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First published online June 11, 2007
Journal of Experimental Biology 210, 2163-2169 (2007)
Published by The Company of Biologists 2007
doi: 10.1242/jeb.02789
A male sex pheromone in a parasitic wasp and control of the behavioral response by the female's mating status
1 Institut für Biologie, Freie Universität Berlin, Haderslebener
Str. 9, D-12163 Berlin, Germany
2 Institut für Biotechnologie, Technische Universität Berlin,
Seestraße 13, D-13353 Berlin, Germany
3 Tierökologie 220c, Universität Hohenheim, D-70593 Stuttgart,
Germany
* Author for correspondence (e-mail: ruther{at}zedat.fu-berlin.de)
Accepted 17 April 2007
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Key words: 5-hydroxy-4-decanolide, Hymenoptera, mating behavior, Nasonia vitripennis, parasitic wasp, parasitoid, Pteromalidae, sex pheromone
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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).
The reproductive success of parasitoid males depends on their ability to
locate and inseminate receptive females. As in most other insects, sex
pheromones are supposed to be of substantial importance during the mate
finding process of parasitic wasps
(Godfray, 1994). However, only
a few sex pheromones have been identified so far (reviewed by
Kainoh, 1999;
Ayasse et al., 2001;
Keeling et al., 2004). These
are exclusively female-derived compounds which are either of high volatility
and attract males over long distances
(Eller et al., 1984;
Swedenborg and Jones, 1992;
Swedenborg et al., 1994) or of
low volatility and mediate arrestment and male courtship behavior at close
range (Shu and Jones, 1993;
Syvertsen et al., 1995;
Sullivan, 2002;
Steiner et al., 2005;
Steiner et al., 2006). Nothing
is known about the chemistry of male-derived sex pheromones in parasitic
wasps, although a few behavioral studies suggest that they exist
(van den Assem et al., 1980;
Gonzalez et al., 1985).
The physiological state of insects can have drastic impacts on their
reproductive behavior. When ejaculating, males not only transfer sperm but
also bioactive molecules, from their accessory glands, that induce a variety
of physiological and behavioral changes in females. Numerous studies [see
Gillott (Gillott, 2003) and
references therein] have shown that these mostly proteinaceous compounds may
not only induce refractoriness (rejection of courting males) but also arrest
biosynthesis and release of female sex pheromones. By this means, males that
gained the first copulation may increase their chance of siring a maximum
number of the female's offspring. Studies on the Mediterranean fruit fly
Ceratitis capitata provided the first evidence that the female mating
status may also influence the responsiveness to olfactory stimuli
(Jang, 1995;
Jang, 2002). After mating or
experimental injection of accessory gland fluid, the female preference
switched from the male sex pheromone to host odors. This behavioral switch of
the females did not occur until 24–48 h after treatment with the
accessory gland fluid (Jang,
1995).
The jewel wasp Nasonia vitripennis Walker (Hymenoptera:
Pteromalidae) is a gregarious parasitoid that attacks pupae of several
cyclorraphous fly species. It is one of the most investigated parasitoid
species (Quicke, 1997) and,
thus, can be considered as a model organism for the study of parasitic wasp
biology. Both male and female sex pheromones have been reported in N.
vitripennis. Males respond to female cuticular hydrocarbons by courtship
behavior (Steiner et al.,
2006) and release a still unknown aphrodisiac from their
mandibular gland that triggers the readiness to copulate in the female
(van den Assem et al., 1980).
Furthermore, males reportedly mark territories chemically after copulation.
These marks are attractive to females and other males
(van den Assem, 1986). In the
course of our recent study on the female courtship pheromone of N.
vitripennis (Steiner et al.,
2006) we found two chemicals in whole body extracts from older
males that were absent in those from females (J.R., unpublished). Here we
report the identification of these compounds and demonstrate that they
function as a male sex pheromone, attracting females. Apart from structure
elucidation, we investigated in which part of the insect the pheromone is
located and whether the pheromone titer depends on the age of the male
parasitoids. Furthermore, we determined release dynamics of pheromone from
individual males and studied whether the mating status of females influences
their responsiveness to the male signal.
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Materials and methods |
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Pheromone extraction and fractionation
Virgin males of different ages [<1 h (N=26), 1 day
(N=19), 2 days (N=17), 3 days (N=15)] and 1-day-old
virgin females (N=15) were killed by freezing, transferred to a 1 ml
glass vial equipped with a 100 µl micro insert, and extracted singly for 30
min with 5 µl of dichloromethane containing 50 ng µl–1
methyl undecanoate (Sigma-Aldrich, Deisenhofen, Germany) as an internal
standard. To identify the site of pheromone storage, 3-day-old unmated males
were dissected with a scalpel into head, thorax and abdomen, and subsequently
tagmata were extracted separately as described above (N=5 for each
segment). Aliquots (1 µl) were analyzed by coupled gas
chromatography–mass spectrometry (GC–MS). Amounts of
(4R,5R)- and
(4R,5S)-5-hydroxy-4-decanolide (HDL) in individuals were
estimated by relating peak areas to the internal standard. For testing
bioactivity of natural (4R,5R)- and
(4R,5S)-HDL, pheromone extracts were fractionated by
adsorption chromatography. Groups (N=20) of 3-day-old males were
killed by freezing and extracted for 30 min with 100 µl of dichloromethane.
After removal of the supernatant, the cadavers were washed twice with 100
µl of dichloromethane. The combined extracts were applied to a silica gel
cartridge (25 mg; International Sorbent Technology, Glamorgan, UK) and rinsed
twice with 250 µl of dichloromethane. The diastereomers of HDL were eluted
with 250 µl of methanol. After removal of the methanol under a gentle
stream of nitrogen the residue was reconstituted in 100 µl of
dichloromethane for bioassay.
Volatile collection
The volatile collection system consisted of a mini vacuum pump (Neolab,
Heidelberg, Germany) that was connected by a piece of Teflon tube to an
adsorption filter (65 mm length, 35 mm diameter; Gränicher and Quartero,
Daumazan, France) designed for closed loop stripping analysis (CLSA)
(Grob and Zürcher, 1976)
and equipped with a 1-mm charcoal layer (5 mg) for volatile adsorption. Single
insects (3-day-old males, N=12) were directly released into the
filter tube and the open end of the tube was connected to another glass tube
(75 mm length, 36 mm diameter) containing 150 mg of charcoal to clean the air
stream before entering the CLSA-tube. An air stream of 40 ml
min–1 was sucked through the tube system for 5 h. Adsorbed
volatiles were eluted with 25 µl of dichloromethane containing 5 ng
µl–1 methyl undecanoate as an internal standard and used
for chemical analysis by GC–MS. Amounts of HDL-diastereomers per sample
were quantified by relating peak areas to the internal standard. To test
whether HDL was released by the males continuously or intermittently, we
repeated the experiment (N=10) but exchanged the adsorption tube
every hour (referred to as 5x1 h). Thereby, it was possible to estimate
HDL amounts released by individual males for each hour separately. Volatile
sampling of N. vitripennis males was performed during the photophase
(10:00 h and 18:00 h), no food or water was offered to the insects to avoid
the danger of contaminations.
GC–MS analysis
Extracts were subjected to GC–MS analysis on a Fisons 8060 gas
chromatograph (Fisons Instruments, Mainz-Kastel, Germany) equipped with a
DB-5ms capillary column (30 mx0.32 mm i.d., 0.25 µm film thickness; J
& W Scientific, Folsom, CA, USA) operated in splitless mode (injector
temperature: 240°C) and coupled to a Fisons MD800 quadrupole MS running in
the electron impact (EI) mode at 70 eV. Helium was used as the carrier gas at
a head pressure of 5 kPa (flow rate 1.0 ml min–1). Initial
oven temperature was 80°C, increased at 5°C min–1 to
280°C and held for 30 min. Linear retention indices (RI) of the
male-specific double peak in natural extracts were estimated by co-injection
of a mixture of n-alkanes with chain lengths between seven and 30 carbon units
(Sigma-Aldrich, Steinheim, Germany) (van
den Dool and Kratz, 1963). The compounds eluting at RI=1592 and
1608 were identified as a pair of diastereomers of HDL by comparison of mass
spectra and RI with those of authentic reference chemicals which were
synthesized as described elsewhere (Garbe
and Tressl, 2003). The two threo-enantiomers,
(4R,5R)- and (4S,5S)-HDL, eluted before
the erythro-enantiomers (4R,5S)- and
(4S,5R)-HDL. Threo- and erythro-enantiomers of HDL were
separated on a chiral ß-DEX 225 GC column (=25%
2,3-di-O-acetyl-6-O-TBDMS-ß-cyclodextrin in
polydimethylsiloxane, 30 mx 0.25 mm diameter, 0.25 µm film thickness;
Supelco, Bellefonte, PA, USA). Hydrogen was used as carrier gas. The flow was
adjusted to 25 cm s–1 at an oven temperature of 120°C.
The GC was operated in splitless mode (15 s) at an injector temperature of
240°C. Initial oven temperature was 80°C, increased at 3°C
min–1 to 220°C and held for 10 min. All four
stereoisomers were separated with the two threo-enantiomers eluting before the
erythro-enantiomers. Threo-enantiomers were only partially resolved with
(4R,5R)-HDL eluting before (4S,5S)-HDL
whereas the erythro-enantiomers were totally resolved with
(4R,5S)-HDL eluting before (4S,5R)-HDL.
The absolute configuration of the natural products was finally established to
be (4R,5R)- and (4R,5S)-HDL by
co-injection of the polar fraction from male extracts with authentic reference
compounds.
Bioassays
The experiments were carried out in a four-chamber static-air-flow
olfactometer at 20±1°C under illumination of a microscope lamp. The
olfactometer consisted of an acrylic cylinder (1.5 cm high, 7 cm diameter)
divided into four chambers by crosswise arranged vertical plates. The top of
the cylinder was covered by plastic gauze (mesh 0.1 mm) functioning as a
walking arena for the parasitoids. A lid consisting of a plastic ring (4 mm
high, 7 cm diameter) and a second gauze (mesh 0.1 mm) was placed on top of the
cylinder to prevent the parasitoids from escaping. Quarters of MN 615 filter
paper discs (5.5 cm diameter; Macherey and Nagel, Düren, Germany) were
placed in each of the four chambers underneath the walking arena. The
following samples were tested: 5 µl of fractions containing natural HDL
diastereomers (representing one male equivalent, see above; experiment 1) or a
synthetic mixture of (4R,5R)- and
(4R,5S)-HDL (ratio 1:1.3) in dichloromethane at doses of 80
or 160 ng HDL (experiment 2). To determine whether the female response is
enantioselective, we also tested 80 ng of either the naturally occurring
(4R,5R)- or the (4S,5S)-enantiomer that
does not occur in the insects (see Results, experiment 3). Samples were
applied to the filter paper of one chamber (test) and equal amounts of the
clean solvent were applied to the filter papers of the remaining chambers. The
opposite chamber was considered as control chamber whereas the remaining two
chambers adjacent to the test chamber were considered as buffer zones.
Parasitic wasps (virgin females, mated females 5 min or 24 h after copulation,
mated females 6 days after copulation with oviposition opportunity, and
unmated males, N=20 for each type) were released singly into the
walking arena using a fine paintbrush. The time spent by wasps in the sectors
above the four chambers was recorded for 300 s using the The Observer 3.0
computer software (Noldus, Wageningen, The Netherlands). To avoid biased
results caused by possible side preferences of the parasitoids, samples were
assigned randomly to one of the chambers and the olfactometer was rotated by
90° after every wasp.
Statistical analysis
Amounts and ratios of (4R,5R)- and
(4R,5S)-HDL in extracts from males of different age were
analyzed by a one-way analysis of variance (ANOVA) followed by least
significant difference test (LSD) for individual comparisons. Amounts of HDL
released by individual males within 5 h were compared to the summed amounts
released within 5x1 h by a Mann–Whitney U-test. Residence
time of males spent above the test and control chamber in the bioassays were
compared by a t-test for dependent samples. Statistical analyses were
done using Statistica 4.5 scientific software (StatSoft, Hamburg,
Germany).
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).
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Virgin females, but not males, were strongly attracted by the natural HDL-diastereomers (1 male equivalent of a whole body extract cleaned up by adsorption chromatography; experiment 1, Fig. 5A), as well as by 80 and 160 ng of the synthetic mixture of (4R,5R)- and (4R,5S)-HDL (experiment 2, Fig. 5B). The response of virgin females was not enantioselective because both the naturally occurring (4R,5R)-enantiomer, as well as the (4S,5S)-enantiomer that does not occur in the parasitoids, were attractive at a dose of 80 ng (experiment 3, Fig. 6).
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Five minutes after copulation females avoided one male equivalent of natural HDL or 160 ng of the synthetic mixture (Fig. 5A,B). Neither preference nor avoidance of all samples offered was shown by mated females after 24 h. Females that had been allowed to oviposit for 6 days, were still neither attracted nor repelled by natural HDL, but there was a tendency to prefer the test field (P=0.06).
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Discussion |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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). One mechanism in male insects to increase the
chance of successful reproduction is the release of sex pheromones that
attract females or elicit sexual acceptance
(Wyatt, 2003). However, in
parasitic wasps the use of female sex pheromones is thought to be more common
(Godfray, 1994) and involvement
of male-derived pheromones has only rarely been demonstrated
(van den Assem et al., 1980;
Gonzalez et al., 1985). The
present study reports the first identification of a male sex pheromone in
parasitic Hymenoptera. Males of N. vitripennis synthesize
HDL-diastereomers in their abdomen and release these chemicals that attract
virgin females, but not males. Nasonia vitripennis is a gregarious
parasitoid developing in groups of 10–20 individuals within a single
host. The protandrous males often wait at the emergence hole of the puparium
they emerged from to mate with their sisters. Thereby, dominant males may
aggressively chase away inferior competitors
(van den Assem, 1986). By
releasing the sex pheromone, males may signal genetic quality and influence
the outcome of this contest. In fact, males may effectively `call' for
females, as indicated by the intermittent release of the pheromone even in the
absence of females. The fact that HDL is biosynthesized in the male abdomen,
suggests that it is not identical with the postulated aphrodisiac that is
released from the mandibular gland of N. vitripennis males during
courtship and triggers the readiness to mate in females
(van den Assem et al., 1980).
This conclusion is supported by the result that males released HDL even when
their mouthparts had been sealed with quick-drying superglue (L.M.S.,
unpublished). Thus, further components of the N. vitripennis chemical
communication system remain to be discovered.
The present study clearly demonstrates that the responsiveness of females
to the male sex attractant is affected by their mating status. Copulation of
N. vitripennis females immediately switched off their attraction to
HDL, and shortly after copulation they even avoided the chemical signal that
indicates the presence of males. A similar mechanism was shown before for the
Mediterranean fruit fly Ceratitis capitata: after copulation, the
female behavioral preference switched from the male sex pheromone to host
fruit odors (Jang, 1995;
Jang, 2002). However, in
C. capitata females did not switch their behavior until 24–48 h
after mating (Jang, 1995) and
it was not determined whether this switch was due to avoidance of the male
pheromone or an increased attractiveness of the host fruit odor. Nevertheless,
the observed phenomenon was clearly shown to be associated with accessory
gland fluids transferred by males to the females during copulation. This might
also be the case in N. vitripennis, although it has been shown that
refractoriness in this species is initiated during post-copulatory courtship
behavior. Van den Assem and Visser (van
den Assem and Visser, 1976) reported that N. vitripennis
females can be provoked to remate by experimentally preventing male
post-copulatory behavior. However, we found the described behavioral switch
concerning HDL also in those females that had copulated but did not experience
post-copulatory courtship (J.R., unpublished). This strengthens the conclusion
that it is the copulation itself rather than post-copulatory courtship that
triggers the observed behavioral switch of N. vitripennis females.
Under normal circumstances, N. vitripennis females mate only once
(van den Assem, 1986) and
therefore, their variable response depending on the mating status makes sense
from an evolutionary perspective. Firstly, it increases the chance of virgins
to be inseminated. Secondly, by terminating the response to HDL or even
avoiding the male pheromone, mated females decrease the probability of
encountering males and being disturbed by their courtship activities when
searching for new oviposition sites. Males in return will be less likely to
engage in unavailing courtship activities towards non-receptive females.
To the best of our knowledge this is the first report of
(4R,5R)- and (4R,5S)-HDL in insects,
although long-chain lactones, including decanolides, are common insect
semiochemicals (e.g. Howard et al.,
1983; Nishida et al.,
1996; Larsson et al.,
2003). The response of insects to chiral lactones can be extremely
enantioselective (Tumlinson, 1977; Leal,
1996). This appears not to be the case in N. vitripennis
since virgin females were also attracted by (4S,5S)-HDL,
which is not released by males. (4S,5R)-HDL has been
described among the fermentation products of Streptomyces griseus
(Graefe et al., 1982).
(+)Vernolic acid
(9Z,12S,13R)-12,13-epoxyoctadec-9-enoic acid) has
been shown to be the precursor of HDL stereoisomers in microorganisms
(Garbe and Tressl, 2003).
Further studies are in progress to investigate whether HDL is biosynthesized
by the same pathway in insects and to characterize the pheromone-producing
gland in the abdomen of N. vitripennis males.
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Acknowledgments |
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|
References |
|---|
|
TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
|---|
Ayasse, M., Paxton, R. J. and Tengö, J. (2001). Mating behaviour and chemical communication in the order Hymenoptera. Annu. Rev. Entomol. 46, 31-78.[CrossRef][Medline]
Choe, J. C. and Crespi, B. J. (1997). The Evolution of Mating Systems of Insects and Arachnids. Cambridge: Cambridge University Press.
Eller, F. J., Bartelt, R. J., Jones, R. L. and Kulman, H. M. (1984). Ethyl (Z)-9-hexadecenoate a sex pheromone of Syndipnus rubiginosus, a sawfly parasitoid. J. Chem. Ecol. 10,291 -300.[CrossRef]
Garbe, L. A. and Tressl, R. (2003). Metabolism of deuterated isomeric 6,7-dihydroxydodecanoic acids in Saccharomyces cerevisiae – diastereo- and enantioselective formation and characterization of 5-hydroxydecano-4-lactone (= 4,5-dihydro-5-(1-hydroxyhexyl)furan-2(3H)-one) isomers. Helv. Chim. Acta 86,2349 -2363.[CrossRef]
Gillott, C. (2003). Male accessory gland secretions: modulators of female reproductive physiology and behavior. Annu. Rev. Entomol. 48,163 -184.[CrossRef][Medline]
Godfray, H. C. J. (1994). Parasitoids. Chichester, USA: Princeton University Press.
Gonzalez, J. M., Matthews, R. W. and Matthews, J. R. (1985). A sex pheromone in males of Mellitobia australica and in M. femorata (Hymenoptera: Eulophidae). Florida Entomol. 68,279 -286.[CrossRef]
Graefe, U., Reinhardt, G., Schade, W., Krebs, D., Eritt, I. and Fleck, W. F. (1982). Isolation and structure of novel autoregulators from Streptomyces griseus. J. Antibiot. 35,609 -614.[Medline]
Grob, K. and Zürcher, F. (1976). Stripping of trace organic substances from water – equipment and procedure. J. Chromatogr. 117,285 -294.[CrossRef]
Howard, D. F., Blum, M. S. and Fales, H. M.
(1983). Defense in thrips: forbidding fruitiness of a lactone.
Science 220,335
-336.
Jang, E. B. (1995). Effects of mating and accessory gland injections on olfactory-mediated behavior in the female Mediterranean fruit fly, Ceratitis capitata. J. Insect Physiol. 41,705 -710.[CrossRef]
Jang, E. B. (2002). Physiology of mating behavior in Mediterranean fruit fly (Diptera: Tephritidae): chemoreception and male accessory gland fluids in females post-mating behavior. Florida Entomol. 85,89 -93.[CrossRef]
Kainoh, Y. (1999). Parasitoids. In Pheromones of Non-Lepidopteran Insects Associated with Agricultural Plants (ed. J. Hardie and A. K. Minks), pp.383 -404. Wallingford: CABI.
Keeling, C. I., Plettner, E. and Slessor, K. N. (2004). Hymenopteran semiochemicals. Top. Curr. Chem. 239,133 -177.
Larsson, M. C., Hedin, J., Svensson, G. P., Tolasch, T. and Francke, W. (2003). Characteristic odor of Osmoderma eremita identified as a male-released pheromone. J. Chem. Ecol. 29,575 -587.[CrossRef][Medline]
Leal, W. S. (1996). Chemical communication in
scrab beetles: reciprocal behavioral agonist-antagonist activities of chiral
pheromones. Proc. Natl. Acad. Sci. USA
93,12112
-12115.
Nishida, R., Schulz, S., Kim, C. S., Fukami, H., Kuwahara, Y., Honda, K. and Hayashi, N. (1996). Male sex pheromone of a giant danaine butterfly, Idea leuconoe. J. Chem. Ecol. 22,949 -972.[CrossRef]
Quicke, D. L. J. (1997). Parasitic Wasps. London: Chapman & Hall.
Shu, S. and Jones, R. L. (1993). Evidence for a multicomponent sex pheromone in Eriborus terebrans (Gravenhorst) (Hym.: Ichneumonidae), a larval parasitoid of the European corn borer. J. Chem. Ecol. 19,2563 -2576.[CrossRef]
Steiner, S., Steidle, J. L. M. and Ruther, J. (2005). Female sex pheromone in immature insect males – a case of pre-emergence chemical mimicry? Behav. Ecol. Sociobiol. 58,111 -120.[CrossRef]
Steiner, S., Hermann, N. and Ruther, J. (2006). Characterization of a female-produced courtship pheromone in the parasitoid Nasonia vitripennis. J. Chem. Ecol. 32,1687 -1702.[CrossRef][Medline]
Sullivan, B. T. (2002). Evidence for a sex pheromone in bark beetle parasitoid Roptrocerus xylophagorum. J. Chem. Ecol. 28,1045 -1063.[CrossRef][Medline]
Swedenborg, P. D. and Jones, R. L. (1992). (Z)-4-Tridecenal, a pheromonally active air oxidation product from a series of (Z,Z)-9,13-dienes in Macrocentrus grandii Goidanich (Hymenoptera: Braconidae). J. Chem. Ecol. 18,1913 -1931.[CrossRef]
Swedenborg, P. D., Jones, R. L., Zhou, H. Q., Shin, I. and Liu, H. W. (1994). Biological activity of (3R,5S,6R)- and (3S,5R,6S)-3,5-dimethyl-6-(methylethyl)-3,4,5,6-tetrahydropyran-2-one, a pheromone of Macrocentrus grandii (Goidanich) (Hymenoptera: Braconidae). J. Chem. Ecol. 20,3373 -3380.[CrossRef]
Syvertsen, T. C., Jackson, L. L., Blomquist, G. J. and Vinson, S. B. (1995). Alkadienes mediating courtship in the parasitoid Cardiochiles nigriceps (Hymenoptera: Braconidae). J. Chem. Ecol. 21,1971 -1989.[CrossRef]
Tumlinson, J. H., Klein, M. G., Doolittle, R. E., Ladd, T. L.
and Proveaux, A. T. (1977). Identification of female Japanese
beetle sex-pheromone – inhibition of male response by an enantiomer.
Science 197,789
-792.
van den Assem, J. (1986). Mating behaviour in parasitic wasps. In Insect Parasitoids (ed. J. Waage and D. Greathead), pp. 137-167. London: Academic Press.
van den Assem, J. and Visser, J. (1976). Aspects of sexual receptivity in female Nasonia vitripennis (Hym., Pteromalidae). Biol. Behav. 1, 37-56.
van den Assem, J., Jachmann, F. and Simbolotti, P. (1980). Courtship behaviour of Nasonia vitripennis (Hym., Pteromalidae): some qualitative experimental evidence for the role of pheromones. Behaviour 75,301 -307.
van den Dool, J. and Kratz, P. D. (1963). A generalization of the retention index system including linear programmed gas-liquid partition chromatography. J. Chromatogr. 11,463 -471.[CrossRef][Medline]
Wyatt, T. D. (2003). Pheromones and Animal Behaviour. Cambridge: Cambridge University Press.
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