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First published online May 2, 2008
Journal of Experimental Biology 211, 1587-1593 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.016725
Effects of the NMDA receptor antagonist MK-801 on female reproduction and juvenile hormone biosynthesis in the cricket Gryllus bimaculatus and the butterfly Bicyclus anynana
1 Department of Animal Ecology I, University of Bayreuth, D-95440 Bayreuth,
Germany
2 Zoological Institute and Museum, University of Greifswald, D-17487 Greifswald,
Germany
* Author for correspondence (e-mail: thorin.geister{at}uni-bayreuth.de)
Accepted 10 March 2008
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Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Key words: fecundity, Corpora allata, glutamate receptor, insects
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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; Gäde et al.,
1997; Nijhout,
1994). Among the different hormones, the juvenile hormones (JHs)
and the ecdysteroids are generally considered the most important ones in
affecting these processes in insects. JHs are sequiterpenoid lipid-like
compounds secreted by the corpora allata (CA), a pair of epithelial glands,
and are well-known for preventing metamorphosis in the insect juvenile stages
and for having pronounced effects on reproduction in the adults
(Gilbert et al., 2000;
Nijhout, 1994;
Ramaswamy et al., 1997). Their
primary function in reproduction is to initiate vitellogenin synthesis in the
fat body and to regulate the uptake of yolk by the ovary
(Hoffmann, 1995). JH
biosynthesis is a tightly regulated process involving stimulating
(allatotropins) and inhibiting (allatostatins) neuropetides secreted by brain
neurosecretory cells (Kataoka et al.,
1989; Stay and Tobe,
2007), and also classical neurotransmitters
(Chiang et al., 2002a;
Granger et al., 2000;
Liu et al., 2005;
Rachinsky and Tobe, 1996).
At least in the cockroach Diploptera punctata, CA function is
controlled by either stimulating ionotropic
(Chiang et al., 2002a) or
inhibiting metabotropic receptors (Liu et
al., 2005). The identified ionotropic
N-methyl-D-aspartate (NMDA) glutamate-gated receptor in
the CA of D. punctata has striking similarities with the vertebrate
NMDA receptor, especially regarding its structure, high Ca2+
permeability, and its response to typical antagonists such as MK-801,
conantokin and Mg2+ (Chiang et
al., 2002a). Interestingly, NMDA receptors in mammals are
important for reproductive control through their effects on the release of the
gonadotropin-releasing hormone required for the initiation of puberty, the
maintenance of reproductive capability and reproductive behaviour
(Mahesh and Brann, 2005).
Similar effects have been described in other vertebrates
(Flynn et al., 2002), and also
in a protochordate species, Ciona intestinalis, suggesting a highly
conserved reproductive function in chordates
(D'Aniello et al., 2003;
Di Fiore et al., 2000).
MK-801, as a high-affinity antagonist of NMDA receptors
(Wong et al., 1986), has been
intensively studied in mammalian models, in particular in connection with its
effects on neuronal plasticity and its neurotoxicity-reducing effects in
ischaemia, epilepsia, brain hypoxia and hypoglycemia
(Ellison, 1995;
Williams et al., 1991;
Wolf, 1998). Furthermore, this
antagonist was used to study NMDA receptor-mediated effects on reproduction in
other vertebrates (Flynn et al.,
2002; Luderer et al.,
1993; Mahesh and Brann,
2005; Melis et al.,
2004). By contrast, in insects MK-801 has thus far only been used
in three species. MK-801 was found to inhibit NMDA-triggered JH biosynthesis
in vitro in the cockroach D. punctata, by reducing levels of
free cytosolic calcium in the CA (Chiang et
al., 2002a; Chiang et al.,
2002b). Furthermore, Begum and co-workers
(Begum et al., 2004) used
MK-801 as an efficient blocker of vitellogenesis in the flesh fly
Neobellieria bullata and the locust Schistocerca gregaria.
However, studies on long-term effects of MK-801 on reproduction and on JH
biosynthesis, involving in vitro and in vivo measurements,
are apparently missing (Begum et al.,
2004). We address these issues here using two insect species: the
hemimetabolous cricket Gryllus bimaculatus and the holometabolous
butterfly Bicyclus anynana, in order to validate the above supposed
mode of action and to test for its generality
(Zera, 2007).
Gryllus bimaculatus has been extensively used to study the
hormonal control of reproduction, which strongly depends on JH
(Hoffmann et al., 1996;
Lorenz, 2003;
Lorenz et al., 1995a;
Lorenz et al., 1995b), thus
making it a highly suitable target for JH manipulation. The butterfly B.
anynana belongs to a group of the Lepidoptera in which vitellogenesis and
choriogenesis seem to depend exclusively on JH
(Ramaswamy et al., 1997).
Reproduction, including different strategies in response to prevailing
temperatures, has been extensively studied in B. anynana
(Fischer et al., 2003a;
Fischer et al., 2004;
Fischer et al., 2003b;
Steigenga et al., 2005), but
its hormonal control is hitherto only poorly understood
(Steigenga et al., 2006),
making this species another suitable model. Given the dependence of
reproduction on JH in both species, we here examine the effect of the NMDA
receptor antagonist MK-801 on lifetime fecundity and egg size, on in
vitro and in vivo JH biosynthesis, and its interactions with JH
mimics.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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). A laboratory
stock population was established at Bayreuth University, Germany, in 2003 from
several hundred individuals derived from a well-established stock population
at Leiden University, The Netherlands. The Leiden population was founded in
1988 from over 80 gravid females caught at a single locality in Malawi.
Several hundred adults are reared in each generation, maintaining high levels
of heterozygosity at neutral loci (Van't
Hof et al., 2005). G. bimaculatus has a global
distribution, spanning Africa, Asia and southern Europe
(Harrison and Bogdanowicz,
1995; Ragge,
1972). The laboratory colony at Bayreuth University was
established with field-caught animals from Italy and Spain in 1995. Regularly,
individuals (also originating from Mediterranean areas) from commercial
suppliers were added to the stock population to maintain high levels of
heterozygosity (Lorenz et al.,
2004).
Insect rearing
Bicyclus anynana was reared in a climate cell at 27°C, 70%
relative humidity, and a photoperiod of 12 h:12 h light:dark. Larvae were fed
on young maize plants in population cages (50 cmx50 cmx80 cm). The
resulting pupae were collected from the plants and transferred to cylindrical
hanging cages. Throughout all experiments, butterflies had access to moist
banana for adult feeding. G. bimaculatus was reared at 27°C,
30–40% relative humidity and a photoperiod of 16 h:8 h light:dark.
Larvae were reared in population cages (45 cmx40 cmx65 cm), fed on
a mixture of commercial rat/mouse, rabbit and cat diets (Altromin GmbH, Lage,
Germany), and supplied with drinking water ad libitum. Newly ecdysed
adults (day 0) were collected daily and transferred to population cages (22
cmx20 cmx37 cm).
Experimental design
To investigate the effects of the NMDA receptor antagonist MK-801 on female
reproduction and juvenile hormone biosynthesis, five different experiments
were performed as outlined below.
Experiment 1: effects of MK-801 on B. anynana reproduction
On the day of eclosion, female butterflies were randomly divided among four
treatment groups, being treated with 0 (control), 10, 20 or 30 µg MK-801 in
4 µl Ringer solution. These solutions were repeatedly injected into the
females' thorax, using a Hamilton syringe, on days 0, 2 and 6 of adult life.
All females were kept together with male butterflies for mating until day 2 of
adult life. After the mating period, females were placed individually in
translucent plastic containers (1 l, covered with gauze) containing a fresh
cutting of maize for egg-laying. Eggs of 
40 females per group were
collected and counted daily until the death of the females. Egg size was
measured as cross-sectional area (mm2) using a digital camera
(Leica DC300, Leica Microsystems, Wetzlar, Germany) connected to a stereo
microscope (Leica MZ 7.5). The resulting images were analysed using Scion
Image public software (Scion Corporation 2000, Frederick, Maryland, USA).
Tight correlations between egg area (applying image analysis) and egg mass as
well as hatchling size confirm that this method provides a highly reliable
measurement of egg size in B. anynana
(Fischer et al., 2002).
Experiment 2: effects of MK-801 on G. bimaculatus reproduction
Adult female crickets were randomly divided among three treatment groups,
being injected with 0 (control), 50, or 150 µg MK-801 in 4 µl
DMSO–Ringer (1:1 v/v) solution (note that MK-801 is not soluble in pure
Ringer at high concentrations). This solution was injected into the lateral
intersegmental membrane between the third and fourth abdominal segment, using
a Hamilton syringe, on days 0 and 3 of adult life. Females were housed
together with males for mating from day 2 until day 4 following ecdysis.
Thereafter, females were placed individually in plastic boxes
(18x13.5x6 cm) and provided moist sand as egg laying substrate.
Eggs were collected, counted and measured (as outlined above) daily for the
following 8 days. For each group about 35 females were used.
Experiment 3: interactive effects between MK-801 and JH mimics in B. anynana and G. bimaculatus
To investigate whether any potential effects of MK-801 on reproductive
traits are mediated through variation in JH titres, JH mimics were applied to
artificially increase JH active compounds in the haemolymph. As mimics,
pyriproxyfen (Dr. Ehrenstorfer GmbH, Augsburg, Germany) was used for B.
anynana, and methoprene (Fluka, Taufkirchen, Germany) for G.
bimaculatus. The compounds are known to work well as JH mimics in these
species (Hoffmann et al.,
1996; Steigenga et al.,
2006). Both species were randomly divided among four treatment
groups, being treated with MK-801, a JH mimic, MK-801 plus JH mimic or the
pure solvent (control). B. anynana females (70–77 per group)
were treated on days 0 and 2 with either 10 µg MK-801 in 6 µl Ringer
(injected), 0.1 µg pyriproyfen in 2 µl acetone (applied topically on the
abdomen using a Hamilton syringe), both compounds or 6 µl Ringer–2
µl acetone (control). Females were kept together with males for mating
until day 2, and were afterwards placed individually in plastic containers as
described above. Egg numbers were determined on day 3 of adult life only.
G. bimaculatus females (33–36 per group) were treated on days 0
and 3 with either 150 µg MK-801 in 4 µl DMSO–Ringer (1:1, v/v), 30
µg methoprene in 4 µl isooctane (applied topically on to the abdomen),
both compounds or 4 µl DMSO–Ringer/4 µl isooctane (control).
Females were kept together with males for mating until day 3 and were then
placed individually in plastic containers as described above. Egg numbers were
determined for days 4–6 following ecdysis. The respective concentrations
and treatment days were chosen on the basis of experiments 1 and 2 as well as
pilot studies.
Experiment 4: effects of MK-801 on in vitro JH biosynthesis in G. bimaculatus
Owing to the small size of the CA and very small amounts of haemolymph in
B. anynana, experiments 4 and 5 were restricted to G.
bimaculatus. Single CA from G. bimaculatus females were used in
a rapid partition assay (Feyereisen and
Tobe, 1981). Methods essentially followed those of Lorenz et al.
(Lorenz et al., 1995b;
Lorenz et al., 1997) with some
modifications: the TC 199 incubation medium (M 7653, Sigma, Deisenhofen,
Germany) with Hank's salts and sodium bicarbonate, without
L-glutamine, buffered with 25 mmol l–1 Hepes,
supplemented with CaCl2 to a final concentration of 3 mmol
l–1, L-methionine to a final concentration of 0.28
mmol l–1 and sodium acetate to a final concentration of 2.5
mmol l–1, fortified with 1% Ficoll 400, was adjusted to pH
7.2. As radiolabelled precursor, [14C2]acetate (MC 213;
Hartmann Analytic, Braunschweig, Germany) was added to a final specific
activity of 64 MBq mmol–1. The resulting total acetate
concentration in the radiolabelled incubation medium was 2.58 mmol
l–1. Single glands without MK-801 were pre-incubated for 90
min to stabilize JH synthesis in the in vitro setup, then transferred
to the first incubation for 120 min and finally assigned to the second
incubation with the respective treatments for 120 min. JH release was examined
in untreated control animals and at 6 MK-801 concentrations ranging from
10–3 to 10–6 mol l–1. JH
release rates are given relative to the initial incubation, to correct for
differences between single CA (N=20–35, but for
10–3 and 10–6 mol l–1,
N=10).
Experiment 5: effects of MK-801 on in vivo JH titres in G. bimaculatus
The JH titres in the haemolymph of G. bimaculatus females were
quantified by liquid chromatography–mass spectrometry (LC–MS)
(Westerlund and Hoffmann,
2004). The experimental design followed the one described for
experiment 2 with 21–24 females for each treatment. Three and 24 h after
the second injection on day 3, 20 µl of haemolymph were collected per
female and extracted (Westerlund and
Hoffmann, 2004). The samples were separated on a C18
reverse-phased column (ReproSil-Pur ODS-3, 5 µm; Dr Maisch GmbH, Germany),
protected by a guard column (C18 cartridge; Phenomex, Aschaffenburg, Germany)
with differing gradients of water–methanol. MS analysis was accomplished
using electrospray ionization (ESI) in positive ion mode using a Shimadzu
LCMS-2010A. As only the relative differences between treatments were of
importance, no additional calibration to estimate the absolute amount of
juvenile hormone was applied.
Data analysis
Differences in egg numbers over time were analyzed using two-way repeated
measurements ANOVAs, with treatment and time (i.e. oviposition day) as
factors. Data on total fecundity, mean egg size (averaged over the oviposition
period) and JH titres were analyzed with standard ANOVAs. As treatment with
MK-801 frequently resulted in the production of zero eggs per day, no repeated
measurements ANOVAs could be calculated for egg sizes. Differences among
treatment groups were analysed using Tukey's HSD. The fecundity data from
G. bimaculatus were square-root transformed prior to analyses to meet
ANOVA requirements. Survival probabilities of B. anynana females over
time were analyzed by survival analyses for multiple groups, based on Gehan's
generalized Wilcoxon test. The dose–response curve for the release of JH
by the CA of G. bimaculatus with regard to MK-801 treatment was
calculated using a sigmoidal 5-parameter fit of SigmaPlot 9.1. All statistical
tests were performed using Statistica 6.1 and values are given as means
±1 s.e.m.
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RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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24% in the 30 µg MK-801
group as compared to the control (F3,156=3.10,
P=0.028; Table 1A).
Again, differences were most pronounced during the first days of the
oviposition period (F3,152=10.43, P<0.001;
Table 1B).
|
|
Egg size generally decreased with increasing female age, but (if averaged
over the whole oviposition period) did not differ significantly between
treatment groups (F3,155=1.83, P=0.14;
Table 1A,
Fig. 1B). However, restricting
the analysis to days 3–7 of adult life shows that mean egg size tended
to decrease with increasing MK-801 concentration
(F3,155=4.00, P=0.009;
Table 1B). MK-801 treatment did
not affect female survival probability (
24=2.5,
P=0.47; Fig. 2).
|
Experiment 2: effects of MK-801 on G. bimaculatus reproduction
Daily egg numbers differed significantly across treatment groups, being
generally lower in the groups treated with MK-801 (repeated measurements
ANOVA: F2,642=5.35, P=0.006; treatment by time
interaction F12,642=0.77, P=0.686;
Fig. 3A). Egg numbers peaked on
day 6 of adult life, followed by a constant decline with female age
(F6,642=67.79, P<0.001). Accordingly, lifetime
fecundity was significantly reduced (by 40%) in the group treated with
150 µg MK-801 as compared with the control group
(F2,104=3.10, P=0.04;
Table 1C). Egg size was not
significantly affected by MK-801 (F2,103=0.54,
P=0.59; Fig. 3B). As
this experiment was terminated on day 12 following ecdysis (coinciding with
the end of egg laying), no longevity data are available, but at least during
this phase mortality rates were very similar (control: 0 individuals; 50 µg
MK-801: 2; 150 µg MK-801: 0).
|
Experiment 3: interactive effects between MK-801 and JH mimics in B. anynana and G. bimaculatus
Egg numbers varied significantly across treatment groups in both species
(B. anynana: F3,270=9.99, P<0.001;
G. bimaculatus: F3,139=10.55, P<0.001;
Fig. 4A,B). They were reduced
in the MK-801-treated groups, but increased in the groups treated with a JH
mimic. Most interestingly, egg numbers were very similar to controls in the
groups treated with both compounds.
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74% from day 3 to 4
(F1,65=29.1, P<0.001; treatment by time
interaction F2,65=1.93, P=0.15). |
DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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).
Furthermore, Steigenga et al. (Steigenga
et al., 2006) demonstrated that applications of the JH mimic
pyriproxifen significantly increased fecundity but decreased longevity,
supporting the notion that in B. anynana JH has pleiotropic effects
on key life-history traits, as has been found for other insects
(Flatt et al., 2005;
Ramaswamy et al., 1997;
Zera et al., 1998). For G.
bimaculatus much more detailed information on JH biosynthesis and the
hormonal control of reproduction, especially egg maturation, is available
(Hoffmann et al., 1996;
Koch and Hoffmann, 1985;
Lorenz et al., 1997).
However, we propose that the overall similar reduction in reproductive
output found in both species is causally related to the inhibitory effects of
MK-801 on JH biosynthesis (Chiang et al.,
2002a). Accordingly, we predicted that negative effects of MK-801
on fecundity can be restored by adding JH active compounds. Indeed this was
found when treating females with both, MK-801 and JH mimics, yielded fecundity
data for both species that were statistically indistinguishable from those of
the control groups. Similarly, Begum et al.
(Begum et al., 2004) showed
that JH treatment could overrule the blocking effect of MK-801 on
vitellogenesis in S. gregaria. Although these findings strongly
suggest that the NMDA receptor is involved in JH biosynthesis, a proof can
only be obtained by in vitro and in vivo analyses
(Begum et al., 2004;
Zera, 2007).
Corresponding analyses in G. bimaculatus (performing the same
measurements in B. anynana was not possible for practical reasons)
showed a reduction of in vitro JH biosynthesis and in vivo
haemolymph JH titres (by up to 48%) in MK-801-treated compared with control
females. JH biosynthesis was inhibited successfully in G. bimaculatus
CA by up to 60%, resembling the results of in vitro measurements of
active CA glands in D. punctata
(Chiang et al., 2002a). In the
experiments of Chiang et al. (Chiang et
al., 2002a) CA glands were incubated with NMDA to compensate for
the missing glutamate stimulus from the severed nerves, with much lower
concentrations of MK-801 needed for this degree of inhibition. The rise of JH
III titres in the haemolymph between days 3 and 4 was expected, as in G.
bimaculatus JH III titres reach their maximum shortly before the onset of
egg laying (Koch and Hoffmann,
1985). Taken together, the available evidence leaves little doubt
that MK-801 affects JH biosynthesis, and concomitantly JH titres, in both
species.
The effects of MK-801 on JH biosynthesis in G. bimaculatus are
possibly mediated through a glutamatergic NMDA receptor, acting on the
Ca2+ flux and thereby on JH biosynthesis. In adults of the
cockroach D. punctata, JH biosynthesis in the CA is initially
sensitive to allatostatins but insensitive to ionotropic glutamate
stimulation, resulting in low rates of JH synthesis. Mating changes this
pattern towards insensitivity of the CA to allatostatins and a high response
to glutamate stimulation, resulting in high rates of JH synthesis
(Chang et al., 2005). G.
bimaculatus allatostatins, by contrast, seem to act less age-dependently
throughout the life cycle, although on days with maximum JH synthesis
allatostatic inhibition is slightly lowered
(Lorenz, 2001). However,
calcium ions [with their influx being regulated by the NMDA receptor in D.
punctata (Chiang et al.,
2002a)], stimulate JH synthesis also in G. bimaculatus
(Klein et al., 1993;
Woodring and Hoffmann, 1994),
and there is no interaction between allatostatins (or allatotropins) and
Ca2+-mediated effects on JH biosynthesis
(Lorenz, 2001). A further
target of glutamate might also be a Na+-dependent transporter
(Kosakai and Yoshino,
2001).
There is no indication of any toxic side effects of the compounds or
solvents used that may have affected our results. For B. anyana,
MK-801 was dissolved in Ringer solution, thereby minimizing any potential
solvent effects. Indeed, lifetime fecundity in the control group was very
similar to values obtained from other studies not involving injections or
applications (Bauerfeind and Fischer,
2005; Bauerfeind et al.,
2007). Furthermore, survival data revealed no difference among
control and MK-801-treated groups, suggesting that MK-801 is a highly specific
compound without any toxic side-effects. For G. bimaculatus it was
necessary to use DMSO as solvent because of the much higher concentrations of
MK-801 employed. Concomitantly, lifetime fecundity was generally lower than in
other studies (Koch and Hoffmann,
1985; Lorenz,
2007; Meyering-Vos et al.,
2006), but again, there was no detectable effect on mortality
rates, although data were restricted to the egg laying period in this
case.
Despite the overall similarity of effects in both species used, there were
also some interesting differences in the effects of MK-801 on fecundity. In
G. bimaculatus egg production was reduced throughout the oviposition
period (at least until day 11 following ecdysis), but in B. anynana
the inhibitory effects of MK-801 were restricted to the first days of the
oviposition period. Furthermore, the dose dependence of effects seems more
pronounced in B. anynana than in to G. bimaculatus. These
findings may suggest some differences in the effects of JH on egg maturation
across species. In G. bimaculatus JH biosynthesis and fecundity can
be manipulated throughout the entire oviposition period by allatostatins and
JH (mimic) injections administered early in life
(Koch and Hoffmann, 1985;
Lorenz, 2001). Therefore, egg
maturation seems to depend on a constant input of JH-mediated signals in
G. bimaculatus. In B. anynana, by contrast, JH seems to be
an important signal for the initiation of egg maturation, which might not be
needed later on (Steigenga et al.,
2006).
In conclusion, the NMDA receptor antagonist MK-801 reduced fecundity in
G. bimaculatus and B. anynana, two species not being
phylogenetically closely related. This effect could be reversed by concurrent
applications of JH mimics. Furthermore, MK-801 inhibited in vitro JH
biosynthesis in the CA and reduced in vivo JH haemolymph titres in a
dose-dependent manner in G. bimaculatus. These results suggest that
in G. bimaculatus JH biosynthesis in the CA is at least in part
controlled by an NMDA receptor with Ca2+ as a second level
messenger, as has been found in the cockroach D. punctata
(Chiang et al., 2002a). As
MK-801 is readily available commercially, is fairly soluble in water and can
be used orally, it obviously represents a convenient tool for manipulating JH
biosynthesis in insects. With the growing knowledge on NMDA receptors in
insects (Chiang et al., 2002a;
Chiang et al., 2002b;
Locatelli et al., 2005;
Xia et al., 2005), such
antagonists may yield new insights into the mechanistic basis of reproduction
and associated trade-offs in insects.
|
Acknowledgments |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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