Introduction
In vitro culture of cumulus-oocyte complexes (COCs) obtained from growing follicles has proven to be a significant technique for studying the processes that regulate the final maturation of mammalian oocytes. In various species, including humans, matured and fertilized oocytes cultured in vitro have successfully developed into healthy progenies. However, it is still observed that the developmental potential of in vitro matured oocytes is lower compared to those matured naturally within the body. Approximately 30–40% of in vitro matured oocytes in large animals can reach the blastocyst stage capable of supporting embryonic development [
1,
2]. In recent times, there have been reports from multiple groups about innovative modifications made to in vitro maturation (IVM) systems. These modifications involve manipulating the intracellular cyclic adenosine monophosphate (cAMP) concentration or adding hormone and growth factor supplements. It has been observed that these changes greatly enhance the developmental competence of cultured oocytes from mice, cattle, and pigs [
3‐
6].
Oocyte developmental competence refers to the ability of a fully grown oocyte to be fertilized, develop into an early preimplantation embryo, and support development until birth [
7]. The acquisition of complete oocyte developmental competence is a gradual process that occurs in stages alongside ovarian follicle growth during oogenesis [
8,
9]. Initially, the oocytes gain the capacity to reach metaphase II and undergo maturation. In the later stages of follicular development, the oocytes gain the ability to support early embryo development. As folliculogenesis progresses toward ovulation, the oocytes acquire full developmental competence, enabling them to support development until birth. The final phase of oogenesis is referred to as “oocyte capacitation” and involves structural changes in organelles within the oocyte itself, along with various molecular events. These changes not only occur within the oocyte but also affect the surrounding cumulus cells, allowing for a response to luteinizing hormone/ receptor (LH/LHR) signaling during ovulation [
10].
In large animal species and humans, the oocytes progressively mature in smaller or medium-sized antral follicles until they are fully developed a few days before ovulation [
11]. Consequently, the follicle’s diameter in adult cycling females and even prepubertal animals serves as a reliable measure of oocyte readiness to complete their maturation process and facilitate embryonic growth. Numerous studies in various animal species, including cows [
9,
12], sheep [
13], goats [
14], horses [
15], monkeys [
16] and humans [
17,
18] have reported a strong association between follicle size and the meiotic and developmental competence of oocytes. In relation to our model organism, the pig, a study by Töpfer et al. (2016) has also confirmed that oocytes isolated from follicles larger than four millimeters exhibit higher developmental competence [
19].
The achievement of oocyte developmental competence is dependent on several factors. The key molecular factors are the activation of the maturation-promoting factor (MPF) in the oocyte cytoplasm and the transition from the G2 phase to the M-phase of the cell cycle, both of which are associated with the resumption of oocyte meiosis [
20]. When investigating why meiotic failure occurs in growing porcine oocytes, it was found that small oocytes have three major problems compared to their larger counterparts: an inactive mitogen-activated protein kinase (MAPK) cascade, a lack of cyclin B synthesis, and insufficient levels of cdc2 kinase [
21,
22]. A study performed in pig oocytes found that inadequate presence of Cdc2 was the primary cause of meiotic failure [
21]. By introducing mRNA encoding c-Mos, which activates the MAPK cascade, cyclin B2 and Cdc2 into the oocyte, it was shown that overexpression of Cdc2 while suppressing the Wee1B kinase - responsible for MPF inactivation - resulted in smaller porcine oocytes (95–105 μm 0.4–1 mm follicle) achieving a GVBD rate of 70%, similar to full-size oocytes [
21].
The achievement of developmental competence is also influenced by cumulus cells because they have a key role in supporting and communicating with the oocyte [
23]. They are necessary for the development and maturation of the oocytes. They provide metabolic assistance to the oocyte by facilitating communication through gap junctions, ensuring an ample supply of ATP [
24]. It was shown that cumulus cells play a key role in maintaining adequate levels of ATP in the oocyte, which is essential for meiotic progression and developmental competence. In addition, the involvement of cumulus cells in regulating oocyte maturation is crucial. They generate different growth factors, including epidermal growth factor (EGF) and transforming growth factor-alpha (TGF-α), that stimulate oocyte maturation. By binding to receptors on the surface of the oocyte, these growth factors initiate internal signalling pathways that facilitate meiotic resumption and cytoplasmic maturation [
25]. The smooth progression of these processes is ensured by the presence of cumulus cells, which also regulate them through the transcriptomic activity of genes and miRNAs that are expressed differently [
26,
27].
A significant increase in maturation and developmental competence has been recently attained in fully gown pig oocytes cultured under in vitro conditions by supplementation of medium containing EGF, gonadotropins (FSH, LH) and three additional cytokines, leukemia inhibitory factor (LIF), insulin-like growth factor-1 (IGF-1), and fibroblast growth factor-2 (FGF-2) [
6,
28]. By using this enriched medium known as FLI medium, it becomes feasible to substitute undefined protein sources like fetal calf serum or follicular fluid with polyvinyl alcohol or bovine serum albumin without decreasing maturation competence [
29].
The goal of this research was to investigate if using FLI medium could enhance the maturity and developmental capability of immature growing pig oocytes obtained from small antral follicles. Various factors such as chromatin remodeling, activation of MAPK3/1, resumption and completion of meiosis, and ability to develop into blastocysts after parthenogenetic activation were evaluated in both growing and fully grown oocytes cultured in control and FLI medium.
Materials and methods
All the procedures with animals were performed according to good veterinary practice for animal welfare according to the relevant Czech laws (No. 246/1992 and 419/2012). All materials were purchased from Thermo Fisher Scientific (Waltham, MA, USA) unless otherwise stated. All chemicals were purchased from Merck (Kenilworth, NJ, USA) unless otherwise stated.
Collection and culture of cumulus-oocyte complexes
Porcine ovaries of prepubertal gilts, 6–8 months old and 90–120 kg in weight, were collected at a local abattoir as a waste material and transported to the laboratory in a thermo-flask at 38 °C. The contents of small (1–2 mm in diameter) and medium-size antral follicles (3–6 mm in diameter) were aspirated with a syringe connected to a 20 G needle, pooled in a test tube, and allowed to sediment for 10 min. The sediment was washed twice with HEPES buffered porcine X medium (PXM-Hepes) [
30], placed in a Petri dish, and the COCs were collected with a pipette. Only COCs surrounded by a compact multi-layered cumulus were selected for experiments. Groups of 50 COCs were cultured for 44 h in four-well dishes (Nunclon, Roskilde, Denmark) in 0.5 ml of culture medium at 38.5 °C in a humidified atmosphere of 5% CO
2. The diameter of some COCs and denuded oocytes isolated from small and medium follicles was measured by Axiocam 208 camera using Zen 3.6 software (Zeiss).
The COCs were cultured either in a control M199 or modified FLI medium [
5]. The composition of the control and FLI medium is given in Table
1.
Table 1
The composition of the control and FLI medium
TCM199 | Sigma, M7528 | TCM199 | TCM199 |
Sodium pyruvate | Sigma, P4562 | 0.2 mM | 0.2 mM |
L-glutamin | Sigma, G8540 | 6.85 mM | 6.85 mM |
Cysteine | Sigma, C7352 | 0.57 mM | 0.57 mM |
Gentamycin | Roth, 0233 | 50 µg/ml | 50 µg/ml |
BSA | Sigma, A7030 | 1 mg/ml | 1 mg/ml |
PMSG | Prospec1, HOR-272 | 10 IU/ml | 10 IU/ml |
hCG | Prospec1, HOR-250 | 10 IU/ml | 10 IU/ml |
EGF | PeproTech2,AF-100-15 | 10 ng/ml | 10 ng/ml |
human LIF | Merck, LIF1005 | − | 2 µl/ml |
human IGF1 | PeproTech, AF-100-11 | − | 20 ng/ml |
human FGF2 | Sigma, F0291 | − | 40 ng/ml |
Assessment of oocyte maturation
To assess their nuclear maturation, oocytes after 44 h of cultivation were stripped of cumulus cells by vortexing. The degenerated oocytes (< 5%) were excluded from the evaluation and the remaining ones were mounted on slides and fixed in an acetic acid-ethanol solution (1:3) for 48 h. Oocytes were then stained with 1% orcein and observed with a light microscope. To confirm the achievement of metaphase II, we focused on determining chromosomes in the equatorial plane and excluded the polar body.
Parthenogenetic activation and culture of embryos
For parthenogenetic activation, cumulus cells were removed from COCs by pipetting and washed twice in PXM-HEPES. Oocytes with recognized polar body were activated by exposure to 10 µM ionomycin in PXM-HEPES for 5 min. After that, they were washed twice in porcine zygote medium 3 (PZM 3) [
31] supplemented with 2 mM 6-DMAP and cultured for 5 h at 38.5 ˚C under a 5% CO
2 atmosphere. Around 50 putative parthenotes were washed twice in PZM 3 and cultured for 6 days in 4-well dishes in 1 ml of PZM 3 medium at 38.5˚C under a 5% CO
2 atmosphere. After 40 h, the cleavage of embryos was assessed and after 144 h, the ability of embryos to reach the blastocyst stage was analyzed.
Immunochemistry
The denuded oocytes collected right after isolation from follicles or after 16, 24, 44 h of maturation were fixed in 4% paraformaldehyde for 40 min at room temperature. Fixed oocytes were processed immediately or stored in PBS supplemented with 2% BSA (PBS/BSA) at 4 °C. After washing in PBS/BSA, oocytes were permeabilized and blocked with PBS supplemented with 0.5% TritonX-100 and 2% BSA for 90 min at room temperature. All subsequent steps were done in PBS/BSA. Oocytes were incubated with mouse anti-lamin antibody (Sigma-Aldrich SAB4200236, St. Louis, MO), diluted 1:100 in PBS/BSA, overnight at 4 °C. After washing twice in PBS/BSA for 30 min at room temperature, oocytes were incubated with secondary goat anti-mouse antibody conjugated with Alexa Fluor 594, diluted 1:350 (Invitrogen, Eugene, OR) in PBS/BSA for 2 h at room temperature in the dark. After washing, the DNA of the nuclei was stained and the oocytes were mounted in Vectashield Vibrance Antifade Mounting Medium with DAPI (4’, 6-Diamidine-2’-phenylindole dihydrochloride, Vector Laboratories, Peterborough, UK). Controls of immunostaining specificity were carried out by omitting the primary antibody. The samples were examined using Leica TCS SP5 (Leica Microsystems AG, Wetzlar, Germany) and the images were processed using Image J software (National Institute of Mental Health, Bethesda, MD, USA).
Immunoblotting
At the selected culture time (GV – 0 h, MI – 28 h, MII – 42 h) groups of 50 denuded oocytes were washed in PBS and solubilized in Laemmli buffer containing 2% sodium dodecyl sulfate (SDS) and 5% 2-mercaptoethanol. Samples were boiled at 100 °C for 3 min and stored frozen at − 20 °C. Subsequently, proteins were separated in 10% acrylamide/SDS gels and transferred to Immobilon-P membranes (Millipore, Bedford, MA, USA). Membranes were blocked in 5% low-fat dry milk in Tris-buffered saline (TBS) with 0.5% Tween 20 for 2 h at room temperature, and then incubated with a primary antibody diluted 1:1000 in 2.5% BSA in TBS-Tween, at 4 °C overnight. The primary antibodies were p-ERK and ERK1 (detecting MAPK3/1), both from Santa Cruz Biotechnology (Santa Cruz, CA, USA). The secondary antibodies (Amersham ECL anti-mouse or anti-rabbit IgG, GE Healthcare, Little Chalfont, UK) were diluted 1:5000 in 2.5% BSA in TBS-Tween. The membranes were incubated with the secondary antibody for 1 h at room temperature and then washed intensively in TBS-Tween. The immune reaction was detected by enhanced chemiluminescence (Pierce, Rockford, IL, USA) according to the manufacturer’s instructions. The intensity of the specific bands on the blots was analyzed by scanning densitometry using the free software Image J Version 1.29 (National Institute of Mental Health, Bethesda MD, USA).
Expression analysis of cumulus cells genes related to oocyte quality RT-qPCR
For our experiments, we utilized the cumulus cells of mature oocytes from individual experimental groups. We collected cumulus cells from 20 oocytes, washed them three times in PBS, and then froze them at -80 °C using buffer from the Ambion RNAqueous-Micro Kit (Thermo Fisher Scientific, Waltham, MA, USA). A group of predicted target genes related to oocyte development and cumulus cells expansion was selected and analyzed in the different experimental groups. Primers for the selected target and quality-related genes were designed using the software Beacon Designer v. 8.21 and listed in Table
2. The one-step RT-qPCR was conducted in a RotorGene 3000 cycler (Corbett Research, Mortlake, Austria) using the QIAGEN OneStep RT-PCR Kit (Qiagen, Germany) in a 20 µl reaction mixture containing 4 µl 5 X reaction buffer, 0.8 µl dNTP mix (10 nM stock), 0.4 µl forward and reverse primers (20 nM stock), 0.125 µl RNasin (20 IU/ml stock, Promega), 0.8 µl enzyme mix, 0.8 µl EvaGreen (Biotium, CA, USA), 3 µl RNA, and nuclease-free water. The reaction conditions were as follows: reverse transcription at 50 °C for 30 min., initial denaturation at 95 °C for 15 min, followed by PCR cycles consisting of denaturation at 94 °C for 15 s, annealing at a temperature specific for each set of primers (Table
2) for 15 s and extension at 72 °C for 20 s; and a final extension at 72 °C for 5 min. Fluorescence data were acquired at the end of each extension step. Products were verified by melting analysis and gel electrophoresis on 1.5% agarose gel with MidoriGreen Direct (Nippon Genetics, Dueren, Germany). Comparative analysis software (Corbett Research) was used for gene expression analyses after normalization to the geometric mean of
YWHAG and
TBP as internal control genes for cumulus cells.
Table 2
List of primers used for real-time RT-PCR
AKT1 | TAC TCC TTC CAG ACC CAC GA CGG AGT GCA GGT AGT CCA AG | 157 | 53 | NM_001159776.1 |
ATP6 | AAT TCC TAT GCT CGT AAT ATG TTG AGT AGT GCT AAT | 141 | 27 | NC_000845 |
CCND2 | CAG TGC TCC TAC TTC AAG ACC TCT TCT TCA CAC TTC | 116 | 58 | NM_214088.1 |
HAS2 | GAA GTC ATG GGC AGG GAC AAT TC TGG CAG GCC CTT TCT ATG TTA | 407 | 54 | NM_214053.1 |
PCNA | TAA TGC AGA CAC CTT GGC ACT GCA AAT TCA CCA GAA GGC ATC | 153 | 55 | NM_001291925.1 |
TBP | ATA GCC TTC CAC CTT ACG CTC ATA GGC TGT GGA GTC AGT CCT | 115 | 58 | XM_021085483.1 |
YWHAG | CAG CCC ACT CAC CCC ATT AG TGC TGA TCG CTT GTC CAG AG | 218 | 58 | XM_005661962.3 |
Statistical analysis
Each experiment was performed in at least three replicates. Oocyte and COC diameter, meiotic competence and the development of embryos, and intensity of the specific bands on immunoblots were analyzed by one-way ANOVA with Holm-Sidak’s post-test (SigmaPlot 12.0, London, UK). The differences in chromatin remodeling between SO and LO were compared by student t-test. Error bars indicate the standard error of the mean (SEM). Probability values < 0.05 were considered to be statistically significant.
Discussion
Most of the oocytes that can be collected from the ovaries of large animals in slaughterhouses by aspiration or dissection are located in small follicles. These oocytes are still growing and have chromatin in a diffuse or partially condensed state, resulting in limited abilities for meiosis and development. Various approaches have been proposed to address this problem and increase oocyte growth potential specifically in preovulatory oocytes cultured in vitro. One approach to improve or maintain communication between cumulus and granulosa cells with the oocyte is to modify the function of gap junctions. By adding cAMP to the culture medium, gap junctional communication between oocytes and cumulus cells can be prolonged, leading to improved meiotic competence in bovine and porcine oocyte cultures [
32,
33]. The addition of factors that are produced in growing ovarian follicles by oocytes or granulosa cells to the culture medium holds promise as a relatively simple method to increase oocyte competence. For example, the combination of amphiregulin (AREG) with cAMP, bone morphogenetic protein 15 (BMP15) and growth differentiation factor 9 (GDF9) resulted in improved oocyte maturation and blastocyst formation in low-competent porcine oocytes obtained from small follicles [
34]. Similarly, the developmental competence of ovine oocytes was increased when C-type natriuretic peptide was combined with AREG and prostaglandin E2 [
13]. After analyzing this information, we hypothesized that the presence of additional growth factors during follicular development, which has been shown to increase the efficiency of fully mature oocytes, may also support the meiotic and developmental capabilities of developing oocytes in in vitro culture. Findings from our research indicate that introducing a combination of FGF2, IGF1, and LIF into the culture medium significantly increases the meiotic and developmental potential of growing porcine oocytes, rivaling fully-grown oocytes.
To our knowledge, this is the initial report suggesting that this combination of growth factors can improve the developmental capacity of growing mammalian oocytes during the in vitro maturation period. Studies to date have shown that FGF2, IGF1, LIF and similar growth factors increase the maturity and developmental potential of fully developed mammalian oocytes. Specifically, it has been well established that epidermal growth factor or EGF-like factors promote both maturation and developmental competence in various animal species, including pigs, cattle, sheep, horses, cats, dogs, rodents, monkeys, as well as human oocytes [
4]. Barros et al. found that the addition of FGF2 to the culture medium resulted in improved nuclear maturation, higher cumulus cell survival and increased extracellular matrix quality in bovine COCs [
35]. The addition of IGF1 has been shown to increase oocyte maturation, leading to improved embryo development and blastocyst formation [
36‐
38]. LIF supplementation in the medium was also found to increase the nuclear maturation of porcine and bovine oocytes as well as blastocyst development [
39‐
41]. The use of FLI medium, consisting of FGF2, LIF and IGF1, allows the elimination of unspecified protein sources such as fetal calf serum or follicular fluid. Instead, they can be replaced with polyvinyl alcohol or bovine serum albumin (BSA), all while maintaining the ability to ripen. Interestingly, this modification in the culture medium significantly increases the quality of porcine oocytes to a level comparable to those that mature naturally in vivo [
6,
28,
42]. We show that this relatively simple approach to promote oocyte competence may increase the efficacy of various biotechnological and medical applications, especially in species such as large animals or humans, where the number of fully-grown oocytes available is limited for physiological, medical or ethical reasons.
The mechanisms of growth-factor enhanced oocyte competence have not been completely elucidated up to now. It appears that an important role in the growth factor/cytokine-promoted oocyte competence play protein kinases such as MAPK3/1 and AKT which regulate proliferation, survival, and gene expression in oocyte surrounding cumulus cells, the function of gap junction between oocyte and cumulus cells as well as translation of specific proteins in oocytes [
5,
43,
44]. All these functions are closely related to the establishment of oocyte developmental competence.
Various changes in oocyte morphology and function are associated with the acquisition of meiotic competence at the final stage of oocyte growth. These changes include various aspects such as cytoplasmic organelles, nuclear membrane, cytoskeletal organization, gap junction communication, metabolism, chromatin remodeling, nuclear compaction and silencing of transcriptional activity at a global level [
45‐
47]. The maturation and readiness of oocytes in all mammalian species are associated with the transformation of their chromatin pattern. This involves a shift from a dispersed nucleolus to a compact nucleolus that is surrounded by chromatin. Oocytes that are ready for final maturation, fertilization, and early embryonic cleavage are characterized by condensed chromatin and cessation of transcriptional activity. At a specific developmental stage unique to each species, transcriptional activity resumes. In vivo, oocytes can remain in this state for several days until they are selected for final maturation or undergo atresia along with the destruction of the entire follicle [
11]. Several studies confirmed this correlation [
48‐
50]. According to several studies, it has been suggested that the transcriptional activity in the nucleus of oocytes gradually decreases as chromatin condenses, eventually stopping completely when oocytes reach full maturity [
47,
51,
52]. However, recent techniques such as RNA-seq have revealed that fully grown oocytes exhibit transcriptional activity during meiotic maturation [
49,
53,
54].
In pigs, the majority of oocytes extracted from 1 to 2 mm follicles showed an NSN (non-surrounded nucleolus) configuration for their chromatin (approximately 50%). Approximately 30% of these oocytes had partially condensed chromatin, while 10% were categorized as SN (surrounded nucleolus). The remaining oocytes were considered defective due to premature chromatin condensation (GV0). Based on a study conducted by Pan et al. in TCM199 medium containing FSH, LH, and EGF, only half of these oocytes were able to successfully mature to the MII stage-consistent with our findings. However, our research shows that by using FLI medium growth factors/cytokines, we can reverse the abnormal chromatin condensation in growing oocytes and facilitate a smooth transition to the MI stage.
Small oocytes obtained from porcine small follicles were found to lack the ability to activate cdc2 and MAPK, as well as to phosphorylate ribosomal S6 kinase (RSK), a downstream target of MAPK. Consequently, these oocytes were unable to resume meiosis when cultured in vitro [
21,
22]. Thus, we hypothesized that the limited rate of maturation observed in small oocytes cultured with the control medium compared to FLI could be attributed to the absence of MAPK activation. However, the findings of our experiment clearly showed that this assumption was incorrect, as small oocytes activated MAPK regardless of the type of medium used. The reason for this discrepancy with previous data is probably the different origin of the considered small oocytes. In previous research, small non-viable oocytes were separated from follicles between 0.5 and 1.5 mm [
22] or 0.4 and 1 mm in size [
21]. However, in our study we extracted small oocytes from follicles measuring 1 to 2 mm, resulting in oocytes with a significantly larger diameter of approximately 113 μm compared to the range of 95–105 μm found previously [
21].
Oocyte development and maturation are influenced by the important role played by the cumulus cells. These specific cells encapsulate the oocyte and offer crucial support and nourishment during the folliculogenesis. Gene expression in cumulus cells of oocytes matured using FLI medium was significantly higher compared to those matured using the control medium. A substantial increase in gene expression was observed in a group of oocytes obtained from small follicles in comparison to large follicles that underwent maturation in FLI medium, indicating an increase in their developmental competence. The role of AKT1 expression in FLI groups is crucial for several important cellular processes such as proliferation, metabolism, cell differentiation and survival [
55].
Research has revealed that activation of AKT1 promotes the expansion of cumulus cells by controlling the expression of hyaluronan synthase 2 (HAS2), an enzyme involved in the synthesis of hyaluronic acid. HAS2 overexpression and cumulus expansion lead to improved oocyte quality and increased fertilization rate [
25]. In addition, overexpression of HAS2 in cumulus cells of human oocytes led to better quality embryos [
56,
57].
The AKT1 has also been found to regulate the expression of proliferating cell nuclear antigen, a marker indicating cumulus cell proliferation [
58]. The active proliferative state of cumulus cells, crucial for oocyte development and support, is demonstrated by increased expression of PCNA. The upregulation of PCNA may be influenced to some extent by the activation of AKT1, as previously explained. Interestingly, recent research has shown that CCND2 expression can be found in the cumulus cells of fully developed oocytes [
59]. This discovery suggests a potential involvement of CCND2 in the control of cumulus cell progression and growth during the cell cycle. Further studies are needed to better understand the exact roles of CCND2 in cumulus cells and its effect on oocyte maturation. ATP6 is part of the mitochondrial ATP synthase complex, which plays a key role in ATP production. Although its exact function in cumulus cells remains unclear, recent studies suggest its potential involvement in energy metabolism. Overexpression of ATP6 in cumulus cells was associated with improved oocyte developmental potential. Higher levels of ATP6 in COCs are associated with increased oocyte quality and their capacity for fertilization and subsequent embryonic development [
60]. Our results align with these findings. We observed increased expression of these specific genes in oocytes matured in FLI medium, particularly SF FLI group. This highlights the impact of cumulus cells and maturation medium on oocyte developmental competence.
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