Effect of Cortisol on Bovine Oocytes Maturation and Further Embryonic Development After In vitro Fertilization
Abstract
Oocyte meiotic maturation and further embryonic development after
fertilization is one of the most important physiological requirements
for species survival. Herein, the aim of the study was to evaluate the
effects of the stressful hormone, cortisol, on the nuclear maturation
and further embryonic development of bovine oocytes after in vitro
fertilization (IVFJ. For such purpose, 1,439 immature oocytes were
collected from slaughtered cows and matured in vitro for 24 hours with
different concentrations of cortisol (0 (control); 50 μM; 150 μM ;250
μM). Afterwards, 412 oocytes were denuded, dyed with aceto-orcein and
evaluated for meiotic development. The other 1027 were submitted to IVF
and cultured for 9 days, being evaluated on day 2, 6 and 9, for
cleavage, morula and blastocyst, respectively. In the control, 85 % of
oocytes reached Metaphase II, decreasing to 49, 32 and 15 % for the
concentration of the cortisol (50, 150, and 250 μM, respectively). For
the embryos, obtained from the oocytes submitted to IVF, in the control
group, 28.3 ± 4.8% reached the stage of blastocyst, while for the
concentrations of cortisol this value decreased to 22.1 ± 5.4%, 15.4 ±
6.0% and 6.5 ± 2.1% for 50, 150 and 250 μM of cortisol, respectively).
Results of the present study clearly demonstrated that animal's stress
and particularly high concentrations of cortisol impair bovine nuclear
maturation as well as the further embryonic development after IVF.
Abbreviations: IVF: In Vitro
Fertilization; GVBD: Germinal Vesicle Breakdown; MPF: Maturation
Promoting Factor; ERKs: Extracellular Signal- Regulated Kinases; GnRH:
Gonadotropin-Releasing Hormone; FSH: Follicle-Stimulating Hormone; LH:
Luteinizing Hormone; HPA: Hypothalamic- Pituitary-Adrenal; DPBS:
Dulbecco's Phosphate Buffered Saline; COCs: Cumulus Oocyte Complexes;
FBS: Foetal Bovine Serum; GV: Germinal Vesicle; GVBD: Germinal Vesicle
Break-Down; NCM: Non-Capacitating HEPES-Buffered Medium; TALP: Tyroide's
Albumin Lactate Pyruvate; TNF: Tumor Necrosis Factor; FasL: Fas Ligand;
NMR: Nuclear Maturation Rate; MAPK: Mitogen-Activated Protein Kinases.
Introduction
Stress is a process stimulus activate the entire system and produces
an organic response generating negative effects on animal health and
production. The hormone mainly produced during stress is the cortisol
(C21H30O5) which is secreted by the upper part of the adrenal gland,
being an useful indicator as a biomarker to detect stress on the animals
[1]. Besides, cortisol plays an important role during the catabolic
phase and it negative effect on several metabolism has been well
described [2], it is not yet clear the role of this hormone in ovaries
and particularly on oocyte nuclear maturation and further embryo
development after fertilization. The immature oocytes begin to develop
in the ovaries, possessing a large nucleus referred to as germinal
vesicle (GV), in which a sequence called germinal vesicle breakdown
(GVBD), initiates the process of nuclear oocyte maturation, finishing at
the stage of metaphase II just before ovulation [3]. Maturation
promoting factor (MPF) is activated at GVBD and increases until it
reaches a plateau at the end of the Metaphase I. A transient decline in
MPF activity takes place during the transition between meiosis I,
arresting at metaphase II.
During oocyte maturation, the extracellular signal-regulated kinases
(ERKs) are activated and a comprehensive, extensive rearrangement of the
cytoskeleton and associated proteins occurs involving a spindle pole
close to the cortex [4-6]. After polar body extrusion, chromosomes
realign progressing to metaphase II. All meiosis developmental stages
occur when follicles are growing from preantral to antral follicles.
Moreover, the ovulation occurs when oocyte is in the metaphase II stage
[7-8]. At the endocrine level, folliculogenesis is regulated by a
central nervous system, anterior pituitary, and ovary cascade mechanism.
Specialized hypothalamic neurons secrete pulses of
gonadotropin-releasing hormone (GnRH) into the portal blood vessels,
which acts on the gonadotrophs to cause a pulsatile release of
follicle-stimulating hormone (FSH) and luteinizing hormone (LH), which
act on ovarian follicle cells to control folliculogenesis. Although
GnRH, FSH, and LH are critically important in regulating
folliculogenesis, hormones and growth factors, which are themselves
products of the follicle, can act locally to modulate (amplify or
attenuate) FSH and LH action [9-10].
This is the autocrine/paracrine system of developing follicles. It is
believed that this local regulatory system plays an important role in
the complex mechanisms governing the timing of folliculogenesis and
whether a follicle becomes dominant or atretic. An important point is
that estradiol produced by the dominant follicle rises production of
GnRH, FSH and LH, increasing follicular growth, leading to its
rupture/ovulation [11-13]. Stress-like levels of cortisol suppress
follicular growth and development and block or delay the preovulatory
surge of LH when cortisol is present during the late luteal and early
follicular phases of the oestrous cycle [14-16]. In fact, since the last
century it has been postulated that stressful stimuli reduce fertility
in domestic species, such climatic extremes, transportation or
laparoscopy as well as psychological stress suppress or delay expression
of behavioural oestrus and ovulation. In addition to reducing
fertility, these stressors also stimulate the activity of the
hypothalamic-pituitary-adrenal (HPA) axis, and a marked increase in
serum concentration of cortisol is commonly associated with
management-related stressors [17-19].
Furthermore, cortisol reduces amplitude of GnRH and LH secretion and
lowers plasma estradiol levels in follicular-phase and for such reason,
high cortisol levels can inhibit the reproduction physiology [20-21].
The effect of cortisol inhibition in the protein ERKs disrupting their
functions in meiotic maturation of full- grown oocytes and/or arrest at
metaphase of meiosis II prior to fertilization [22-23]. Although the
causal link between stress and infertility has not been precisely
defined, several studies indicate that glucocorticoids in general and
cortisol in particular may contribute to the anti-gonadal effect of
stress [24-25]. Additionally, the increasing of cortisol level reduces
estradiol production possibly by affecting the granulosa cell functions
within the follicle, which results deterioration in oocyte quality,
leading to a poorest ability to develop after fertilization [17]. The
aim of the present study is to evaluate the role of this hormone on
bovine in vitro oocyte nuclear maturation and further embryo development
after fertilization.
Materials and Methods
Chemicals
All the chemicals and reagents used in this study were obtained from Sigma-Aldrich (St. Louis, Mo, USA) unless stated otherwise.
Ovaries
Ovaries (n = 350) were obtained at a local abattoir from adult
animals, trimmed of adhering tissue and transported to the laboratory in
Dulbecco's phosphate buffered saline (DPBS), at temperature ranging
from 35 to 37°C within 2 hours postslaughtering.
Experimental design
In Vitro Oocyte Nuclear Maturation
Cumulus oocyte complexes (COCs) were washed twice in TCM- 199 medium
supplemented with 2% Foetal Bovine Serum (FBS), 0.3 mg/ml glutamine and
50 mg/ml gentamicin and then washed twice in maturation medium
supplemented with 10% FBS, 5 μg/ ml of FSH-LH, 1μg/ml estradiol-17te,
0.15 mg/ml glutamine, 22 μg/ ml Na-pyruvate, 50 μg/ml gentamicin. Then,
COCs were transferred to sterile Petri dishes containing 100 μl of
maturation medium supplemented with cortisol, previously diluted in
ethanol at 0 (control) 50, 150 and 250 μM final concentration (10-15
oocytes/ droplet) at in an incubator (Lab line instrument Inc. USA) at
38.5 °C for 22-24 hours with saturated humidity and 5% of CO2,
for maturation. Afterwards, COCs were selected, and divided into two
groups: (1 and 2). The ones considered in the group A (n=412) were
fixated and stained for meiosis development evaluation, while the ones
considered in the group B (n=1027) were used for IVF.
Oocyte Fixation and Nuclear Staining
For meiosis development evaluation, COCs were selected, denuded by
vortexing for 2 min and fixated in 3:1 (Methanol: glacial acetic acid)
solution for 24 h at room temperature in petri dishes sealed with
parafilm and then dyed with 1% Orcein. Meiosis stages were recorded as
previously described [26] under a phase contrast microscope at 400x
magnification. Meiotic stages were classified as germinal vesicle (GV),
germinal vesicle break-down (GVBD), metaphase I (MI), anaphase I (Al),
telophase I (TI), and metaphase II (MII) [27], being considered as
mature those evaluated on Telophase I to Metaphase II.
IVF
After 24 hours of maturation, oocytes designated to IVF were selected
under the stereomicroscope, transferred into a Petri dish containing
maturation medium and washed twice in IVF medium. After thawing, semen
was washed twice by centrifuge at 320xg for 5 minutes each, in
non-capacitating HEPES-buffered medium (NCM) sperm washing medium (5 ml
each time). After removing the supernatant, sperm pellet was homogenized
by pipetting in the remaining NCM Sperm wash medium (0.25-0.5 ml) for
adjusting the sperm concentration and motility. A volume of 20 μl of the
semen (11.5 x 106) was uploaded on a slide, covered with a cover slip
and the motility of the sperms was checked under the inverted
microscope. To adjust the semen concentration, 5 μl from the semen were
added to 95 μl distilled water in an Eppendorf tube, and then exposed to
direct light until the semen died. Oocytes and sperms were then
co-cultured in 500 μl of IVF Tyroide's Albumin Lactate Pyruvate (TALP)
for 22-24 hours at 38.5°C in the incubator with saturated humidity and
5% of CO2
In Vitro Embryo-Culture (IVC)
Twenty-four hours from the fertilization, presumptive zygotes were
transferred to a glass tube containing 1 ml of washing medium and
vortexed to remove granulosa cells attached them. Then the embryos were
checked under the microscope, washed twice in culture medium and
cultured for 9 days.
Statistical Analysis
Data are expressed as percentages, and they were subjected to arcsine
transformation when required by X'= arcsinVx All the statistical
analyses were performed by one-way ANOVA in SPSS vs 22. When significant
differences were found, comparison between treatments was made using
either the post hoc, to verify differences between the groups, followed
by the LSD test between groups when parametric assumptions were not
fulfilled. Results are expressed as mean ± SEM. Probability values less
than 0.05 were considered statistically different.
Results and Discussion
]In the present study the effect of several concentrations of
cortisol, ranging from 0 to 250 μM was evaluated on the nuclear and
further in vitro development of bovine oocytes after IVF. As
known, cortisol is a glucocorticoid hormone, which plays an important
role in numerous processes including metabolism, blood pressure, and
immune response regulation, and thus has proved a reliable biological
correlate of many adverse health outcomes [33]. In that manner, as
cortisol is considered a stressful hormone an effective negatively for
the maturation oocytes would be expected on oocytes maturation and
further embryonic development after IVF [34]. In fact, several studies
have observed exposing oocytes to high concentration of cortisol
decreased their competence, undergo impair oocyte developmental
potential by triggering apoptosis of ovarian cells via activating a
transmembrane protein belonging to the tumor necrosis factor (TNF)
usually known as Fas ligand (FasL). Research developed on mice were
injected with cortisol, indicated a clear negative impact of cortisol on
oocyte's nuclear maturation rate (NMR), blastocyst rates and the cell
number per blastocyst [35-36].
Furthermore, related for pigs that significant high concentration of
cortisol in unfertilized oocytes leads to its relative decrease in the
NMR, fertilization or embryo cleavage [37]. Several research developed
in vivo show cortisol as a stressful hormone, affects bovine metabolism,
in general, and reproduction in particular [30-31]. Previously studies
showed that in the Azores, fertility of bovine decreases drastically to
35% in the summer period, achieving 78% in the non-hot periods as spring
and autumn [4445]. Several hypotheses have been purposed to explain
this shut in the hot periods [18, 32, 45]. Heat stress genes, such
HASP14 and Cx34 are activated during summer, when outside temperature
rises over 25 °C. As these genes are also related to the apoptosis, one
can speculate that, among other mechanisms, apoptosis can play a crucial
role in the embryonic as well as in the follicle/oocyte development
from the beginning to metaphase II [32, 45]. Besides in the literature,
cortisol levels on cattle are not very clear, these values were chosen
according several authors in which cortisol can reach a maximum of about
250 μM when cattle are exposed for long time to stress conditions such
high environmental temperature [28-29].
From the 1439 oocytes used in this experiment, results revealed that
those (n=412) employed for maturation rate, a statistical decreased was
observed when cortisol levels increased in the maturation medium. For
cortisol levels of 0 (control); 50 μM; 150 μM; 250 μM groups, rate of
maturation was respectively 85.0; 49.0; 32.0 and 15.0 (Table 1). A
negative correlation (R2 = 0.991) was observed between these two
parameters (P<0.01) (Figure 1). For the 1027 oocytes used for IVF, a
statistical (p<0.01) negative dose- response was observed between the
number of produced embryos in the stage of blastocysts and the cortisol
concentrations (Table 2).
Figure 1: Correlation between mature oocytes and the different concentrations of cortisol. (Y=1.02 + -47.6*X+5*X2, R2 = 0.991 p<0.01).
In our study, cortisol significantly affected NMR decreasing to 15.0%
and blastocyst production to 6.5% when oocytes were exposed to 250 μM
of cortisol (P<0.01), which values are in agreement with those
published also working with cattle [38]. Moreover, in an endeavour to
explain the clear inhibitory effect of cortisol, Gonzalez and
collaborators [2] explained that corticosterone decreases phosphorylated
forms of extracellular signal-regulated kinases (ERKs), phospho-ERK
(p-ERK)-1 and p-ERK-2 in exposed oocytes and this could represent an
alteration in molecular mechanisms underlying oocyte maturation and
competence for subsequent development.
The ERKs are members of the mitogen-activated protein kinases (MAPK)
family activated during oocyte maturation. The MAPKs together with
maturation/metaphase-promoting factor (MPF complex), the two important
protein kinases for oocyte meiosis, interact intimately and perform
essential regulating roles in meiotic maturation and fertilization [39].
Additionally, in mammalian oocytes, several kinases, such as Plk1- and
Akt-induced, regulates the MPF activation, which plays a key role in the
events of GVBD. Moreover, PKA can activate Wee1B (Wee1-like protein
kinase 1B) or inhibit CDC25B, which downregulates MPF activity and
prevents GVBD [40-41]. This mechanism is independent of MAPK activation
inside oocytes [42]. In porcine oocytes, the inhibitory action of
cortisol on meiotic maturation could be due to the reduction in
p34cdc2-cyclin B1 complex, one of the components of MPF [43]. In
addition, results presented and demonstrated that the effect of high
ambient temperatures on reproductive processes, decrease the bovine
fertility to 36.8% in the summer period, affecting also the
physiological mechanisms, inhibiting the in vitro oocytes maturation
rate to 44.3% while the in vitro embryonic development in that period
was 19.6% [44].
In another research developed by our working group, these authors,
showed that heat stress influences the expression on some genes related
to growth and develop embryos such Cx43, CDH1, DNMT1, HSPA14, in which
the lower maturation rate could may be due to the down-regulation of
these genes. Whereas, HSPA14 gene is an important part of the cell's
machinery for folding, unfolding, transport, localization of proteins
and differentiation, regulation of the embryonic cell cycle and helping
to protect cells from stress. Therefore, HSPA14 is an apoptotic gene
induced by heat shock is associated with embryonic loss, playing an
important role of control mechanism of processes involved in growth,
cellular differentiation, and embryonic development [45]. Furthermore,
Cx43 is expressed in numerous tissues including gonads, act as a
mediator of heat stress effect on cells [18]. Additionally, plasma
concentrations of cortisol significantly increased following exposure to
heat stress [18, 32]. Under conditions of prolonged heat exposed to a
moderate heat stress (35 °C) cow's plasma cortisol increased
significantly (P<0.05).
Therefore, plasma cortisol may increase within 20 min of exposure to
acute heat stress and reach a plateau within 2h [46]. Previously
research demonstrated clear the viewpoint of animal welfare in both of
the high ambient temperatures, high direct and indirect solar radiation,
showing an unequivocal evidence that hyperthermia is deleterious to any
form of productivity [47]. Further, numerous studies that use
behavioural indicators of welfare show that behavioural changes can be
interpreted as either good or poor welfare and can be defined by
discrete measures, such as changes in hormone level, body temperature,
and normal behaviour [48]. The type of biological defence an animal
utilizes is not important but the resulting change in biological
function determines if there is a threat to the animal welfare [49].
Conclusion
Results of the present research clearly demonstrated that animal's
stress and particularly cortisol levels might have impaired ovulation
and oocyte potential, influencing negatively their ability to develop to
the stage of blastocyst after fertilisation. Management practices such
as handling, weaning, housing conditions and transportation are
essential to reproduction efficiency of cattle.
Acknowledgment
This project was financed in 85% by FEDER and in 15% with regional
funds through the Programa Operacional Azores 2020 (Operational Program
Azores 2020), in scope of the project «BEMAP-ET -
AC0RES-01-0145-FEDER-000026».
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