on coxA sequences, the Chysopa perla sample ‘CPer7’ clustered within the ‘Transitional’ group of Rickettsia strains (Additional file 3: Figure S1), as did all other strains from Chrysopa perla (Fig. 2). However, the 16S sequence of this strain was most similar to strains of the ‘Torix’ group (Additional file 3: Figure S1). We consequently excluded this sample from the supermatrix analysis. Of the seven distinct lineages of Rickettsia within lacewings, most are represented by multiple samples and/or loci, and recombination did thus likely not affect their phylogenetic placement. However, the sample Chrysotropia ciliata 15,084 was only represented by a single 16S sequence in our dataset, and as the only member of Rickettsia lineage ‘I’ (Fig. 2), we cannot exclude the possibility that this lineage only appears to be distinct due to a recombination artifact.

Examples for other taxa frequently associated with Rickettsia include ladybirds [3, 14], spiders [44, 45], and water beetles of the genus Deronectes [46], as well as species in the dipteran families Dolichopodidae, Empidae, and Hyobotidae [47]. Strikingly, all of these taxa, and the chrysopids investigated here, are predaceous. Hence, the question arises whether our and previous reports of Rickettsia PCR positives represent true symbiotic associations, or rather contaminants from symbionts of prey taxa. However, multiple lines of evidence support the view that Rickettsia are vertically transmitted symbionts in lacewings: 1) The main prey of green lacewing larvae are aphids, and the low prevalence of Rickettsia in aphids [48] cannot account for the high incidence of this symbiont in lacewings. 2) Rickettsia strains from lacewings are genetically very diverse and host-specific (only a single Rickettsia strain per species, Fig. 2). It is very unlikely that individuals of a single species sampled at various locations and times acquired identical Rickettsia strains from their prey (or environment) by chance alone. A more parsimonious explanation is that the association of Rickettsia with lacewings is evolutionarily stable and pre-dates the geographic distribution of host populations sampled here. 3) We found that closely related lacewing species (e.g., Chrysoperla sp. & Pseudomallada sp.) harbor similar Rickettsia strains that are genetically distinct from other strains. Again, it is unlikely that such patterns arise by chance. Rather, we think it is best explained by the presence of a vertically transmitted Rickettsia symbiont in the last common ancestor of the recently diverged host species (Fig. 1).

Rickettsia is one of four symbionts reported from green lacewings to date. It has been recognized for nearly 50 years that some chrysopids are associated with symbiotic yeasts [49, 50]. Special morphological structures appear to have evolved in response to the presence of yeasts and are present only in lacewings that feed on pollen, nectar, and honeydew as adults, but not in species with predaceous adults [51]. It has consequently been suggested that symbiosis with yeasts is obligate for these lacewings, and that yeasts may provide essential nutrients for non-predaceous adult chrysopids [49]. However, evidence for nutritional supplementation is ambiguous [52] and the role of yeasts in lacewings remains unclear [53]. Furthermore, high densities of bacterial cells have been reported from microscopic investigations of the midgut of Chrysoperla carnea, potentially indicating a nutritional role for these bacteria [54]. However, it has also been suggested that midgut-associated bacteria in lacewings are transient, rather than symbiotic [55]. A “true” symbiont reported from lacewings is Spiroplasma (Mollicutes). Hayashi et al. detected this bacterium in a Japanese population of the chrysopid Mallada desjardinsi and further observed that Spiroplasma presence in mothers is strongly correlated with all-female broods [56]. Spiroplasma thus may act as a male-killer in this chrysopid, as has been reported previously from e.g., buprestid and ladybird beetles [5, 57]. The Hayashi group also detected Rickettsia in Mallada desjardinsi, but did not find evidence for sex-ratio distortion in this green lacewing species [56].

These examples illustrate how symbionts can profoundly impact lacewing biology. While past research has focused on the role of yeasts, the incidence and diversity of the bacterial symbiont Rickettsia as reported here warrant investigations of its effects in lacewings. This is not only interesting from evolutionary and ecological perspectives, but also important for the application of green lacewings in biological pest control. Larval chrysopids are efficient predators of aphids, psyllids, whiteflies, and other crop pests, and a number of species are currently used as biological control agents [58]. Many traits that are typically encoded by symbionts could potentially impact the effectiveness of chrysopids in that respect: nutritional supplementation, reproductive manipulations or protection from viruses and parasitoids. Understanding the interactions of Rickettsia and other symbionts with lacewings would therefore facilitate a targeted manipulation of the biological properties of lacewings, and thus improve their value in biological control.

Conclusion

Rickettsia are common symbionts of green lacewings (Chrysopidae). While the importance of these symbiotic associations remain to be determined, the large genetic diversity of Rickettsia in lacewings, species-specific distributions, and previous reports on symbiont-mediated sex ratio distortion suggest they are relevant to lacewing biology. Several green lacewing species are being reared efficiently in large numbers for the purpose of biological pest control. These species are clear candidates for use in investigating the characteristics of rickettsial symbiosis in lacewings.

Sampling information for all individuals investigated in this study. (ODS 26 kb)

NCBI accession numbers for all sequences created in this study. Missing accession numbers indicate that PCR was not successful for corresponding fragment. (ODS 24 kb)

Recombination in Rickettsia from lacewings. Maximum likelihood trees for both CoxA and 16S rRNA are shown. Presumed recombinant Rickettsia strain is highlighted with an arrow in both trees. (PDF 62 kb)