https://doi.org/10.52973/rcfcv-e33212

Received: 07/06/2023 Accepted: 01/08/2023 Published: 17/08/2023

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Revista Científica, FCV-LUZ / Vol. XXXIII, rcfcv-e33212

ABSTRACT

Oocyte maturation is a critical step for in vitro embryo production.

In female cats, ndings on the inuence of the estrous cycle stage

on oocyte quality and maturation are contradictory. Little is known

about this phenomenon in female cats in the tropics. This study aimed

to assess the effect of the estrous cycle stage on oocyte quality and

subsequent capacity to complete nuclear maturation in cats in a

tropical environment. Ovaries from 18 sexually matured cats were

collected during ovariohysterectomy. Cumulus–oocyte complexes

(COCs) were released from follicles by slicing and fragmentation of

the ovarian cortex. According to morphological characteristics, COCs

were classied into grades I–II (suitable) and III–IV (no suitable). Only

suitable COCs from each cat were cultured for in vitro maturation.

Nuclear oocyte maturation was assessed by the presence of a

telophase I or metaphase II plate with extrusion of the rst polar

corpuscle. A signicantly greater number of oocytes per ovary were

collected from queens in inactive than in follicular or luteal phase.

Proportions of suitable COCs were similar among groups. Rate of

oocyte maturation did not differ among stages of the estrous cycle,

nor did the proportion of non–matured or degenerated oocytes. The

age of the queens did not affect the percentage of oocyte maturation.

In conclusion, the quality and rate of oocytes maturation were similar

in the three stages of estrous cycle examined.

Key words: Cat, reproduction; biotechnology; in vitro system;

tropics

RESUMEN

La maduración de los ovocitos es un paso crítico para la producción

de embriones in vitro. En las gatas, los hallazgos sobre la inuencia de

la fase del ciclo estral en la calidad y maduración de los ovocitos son

contradictorios. Se sabe poco sobre este fenómeno en las gatas en los

trópicos. El objetivo de este estudio fue evaluar el efecto de la fase del

ciclo estral sobre la calidad de los ovocitos y la posterior capacidad de

completar la maduración nuclear en gatas de un ambiente tropical.

Se recogieron ovarios de 18 gatas sexualmente maduras durante la

ovariohisterectomía. Los complejos cúmulo–ovocito (COCs) fueron

obtenidos de los folículos mediante el corte y la fragmentación de la

corteza ovárica. Según sus características morfológicas, los COCs se

clasicaron en grados I–II (aptos) y III–IV (no aptos). Sólo los COCs de

buena calidad de cada gata se cultivaron para su maduración in vitro.

La maduración nuclear de los ovocitos se evaluó por la presencia

de una placa en telofase I o metafase II con extrusión del primer

corpúsculo polar. Se obtuvo un número signicativamente mayor

de ovocitos por ovario en las gatas en fase inactiva que en fase

folicular o lútea. Las proporciones de COCs fueron similares entre

los grupos. La tasa de maduración de los ovocitos no dirió entre

las fases del ciclo estral, ni tampoco la proporción de ovocitos no

maduros o degenerados. La edad de las gatas no afectó al porcentaje

de maduración de los ovocitos. En conclusión, la calidad y la tasa de

maduración de los ovocitos fueron similares en las tres etapas del

ciclo estral examinadas.

Palabras clave: Gata; reproducción; biotecnología; sistema in vitro;

trópico

Effect of estrous cycle stage on oocyte in vitro maturation of domestic cats

reared under tropical conditions

Efecto de la fase del ciclo estral en la maduración in vitro de ovocitos de gatas domésticas

criadas en condiciones tropicales

Enmar Monasterio–Alemán

, Luis Monasterio–Oquendo

, Liset Zambrano–Vivas

, Verónica Arboleda–Caldera

, Carla Osorio–Melendez

José Aranguren–Méndez

, Fernando Perea–Ganchou

* , Hugo Hernández–Fonseca

Universidad del Zulia, Facultad de Ciencias Veterinarias. Maracaibo, Venezuela.

Universidad del Zulia, Facultad de Ciencias Veterinarias, Unidad de Investigación en Biotecnología Animal. Maracaibo, Venezuela.

Universidad de Cuenca, Facultad de Ciencias Agropecuarias. Cuenca, Ecuador.

Saint George's University, School of Veterinary Medicine, Anatomy, Physiology and Pharmacology Department. True Blue, St. George's, Grenada, WI.

*Corresponding author: fernando.perea@ucuenca.edu.ec

Estrous cycle stage and in vitro maturation of cat oocytes in tropical countries/ Monasterio-Alemán et al. ________________________

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INTRODUCTION

Domestic cats (Felis catus) are very prolic and fertile animals, so

the main efforts to develop an ecient in vitro system for embryo

production have been the multiplication and preservation of wild

species of felines threatened by extinction [1]. Thus, domestic cats

have been used as an experimental model [2, 3] for the development

of an in vitro embryo production system to generate information

applicable to the reproduction of wild cats [4, 5].

In vitro studies in small animals are scarce, particularly in domestic

cats. In felines, as in other domestic species, in vitro oocyte

maturation has been considered a critical step for the advancement

of this biotechnology in terms of production of transferable embryos

[6]. Different methodologies and media for in vitro maturation (IVM)

and in vitro fertilization (IVF) in cat oocytes have been described [3,

7, 8, 9, 10, 11, 12, 13].

The goal of an optimal in vitro maturation media is to allow the

developmental competence of the oocytes to be fully expressed.

Oocyte competence is crucial for the success of in vitro maturation

and subsequent embryo development. This capacity is inuenced

by several factors such as the presence of cumulus cells around the

oocyte [14], reproductive season [15], the diameter of the follicle

from which the oocyte is derived [16] and stage of the estrous cycle

at the time of oocyte retrieval [13].

In cats, the estrous cycle progresses throughout different phases:

proestrus, estrus, interestrus, diestrus (if copulation and induced

ovulation occur), and anestrus [17]. In each phase, there is absence

(anestrus), low (interestrus) or high concentration of estrogens

(proestrus, estrus), and high (diestrus) or low (proestrus, estrus)

concentration of Progesterone. These gonadal hormones modulate

the physiological characteristics of the ovaries, oviduct and uterus,

and determine changes in the cellular morphology of the vagina [17].

The variation in the developmental capacity of cat oocytes by the

influence of the estrous cycle stage has been poorly studied and

controversial. Progesterone and or other substances produced by the

corpus luteum (CL) seem to affect the ability of oocytes to complete

nuclear maturation. Oocytes retrieved during the follicular phase

completed metaphase II in a greater proportion, to those recovered

from ovaries with a luteal structure [13, 18]. However, other studies found

no effects of the stage of the estrous cycle on the maturation rate of

cat oocytes, or the cleavage rate and blastocyst development [19, 20].

The studies mentioned above were conducted in regions where

cats exhibit seasonal polyestrous reproductive conduct [21]. In

the tropics, daylight hours do not vary greatly throughout the year,

and cat reproduction is continuously polyestrous [22]. There is no

published information about the inuence of estrous cycle stages

on oocyte quality and nuclear maturation in tropical regions in cats.

Therefore, this study aimed to assess the effect of the estrous cycle

stage on oocyte quality and subsequent capacity to complete nuclear

maturation in cats under a tropical environment.

MATERIAL AND METHODS

All chemicals were purchased from Sigma (St Louis, MO, USA),

unless otherwise mentioned.

Animals and surgery

It was studied 18 domestic cat females, sexually matured, aged

between 8 and 30 months, of different breeds and crossbreeds. Cats

(2.4 kg weight) were in satisfactory physical and health condition

before being included in the study. The surgical procedure was

performed at the Veterinary Polyclinic of the University of Zulia,

Maracaibo, Venezuela. For surgery was used the Hedlund's surgical

technique [23]. The study was conducted between March and May

2017. Vaginal smears were taken before surgery to corroborate the

stage of the estrous cycle. Ovaries were collected from each female

during ovariohysterectomy. Cats were allocated to one of three stages

of the estrus cycle, according to the structures found in the ovaries:

1) follicular stage: one or more follicles greater than or equal to 2 mm

in diameter in one or both ovaries; 2) luteal stage: presence of one or

more CL in one or both ovaries; 3) inactive stage: ovaries without CL

and with no follicles greater than or equal to 2 mm in diameter [20].

Ovary collection and oocyte recovery were transported to the

in vitro fertilization (IVF) laboratory in sterile saline (0.9% NaCl) at

38°C within one h after surgery. Immediately after arriving at the

laboratory, ovaries were rinsed twice in a sterile warmed washing

medium (NaHCO

0.55 g; Heparin 0.00277 g; TCM–199 3.9 g; Gentamicin

sulphate 50 mg·mL

-1

, 0.4 % Bovine Serum Albumin (BSA), Sodium

Pyruvate 20 µL; embryo tested ultra–pure water 250 mL). Surrounding

tissues were removed from the ovaries. Ovaries were placed in a

sterile 100 mm petri dish containing washing medium, and cumulus

oocytes complexes (COCs) were released from follicles by slicing and

fragmentation of the ovarian cortex.

COCs were classied according to morphological features under

stereoscopic magnication 20X (Nikon, SMZ–2B, Tokyo, Japan) into

four categories [24]: 1) Grade I: oocytes with uniform, dark cytoplasm,

eccentric spherical nuclei, and five or more compact layers of

cumulus cells; 2) Grade II: oocytes with uniform, dark cytoplasm,

less than ve compact layers of cumulus cells; 3) Grade III: oocytes

with inhomogeneous cytoplasm, partially surrounded by not so

compact cumulus cells; 4) Grade IV: oocytes with heterogeneous or

fragmented cytoplasm, with few or no cumulus cells around them.

Grade I and II oocytes were considered suitable and grades III and IV

were unsuitable. Only the former group of oocytes (grades I and II)

was submitted to Maturation in vitro (IVM).

In vitro maturation

Cumulus oocytes complexes from each cat were cultured separately

for IVM in groups no greater than 20 structures in 90–µL droplets,

covered with mineral oil. IVM medium was composed of TCM–199

supplemented with 1 µg·mL

-1

of estradiol 17–ß; 0.02 UI·mL

-1

of FSH;

0.02 UI·mL

-1

of LH 50 µL; 0.3 mM sodium pyruvate; 4 mg·mL

-1

BSA; 5%

fetal bovine serum; and 50 μg·mL

-1

of Gentamicin. Incubation (Thermo

Scientic, modelo 3010, Waltham, MA, USA) was performed for 30 h

at 38.5 °C in a humidied atmosphere of 5% CO

Oocyte nuclear maturation

After maturation, COCs from each cat were denuded from cumulus

cells by gentle pipetting in the maturation medium. Denuded oocytes

were xed in a solution of acetic acid–ethanol (1:3) for 24–48 h at

4°C and then placed on a sterile slide covered with a cover slide

setting. Oocytes stained with 1% aceto–orcein solution for 30

min, were rinsed in acetic acid and glycerol solution and left to

dry. Nuclear oocyte maturation was assessed by the presence of

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a telophase I or metaphase II plate and the extrusion of the rst

polar corpuscle. Oocytes without the above characteristics were

considered immature. Fragmented or irregularly shaped oocytes

were considered degenerated [25].

Statistical analysis

The number of oocytes recovered per ovary was analyzed by the

general linear model of SAS (SAS

; Version 9.3; SAS Institute, Inc.,

Cary, NC, USA). Means differences were compared by Tukey’s multiple

comparison test. Proportions of suitable, matured or immatured/

degenerated oocytes were analyzed by Chi–square of SAS.

RESULTS AND DISCUSSION

In general, 601 COCs were recovered from female cats in follicular

(n=7), luteal (n=9) or inactive (n=2) stage. A signicantly greater

(P<0.05) number of oocytes per ovary were obtained from queens

in inactive than in the follicular or luteal phases. This difference was

because one queen in the inactive stage yielded 100 COCs and the

other 21. Similar proportions of suitable COCs were quantied among

groups of ovaries (TABLE I).

Proportionally more COCs per ovary were retrieved from ovaries in

the inactive than in the luteal or follicular stages. Although only two

queens with inactive phase ovaries were part of the current study,

and the ovaries from one of them produced 5 fold more COCs than

the second, the average number of oocytes recovered was close to

doubling the average number of oocytes recovered from the other

groups. In relation to this issue, there are opposite ndings. Naoi et al.

[20] reported obtaining a greater number of COCs from inactive than

from follicular or luteal ovaries, which agrees with the outcomes of

Freistedt et al. [26] and the present study in South America. However,

no difference was found in the number of COC retrieved in different

stages of the reproductive cycle [19]. It was found similar proportions

of suitable (grade I and II) COCs among groups of ovaries; however,

signicant differences in the proportions of grade I oocytes was

observed between the follicular and luteal stages [20].

In this study conducted in a tropical region, where cats exhibit

reproductive cyclicity throughout the entire year, maturation

rates were statistically similar among stages of the estrous cycle.

However, it is important to note that the maturation rate was 5 and 9.7

percentage points greater (P>0.05) in oocytes obtained in luteal than

in follicular or inactive phase, respectively. The rate of maturation in

this study was considerably lower than that found in other studies [13,

19]. There is no precise explanation for this nding; however, the donor

cats included in this study came from widely varied households with

varying levels of medical care, husbandry, and nutrition. In general,

cats in tropical environments are freer to be outside the house and,

therefore, are more exposed to stressful situations and environmental

cues that may affect the oocyte developmental competence [27, 28].

The outcomes of previously published studies in felines about

oocyte competence and how it is affected by the stages of the

reproductive cycle have been variables, but not enough evidence

has been gathered. For instance, noticeable differences in oocyte

maturation between follicular and luteal stages were found, with

maturation rates of 50 percentage points greater in the former than

in the later stage [13]. This difference did not change by adding IGF–I,

EGF, or both growth factors, in the maturation media [13].

Supporting the previous nding, substances produced by luteal

tissue, likely Progesterone, seem to have adverse effects on oocyte

competence, because maturation rate was lower when the oocytes

were collected during the luteal stage or from ovaries of pregnant

cats than in the follicular or inactive stage [18]. However, in ruminants,

the CL had favorable effects on oocyte competence and embryonic

development [29, 30].

On the other hand, other studies found no difference in the

maturation rate [19] or blastocyst development [20] from cat

oocytes collected at different stages of the estrous cycle. However,

proportionally more oocytes obtained from the luteal or inactive or

TABLE I

Effect of stage of estrous cycle on the quantity and

quality of oocytes recovered from cat ovaries

Estrous cycle

stage

No. oocytes

recovered

Oocytes/ovary

(mean ± EE)

Suitable

oocytes n (%)

Follicular 228 16.3 ± 6.7

173 (75.9)

Luteal 252 14.0 ± 6.2

188 (74.6)

Inactive 121 30.2 ± 27.9

90 (74.4)

Total 601 16.7 ± 10.2

a, b

: Values with different letters in the same column differ. P<0.05

TABLE II

Effect of stage of estrous cycle on nuclear maturation

of oocytes recovered from cat ovaries

Estrous cycle

stage

No. oocytes

examined

Matured

oocytes n (%)

Immature/

degenerated

oocytes n (%)

Follicular 89 11 (12.4) 78 (87.6)

Luteal 144 25 (17.4) 119 (82.6)

Inactive 65 5 (7.7) 60 (92.3)

Total 298 41 (13.7) 257 (86.2)

TABLE III

Chi–square value and odds ratios for oocyte

maturation among stages of estrous cycle

Estrous cycle

stage

P–value

Odds ratio

(95% CI)

Luteal × Follicular 1.05 0.305 1.49 (0.69–3.19)

Luteal × Inactive 0.87 0.349 1.69 (0.56–5.13)

Luteal × Inactive 3.40 0.065 2.52 (0.91–6.91)

Maturation rate was greater (P>0.05) in oocytes from cats in luteal

than in follicular or inactive stage (TABLE II). A similar proportion of

immature/degenerated oocyte was observed among groups. The

odds ratios for oocyte maturation between two groups in different

stages of the estrous cycle showed a greater probability of oocyte

maturation in luteal than in follicular phase, and in follicular or in

luteal than in inactive stage (TABLE III). According to the cat’s age,

categorized as ≤ 12 (10.1 ± 1.7; n=8) and >12 (20.4 ± 4.2; n=10) months,

the rate of maturation did not differ among stages of estrous cycle

(data not shown).

Estrous cycle stage and in vitro maturation of cat oocytes in tropical countries/ Monasterio-Alemán et al. ________________________

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intermediate phase cleaved and became blastocysts after IVF than

those recovered in the follicular stage [19, 28].

At different stages of the estrous cycle, oocytes are exposed to

varying concentrations of gonadal steroids and other substances

produced inside or outside the ovary [31, 32, 33, 34]. Therefore,

it is plausible that the developmental competence of the oocytes

changes throughout the reproductive cycle. Progesterone is essential

in determining uterine receptivity in mammals but also plays a relevant

role in oocyte maturation and subsequent embryo development [29,

35, 36]. Follicular size, which is related to the stage of the estrous

cycle, may affect maturation and blastocyst rates [37, 38]. Even

varying rates of oocyte maturation, cleavage, and embryo production

in cats in the same stages of the estrous cycle may be supported by

numerous factors modifying the oocyte developmental capacity [26,

27, 39, 40, 41, 42, 43].

CONCLUSION

The quality and rate of oocyte maturation were not affected by the

estrous cycle stage. Nonetheless there was a greater probability for

oocytes obtained from queens in the luteal phase to reach maturation

after IVM . Eventhough, there is some indication that the number of

recovered COCs increased in the inactive than in the follicular or luteal

stage, it cannot at this time conclude this due to the small number

of cats in this group and further research should be conducted using

cats between 12–24 months of known parity.

Conicts of Interest

The authors have no potential conicts of interest with respect to

the research, authorship or publication of this article.

BIBLIOGRAPHICS REFERENCES

[1] Veraguas D, Echeverry D, Castro FO, Rodriguez–Alvarez Ll.

Applied biotechnologies in the conservation of wild felids: In

vitro embryo production and cellular regenerative therapies. In:

Shrivastav AB, Singh KP, editors. Big Cats [Internet]. London:

Intech. Open. 2017. p. 47–71. doi: https://doi.org/kpcj

[2] Pope CE. Aspects of in vivo oocyte production, blastocyst

development, and embryo transfer in the cat. Theriogenol.

[Internet]. 2014; 81(1):126–37. doi: https://doi.org/kpck

[3] Pope CE. Thirty years of assisted reproductive technology in the

domestic cat: A selected summary. Rev. Bras. Reprod. Anim.

2019; 43(2):129–136.

[4] Farstad W. Current state in biotechnology in canine and feline

reproduction. Anim. Reprod. Sci. [Internet]. 2000; 60–61:375–

387. doi: https://doi.org/cmfnmk

[5] Luvoni GC. Current progress on assisted reproduction in

dogs and cats: in vitro embryo production. Reprod. Nutr. Dev.

[Internet]. 2000; 40:505–512. doi: https://doi.org/bd9sqp

[6] Sánchez A; López L; Silva M; Berland M. Maduración in vitro de

ovocitos de gatas tratadas con hormona folículo estimulante

(FSH). Rev. Cientif. FCV–LUZ. 2006; 26(2):124–128.

[7] Goodrowe KL, Hay M, King W. Nuclear maturation of domestic cat

ovarian oocytes in vitro. Biol. Reprod. [Internet]. 1991; 45:466–

470. doi: https://doi.org/bhz65s

[8] Johnston L, Donoghue A, O´Brien S, Wildt D. Culture medium

and protein supplementation inuence in vitro fertilization

and embryo development in the domestic cat. J. Exp. Zool.

[Internet]. 1991; 257:350–359. doi: https://doi.org/bfpvkg

[9] Roth T, Swanson W, Wildt D. Development competence of

domestic cat embryos fertilized in vivo versus in vitro. Biol.

Reprod. [Internet]. 1994; 51:441–451. doi: https://doi.org/c9ss9b

[10] Prochowska S, Nizanski W, Partyka A, Kochan J, Młodawska W,

Nowak A, Skotnicki J, Grega T, Pałys M. The use of human and

bovine commercial media for oocyte maturation and embryo

development in the domestic cat (Felis catus). Reprod. Domest.

Anim. [Internet]. 2019; 54(4):719–726. doi: https://doi.org/kpcm

[11] Wlodarczyk R, Bukowska D, Jackowska M, Mucha S, Jaskowski

JM. In vitro maturation and degeneration of domestic cat oocytes

collected from ovaries stored at various temperatures. Vet. Med.

[Internet]. 2009; 54(10):491–497. doi: https://doi.org/kpcn

[12] Wolfe B, Wildt D. Development to blastocyst of domestic cat

oocytes matured and fertilized in vitro after prolonged cold

storage. J. Reprod. Fert. [Internet]. 1996; 106:135–141. doi:

https://doi.org/bb5g96

[13] Yildirim K, Vural MR, Küplülü S, Ozcan Z, Polat I.M. The effects of

EGF and IGF–1 on FSH–mediated in vitro maturation of domestic

cat oocytes derived from follicular and luteal stages. Reprod.

Biol. [Internet]. 2014; 14(2):122–127. doi: https://doi.org/f59bxx

[14] Sowińska N, Frankowska K, Filipczyk A, Adamaszek A, Nalik K,

Fic K, Pietsch–Fulbiszewska A. The effect of cumulus cells on

domestic cat (Felis catus) oocytes during in vitro maturation and

fertilization. Reprod. Domest. Anim. [Internet]. 2017; 52(Suppl

2):108–113. doi: https://doi.org/kpcq

[15] Martins LM, Fernandes CB, Villaverde A, Landim–Alveranga

FC, Lopes MD. The seasonal and ovarian status effects on in

vitro production of domestic cat embryos between Equator

and Tropic of Capricorn. Pesq. Vet. Bras. 2014; 34(3):277–280.

[16] Uchikura K, Nagano M, Hishinuma M. The effect of ovarian status

and follicular diameter on maturational ability of domestic cat

oocytes. J. Vet. Med. Sci. [Internet]. 2011; 73(5):561–566. doi:

https://doi.org/cjw2nz

[17] Feldman EC, Nelson RW, Reusch C, Scott–Moncrieff, JC. Canine and

Feline Endocrinology. 4th ed. Philadelphia: Saunders; 2014. 688 p.

[18] Johnston LA, O'brien SJ, Wildt DE. In vitro maturation and

fertilization of domestic cat follicular oocytes. Gamete Res.

[Internet]. 1989; 24(3):343–56. doi: https://doi.org/bhrqrg

[19] Karja N, Otoi T, Murakami M, Fahrudin M, Suzuki T. In vitro

maturation, fertilization and development of domestic cat

oocytes recovered from ovaries collected at three stages of the

reproductive cycle. Theriogenol. [Internet]. 2002; 57(9):2289–

2298. doi: https://doi.org/d2bzdr

[20] Naoi H, Agung B, Karja NW, Wongsrikeao P, Shimizu R, Taniguchi

M, Otoi T. Effects of the reproductive status on morphological

oocyte quality and developmental competence of oocytes after

in vitro fertilization and somatic cell nuclear transfer in cat.

Reprod. Domest. Anim. 2008; 43(2):157–161.

______________________________________________________________________Revista Cientifica, FCV-LUZ / Vol. XXXIII, rcfcv-e33212

5 of 5

[21] Schmidt PM. Feline breeding management. Vet. Clin. North Am.

Small Anim. Pract. [Internet]. 1986; 16(3):435–451. doi: https://

doi.org/bj54bs

[22] Hurni H. Daylength and breeding in the domestic cat. Lab. Anim.

[Internet]. 1981; 15(3):229–233. doi: https://doi.org/b739d7

[23] Hedlund CH. Surgery of the reproductive and genital systems.

In: Fossun TW, editor. Small Animal Surgery. 2nd ed. St Louis,

USA: Mosby. 2002. 122 p.

[24] Wood T, Wildt D. Effect of the quality of the cumulus–oocyte

complex in the domestic cat on the ability of oocytes to mature,

fertilize and develop into blastocysts in vitro. J. Reprod.

[Internet]. Fert. 1997; 110:355–360. doi: https://doi.org/dhfqw8

[25] Wood T, Montali R, Wildt D. Follicle–oocyte atresia and temporal

taphonomy in cold–stored domestic cat ovaries. Mol. Reprod.

Dev. [Internet]. 1997; 46:190–200. doi: https://doi.org/cgzcs6

[26] Freistedt P, Stojkovic M, Wolf E. Ecient in vitro production

of cat embryos in modied synthetic oviduct uid medium:

effects of season and ovarian status. Biol. Reprod. [Internet].

2001; 65(1):9–13. doi: https://doi.org/fnjjwk

[27] Brevini TA, Cillo F, Antonini S, Gandol F. Effects of endocrine

disrupters on the oocytes and embryos of farm animals. Reprod.

Dom. Anim. [Internet]. 2005; 40(4):291–299. doi: https://doi.

org/d69j7p

[28] Gao Y, Chen F, Kong Qq, Ning Sf, Yuan Hj, Lian Hy, Luo Mj, Tan Jh.

Stresses on female mice impair oocyte developmental potential:

effects of stress severity and duration on oocytes at the growing

follicle stage. Reprod. Sci. [Internet]. 2016; 23(9):1148–1157. doi:

https://doi.org/kpcw

[29] Argudo DE, Tenemaza MA, Merchán Sl, Balvoa JA, Méndez MS,

Soria ME, Galarza LR, Ayala LE, Hernández–Fonseca HJ, Perea

MS, Perea FP. Intraovarian inuence of bovine corpus luteum on

oocyte morphometry and developmental competence, embryo

production and cryotolerance. Theriogenol. [Internet]. 2020;

155:232–239. doi: https://doi.org/kpcx

[30] Gonzalez–Bulnes A, Berlinguer F, Cocero MJ, Garcia–Garcia RM,

Leoni G, Naitana S, Rosati I, Succu S., Veiga–Lopez A. Induction

of the presence of corpus luteum during superovulatory

treatments enhances in vivo and in vitro blastocysts output in

sheep. Theriogenol. [Internet]. 2005; 64:1392–1403. doi: https://

doi.org/fds7zc

[31] Cotterill M, Catt Sl, Picton HM. Characterisation of the cellular

and molecular responses of ovine oocytes and their supporting

somatic cells to pre–ovulatory levels of LH and FSH during in

vitro maturation. Reprod. [Internet]. 2012; 144(2):195–207. doi:

https://doi.org/kpcz

[32] Knight PG, Satchell L, Glister C. Intra–ovarian roles of activins and

inhibins. Mol. Cell Endocrinol. [Internet]. 2012; 359(1–2):53–65.

doi: https://doi.org/fpxg4x

[33] Richani D, Gilchrist RB. The epidermal growth factor network: role

in oocyte growth, maturation and developmental competence.

Hum. Reprod. Update. [Internet]. 2018; 24(1):1–14. doi: https://

doi.org/gczkxr

[34] Webb R, Garnsworthy PC, Campbell B, Hunter MG. Intra–ovarian

regulation of follicular development and oocyte competence in

farm animals. Theriogenol. [Internet]. 2007; 68 (Suppl.1):S22–29.

doi: https://doi.org/ctd9v8

[35] Fair T, Lonergan P. The role of progesterone in oocyte acquisition

of developmental competence. Reprod. Domest. Anim. [Internet].

2012; 47(Suppl 4):142–147. doi: https://doi.org/f36jgn

[36] Menchaca A, Cuadro F, Dos Santos–Neto Pc, Bosolasco D, Barrera

N, De Brun V, Crispo M. Oocyte developmental competence

is improved by relatively greater circulating progesterone

concentrations during preovulatory follicular growth. Anim.

Reprod. Sci. 2018; 195:321–328. doi: https://doi.org/gd2hgh

[37] Manjunatha BM, Gupta PS, Ravindra JP, Devaraj M, Ramesh HS,

Nandi S. In vitro developmental competence of buffalo oocytes

collected at various stages of the estrous cycle. Theriogenol.

2007; 68(6):882–88.

[38] Rosen MP, Shen S, Dobson AT, Rinaudo PF, Mcculloch CE,

Cedars MI. A quantitative assessment of follicle size on oocyte

developmental competence. Fertil. Steril. [Internet]. 2008;

90(3):684–690. doi: https://doi.org/bns4wz

[39] Ahmadi E, Nazari H, Hossini–Fahraji H. Low developmental

competence and high tolerance to thermal stress of ovine oocytes

in the warm compared with the cold season. Trop. Anim. Health

Prod. [Internet]. 2019; 51(6):1611–1618. doi: https://doi.org/kpc2

[40] Almeida FR, Mao J, Novak S, Cosgrove JR, Foxcroft GR. Effects

of different patterns of feed restriction and insulin treatment

during the luteal phase on reproductive, metabolic, and

endocrine parameters in cyclic gilts. J. Anim. Sci. [Internet].

2001; 79(1):200–212. doi: https://doi.org/kpc3

[41] Armstrong DT. Effects of maternal age on oocyte developmental

competence. Theriogenol. [Internet]. 2001; 55(6):1303–1322.

doi: https://doi.org/btrmzc

[42] Igosheva N, Abramov AY, Poston L, Eckert JJ, Fleming TP, Duchee

MR, Mcconnell J. Maternal diet–induced obesity alters mitochondrial

activity and redox status in mouse oocytes and zygotes. Plos One.

[Internet]. 2010; 5(4):e10074. doi: https://doi.org/c6pqw7

[43] Magata F, Shimizu T. Effect of lipopolysaccharide on

developmental competence of oocytes. Reprod. Toxicol.

[Internet]. 2017; 71:1–7. doi: https://doi.org/gbrqb4