Post-copulatory interactions between males and females involve highly coordinated, complex traits that are often rapidly evolving and divergent between species. Failure to produce and deposit eggs may be a common post-mating prezygotic barrier, yet little is known about what prevents the induction of egg-laying between species. The field crickets, Gryllus firmus and G. pennsylvanicus are isolated by a one-way reproductive incompatibility; G. pennsylvanicus males fail to fertilize G. firmus eggs or to induce normal egg-laying in G. firmus females. We use experimental crosses to elucidate the role of accessory gland-derived vs. testis-derived components of the G. firmus male ejaculate on egg-laying in conspecific and heterospecific crosses. Using surgical castrations to create ‘spermless’ males that transfer only seminal fluid proteins (SFPs) we test whether G. firmus male SFPs can induce egg-laying in conspecific crosses and rescue egg-laying in crosses between G. pennsylvanicus males and G. firmus females. We find G. firmus SFPs induce only a small short-term egg-laying response and that SFPs alone cannot explain the normal induction of egg-laying. Gryllus firmus SFPs also do not rescue the heterospecific cross. Testis-derived components, such as sperm or prostaglandins, most likely stimulate egg-laying or act as transporters for SFPs to targets in the female reproductive tract. These results highlight the utility of experimental approaches for investigating the phenotypes that act as barriers between species and suggest that future work on the molecular basis of the one-way incompatibility between G. firmus and G. pennsylvanicus should focus on divergent testis-derived compounds or proteins in addition to SFPs.
Citation: Larson EL, Andrés JA, Harrison RG (2012) Influence of the Male Ejaculate on Post-Mating Prezygotic Barriers in Field Crickets. PLoS ONE 7(10): e46202. https://doi.org/10.1371/journal.pone.0046202
Editor: Therésa M. Jones, University of Melbourne, Australia
Received: May 22, 2012; Accepted: August 29, 2012; Published: October 10, 2012
Copyright: © Larson et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: This work was funded by a National Science Foundation grant (DEB-0639904) to RGH and an American Association for Women in Science American Fellowship to ELL. The funders had no role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Traits that mediate interactions between males and females are critical for reproduction and yet often evolve rapidly and are highly divergent between species. Therefore, these traits may be particularly important in the early divergence of isolated populations and in speciation –. Although we are often struck by the diversity of conspicuous behaviors involved in courtship and mate recognition, post-copulatory interactions between males and females are equally diverse and complex , . As a result, fertilization in a heterospecific cross can fail at a number of critical steps, resulting in post-mating prezygotic barriers between species. These barriers can range from traits that prevent sperm and eggs from meeting (e.g. sperm transfer, sperm storage, sperm utilization, egg-laying, sperm binding) to intracellular traits that prevent the sperm nucleus and egg nucleus from fusing (e.g. incomplete sperm entry, sperm folding) , –.
Egg-laying in insects provides an example of the complexity of male-female interactions. Egg-laying is a multi-step process that involves egg production within the ovary (oogenesis), release of the egg from ovary into the oviducts (ovulation), progression of the egg down the oviducts, union of the sperm and egg within the genital chamber (fertilization) and the deposition of the egg into a particular substrate (oviposition). These steps are tightly linked to the proper transfer and storage of the male ejaculate. Oogenesis is increased when sperm is stored within the female storage organ, and ovulation interacts with sperm storage and sperm release from storage to facilitate successful fertilization (Fig. 1, reviewed in ). A reduction in the efficiency or a failure at any of these steps can lead to reproductive incompatibilities in insects.
Diagram showing the steps involved in egg-laying in female insects (solid lines) and the interactions that may stimulate increased egg-laying (dashed lines). In boxes are steps that may be mediated by seminal fluid proteins. The interaction between sperm storage and ovulation is hypothesized based on the observation that sperm transfer may increase ovulation and sperm depletion, thereby affecting the number of eggs laid. The figure is re-drawn from Bloch Qazi et al. (2003).
The failure of the male ejaculate to stimulate egg-laying between species has been observed in fruit flies , , beetles , katydids , lacewings  and ground crickets . A similar phenomenon is sometimes observed between populations within a single species , . Failure to produce and deposit eggs may be a common post-mating prezygotic barrier, yet little is known about what prevents the induction of egg-laying between species. We do know which components of the male ejaculate (testis-derived vs. accessory gland- derived) induce intraspecific egg-laying in a variety of insect species , and the molecular interactions of the male ejaculate and female reproductive tract that induce egg-laying in Drosophila melanogaster are now well understood , , , . By characterizing the intraspecific mechanisms that result in egg-laying, we can begin to make inferences about how egg-laying breaks down between species. Here, we use experimental crosses both within and between species to test the influence of components of the male ejaculate on egg-laying and fertilization between two closely related species of field cricket.
Post-mating prezygotic barriers in field crickets
The field crickets, Gryllus firmus and G. pennsylvanicus, are recently diverged species (<0.5% mtDNA divergence ) that interact in a hybrid zone in the northeastern United States, extending from Massachusetts south into Virginia . The cricket species have diverged both ecologically – and behaviorally –, but an important barrier between these species is a one-way incompatibility between G. firmus females and G. pennsylvanicus males . Despite normal sperm transfer and storage, G. firmus females mated with G. pennsylvanicus males do not produce fertilized eggs , . Fertilization appears to break down in this cross somewhere between the release of sperm from storage and the sperm entering the egg . There is an equally striking reduction in egg-laying for these females. A G. firmus female mated with conspecifics will lay approximately 700 eggs over her lifetime, while a virgin female will produce less than 50 eggs and typically only late in life. Gryllus firmus females mated with G. pennsylvanicus males will lay about twice the number of eggs as virgin females, but significantly fewer eggs than a female mated to a conspecific . In contrast, the reciprocal cross produces viable, fertile offspring in numbers indistinguishable from conspecific matings , .
Seminal fluid proteins (SFPs), which are synthesized and secreted from the male accessory gland and transferred to females during copulation, are known to play a role in many of the processes that may underlie a breakdown in egg-laying and fertilization, including ovulation, sperm storage, and sperm release (Fig. 1). Accessory gland genes from G. firmus and G. pennsylvanicus have been characterized through transcriptome sequencing ,  and proteomics of the seminal fluid . Many of the SFPs are found to be rapidly evolving under positive selection. However, there is currently no direct functional link between the divergence we observe in Gryllus SFPs and the post-mating prezygotic barriers that isolate these taxa. One step towards exploring this connection is to characterize the intraspecific and interspecific mechanism(s) that induce egg-laying and fertilization.
We attempt to elucidate the roles of accessory gland-derived vs. testis-derived components of the male ejaculate on these two barriers by asking whether G. firmus male SFPs induce egg-laying in G. firmus females and can “rescue” the cross between G. firmus females and G. pennsylvanicus males. We test the influence of G. firmus SFPs by mating females to surgically castrated (“spermless”) conspecific males that transfer only SFPs. We find that SFPs induce only a modest short-term egg-laying response and that SFPs alone cannot explain the normal induction of egg-laying. We also try to rescue the incompatibility by mating G. firmus females to males of both species. Again, we find no evidence that G. firmus SFPs can rescue the one-way incompatibility.
Materials and Methods
We collected crickets in August of 2006, 2009 and 2011 from pure populations of G. firmus in Guilford, CT, USA (N 41°16′9″; W 72°39′59″); near Hammonasset Beach State Park, CT, USA (N 41°16′4″; W 72°34′14″); and Milford, CT, USA (N 41°11′48″; W 73°4′30″) and G. pennsylvanicus in Ithaca, NY, USA (42°24′35″; −76°32′46″). Crickets were collected as late instar nymphs, separated by sex and maintained in large laboratory colonies with food (cat and rabbit food), water vials and egg flats for shelter, under a 12∶12 h light/dark cycle at 28°C. Every two days we isolated crickets that had become adults and maintained them in same-sex groups of 6–8 crickets in plastic containers (30×16×9 cm). No specific permits were required for the described collections because the study organisms are not endangered or protected species and the collection locations are not privately own or protected.
For each experiment, virgin adult crickets between 6–10 days post-eclosion were randomly assigned to treatment (described below). We abbreviate treatments to indicate species (F = G. firmus, P = G. pennsylvanicus) and the order females were mated, with the first letter representing the female and subsequent letters representing the males with which she mated (e.g., FFP represents a G. firmus female that mated with a G. firmus male followed by a G. pennsylvanicus male). Subscripts represent specific manipulations of male crickets described in the following section (e.g. FFC represents a G. firmus female mated with a G. firmus male that was surgically castrated).
For each cross, cricket pairs were placed in petri dishes (9 cm) lined with moistened filter paper to provide traction. We considered matings complete when the male was observed to successfully transfer and properly attach the spermatophore to the female genital opening. To standardize the spermatophore attachment time and allow the spermatophore contents to be transferred completely, we left mated pairs undisturbed, allowing males to guard females and prevent early spermatophore removal. After males reinitiated courtship (approximately 45 min) we removed males from the mating chamber and females were either presented with a second male or were isolated in individual chambers depending on the experiment. Females that did not mate within 60 minutes of adding either a first or second male to the mating chamber were removed from the experiment.
Following matings, females were isolated in individual containers (30×16×9 cm) and provided with food, water, shelter and a petri dish (9 cm) filled with a mixture of moistened sand and soil as oviposition substrate. Food and water were replaced twice a week, oviposition substrate was periodically moistened, and mortality was scored every two days.
To isolate the roles of testis-derived and accessory gland-derived components of the male ejaculate, we created spermless males using surgical castrations. Surgeries were performed on adult males 5–6 days post-eclosion, after the cuticle had hardened (surgeries performed too soon after eclosion result in high mortality rates). Males were divided into two categories: males that would be surgically castrated (FC) and males that would undergo a sham castration (FS) to serve as a control for effects of surgery on the male ejaculate production or content. Prior to surgery, males were anesthetized by chilling at 4°C for at least 30 minutes. Using fine forceps, we made an incision across the dorsal side through the intersegmental membrane between the 2nd and 3rd abdominal segments and gently teased open the wound. For FC males we completely removed each testis and severed the vas deferens (Fig. 2), while for FS males we probed the wound and body cavity to try to mimic testis removal. We then sealed the wound with Vetbond™Tissue Adhesive (3 M, St. Paul, MN, USA), which polymerizes after contact with tissue and body fluids, binding the wound edges together. Following surgery, males were placed in a sterile petri dish with moistened cotton for water, and allowed two days to recover. Males in both categories had a high survival rate following surgery (FC N = 83, 86.7% survived; FS = 69, 89.8% survived). After the recovery period males resumed normal mate calling and courtship behaviors. Males were then transferred to individual containers and provided with food, shelter and water and the containers were cleaned every day.
The incision is made between the dorsal 2nd and 3rd segments, and each testis (arrow) is gently removed.
Following the recovery period, males that were surgically castrated were placed in a petri dish with a single virgin G. firmus female, and allowed to mate repeatedly in order to deplete stores of mature sperm from the seminal vesicles. After two days of repeated matings, we checked males for remaining stored sperm by removing his spermatophore immediately after attachment to the female and examining the spermatophore contents under a compound light microscope (400×). Spermatophores were gently removed so that all components of the spermatophore remained intact, placed on a microscope slide in a drop of phosphate buffered saline (PBS), and then gently squashed with a coverslip. When normal spermatophores were observed in this manner, a viscous liquid could be observed evacuating the spermatophore tube, followed immediately by long, thread-like sperm. If sperm were observed, males were allowed to mate repeatedly for another eight hours and were checked again the following day. If males were depleted of stored sperm, the viscous seminal fluid was still observed evacuating the spermatophore tube. If no sperm were observed in a male's spermatophore for three consecutive days, we considered the male spermless. Males were kept a minimum of 4 days during which they mated only once a day; this treatment allowed full recovery from repeated matings. Of the 72 males that survived surgical castrations, 57 were successfully cleared of sperm.
To validate that surgically castrated males still transferred SFPs we used two-dimensional electrophoresis (2D–E) to visualize the protein content of the spermless ejaculates. We collected two independent samples of both spermless spermatophores and normal spermatophores in liquid nitrogen, for a total of 4 samples (N = 25 males per sample). We homogenized each sample in 100 ul of ice-cold PBS and centrifuged (14,000 rpm for 1 min at 4°C) to separate the ejaculate from most sperm and spermatophore debris. The 2D–E analysis, including sample preparation and quantification, first and second dimension separations using isoelectric focusing and Tris-SDS-PAGE electrophoresis, gel staining, image capture and analysis were carried out by the Cornell Core Laboratories Center for Proteomics and Mass Spectrometry.
Influence of the G. firmus ejaculate on egg-laying and longevity
To test the effects of seminal fluids on egg-laying in G. firmus females, we measured the total number of eggs produced by G. firmus females that 1) remained unmated (F = 57), 2) were mated to G. firmus males that were surgically castrated (FFC = 56), 3) G. firmus males that underwent a sham castration (FFS = 61), and 4) normal G. firmus males (FF = 60). By surgically castrating the G. firmus males, we could compare the effects on egg-laying of SFPs alone with the effects of the complete male ejaculate.
In other insects (including crickets) components of the male ejaculate typically elicit a short-term egg-laying response within 24 h of mating. To estimate both the initial egg-laying response and a female's lifetime fecundity, we collected oviposition substrates at both 48 h following mating and at the end of the female's lifespan. We collected substrates at 48 h to allow each female time to adjust following transfer to a new container and provide sufficient time for egg-laying; G. firmus females that are frequently disturbed are less inclined to oviposit (EL Larson personal observation). Eggs were separated from the oviposition substrate using a series of sieves and we counted the total number of eggs for each time point (within 48 h and after 48 h).
Influence of the G. firmus ejaculate on the one-way incompatibility
We performed two experiments to test whether the presence of a G. firmus male's ejaculate within the female reproductive tract could “rescue” the incompatibility (reduced egg-laying, no fertilization) between G. firmus females and G. pennsylvanicus males. For the first experiment G. firmus females were either mated to a normal G. firmus male immediately followed by a G. pennsylvanicus male (FFP = 9) or were mated first to a G. pennsylvanicus male followed by a normal G. firmus male (FPF = 11). Females were provided with oviposition substrate immediately after mating, and then allowed to oviposit for three weeks. Eggs were incubated at 28°C for 21 days and then at 4°C for 102 days to break diapause conditions and ensure synchronous hatching . Eggs were then removed from chilled conditions and incubated at 28°C until hatching (approximately 17 days). We collected all hatchlings (1st instar nymphs) each morning until all eggs hatched and stored nymphs at −80°C for paternity analysis. We randomly selected 20 nymphs per cross for genotyping.
For paternity analysis, we used highly polymorphic microsatellite markers (PGI, Gr143, G3 and G28). Two of these loci were developed from G. pennsylvanicus, and have been previously described . The remaining two loci were developed from G. firmus using methods described in Hamilton et al.  and Larson et al.  with the addition of an enrichment by hybridization with biotinylated dimeric, trimeric and tetrameric nucleotide repeats. We quantified genetic variation for these new loci in one population of each species (G. pennsylvanicus: Ithaca, NY, USA; G. firmus: Guilford, CT, USA) (Table 1). Tests for linkage disequilibrium and deviation from Hardy-Weinberg equilibrium were performed using Genepop v. 4.1  and we adjusted significance thresholds using the false discovery rate procedure . Cervus v 3.0  was used to test parentage exclusion probabilities, estimate null alleles and the polymorphic information content of the markers.
Parental genomic DNA extractions from single femurs were performed using the DNeasy Blood and Tissue Kit (QIAGEN Inc., Valencia, CA, USA); offspring genomic DNA was extracted from entire nymphs using the DNAdvance Genomic DNA Isolation Kit (Agencourt, Beverly, MA, USA). The forward primer of each primer pair was labeled with a 5′ fluorescent tag (6-FAM, PET, NED, or VIC). We amplified these microsatellite loci using the Type-it Micosatellite PCR Kit (QIAGEN) following manufacturer's protocol with the addition of a touchdown protocol of 28 cycles of 95°C for 30 s, 59–53°C for 90 s (the annealing temperature decreased by 1°C each cycle for the first 6 cycles and remained at 53°C for the remaining 22 cycles) and 72°C for 30 s. Fluorescent PCR products were diluted 1∶15 in water, mixed with formamide and Genescan LIZ-500 size standard (Applied Biosystems Inc. Foster City, CA, USA) and run on an ABI Automated 3730 DNA Analyzer at the Cornell University Life Sciences Core Laboratories Center (CLC). Alleles were called using Genemapper (Applied Biosystems) and then verified by eye. The high level of polymorphism in our markers allowed us to assign paternity by eye.
For the second experiment G. firmus females were either mated to a surgically castrated male G. firmus male immediately followed by a G. pennsylvanicus male (FFCP = 3), a G. pennsylvanicus male immediately followed by a surgically castrated G. firmus male (FPFC = 12), or a normal G. pennsylvanicus male (FP = 10). After mating, females were provided with oviposition substrate and allowed to oviposit for 48 h. We then counted the total number of eggs laid by each female.
To investigate the influence of G. firmus SFPs on G. firmus female egg-laying within 48 h of mating and after 48 h of mating, we constructed generalized linear mixed model (GLMM) contrasts to test the following hypotheses: Model 1: females mated with normal males (FF) will lay more eggs than females mated with males that that underwent sham castration (FFS); Model 2: females mated with surgically castrated males (FFC) will lay more eggs than unmated females (F); and Model 3: females in treatments without sperm (F, FFC) will lay fewer eggs than females in treatments with sperm (FF, FFS). Differences between collecting locations were controlled by including a random effect of population identity. Using the R package ‘lme4’ , we modeled the proportion of females that laid eggs within 48 h with GLMMs fitted with a binomial error structure and a logit link function and the male treatment as the predictor. The egg-count data were highly over-dispersed; therefore, we modeled the total number of eggs laid by G. firmus females after 48 h using GLMMs with a Poisson distribution, individual-level random effects , and male treatment as the predictor. To compare longevity of females between mating treatments we estimated survival curves using the Kaplan-Meier method and compared differences between treatments using the log-rank test in the R package ‘survival’ .
To test the influence of the G. firmus ejaculate on the one-way incompatibility, we modeled the effect of male species on the proportion of offspring sired by the second male (P2) for G. firmus females mated sequentially to both G. firmus and G. pennsylvanicus males. We constructed a GLM with binomial error structure and a logit link function using P2 as the response variable and the male species as the predictor. For the second experiment involving G. firmus females mated with surgically castrated G. firmus males and G. pennsylvanicus males no statistics were required to interpret the results. Figures were constructed using the R packages ‘plotrix’  and ‘gplots’ . All analyses were performed using the statistical package R version 2.12.0 .
Seminal fluid protein content of spermless spermatophores
Representative examples of the 2D–E gels for the normal ejaculates (with sperm removed via centrifugation) and a spermless ejaculates are presented in Figure 3. Each spot represents a protein isoform. Overall, we estimate that there are about 630 protein spots present in all four samples. The patterns seen for normal and spermless spermatophore are very similar. Extra spots seen in the normal spermatophore extracts are presumably due to contamination from residual sperm.
Protein gels of a normal male ejaculate (left) and a spermless male ejaculate (right). Spermatophore samples were ground and centrifuged to remove spermatophore debris and sperm. Proteins were separated based on their isoelectric point in the first dimension and molecular weight in the second.
Influence of the G. firmus ejaculate on egg-laying
When sperm are transferred to females (FF vs FFS), there is no effect of sham castration on either the proportion of females that laid eggs within 48 h (Fig. 4, GLMM: z = −0.451, df = 6, p = 0.652) or the number of eggs laid after 48 h (Fig. 5, GLMM: z = −1.12, df = 6, p = 0.263). A greater proportion of females mated with surgically castrated males (FFC) laid eggs in 48 h compared to females that remained unmated (F) (GLMM: z = 2.442, df = 6, p = 0.015); however, there was no significant difference in the number of eggs laid after 48 h (GLMM: z = −1.38, df = 6, p = 0.167). Comparisons between females mated with males that transferred sperm (FF, FFS) and females that did not receive sperm (FFC, F) revealed that in the former group there was both a greater proportion of females that laid eggs within 48 h (GLMM: z = 7.155, df = 6, p = <0.001) and females laid more eggs after 48 h (GLMM: z = −10.15, df = 6, p = <0.001).
Females were mated with (1) a normal G. firmus male (FF), (2) a G. firmus male that underwent sham testes removal surgery (FFS), (3) a G. firmus male surgically castrated (FFC) or (4) remained unmated (F).
Box plot of egg production A) 48 h following mating and B) total lifetime for G. firmus females that (1) mated with a normal G. firmus male (FF), (2) mated with a G. firmus male that underwent sham testes removal surgery (FFS), (3) mated with a G. firmus male surgically castrated (FFC) or (4) remained unmated (F).
Influence of the G. firmus ejaculate on female longevity
Female life span ranged from 7–84 days following mating (FF: 7–71; FFS: 17–84; FFC: 17–69; F: 17–73) with an average lifespan of 44 days (FF: 45.8; FFS: 41.8; FFC: 42.7; 47.6). There was no difference in lifespan among the four mating treatments (Fig. 6, log-rank: χ2 = 0.2, df = 3, p = 0.972).
Survivorship curves of G. firmus females (1) mated with a normal G. firmus male (FF), (2) mated with a G. firmus male that underwent sham testes removal surgery (FFS), (3) mated with a G. firmus male surgically castrated (FFC) or (4) remained unmated (F).
Influence of the G. firmus ejaculate on one-way incompatibility
None of the microsatellite loci used in this study deviated from Hardy-Weinberg equilibrium following false discovery rate correction and there was no evidence of linkage disequilibrium between any pair of loci (Table 1). Despite the presence of null alleles in two of these loci (PGI and G28), the combined nonexclusion probability of the second parent across all four loci was 0.004 and 0.006 for G. firmus and G. pennsylvanicus, respectively, indicating that these markers are appropriate for assigning paternity. Of the 474 nymphs selected for genotyping, 98.9% were genotyped and assigned paternity successfully. The remaining 1.1% had poor microsatellite amplification, most likely due to low quantities of DNA as a result of little starting material. We did not observe any non-parental alleles in the offspring. Gryllus firmus females mated sequentially to G. firmus and G. pennsylvanicus males (FFP, FPF) produced offspring that were sired only by G. firmus males regardless of mating order (t = −8.05×1015, df = 1, p = <0.001). Gryllus firmus females mated sequentially to surgically castrated G. firmus males and G. pennsylvanicus males (FFCP, FPFC) and G. firmus females mated only to G. pennsylvanicus males (FP) laid no eggs within a 48 h period.
Gryllus firmus seminal fluid proteins induce only a marginal egg-laying response
Following mating, female insects undergo numerous physiological and behavioral changes. Pre-mating courtship or the mechanical stimulus of copulation can cause these changes, but the majority of changes are induced by components of the male ejaculate. In insects, sperm clearly play a critical role in fertilization, but many aspects of sperm function (viability, storage, activation, competition) and female response to mating (mating refractoriness, oogenesis, sperm utilization, ovulation, oviposition) are mediated by SFPs secreted from the male accessory glands or ejaculatory duct , , , , . Seminal fluid proteins were first linked to these post-mating changes via whole tissue transplantation experiments in Drosophila melanogaster, where portions of the male accessory glands or testes were transplanted into the abdomens of virgin females , . Subsequently, methods to isolate the roles of SFPs in fertilization have ranged from simple injections of SFP extracts into virgin females to the creation of “spermless” or “accessory glandless” males and the targeted knockdown of specific SFPs using RNAi , , .
Much of this effort has focused on how components of the male ejaculate elevate egg-laying in mated females. In Drosophila, where egg-laying is best understood, the male ejaculate alters a female's reproductive physiology over different timescales. Initially, there is a short-term increase in the number of eggs laid within the first 24 h of mating , . This short-term response is induced by the presence of at least three SFPs in the female reproductive tract, sex peptide (SP, Acp70A), the prohormone ovulin (Acp26Aa) and CG33943 –. However, this response is transient, and the presence of both sperm and SFPs in the sperm storage organ is required to maintain elevated levels of egg-laying , . This so-called sperm effect or long-term post-mating response was thought to be induced by sperm-binding receptors or stretch receptors within the female sperm storage organ . It is now clear that the sperm effect, at least in Drosophila, is actually an SFP effect, mediated in part by the SFP sex peptide , . Sex peptide binds to the tails of sperm and is slowly released from sperm within the female storage organ , , . It appears that sperm may act as both carriers and reservoirs for SFPs, enabling sperm to reach target cells within the female reproductive tract and maintaining their effects on female reproduction over an extended period. At least four other SFPs have been identified that act in concert with sex peptide to sustain the long-term post-mating response, and at least one of these proteins also binds to sperm , .
Drosophila has been a model for understanding post-mating male and female interactions, and from this work it has become clear that seminal fluid proteins stimulate egg-laying in mated females but that to do so they must interact with sperm. However, this picture of reproduction appears to vary greatly across taxa. In other Dipterans there is evidence that SFPs alone can induce egg-laying in mated females , , whereas in Lepidoptera egg-laying is often triggered by the presence of eupyrene sperm in the spermatheca –, but there is at least one case of SFPs inducing partial egg-laying . There are few examples from the Coleoptera, but in at least two species both components of the testis/seminal vesicle and the accessory gland induce egg-laying, although the accessory gland extracts had a minimal influence .
In Orthoptera, the picture is even less clear. Egg-laying is stimulated by SFPs in some grasshoppers – and in ground crickets , while in at least one grasshopper the combination of mechanical stimulus and testis derived components can induce egg-laying . In the field crickets, Acheta domesticus and Teleogryllus commodus egg-laying is initially induced by prostaglandins, autocrine hormones transferred to females as part of the seminal fluid –, but the presence of sperm in the spermatheca is required to maintain long term egg-laying (similar to Drosophila) , . Prostaglandins or prostaglandin precursors have been found to be synthesized in both the testes (T. commodus and A. domesticus) and the accessory glands (A. domesticus and Locusta migratoria) of Orthoptera, although the prostaglandins found in L. migratoria do not appear to be involved in egg-laying . The only study to attempt to induce egg-laying in field crickets using whole ejaculatory-fluid extracts failed to see a response . However, in that study ejaculate extracts were injected into the abdominal cavity and may have failed to elicit an egg-laying response because SFPs did not reach target receptors within the female reproductive tract.
Our use of castrated males to transfer SFPs to virgin females is a more effective way of delivering SFPs directly into the female reproductive tract while controlling for any effects of mating. Still, we found that SFPs without the presence of sperm or other testis-derived compounds induced only a modest short-term egg-laying response in the field cricket G. firmus. This response is small compared to egg-laying in normally mated females, a result in stark contrast to the induction of egg-laying seen in other taxa. In the long-term, there was no difference in the fecundity of virgin females and those that received SFPs. This suggests that SFPs indeed play some role in eliciting egg-laying behavior over the short term, but that testis derived factors are required for both the short and long term post-mating egg-laying response in G. firmus.
It might be argued that the “effectors” of egg-laying did not reach their targets in the female reproductive tract. However, we know that spermatophores of surgically castrated males transfer seminal fluid. Seminal fluid can be directly observed evacuating the spermatophore tube of spermless spermatophores (see Methods). Furthermore, analysis of this fluid using 2-D gel electrophoresis clearly reveals the same pattern of protein spots that are seen in extracts from normal spermatophores (Fig. 3).
There is also no reason to believe that the multiple matings required to create the spermless males adversely affect SFP volume or content. Field crickets are highly promiscuous and males mate repeatedly both in the wild and the laboratory –. Males will only re-mate when a fully formed spermatophore is present in their spermatophore pouch , . As a result, both the timing and the frequency of matings in field crickets are dependent on spermatophore production, which in Gryllus firmus males is approximately every 45 minutes throughout the day , . Both the spermatophore and the seminal fluid are composed of proteins secreted by the male accessory gland ,  and it is unlikely that a male would have sufficient accessory gland function to produce a spermatophore, but not the seminal fluid proteins. There is also evidence that male insect ejaculate content is consistent across repeated matings  and throughout their lifetime , . In our protocol, castrated males were mated repeatedly only during the first two days following surgery recovery. Subsequently, they only mated once a day for a minimum of four days, well below the expected number of matings for a male field cricket. Thus, our treatment should not compromise SFP production.
Given our observation of SFPs in the seminal fluid of spermless spermatophores and our delivery method of SFPs directly into the female reproductive tract (as opposed to abdominal injections), our failure to find any large or long term egg-laying response induced by SFPs suggests that SFPs alone are not sufficient to stimulate egg-laying in G. firmus. This is consistent with a similar failure of SFPs to induce egg-laying in G. bimaculatus . It is possible, even very likely, that we see a failure of SFPs to induce egg-laying in field crickets because key SFPs bind to the sperm for transport into the female reproductive tract as has been demonstrated in Drosophila , , , , , .
The question of what components of the male ejaculate stimulate egg-laying is an important one, not simply for a better understanding of insect reproduction, but because these components, if diverged, may constitute a barrier to gene exchange between closely related taxa. To our knowledge, only one study, in Drosophila pulchrella and D. suzukii, has attempted to differentiate between the components of the male ejaculate that induce egg-laying in heterospecific crosses. In that case, a one-way incompatibility between D. pulchrella females and D. suzukii males is a result of both low sperm storage and severely reduced egg-laying. When D. pulchrella females are implanted with accessory gland tissue from conspecifics they have an ovulation rate that is 75% of a normally mated female, whereas females implanted with heterospecific accessory glands have an ovulation rate of only 54% , .
Gryllus firmus seminal fluids do not affect female lifespan
Mating is often costly to females and results in decreased lifespan due to SFPs that are toxic to females. For example in Drosophila, females that receive SFPs during mating have a reduced lifespan , but these SFPs serve to increase male mating success . In species, such as crickets, that are promiscuous and mate more often than is required for fertilization of their eggs, the male ejaculate may actually increase female lifespan , or have no effect . In one case, female lifespan in the cricket G. bimaculatus was reduced as a result of the injection of SFPs into the female abdomen, but it is difficult to determine whether this is a normal effect of SFPs or a result of SFPs present in the body cavity where they may be toxic . We found no effect of SFPs on female lifespan. This is consistent with similar studies in Gryllus firmus and G. pennsylvanicus that found no difference in the lifespan of singly mated, doubly mated and virgin females , despite the fact that virgin females and females mated with surgically castrated males are often ‘bursting’ with eggs (EL Larson personal observation). It is possible that there are lifespan benefits or costs to mating, but that a greater number of matings is required to see an effect in G. firmus.
Gryllus firmus seminal fluid proteins alone do not rescue the one-way incompatibility
In Drosophila, sperm function is dependent on the presence of SFPs, and males that transfer only sperm (prd males) are completely sterile. However, females mated to prd males and subsequently mated to males transferring only SFPs (tud males) can occasionally lay fertile eggs . The number of rescued crosses is very low (less than 1%). Nonetheless, this suggests that SFPs from one male can facilitate fertilization by the sperm of a second male. Alternatively, SFPs could act as a specific stimulus, only affecting sperm from the same male, or complementation may only be possible within species and SFPs may not interact with heterospecific sperm.
Our results suggest that in G. firmus, the latter is the case. The G. firmus male ejaculate was unable to facilitate fertilization for heterospecific sperm and G. firmus males sired all offspring in females mated sequentially with both species. Similar results have been observed in double matings of the lacewing species Chrysopa quadripunctata and C. slossonae, but in these taxa, there are fewer heterospecific sperm stored . Gryllus firmus male SFPs also failed to induce egg-laying when G. pennsylvanicus sperm were present in the spermatheca. Therefore, failure of G. firmus SFPs alone to stimulate normal egg-laying in G. firmus females is not simply a result of mechanical stimulus (e.g., stretch receptors in the spermatheca). SFPs may need to act in concert with sperm to induce egg-laying in G. firmus females. Unfortunately, we are not able to test whether testis-derived compounds alone can induce oviposition. Surgical removal of accessory glands would prevent the formation of the spermatophore necessary to transfer sperm to a female.
Our results highlight the utility of experimental approaches for investigating the phenotypes that act as barriers between species and provide new directions for investigating the molecular changes that lead to these barriers. The nature of the one-way incompatibility between G. firmus females and G. pennsylvanicus males suggests a role for SFPs, and both egg-laying and fertilization are traits that are often mediated by SFPs in other taxa. In addition, many SFPs are highly divergent between G. firmus and G. pennsylvanicus and appear to be evolving as a result of positive selection , . Although the results of this study do not exclude a role for SFPs in these barriers, they do suggest that SFPs are not solely responsible for successful egg-laying. In particular, testis derived components, such as sperm or prostaglandins, either stimulate egg-laying or act as transporters for SFPs to targets in the female reproductive tract. Future work on the molecular basis of the one-way incompatibility between G. firmus and G. pennsylvanicus should focus on divergent testis-derived compounds or proteins.
A great deal of research on post-mating prezygotic barriers in internal fertilizers has concentrated on the role of SFPs –, but our results suggest that focusing on SFPs alone is too narrow. Although there are now numerous examples of rapid divergence in SFPs between closely related species across diverse taxonomic groups  and there is some evidence of post-mating prezygotic barriers between several of these species , , there are few studies that provide a functional link between the rapid evolution of SFPs and post-mating prezygotic barriers. While documenting patterns of divergence between species is an important step, functional studies through experimental crosses are needed to determine whether divergent genes play a role in reproductive barriers between species.
We thank Nicholas Saleh and Eliana Bondra for assistance with data collection, Joseph Simonis for assistance with statistical analyses and members of the Harrison laboratory for thoughtful comments on the manuscript.
Conceived and designed the experiments: ELL JAA RGH. Performed the experiments: ELL. Analyzed the data: ELL JAA. Contributed reagents/materials/analysis tools: ELL JAA RGH. Wrote the paper: ELL JAA RGH.
- 1. West-Eberhard MJ (1983) Sexual selection, social competition, and speciation. Q Rev Biol 58: 155–183.
- 2. Andersson M (1994) Sexual selection. Princeton: Princeton University Press. 588 p.
- 3. Civetta A, Singh RS (1998) Sex-related genes, directional sexual selection, and speciation. Mol Biol Evol 15: 901–909.
- 4. Panhuis TM, Butlin R, Zuk M, Tregenza T (2001) Sexual selection and speciation. Trends Ecol Evol 16: 364–371.
- 5. Ritchie MG (2007) Sexual selection and speciation. Annu Rev Ecol Syst 38: 79–102.
- 6. Snook R, Chapman T, Moore P, Wedell N, Crudgington H (2009) Interactions between the sexes: new perspectives on sexual selection and reproductive isolation. Evol Ecol 23: 71–91.
- 7. Wolfner MF (1997) Tokens of love: functions and regulation of Drosophila male accessory gland products. Insect Biochem Mol Biol 27: 179–192.
- 8. Wolfner MF (2009) Battle and ballet: molecular interactions between the sexes in Drosophila. J Hered 100: 399–410.
- 9. Howard DJ (1999) Conspecific sperm and pollen precedence and speciation. Annu Rev Ecol Syst 30: 109–132.
- 10. Howard DJ, Palumbi SR, Birge LM, Manier MK (2009) Sperm and speciation. In: Birkhead TR, Hosken DJ, Pitnick S, editors. Sperm Biology: An Evolutionary Perspective. Burlington, MAUSA: Academic Press. pp. 267–403.
- 11. Larson EL, Hume GL, Andrés JA, Harrison RG (2012) Post-mating prezygotic barriers to gene exchange between hybridizing field crickets. J Evol Biol 25: 174–186.
- 12. Bloch Qazi M, Heifetz Y, Wolfner MF (2003) The developments between gametogenesis and fertilization: ovulation and female sperm storage in Drosophila melanogaster. Dev Biol 256: 195–211.
- 13. Fuyama Y (1983) Species-specificity of paragonial substances as an isolating mechanism in Drosophila. Experientia 39: 190–192.
- 14. Price CSC, Kim CH, Gronlund CJ, Coyne JA (2001) Cryptic reproductive isolation in the Drosophila simulans species complex. Evolution 55: 81–92.
- 15. Wade MJ, Patterson H, Chang NW, Johnson NA (1994) Postcopulatory, prezygotic isolation in flour beetles. Heredity 72: 163–167.
- 16. Shapiro LH (2000) Reproductive costs to heterospecific mating between two hybridizing katydids (Orthoptera: Tettigoniidae). Ann Entomol Soc Am 93: 440–446.
- 17. Albuquerque G, Tauber C, Tauber M (1996) Postmating reproductive isolation between Chrysopa quadripunctata and Chrysopa slossonae: Mechanisms and geographic variation. Evolution 50: 1598–1606.
- 18. Gregory PG, Howard DJ (1993) Laboratory hybridization studies of Allonemobius fasciatus and A. socius (Orthoptera, Gryllidae). Ann Entomol Soc Am 86: 694–701.
- 19. Brown DV, Eady PE (2001) Functional incompatibility between the fertilization systems of two allopatric populations of Callosobruchus maculatus (Coleoptera: Bruchidae). Evolution 55: 2257–2262.
- 20. Messina FJ, Bloxham AJ, Seargent AJ (2007) Mating compatibility between geographic populations of the seed beetle Callosobruchus maculatus. J Insect Behav 20: 489–501.
- 21. Leopold RA (1976) Role of male accessory glands in insect reproduction. Annu Rev Entomol 21: 199–221.
- 22. Kubli E (2003) Sex-peptides: seminal peptides of the Drosophila male. Cell Mol Life Sci 60: 1689–1704.
- 23. Willett CS, Ford MJ, Harrison RG (1997) Inferences about the origin of a field cricket hybrid zone from a mitochondrial DNA phylogeny. Heredity 79: 484–494.
- 24. Harrison R, Arnold SJ (1982) A narrow hybrid zone between closely related cricket species. Evolution 36: 535–552.
- 25. Harrison RG (1985) Barriers to gene exchange between closely related cricket species. II. life-cycle variation and temporal isolation. Evolution 39: 244–259.
- 26. Rand DM, Harrison RG (1989) Ecological genetics of a mosaic hybrid zone - mitochondrial, nuclear, and reproductive differentiation of crickets by soil type. Evolution 43: 432–449.
- 27. Ross CL, Harrison RG (2002) A fine-scale spatial analysis of the mosaic hybrid zone between Gryllus firmus and Gryllus pennsylvanicus. Evolution 56: 2296–2312.
- 28. Ross CL, Harrison RG (2006) Viability selection on overwintering eggs in a field cricket mosaic hybrid zone. Oikos 115: 53–68.
- 29. Harrison RG, Rand DM (1989) Mosaic hybrid zones and the nature of species boundaries. In: Otte D, Endler JA, editors. Speciation and its Consequences. Sunderland, MA: Sinauer. pp. 111–133.
- 30. Doherty JA, Storz MM (1992) Calling song and selective phonotaxis in the field crickets, Gryllus firmus and G. pennsylvanicus (Orthoptera, Gryllidae). J Insect Behav 5: 555–569.
- 31. Maroja LS, Andrés JA, Walters JR, Harrison RG (2009) Multiple barriers to gene exchange in a field cricket hybrid zone. Biol J Linn Soc 97: 390–402.
- 32. Harrison RG (1983) Barriers to gene exchange between closely related cricket species. I. laboratory hybridization studies. Evolution 37: 245–251.
- 33. Maroja LS, Clark ME, Harrison RG (2008) Wolbachia plays no role in the one-way reproductive incompatibility between the hybridizing field crickets Gryllus firmus and G. pennsylvanicus. Heredity 101: 435–444.
- 34. Andrés JA, Maroja LS, Bogdanowicz SM, Swanson WJ, Harrison RG (2006) Molecular evolution of seminal proteins in field crickets. Mol Biol Evol 23: 1574–1584.
- 35. Braswell WE, Andres JA, Maroja LS, Harrison RG, Howard DJ, et al. (2006) Identification and comparative analysis of accessory gland proteins in Orthoptera. Genome 49: 1069–1080.
- 36. Andrés JA, Maroja LS, Harrison RG (2008) Searching for candidate speciation genes using a proteomic approach: seminal proteins in field crickets. Proc R Soc Lond, Ser B: Biol Sci 275: 1975–1983.
- 37. Hamilton MB, Pincus EL, Di Fiore A, Fleischer RC (1999) Universal linker and ligation procedures for construction of genomic DNA libraries enriched for microsatellites. BioTechniques 27: 500–507.
- 38. Raymond M, Rousset F (1995) Genepop (version-1.2) - population-genetics software for exact tests and ecumenicism. J Hered 86: 248–249.
- 39. Benjamini Y, Hochberg Y (1995) Controlling the false discovery rate: a practical and powerful approach to multiple testing. J Roy Stat Soc Ser B (Stat Method) 57: 289–300.
- 40. Kalinowski ST, Taper ML, Marshall TC (2007) Revising how the computer program cervus accommodates genotyping error increases success in paternity assignment. Mol Ecol 16: 1099–1106.
- 41. Bates D, Maechler M, Bolker B (2011) lme4: Linear mixed-effects models using S4 classes. Vienna, Austria: R Foundation for Statistical Computing.
- 42. Therneau T (2011) survival: Survival analysis, including penalised likelihood. Vienna, Austria: R Foundation for Statistical Computing.
- 43. Lemon J (2006) Plotrix: a package in the red light district of R. R-News 6: 8–12.
- 44. Warnes GR (2010) gplots: Various R programming tools for plotting data. Vienna, Austria: R Foundation for Statistical Computing.
- 45. R Core Development Team (2010) R: A language and environment for statistical computing. 2.12.0 ed. Vienna, Austria: R Foundation for Statistical Computing.
- 46. Engelmann F (1970) The physiology of insect reproduction: Pergamon Press. 307 p.
- 47. Gillott C (2003) Male accessory gland secretions: modulators of female reproductive physiology and behavior. Annu Rev Entomol 48: 163–184.
- 48. Garcia-Bellido A (1964) Das sekret der paragonien als stimulus der fekunditat bei weibchen von Drosophila melanogaster. Zeitschrift Fur Naturforschung Part B-Chemie Biochemie Biophysik Biologie Und Verwandten Gebiete B 19: 491–495.
- 49. Merle J (1968) Ovarian functioning and sexual receptiveness of Drosophila melanogaster after implantation of male genital fragments. J Insect Physiol 14: 1159–1168.
- 50. Kalb JM, Dibenedetto AJ, Wolfner MF (1993) Probing the function of Drosophila melanogaster accessory glands by directed cell ablation. Proc Natl Acad Sci U S A 90: 8093–8097.
- 51. Herndon LA, Wolfner MF (1995) A Drosophila seminal fluid protein, Acp26Aa, stimulate egg-laying in females for one day after mating. Proc Natl Acad Sci U S A 92: 10114–10118.
- 52. Heifetz Y, Lung O, Frongillo EA Jr, Wolfner MF (2000) The Drosophila seminal fluid protein Acp26Aa stimulates release of oocytes by the ovary. Curr Biol 10: 99–102.
- 53. Chapman T, Bangham J, Vinti G, Seifried B, Lung O, et al. (2003) The sex peptide of Drosophila melanogaster: female post-mating responses analyzed by using RNA interference. Proc Natl Acad Sci U S A 100: 9923–9928.
- 54. Liu HF, Kubli E (2003) Sex-peptide is the molecular basis of the sperm effect in Drosophila melanogaster. Proc Natl Acad Sci U S A 100: 9929–9933.
- 55. Ram KR, Wolfner MF (2007) Sustained post-mating response in Drosophila melanogaster requires multiple seminal fluid proteins. PLoS Genet 3: 2428–2438.
- 56. Manning A (1962) Sperm factor affecting receptivity of Drosophila melanogaster females. Nature 194: 252–253.
- 57. Manning A (1967) Control of sexual receptivity in female Drosophila. Anim Behav 15: 239–250.
- 58. Kubli E (1992) My favorite molecule. The sex-peptide. Bioessays 14: 779–784.
- 59. Peng J, Chen S, Büsser S, Liu H, Honegger T, et al. (2005) Gradual release of sperm bound sex-peptide controls female postmating behavior in Drosophila. Curr Biol 15: 207–213.
- 60. Ram KR, Wolfner MF (2009) A network of interactions among seminal proteins underlies the long-term postmating response in Drosophila. Proc Natl Acad Sci U S A 106: 15384–15389.
- 61. Leahy MG, Craig GB (1965) Accessory gland substance as a stimulant for oviposition in Aedes aegypti and Aedes albopictus. Mosq News 25: 448–452.
- 62. Thailayil J, Magnusson K, Godfray HCJ, Crisanti A, Catteruccia F (2011) Spermless males elicit large-scale female responses to mating in the malaria mosquito Anopheles gambiae. Proc Natl Acad Sci U S A 108: 13677–13681.
- 63. Thibout E (1979) Stimulation of reproductive activity of females of Acrolepiosis assectella (Lepidoptera, Hyponomeutoidea) by the presence of eupyrene spermatozoa in the spermatheca. Entomol Exp Appl 26: 279–290.
- 64. Karube F, Kobayashi M (1999) Presence of eupyrene spermatozoa in vestibulum accelerates oviposition in the silkworm moth, Bombyx mori. J Insect Physiol 45: 947–957.
- 65. Xu J, Wang Q (2011) Seminal fluid reduces female longevity and stimulates egg production and sperm trigger oviposition in a moth. J Insect Physiol 57: 385–390.
- 66. Jin Z-Y, Gong H (2001) Male accessory gland derived factors can stimulate oogenesis and enhance oviposition in Helicoverpa armigera (Lepidoptera: Noctuidae). Arch Insect Biochem Physiol 46: 175–185.
- 67. Yamane T, Miyatake T (2010) Induction of oviposition by injection of male-derived extracts in two Callosobruchus species. J Insect Physiol 56: 1783–1788.
- 68. Pickford R, Ewen AB, Gillott C (1969) Male accessory gland substance: an egg-laying stimulant in Melanoplus sanguinipes (F)(Orthoptera, Acrididae). Can J Zool 47: 1199–1203.
- 69. Leahy MG (1973) Oviposition of virgin Schistocerca gregaria (Forskal) (Orthoptera, Acrididae) after implant of male accessory gland complex. J Entomol Ser A Physiol Behav 48: 69–78.
- 70. Friedel T, Gillott C (1976) Male accessory gland substance of Melanoplus sanguinipes: ovipostion stimulant under control of corpus allatum. J Insect Physiol 22: 489–&.
- 71. Lange AB, Loughton BG (1985) An oviposition-stimulating factor in the male accessory reproductive gland of the locust, Locusta migratoria. Gen Comp Endocrinol 57: 208–215.
- 72. Yi SX, Gillott C (1999) Purification and characterization of an oviposition-stimulating protein of the long hyaline tubules in the male migratory grasshopper, Melanoplus sanguinipes. J Insect Physiol 45: 143–150.
- 73. Marshall JL, Huestis DL, Hiromasa Y, Wheeler S, Oppert C, et al. (2009) Identification, RNAi knockdown, and functional analysis of an ejaculate protein that mediates a postmating, prezygotic phenotype in a cricket. PLoS ONE 4: e7537.
- 74. Quo F (1959) Studies on the reproduction of the Oriental migratory locust: The physiological effects of castration and copulation. Acta Ent Sinica 9: 464–476.
- 75. Destephano DB, Brady UE (1977) Prostaglandin and prostaglandin synthetase in the cricket, Acheta domesticus. J Insect Physiol 23: 905–911.
- 76. Loher W (1979) The influence of prostaglandin E2 on oviposition in Teleogryllus commodus. Entomol Exp Appl 25: 107–109.
- 77. Loher W, Ganjian I, Kubo I, Stanleysamuelson D, Tobe SS (1981) Prostaglandins - their role in egg-laying of the cricket Teleogryllus commodus. Proc Natl Acad Sci U S A 78: 7835–7838.
- 78. Lange AB (1984) The transfer of prostaglandin-synthesizing activity during mating in Locusta migratoria. Insect Biochem 14: 551–556.
- 79. Stanley-Samuelson DW, Peloquin JJ (1986) Egg-laying in response to prostaglandid injections in the Australian field cricket, Telelgryllus commodus. Physiol Entomol 11: 213–219.
- 80. Murtaugh MP, Denlinger DL (1985) Physiological regulation of long-term oviposition in the house cricket, Acheta domesticus. J Insect Physiol 31: 611–617.
- 81. Murtaugh MP, Denlinger DL (1987) Regulation of long-term oviposition in the house cricket, Acheta domesticus: roles of prostaglandin and factors associated with sperm. Arch Insect Biochem Physiol 6: 59–72.
- 82. Stanley D, Kim Y (2011) Prostaglandins and their receptors in insect biology. Front Endocrinol 2: 1–11.
- 83. Green K, Tregenza T (2009) The influence of male ejaculates on female mate search behaviour, oviposition and longevity in crickets. Anim Behav 77: 887–892.
- 84. Alexander R, Otte D (1967) The evolution of genitalia and mating behavior in crickets (Gryllidae) and other Orthoptera. Misc Publ Mus Zool Univ Mich 133: 1–62.
- 85. Bretman A, Tregenza T (2005) Measuring polyandry in wild populations: a case study using promiscuous crickets. Mol Ecol 14: 2169–2179.
- 86. Rodriguez-Munoz R, Bretman A, Slate J, Walling CA, Tregenza T (2010) Natural and sexual selection in a wild insect population. Science 328: 1269–1272.
- 87. Sakaluk SK (1987) Reproductive-behavior of the decorated cricket, Gryllodes supplicans (Orthoptera, Gryllidae)- calling schedules, spatial-distribution, and mating. Behaviour 100: 202–225.
- 88. Sakaluk SK, Schaus JM, Eggert AK, Snedden WA, Brady PL (2002) Polyandry and fitness of offspring reared under varying nutritional stress in decorated crickets. Evolution 56: 1999–2007.
- 89. Simmons LW (1988) Male size, mating potential and lifetime reproductive success in the field cricket, Gryllus bimaculatus (Degeer). Anim Behav 36: 372–379.
- 90. Tregenza T, Wedell N (1998) Benefits of multiple mates in the cricket Gryllus bimaculatus. Evolution 52: 1726–1730.
- 91. Wagner WE, Harper CJ (2003) Female life span and fertility are increased by the ejaculates of preferred males. Evolution 57: 2054–2066.
- 92. Wagner WE, Kelley RJ, Tucker KR, Harper CJ (2001) Females receive a life-span benefit from male ejaculates in a field cricket. Evolution 55: 994–1001.
- 93. Loher W, Dambach M (1989) Reproductive Behavior. In: Huber F, Moore TE, Loher W, editors. Cricket Behavior and Neurobiology. Ithaca, NY: Cornell University Press. pp. 43–82.
- 94. Zuk M, Simmons L (1997) Reproductive strategies of the crickets (Orthoptera: Gryllidae). In: Choe J, Crespi B, editors. The Evolution of Mating Systems in Insects and Arachnids. Cambridge: Cambridge University Press. pp. 89–109.
- 95. Chapman RF (1998) The Insects: Structure and Function. New York: Cambridge University Press. 819 p.
- 96. Heller KG, Faltin S, Fleischmann P, von Helversen O (1998) The chemical composition of the spermatophore in some species of phaneropterid bushcrickets (Orthoptera: Tettigonioidea). J Insect Physiol 44: 1001–1008.
- 97. Schaus JM, Sakaluk SK (2002) Repeatability of sperm number across multiple matings in three cricket species, Gryllodes sigillatus, Gryllus veletis, and Gryllus texensis (Orthoptera: Gryllidae). Can J Zool 80: 582–585.
- 98. Monsma SA, Harada HA, Wolfner MF (1990) Synthesis of two Drosophila male accessory gland proteins and their fate after transfer to the female during mating. Dev Biol 142: 465–475.
- 99. Chapman KB, Wolfner MF (1988) Determination of male-specific gene expression in Drosophila accessory glands. Dev Biol 126: 195–202.
- 100. Neubaum DM, Wolfner MF (1999) Mated Drosophila melanogaster females require a seminal fluid protein, Acp36DE, to store sperm efficiently. Genetics 153: 845–857.
- 101. Ohashi YY, Hainofukushima K, Fuyama Y (1991) Purification and characterization of an ovulation stimulating substance from the male accessory glands of Drosophila suzukii. Insect Biochem 21: 413–419.
- 102. Chapman T, Liddle LF, Kalb JM, Wolfner MF, Partridge L (1995) Cost of mating in Drosophila melanogaster females is mediated by male accessory gland products. Nature 373: 241–244.
- 103. Clark AG, Aguade M, Prout T, Harshman LG, Langley CH (1995) Variation in sperm displacement and its association with accessory-gland protein loci in Drosophila-melanogaster. Genetics 139: 189–201.
- 104. Bateman PW, Ferguson JWH, Yetman CA (2006) Courtship and copulation, but not ejaculates, reduce the longevity of female field crickets (Gryllus bimaculatus). J Zool 268: 341–346.
- 105. Xue L, Noll M (2000) Drosophila female sexual behavior induced by sterile males showing copulation complementation. Proc Natl Acad Sci U S A 97: 3272–3275.
- 106. Swanson WJ, Vacquier VD (2002) Reproductive protein evolution. Annu Rev Ecol Syst 33: 161–179.
- 107. Clark NL, Aagaard JE, Swanson WJ (2006) Evolution of reproductive proteins from animals and plants. Reproduction 131: 11–22.
- 108. Turner LM, Hoekstra HE (2008) Causes and consequences of the evolution of reproductive proteins. Int J Dev Biol 52: 769–780.
- 109. Marshall JL, Huestis DL, Garcia C, Hiromasa Y, Wheeler S, et al. (2011) Comparative proteomics uncovers the signature of natural selection acting on the ejaculate proteomes of two cricket species isolated by postmating, prezygotic phenotypes. Mol Biol Evol 28: 423–435.