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First published online January 18, 2008
Journal of Experimental Biology 211, 400-408 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.011205
Hematological changes associated with egg production: estrogen dependence and repeatability
1 Women's Health Research Institute, E204-4500 Oak Street, Box 42, Vancouver,
British Columbia, V6H 3N1, Canada
2 School of Criminology, Simon Fraser University, 8888 University Drive,
Burnaby, British Columbia, V5A 1S6, Canada
3 Department of Biology, Queen's University, Kingston, Ontario, Canada, K7L
3N6
4 Department of Biological Sciences, Simon Fraser University, 8888 University
Drive, Burnaby, British Columbia, V5A 1S6, Canada
* Author for correspondence (e-mail: ewagner3{at}cw.bc.ca)
Accepted 2 December 2007
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Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Key words: hematocrit, cost of reproduction, egg production, erythropoiesis, estrogen, zebra finch
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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). Studies where investment in egg production has been
experimentally manipulated have provided considerable empirical evidence in
support of this concept (Monaghan et al.,
1995; Daan et al.,
1996; Monaghan and Nager,
1997; Monaghan et al.,
1998; Nager et al.,
2001). However, we still know very little about the physiological
mechanism(s) underlying such costs
(Williams, 2005;
Harshman and Zera, 2007;
Zera et al., 2007). Most
studies to date have focused on relatively simple models of resource-based
allocation trade-offs (e.g. Gustafsson et
al., 1994; Houston et al.,
1995; Oppliger et al.,
1997; Veasey et al.,
2001; Kullberg et al.,
2002; Martin et al.,
2003), in which energy and/or nutrients are reallocated to egg
production and away from other physiological functions with negative
consequences. More recently, it has been suggested that costs of reproduction
might also be caused by the reproductive process itself or the regulatory
(hormonal) mechanisms underlying reproduction (e.g.
Partridge et al., 2005;
Harshman and Zera, 2007).
Hormones are particularly strong candidates for regulating such trade-offs due
to their many pleiotropic effects, both positive and negative
(Ketterson and Nolan, 1992;
Finch and Rose, 1995;
Rose and Bradley, 1998;
Ketterson and Nolan, 1999;
Reed et al., 2006).
Here we test the hypothesis that decreased hematocrit during egg production
reflects a pleiotropic effect of estrogen, the principle female reproductive
hormone, which otherwise has essential functions during egg production.
Numerous studies in birds have documented a reduction in hematocrit,
hemoglobin concentration, and red blood cell counts during egg production
(Jones, 1983;
Keys et al., 1986;
Morton, 1994;
Merino and Barbosa, 1997;
Horak et al., 1998;
Davey et al., 2000;
Sheridan et al., 2004;
Gayathri and Hegde, 2006). In
some cases, the reduction in hematocrit may persist through incubation and
chick rearing stages (Williams et al.,
2004a). Williams et al.
(Williams et al., 2004a)
proposed that these associated changes in hematological parameters may play a
role in shaping the costs of egg production via reducing the total
oxygen carrying capacity of the blood, which could negatively impact aerobic
performance during subsequent energetically demanding reproductive stages such
as chick provisioning (Monaghan et al.,
1998; Nager et al.,
2001).
Kern et al. (Kern et al.,
1972) suggested that the decrease in hematocrit during initial
stages of egg production is most likely due to osmoregulatory processes
(hemodilution) associated with estrogen-dependent changes in lipid metabolism
and the rapid increase of yolk precursors in the blood
(Challenger et al., 2001),
which induces a compensatory increase in total plasma volume
(Kern et al., 1972;
Reynolds and Waldron, 1999).
However, plasma concentrations of yolk precursors decrease rapidly upon
ovulation of the last follicle, reaching non-breeding levels at clutch
completion (Challenger et al.,
2001; Salvante and Williams,
2002). If the observed reduction in hematocrit was due to
hemodilution alone, then hematocrit should be restored to normal
(non-breeding) levels at clutch completion, which is not the case
(Williams et al., 2004a;
Williams, 2005). One
explanation for the persistence of the decrease in hematocrit is that the high
levels of estrogens required to drive egg production also have a transient
inhibitory effect on erythropoietic (red blood cell) stem cells
(Clermont and Schraer, 1979).
Estrogen treatment has been shown to induce anemia in several mammalian and
avian species (reviewed by Blobel and
Orkin, 1996) and molecular studies have demonstrated that estrogen
inhibits erythroid gene expression, delays progenitor cell maturation, and
induces apoptosis in erythroid cell lineages in vitro
(Blobel et al., 1995;
Blobel and Orkin, 1996;
Perry et al., 2000). Since the
estimated lifespan of avian red blood cells is 30–42 days
(Rodnan et al., 1957),
transient suppression of erythropoiesis during egg production could have
relatively long-lasting effects on the proportion of red blood cells in
circulation due to continued cell turnover.
In this study, we investigated whether the reduction in hematocrit during egg production is estrogen dependent in the female zebra finch (Taeniopygia guttata) using experimental manipulations with 17β-estradiol and the anti-estrogen tamoxifen citrate, and a robust repeated-measures breeding design (i.e. each individual female acted as her own control). We predicted that treatment with exogenous 17β-estradiol would result in a larger reduction in hematocrit during egg production, whereas treatment with tamoxifen citrate would result in a smaller reduction in hematocrit at the onset of egg-laying with reference to unmanipulated and sham-treatment breeding trials for each female. Utilizing the repeated-measures experimental design, we also examined individual variability and repeatability of hematological parameters (hematocrit, hemoglobin, red blood cell size and number) and of the change in hematocrit associated with egg production.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Experimental protocol
A repeated-measures design was used to control for variation among
individual females in the traits of interest (i.e. hematological and
reproductive variables). Twenty-nine inexperienced females were randomly
paired with 29 inexperienced males, and the same matched breeding pairs were
used in four successive breeding attempts (experimental trials), alternating
with 3-week rest periods. (1) Unmanipulated (N=23): females did not
receive injections; (2) estradiol treatment (N=24): females were
injected intramuscularly (i.m.) every other day from pairing until clutch
completion with 25.5 µg 17β-estradiol (E8875 Sigma-Aldrich Canada
Ltd., Oakville ON, Canada) in 30 µl canola oil (1.5 µg
g–1 body mass); (3) sham treatment (N=26): females
were injected i.m. every other day from pairing until clutch completion with
30 µl canola oil; and (4) tamoxifen treatment (N=21): females were
injected i.m. every other day from pairing until clutch completion with 170
µg of tamoxifen citrate (T9262 Sigma-Aldrich Canada Ltd.) in 30 µl
1,2-propanediol (10 µg g–1 body mass). Treatment doses
were based on our previous work, which found that injections of 25.5 µg
17β-estradiol every other day increased estrogen concentration in laying
females twofold in comparison to control females but remained within the
physiological range of this species
(Williams et al., 2005), and
that injections of 170 µg of tamoxifen citrate every other day reduced egg
size by 
10% but did not alter clutch size or negatively impact maternal
condition, whereas more frequent injections negatively affected egg quality,
hatchability and offspring growth (Wagner
and Williams, 2007) (T.D.W., unpublished data).
In each experimental trial, pre-breeding blood samples were collected from females on the day of pairing to measure hematological parameters (hematocrit, hemoglobin concentration, red blood cell number, mean red cell volume). A second blood sample was collected at the 1-egg stage (i.e. on the day that the first egg was laid) to measure the same hematological parameters as well as plasma estradiol levels. If blood samples collected at the 1-egg stage were of insufficient volume to permit all analyses listed above, priority was given to measuring hematocrit and aliquoting necessary plasma for estradiol determination (final sample sizes are listed in Table 1). All blood samples were collected from the brachial vein within 3 min of capture (to avoid potential capture-related stress effects) on hematological parameters between 09:30 h and 11:30 h.
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Hematological analyses
Hematological variables were measured with standard techniques developed
for human blood and commonly used on birds
(Campbell, 1995). Hematocrit
(Hct; %) was measured following centrifugation of whole blood for 3 min at 13
000 g. Hemoglobin (Hb; g 100 ml–1 whole blood) was measured
using the cyanomethemoglobin method
(Drabkin and Austin, 1932)
modified for use with a microplate spectrophotometer (BioTek Powerwave 340,
BioTek Instruments, Ltd., Winooski, VT, USA), using 5 µl whole blood
diluted in 1.25 ml Drabkin's reagent (D5941 Sigma-Aldrich Canada Ltd.) with
absorbance measured at 540 nm. Intra- and inter-assay coefficients were 1.71%
and 3.90%, respectively. Erythrocyte counts (RBC; number of
cellsx106 µl–1) were determined from
duplicate samples [1 µl blood diluted 1/200 with modified Natt and
Herrick's solution (Natt and Herrick,
1952; Robertson and Maxwell,
1990)] with an improved Neubauer hemocytometer (Fisher Scientific,
Ottawa, ON, Canada). The average variation among duplicate RBC samples from
the same bird was 6.9%, and measurement error (determined from repeated
sampling) was 8.9%, which is expected with this technique
(Campbell, 1995). As the same
examiner (E.C.W.) scored all red blood cell counts, we expect the measurement
error to be consistent across different breeding stages and experimental
trials. From these measurements we calculated mean red cell volume (MCV; in
fl) with the formula Hct/RBC=MCV (Archer,
1965). For breeding birds, additional blood collected was
centrifuged at 2200 g for 10 min to separate the plasma layer,
which was decanted and frozen at –20°C until assayed for
estradiol.
Estradiol determination
Plasma samples and controls were passed through C18 columns
(octadecylsilane; CUC18156, United Chemical Technologies SPE columns,
Chromatographic Specialties Inc., Brockville, ON, Canada) following the
procedure described (Williams et al.,
2005). Prior to the solid phase extraction procedure, 1 ml of
doubly distilled (dd) water was added to each plasma sample (50 µl unless
sample volume could only provide 25 µl or 10 µl). Using vacuum
filtration, each column was primed with 3 ml of HPLC-grade methanol, followed
by 10 ml of dd water, followed by the entire diluted plasma sample, and then
washed with 10 ml of dd water. Estradiol was eluted with 5 ml of 80% methanol
into 7 ml borosilicate vials (03-337-26, Fisher Scientific, Ottawa, ON,
Canada). Each sample was then evaporated to dryness under vacuum with gentle
shaking and reconstituted in 300 µl of 10% methanol.
A pool of zebra finch plasma was used to quantify the recovery of estradiol. Following vortexing, the plasma pool was divided into three aliquots, each containing 500 µl of plasma. One aliquot was diluted with 400 µl of the assay buffer, one was spiked with 400 µl of the 1 ng ml–1 standard (400 pg spike) and the third remained as raw plasma. Each solid phase extraction run (N=6) contained one 50 µl raw sample, two 50 µl diluted samples and one 50 µl spiked sample. Recovery, calculated as the proportion of the 3.7 pg spike in the assay well that was recovered (duplicate determinations for each of six quantifications of the spiked sample – average of 12 diluted sample duplicate determinations across three plates) was 89%.
The concentration of estradiol in each extracted sample was then determined using a 17β-estradiol enzyme immunoassay kit (Ecologiena/Japan EnviroChemicals Ltd., Abraxis LLC, Warminster, PA, USA) exactly as indicated in the instructions. In duplicate, 100 µl of reconstituted sample (equivalent to 16.7 µl, 8.3 µl or 3.3 µl of the original plasma) was mixed with 100 µl of antigen-enzyme conjugate solution to yield a 5% methanol solution. Of that 200 µl, 100 µl (equivalent to 8.3 µl, 4.2 µl or 1.7 µl of the original plasma sample of 50 µl, 25 µl, or 10 µl, respectively) was then transferred into an antibody-coated plate for quantification. A total of three assay plates were run, each of which included all samples, in duplicate, from two solid phase extraction runs. One sample fell outside the range of assay sensitivity and was further diluted prior to re-analysis on a subsequent plate. Assay variability was calculated from controls at 9 pg/well and 21.5 pg/well, yielding intra-assay coefficients of variability of 2.3% and 5.3% and inter-assay coefficients of variability of 5.3% and 6.7%, respectively.
Statistical analysis
All statistical analyses were carried out using SAS software version 9.1
(SAS Institute, 2003). A
repeated-measures mixed linear model (MIXED procedure) was used to compare
temporal variation in body mass and hematological parameters across trials,
with reproductive stage, treatment and stagextreatment interaction
included in the model as fixed effects and individual as a random effect.
Treatment effects on plasma estradiol concentration and reproductive traits
were analyzed using repeated-measures mixed linear models, with treatment
included as a fixed effect and individual as a random effect in the model. The
effect of reproductive stage on hematocrit was analyzed separately for each
trial using generalized linear models (GLM procedure). Post-hoc tests
for differences between means were adjusted for multiple comparisons following
the Tukey–Kramer method. Repeatability of pre-breeding hematological
parameters and the change in hematocrit from pre-breeding to the 1-egg stage
were determined using nested ANOVA (NESTED procedure) following Lessells and
Boag (Lessells and Boag,
1987). Clutch size was the only variable that was not
approximately normal in distribution (Kruskal–Wallis test; UNIVARIATE
procedure) and was therefore log-transformed prior to analyses. All values
presented are least-squares means ± s.e.m. unless otherwise stated.
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RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Excluding pre-breeding data from the first, unmanipulated trial (but not data for clutch completion for this trial, see Discussion for rationale), there was no difference in mean body mass at pre-breeding (F2,67=0.34, P>0.7) and clutch completion stages (F3,85=1.34, P>0.25) between treatments, indicating that female condition was not adversely affected by hormonal manipulations or successive breeding attempts. In addition, all hematological parameters (hematocrit, hemoglobin concentration, red blood cell count and mean cell volume) were independent of pre-breeding body mass (P>0.1 in all cases), and plasma estradiol concentration was independent of 1-egg stage body mass (P>0.1 for all trials).
Variation in plasma estradiol concentration and reproductive output
Experimental treatment had a highly significant effect on mean plasma
estradiol concentration at the 1-egg stage (F3,59=8.48,
P<0.0001; Table 2).
There was no difference in plasma estradiol levels at the 1-egg stage among
unmanipulated, sham-treated and tamoxifen-treated females (P>0.7
for all comparisons, 95% CI=1.02–1.22 ng ml–1).
However, plasma estradiol levels were significantly elevated in the
estrogen-treated females (P<0.001 for all pairwise comparisons;
95% CI=2.22–3.77 ng ml–1).
Controlling for differences in female body mass at laying, experimental treatment had a significant effect on mean egg mass (F3,66=10.2, P<0.0001; Table 2); mean egg mass was reduced by approximately 10% in tamoxifen-treated females compared with all other breeding trials. However, treatment had no effect on clutch size (controlling for differences in laying interval: F3,48=0.94, P>0.45; Table 2) or clutch mass (F3,46=2.66, P>0.05; Table 2). Controlling for differences in clutch size, laying interval was significantly longer in the first, unmanipulated trial compared with all other trials (F3,42=3.16, P<0.035; Table 2).
Treatment effects on hematological parameters
The change in hematological parameters from pre-breeding to the 1-egg stage
was independent of the number of days elapsed between blood samples for all
four experimental trials (P>0.15 for all). Among individual
females, pre-breeding measurements of hematocrit
(F3,53=2.14, P>0.1), hemoglobin
(F2,43=2.06, P>0.1), red blood cell number
(F3,68=0.46, P>0.7), and mean cell volume
(F3,71=0.52, P>0.65) did not differ between
trials indicating that hematological variables recovered to baseline,
pre-breeding levels during the 3-week recovery period between the four
successive breeding trials, and that treatment order, breeding experience and
age did not alter these parameters (Table
3).
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There was a highly significant treatment–reproductive stage interaction for hematocrit (F3,35=7.32, P<0.0006) and this was due to maintenance of a higher hematocrit at the 1-egg stage in tamoxifen-treated females (Table 3). Hematocrit decreased significantly from pre-breeding to the 1-egg stage in the unmanipulated (–4.3±1.1%; F1,21=14.54, P<0.001; Fig. 1A), estradiol-treated (–5.5±0.7%; F1,22=60.83, P<0.0001; Fig. 1B) and sham-treated females (–5.3±0.7%; F1,25=66.41, P<0.0001; Fig. 1C), but there was no significant difference in hematocrit from pre-breeding to the 1-egg stage in the tamoxifen-treated females (F1,17=3.77, P>0.07; Fig. 1D).
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Individual variation and repeatability of hematological parameters
Pre-breeding hematocrit was highly variable among individuals
(45–63%; Fig. 1) but was
also highly repeatable with individual female, explaining 63.4% of the total
variation (F13,42=7.93, P<0.0001).
Pre-breeding hemoglobin concentration across the estradiol-treatment,
sham-treatment and tamoxifen-treatment trials was also repeatable with
individual female explaining 35.9% of the total variation
(F13,28=2.68, P<0.015; hemoglobin data were
not available for the first, unmanipulated trial). However, pre-breeding
measurements of red blood cell number (F13,42=0.93,
P=0.5) and mean cell volume (F13,42=1.26,
P=0.3) were not repeatable across trials.
With the exception of tamoxifen-treated females, the majority of individual females showed a robust and consistent decrease in hematocrit between pre-breeding and the 1-egg stage (Fig. 1). Pre-breeding and 1-egg hematocrit were positively correlated in the estradiol-(r23=0.60, P<0.0025; Fig. 2B) and sham-treated females (r26=0.73, P<0.0001; Fig. 2C), and this relationship was positive but not significant in unmanipulated females (r22=0.31, P=0.16; Fig. 2A) and tamoxifen-treated females (r18=0.44, P<0.07; Fig. 2D). There was some variation among individual females in the magnitude of the decrease in hematocrit (calculated as 1-egg to pre-breeding values) within experimental trials: the change in hematocrit ranged from –17.3 to +3.8% in the unmanipulated trial, –13.0 to +1.1% in the estradiol-treatment trial, –11.3 to +2.1% in the sham-treatment trial and –13.3 to +6.0% in the tamoxifen-treatment trial (Fig. 3). Furthermore, the change in hematocrit was negatively correlated with pre-breeding hematocrit for all trials (unmanipulated: r22=–0.74, P<0.0001; estradiol-treatment r23=–0.61, P<0.002; sham-treatment: r26=–0.51, P<0.007; tamoxifen-treatment: r18=–0.57, P<0.015), i.e. females with the highest pre-breeding hematocrit values tended to show the largest decrease in hematocrit during egg production (Fig. 3). Nevertheless, for all experimental trials the change in hematocrit from pre-breeding to the 1-egg stage was repeatable, with individual female explaining 31.6% of the total variation (F13,42=2.85, P=0.005). Excluding the tamoxifen-treatment and unmanipulated trials (see Discussion), repeatability of the reduction in hematocrit for the sham- and estradiol-treatment trials was 66.7% (F13,14=5.0, P<0.003).
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DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Body mass variation, estradiol and tamoxifen treatment effects on
reproductive traits in the present study were similar to those reported in our
previous studies (Williams,
1996a; Christians and Williams,
1999; Williams,
1999; Williams,
2000; Wagner and Williams,
2007). In our experiment, all females were exposed to the four
treatments in the same sequential order, and it is possible that treatment
order, age, or breeding experience might have influenced our results. However,
we do not believe that this was the case for the following reasons. First,
effects of estradiol and tamoxifen injections at the physiological doses we
used are short-term and transient (Johnson
and van Tienhoven, 1981; Tsang
and Grunder, 1984; Williams,
2000). We also demonstrated directly that hematological parameters
returned to `baseline' pre-breeding values during each of the 3-week recovery
periods, and that these pre-breeding hematological variables were repeatable
across trials. Second, Williams (Williams,
1996b) has shown that successive breeding attempts with no
recovery period between laying bouts does not affect egg and clutch size. In
addition, Williams and Christians
(Williams and Christians,
2003) demonstrated that age and breeding experience do not
significantly influence primary reproductive effort (egg size, clutch size) in
this population of zebra finches, the only exception being a longer laying
interval in the first breeding attempt, which is consistent with the results
of this experiment. During the initial reproductive bout (unmanipulated trial)
of the current experiment, females also showed changes in body mass typical of
inexperienced breeders (Williams,
1996a) (E.C.W., unpublished data): pre-breeding body mass was
significantly higher than all other trials, and in contrast to the pattern
observed in estradiol- and sham-treatment trials, females showed a linear
decline in body mass from pre-breeding to clutch completion. There was some
evidence that hematocrit was similarly affected by breeding inexperience, but
for the first trial only. In comparison to the estradiol- and sham-treatment
trial, the mean change in hematocrit from pre-breeding to the 1-egg stage was
slightly less (1%) and there was a greater range in the magnitude of this
change among individuals, suggesting that breeding experience may alter body
condition somewhat through unknown mechanisms. However, the effects of
estradiol and tamoxifen were consistent in comparison with both the
unmanipulated and sham-treatment groups, and the latter group was included
specifically to control for breeding experience. Third, in our study only
females in the last (tamoxifen) treatment showed any treatment effect and this
was a reduction of the decrease in hematocrit: the opposite to what would be
predicted if successive breeding attempts were causing a decline in
hematological variables (e.g. maternal condition). Reproductive traits did not
vary significantly across the first three trials as might be expected if birds
were experiencing `reproductive exhaustion', and the specific
tamoxifen-induced decrease in egg size (with no change in clutch size) in the
last trial is entirely consistent with the direct effects of tamoxifen shown
in previous studies (Williams,
2000; Williams,
2001; Wagner and Williams,
2007). Finally, in a preliminary experiment (E.C.W., unpublished
data) utilizing a different treatment order we obtained results that are
consistent with those reported here.
In the present study, tamoxifen inhibited the reduction in hematocrit but
estradiol did not enhance the reduction in hematocrit during egg production,
and initially these results appear to be contradictory. However, similar
differential effects on estrogen-dependent reproductive traits have been
documented here and in previous studies: tamoxifen treatment causes a robust
decrease in egg size (Williams,
2000; Williams,
2001; Wagner and Williams,
2007), whereas exogenous estradiol does not increase egg size
(Christians and Williams, 1999;
Williams, 1999). Although
previous studies have reported that estradiol treatment induces anemia (range
–2 to –15%) in domestic fowl
(Domm and Taber, 1946;
Sturkie and Eiel, 1966),
pilgrim geese (Hunsaker,
1968), Japanese quail
(Nirmalan and Robinson, 1972;
Nirmalan and Robinson, 1973;
Garcia et al., 1984), rain
quail (Deshmukh and Suryawanshi,
1982) and white-crowned sparrows
(Kern et al., 1972), these
studies all used non-breeding birds, which would have low baseline levels of
endogenous estrogens. To our knowledge, our study is the first to assess
effects of physiological levels of estradiol on hematological parameters in
laying females specifically within the context of egg production. We suggest
two reasons for the differential effects of anti-estrogen treatment
(tamoxifen) versus estrogen treatment on hematocrit: (1)
estrogen-mediated physiological effects might be effectively `maximized' at
normal endogenous plasma estradiol concentrations, or (2) despite the
experimentally induced increase in circulating estrogens, homeostatic
mechanisms may act to maintain hematocrit above some minimum `threshold' level
to maintain a minimum oxygen-carrying capacity required to meet enhanced
metabolic demands and/or to facilitate transport of egg constituents to the
oviduct. It is possible that in egg-laying females estrogen receptors in bone
marrow (the site of erythropoiesis) might be saturated at endogenous estrogen
concentrations and thus unresponsive to estrogen supplementation, and/or that
estrogen receptor number or receptor sensitivity might be downregulated to
modulate pleiotropic effects of the high levels of endogenous estrogens
present during egg production (Williams et
al., 2004b; Williams et al.,
2005). This is consistent with previous work demonstrating that
exogenous estradiol treatment stimulates estrogenic processes in non-breeding
birds, but does not enhance the same processes in breeding females, e.g.
hepatic synthesis and release of yolk precursors
(Williams, 1999).
Alternatively, homeostatic mechanisms (hemoconcentration or hemodilution) may
act to maintain hematocrit within an optimum range that best meets the
increased metabolic demands during egg production
(Vezina et al., 2003;
Vezina et al., 2006);
therefore, any inhibitory effects of exogenous estradiol on erythropoiesis may
be masked as a result. Given that hematocrit is a critical determinant of
blood viscosity (Gaudard et al.,
2003), it may not be advantageous for females to deviate from a
set range because this would compromise blood flow dynamics and influence
efficiency of oxygen and/or nutrient delivery to tissues
(Nikinmaa, 1990;
Hebert et al., 1997) during
key reproductive stages. In addition, hematocrit might be maintained within a
set range to maximize transfer efficiency of proteins, lipids, water and trace
elements from the plasma reservoir to the oviduct
(Reynolds and Waldron, 1999).
This idea of some minimum threshold at which egg-producing females maintain
hematocrit is supported by our observation that females with relatively low
pre-breeding hematocrit showed the smallest change in hematocrit during egg
production. However, the fact that decrease in hematocrit itself was
repeatable suggests that any threshold hematocrit level might vary among
individuals and that the decrease in hematocrit during egg-laying may be
`programmed' both within- and among-individual females, possibly reflecting
individual variation in a lower physiological limit below which aerobic
capacity would be compromised.
Our study supports the hypothesis that the reduction in hematological
parameters during egg production is dependent on the receptor-mediated action
of endogenous estrogens, and thus we suggest that this mechanism is a good
candidate for a regulatory-network-based trade-off involving antagonistic
pleiotropic effects of estrogens, which otherwise have essential reproductive
functions during egg production. However, the present study does not
distinguish between the specific proximate mechanisms underlying these changes
in hematological parameters that were potentially disrupted by tamoxifen
treatment. Our main objective was to manipulate hematocrit levels at the onset
of egg-laying, and because of our experimental design, we did not investigate
potential long-term effects of changes in hematocrit at later stages of egg
production and incubation. Therefore, we could not separate estrogen-dependent
hemodilution effects from direct inhibition of erythropoiesis, and we did not
capture any delayed effects of estradiol on red blood cell production, e.g.
estradiol suppression of erythrocyte production at multiple points in the
maturation pathway, such as gene transcription, cell differentiation and
hemoglobin production (Blobel and Orkin,
1996). Future studies could clarify this issue by collecting blood
samples from estradiol- and tamoxifen-treated females at later stages in the
reproductive cycle. In addition, whereas tamoxifen prevented a decrease in
hematocrit during egg production, we did not detect any treatment effects on
other hematological parameters (i.e. there was no difference in the decrease
in hemoglobin and red blood cell number in tamoxifen-treated females). Whether
this is the result of too small sample numbers of these more variable, less
repeatable traits or whether this reflects differential actions of estrogens,
e.g. estrogen-independent components of the hematological response, remains to
be determined.
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Acknowledgments |
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References |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Archer, R. K. (1965). Hematological Techniques for use on Animals. Oxford: Blackwell Scientific Publishing.
Blobel, G. A. and Orkin, S. H. (1996). Estrogen-induced apoptosis by inhibition of the erythroid transcription factor GATA-1. Mol. Cell. Biol. 16,1687 -1694.[Abstract]
Blobel, G. A., Sieff, C. A. and Orkin, S. H. (1995). Ligand-dependent repression of the erythroid transcription factor GATA-1 by the estrogen-receptor. Mol. Cell. Biol. 15,3147 -3153.[Abstract]
Campbell, T. W. (1995). Avian Hematology and Cytology (2nd edn). Ames: Iowa State Press.
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