Oocyte Aging: A Multifactorial Phenomenon in A Unique Cell

The oocyte is considered to be the largest cell in mammalian species. Women hoping to become pregnant face a ticking biological clock. This is becoming increasingly challenging as an increase in life expectancy is accompanied by the tendency to conceive at older ages. With advancing maternal age, the fertilized egg will exhibit lower quality and developmental competence, which contributes to increased chances of miscarriage due to several causes such as aneuploidy, oxidative stress, epigenetics, or metabolic disorders. In particular, heterochromatin in oocytes and with it, the DNA methylation landscape undergoes changes. Further, obesity is a well-known and ever-increasing global problem as it is associated with several metabolic disorders. More importantly, both obesity and aging negatively affect female reproduction. However, among women, there is immense variability in age-related decline of oocytes’ quantity, developmental competence, or quality. Herein, the relevance of obesity and DNA-methylation will be discussed as these aspects have a tremendous effect on female fertility, and it is a topic of continuous and widespread interest that has yet to be fully addressed for the mammalian oocyte.


Introduction
The oocyte is considered to be the largest cell in mammalian species, and very unique with regard to its lifespan since aging-related changes in ovaries are detectable very early in life [1].Women are born with a large pool of oocytes in primordial follicles, arrested in prophase of the first meiotic division (Fig. 1).Because oocytes are metabolically active, they experience the effects of chronic exposure to environmental influences.Due to attrition, ovulation, and apoptosis, the number of eggs decreases continuously throughout life, to approximately 300,000 at menarche.This number drops to nearly complete exhaustion by menopause.With important implications, women around the world increasingly postpone childbearing, leading to reduced fertility, more abortions, fetal abnormalities, and fewer children per family on average [2,3].In parallel, the utilization of in vitro fertilization (IVF) has increased, along with a significant economic burden on society.There is an obvious lack of research on how to improve fertility in older women and most IVF centers routinely refer women to third-party egg donation after ages 42-43 years [4].Therefore, novel biomarkers of ovarian aging and new intervention techniques, would be desirable and epigenetics could play a significant role in this process.Despite rapidly improving our knowledge about the aging methylome, we have yet to fully understand the underlying mechanisms that underpin age-related epigenetic alterations that constitute one of the primary hallmarks of aging [5].The methylation of cytosines (Fig. 1) has, for example, been well-investigated [6,7].5methyl cytosine (5mC) on promoters of genes almost invariably relate to transcriptional repression, in concert with other transcriptional silencing mechanisms such as the histone modifications.DNA methylation (DNAm) contributes to a multitude of biological processes, including regulation of gene expression, X-chromosome inactivation, and aging [7].As the methylome acts as one of the important interfaces between the genome and the environment, it also responds to environmental stimuli from lifestyle factors such as diet and smoking [4].The recent development of novel DNA methylation microarrays enabled the investigation of DNA methylation in different mammalian species and cell types and has opened the possibility of developing third generation (multi-species) epigenetic clocks, which can serve as powerful tools to measure biological aging [6,7].These methylation arrays can also be used for numerous purposes in reproductive medicine to advance the field and open new possibilities.Furthermore, obesity has been reported to be a risk factor for developing deficiencies [8,9].Decreased embryo quality and impaired folliculoand steroidogenesis are the main changes that occur in the female reproductive system as a result of obesity [10,11].There is no doubt that due to ethical and legal issues, and limited availability, research on human oocytes is restricted in numerous countries.Therefore, quite often an adequate animal model is needed.Both bovine and murine oocytes are an attractive animal model but the degree of similarity to human oocytes differs.For instance, the murine IVF system and embryo culture are frequently taken into consideration as a model for human IVF [12].With regard to DNA methylation, it is widely accepted that the oocyte undergoes re-and de-methylation during oocyte development.Noteworthy, there are two waves of genome-wide reprogramming in mammals, namely in germ cells and in preimplantation embryos.Interestingly, the step of epigenetic reprogramming in germline cells, including the egg cell, is essential for the phenomenon of imprinting [13].Noteworthy, the big hyper-and hypomethylated domains which are associated with transcription appear to be similar in human and murine eggs.However, there is a significant difference with regard to the methylated regions in human and murine egg cells, reflecting contrary transcriptome profiles.In addition, the maternal genome appears to be demethylated at a lower level in human blastocysts when compared to murine counterparts (Fig. 2), and the active DNA demethylation by TET enzymes is conserved but is less pronounced in human zygotes [14].Furthermore, it is well known that there are specific regulators which control global DNA methylation, histone modification, transposon elements, and the energy metabolism of the oocyte [15][16][17][18].
Therefore, in this Review, we aim to provide a summary of recent research related to maternal aging, obesity, and DNA methylation in regard to their impact on the mammalian oocytethe crucial female cell for procreation.

Epigenetic alterations as a hallmark of oocyte development and aging
The epigenome and specifically, the DNA methylome undergoes very significant changes with oocyte growth and development.DNA of primordial germ cells is highly methylated.When these cells enter the genital ridge, global DNA methylation decreases drastically, except for primary imprinted regions, which escape this process, and retain their DNA methylation state.During gametogenesis, at the time when oocytes are formed, de novo methylation of DNA occurs gradually with oocyte growth.This genome-wide demethylation and remethylation are defined as the first round of epigenetic reprogramming.The second round of such reprogramming occurs in the embryo after fertilization.DNA demethylation after fertilization occurs both actively and passively.Active demethylation is promoted by the ten-eleven translocation (TET) enzymes (Fig. 1) which catalyze the conversion of 5MC to 5hydroxmethylcytosine (5hMC).From the very early stage of development, methylation and demethylation of the DNA occur in very specific manner and locations.Depending on the specific chromatin context, some genomic loci gain heterochromatin and DNA methylation, and some heterochromatic regions lose their repressive marks with resulting de-repression of the locus [19].For example, CpGs located in polycomb repressor type 2 complex targets tend to gain methylation with age, -particularly in peripheral tissues [6].Strikingly, a recent study revealed that oocytes do not follow this pattern [20] suggesting a distinct epigenetic aging pattern in comparison to other organs.This may be related to the specific and specialized pattern of DNA methylation in oocytes.Interestingly, histone modifications dramatically change with age in oocytes.As demonstrated recently, mouse and human oocytes lose heterochromatin histone markers with age [19].This loss results in a massive activation of transposable elements and retrotransposons which result in DNA damage.Consistent with this, it has been demonstrated that inhibition of reverse-transcriptase activity or artificially increasing heterochromatin levels in aging oocytes abrogates DNA damage and improves oocyte in-vitro maturation efficiency when applied to aged oocytes [19].In addition, post-translational histone modifications (PTMs) modulate transcriptional activity [21] in the egg and, as part of their meiotic function, they are of importance for the processes of kinetochore formation and chromosome segregation [22].Noteworthy, changes in histone PTM patterns and DNA methylation are typical for oocyte oogenesis and maturation [23], and appear to be sensitive in response to stress, stimulation, and aging [22].A recent study provided evidence that the chromatin structure in postpubertal murine oocytes has fewer chromocenters than prepubertal counterparts, and heterochromatin marker values, such as H3K9me2, H3K27me3, or H4K20me1 increase significantly at the onset of puberty [22].In contrast to the latter-mentioned phenomenon, euchromatic markers behave in a different fashion, namely, H3K4me3 levels are elevated during puberty, whereas H3K27Ac shows lower values [22].Moreover, the same study revealed that the application of folliclestimulating hormone (FSH) to pre-pubertal oocytes for 24h impacts their chromatin structure to a post-pubertal configuration and elevates their histone methylation levels.In consequence, it appears that FSH plays a key role in chromatin regulation during the pubertal transition [22].In addition, H3K9me3 is linked to transcriptionally silent heterochromatin, and it has been shown that KDM4A alters the entire H3K9me3 landscape in mature eggs at sites occupied by bdH3K4me3, emphasizing the crucial role of KDM4A in maintaining the integrity of the maternal epigenome, which is a prerequisite for adequate zygotic genome activation and the transfer of developmental control to the embryo [24].It is worth mentioning that ribosomal DNA (rDNA) methylation seems to reflect functional changes in nucleolus biology during aging and aging-related pathologies [25], and aging-related rDNA methylation has been proposed as a universal predictor of age [26].A recent study provided evidence that there is an aging-related elevation of rDNA methylation levels in murine eggs generated from advanced-age mothers [27].In consequence, ovarian aging appears to be associated with increased values of rDNA methylation in meiotically arrested oocytes.However, eggs from the same woman can have different levels of rDNA methylation and, by extrapolation, different epigenetic age [27].The latter-mentioned fact contributes among others to the variability of oocytes' developmental competence even when generated from the same woman.As already mentioned in the Introduction, previous research provided evidence that transcriptional and epigenetic changes, particularly DNA methylation, appear to contribute to the deterioration in oocyte quality with regard to maternal age [28].With advancing maternal age, there is a chronic exposure of oocytes in the ovary to a changing environment, such as altered hormone levels and changes in energy and single-carbon metabolism, which affect gene expression and epigenetic processes, and in consequence, may contribute to lower viability of oocytes [29].The impact on the epigenetic quality of the oocyte is also important since it can potentially be inherited by the embryo, which is manifested in the later developmental outcomes of the offspring.Besides, one should keep in mind that gene expression in the oocyte is unique in that it contains many oocyte-specific transcripts that regulate pathways and functions not only in the oocyte itself but also during early embryonic development [30].This has been emphasized in a recent study [30], in which a diminished complexity and elevated variability in the transcriptome of eggs from older women have been described.The transcriptome heterogeneity allows the division of oocytes with an immature chromatin configuration transcriptome into two groups.The first group is composed of those oocytes with reduced developmental competence, which is indicated by lower expression of maternal effect genes, and the other group contains those oocytes with a juvenile transcriptome.The same study revealed that oocytes from older women had, on average, reduced CpG methylation, but the characteristic landscape of bimodal oocyte methylation was preserved [30].For most differentially expressed transcripts, the lack of related methylation changes suggests that most age-related effects on the transcriptome are on a post-transcriptional basis.Interestingly, the oocytes differed in the expression and methylation of genes, which may have contributed to the differential oocyte competence or penetrance of agerelated maternal phenotypes in the offspring [30].

An oocyte epigenetic estimator of chronological age
Researchers have taken advantage of age-related DNA methylation changes to develop epigenetic estimators of chronological age, known as epigenetic clocks.Epigenetic age, which is the quantitative prediction of such clocks appears to capture some elements of biological age [20].Epidemiological studies revealed that individuals with epigenetic ages that are older than their chronological ages have increased risks of various chronic diseases [31].The application of epigenetic clocks is not limited to humans but can be extended to different mammalian species [32,33].Recently, a universal mammalian methylation clock, based on highly conserved CpGs across mammals, was developed.This clock is able to estimate biological age of all mammalian species from DNA derived from different tissues and organs [6].Due to ethical restrictions for research on human eggs [1], bovine eggs are a good model to facilitate future studies into the epigenetic underpinnings of human female reproductive aging.It has been observed that germinal vesicle stage oocytes exhibit a slower rate of epigenetic aging, but surprisingly, they start with an older developmental epigenetic age than a non-germline tissue such as blood [20].This observation parallels our prior statement about a lack of methylation gain in the oocyte's promoter regions, shedding new light on the phenomenon of oocyte aging.Evidently, oocytes are somehow protected from the gain of methylation in the regulatory regions.This observation also matches the reported oocyte protection against mitochondrial DNA point mutations and differs from aging of somatic tissues [34].It thus appears that the epigenetic clock ticks differently in oocytes, even early in life, suggesting a rejuvenation event during early embryonic cleavage stages followed by aging, as shown in a recent study [35].In this study, zygotes were reported to be epigenetically older than cells from blastocysts (Fig. 1).With the help of these new insights into the epigenetic age of mammalian oocytes, researchers will hopefully be able to address several open questions regarding the nature of reproductive aging in women.A blood-based oocyte epigenetic clock can be a scalable measure to examine oocyte aging and identify genetic variants or environmental factors (e.g., lifestyle and diet) contributing to healthy and extended reproductive lifespans.Reproductive aging does not only have significant relevance for women's health but also profoundly affects society.Moreover, studies of reproductive aging may result in new knowledge about more fundamental pathways of aging involving epigenetic reprogramming, and genomic imprinting.To what extent epigenetic modifications in oocytes are driven by lifestyle changes, different environmental conditions, and the use of reproductive biotechnologies is important to understand.Interestingly, a recent mouse model provided evidence that the oocyte's methylome is robust and is not drastically altered by artificial reproductive techniques (ART) [36].To achieve breakthroughs, future studies of oocyte epigenetics should be directed toward epigenetic reprogramming and how oocytes are able to encode and store epigenetic information which has been set very early, even before birth.

Relevance of Stella, TET3, UHRF1 for DNA methylation and the oocyte
DNA methylation is not necessarily associated with oocyte developmental competence however, it is an essential factor for genomic imprinting [37], and disorders associated with abnormal methylation of given loci, cause disorders related to metabolism, placental and fetal growth [37].This regulation takes place at so-called imprinting control regions, where the higher methylation of given loci, the more strongly the inhibition of a given gene is expressed.Therefore, the proper methylome status is crucial for genomic imprinting [38,39].The DNA methyltransferase (DNMT) family, which consists of 6 pillars, is responsible for maintaining the proper methylome status of both specific imprinting control loci and other genes: DNMT1, DNMT2, DNMT3A, DNMT3B, DNMT3L, and the male-specific DNMT3C.Altogether, they are crucial for epigenetic regulation [40].DNMT3A and DNMT3B are known to be enzymes required for de novo methylation, but their knockout does not alter already established methylation patterns.DNMTL3 is known more as a cofactor for the previous two because it lacks active catalytic sites [41], but interestingly, it has a site on its C-terminal chain for DNMT3A and DNMT3B binding increasing its ability to bind chromatin in the oocyte which significantly improves their catalytic activity [42].In the female oocyte, the knockout of DNMT3A and DNMTL3 binding gene is associated with the loss of maternal phenotype and the failure of genomic imprinting [43].Another enzyme responsible for de novo methylation is DNMT3C, but its action is reduced to male lineage methylation of evolutionarily young retrotransposons [44].Moreover, mutation of this gene in mice can lead to diseases found in humans [45].DNMT's role in epigenetic regulation is crucial for maintaining methylome balance and thus proper oocyte growth at least up to the metaphase II stage [46].
The Stella protein, also known as Dppa3 and Pgc7, is highly expressed in primordial germ cells [16,47].Its main action is based on the specific control of global DNA demethylation enabling the epigenetic remodelling process immediately after fertilisation [48].While demethylation in the male pronuclei is almost instantaneous, this process is delayed in the female pronuclei of the zygote [18,49].Thus, a model of epigenetic asymmetry between the female and male pronuclei is drawn.The establishment of global hypomethylation occurs through the oxidation of 5methylcytosine (5-mc) to 5-hydroxymethylcytosine (5hmc) [17,50].This reaction is tightly controlled by the Stella protein by which an extended demethylation time is possible (Fig. 2) [16].Oocytes from mice fed on a highfat diet (HFD) have shown a strong signal for 5-mc, while the signal for 5-hmc was markedly reduced, suggesting a severe disruption of DNA demethylation [18].Some research reported that the conversion of 5-mc to 5-hmc is possible due to the binding of Stella to demethylated lysine 9 on histone H3 (H3K9me2) [51], which was not confirmed by other studies, indicating that H3K9me2 does not appear to be the main fraction interacting with Stella in delayed DNA demethylation.There is no doubt that adequate levels of maternal global DNA methylation are crucial for proper oocyte development and survival [52].In early embryos, transposable elements play a particular role by dynamically re-organising the arrangement of available chromatin [53].Given the critical role of the Stella protein for the oocyte, its deficiency in a HFD mouse model has led to hypomethylation of transposable elements [54].Interestingly, inducing overexpression of the Stella protein may prevent the above defects to some extent by inhibiting overaccumulation of 5-hmc, but some genomic loci did not respond to the increase in Stella activity [55].These data suggest that despite the important function of Stella in maintaining DNA methylation, there may be other factors contributing to global hypomethylation in oocytes of obese mothers.The TET3 dioxygenase is considered to be one of the critical control points catalysing the conversion of 5-mc to 5-hmc only in the male pronucleus (Fig. 3) [49].In addition to its catalytic function, TET enzymes play a key role in the expression of transposable elements as well as chimeric transcripts, both of which are important processes for the completion of zygotic genome activation (ZGA) [56].HFD-fed mouse oocytes showed increased levels of TET3, suggesting that reduced Stella expression in HFD oocytes contributes to the activation of pathways for TET3 leading to overly rapid demethylation of the transgenome [55].Additionally, after deletion of the gene encoding for TET3, a reduction in γ-H2AX was observed [55], which, in consequence, illustrates the extent of double-strand DNA damage in mouse oocytes [57].
Uhrf1 (ubiquitin-like, containing PHD and RING finger domains 1), also known as NP95 in mice and ICBP90 in humans, is a protein involved in DNA methylation.To maintain an appropriate level of DNA methylation, the interaction of UHRF1 protein with DNA methyltransferase 1 (DNMT1) takes place [15].It has been shown that the Stella protein can attenuate the action of UHRF1 protein thus indicating another pathway for the regulation of global DNA methylation in mouse oocytes [47].Recently, attempts have been made to understand the exact interaction between the Stella protein and UHRF1 protein.Interestingly, the knockout of the gene encoding for Stella resulted in a marked increase in global DNA methylation, where 22% of the CpG islands were hypermethylated, and the location of UHRF1 protein was detected almost exclusively in the nucleus [58].Such an increase in global DNA methylation may be due to occupying binding sites of inactive regions of the transgene by DNMT1 during oocyte maturation [58,59].In addition, there is another mechanism whereby the PHD-UHRF1 domain and the Stella protein compete for the same binding site on the Histone H3K9 tail, particularly the trimethylated one [47].Interestingly, it has been revealed that the Stella protein through a strong binding to the PHD-UHRF1 domain, displaces the lattermentioned complex from its binding site on H3K9me0-3, thus preventing DNA methylation [47].Ectopic overexpression of Stella has been shown to largely restore the normal state of global DNA methylation in oocytes [58].Stella protein deficiencies may also lead to severe consequences in the pre-implantation period (Fig. 2).Stella knockout led to a developmental interruption of two-cell embryos, and only 15% developed into blastocysts [58,60], which is consistent in another research [61].In summary, the before-mentioned results indicate that the absence of Stella leads to an excessive DNA methylated oocyte.Knowing the importance of the interaction between the Stella protein and UHRF1 protein in future studies will be worthwhile to highlight the state of global methylation regulated by UHRF1.For instance, by using a HFD mouse model, this could further elucidate the defective mechanisms of global DNA methylation regulated by Stella in obese mothers.

N6-methyladenosine:
An epitranscriptomic mRNA modification During oocyte development, mRNA undergoes continuous epigenetic modifications which enable normal embryonic growth and development [62].Through methylation of the relevant nucleobase pairs, tight control of gene expression is possible [62].The most abundant modification is the methylation of the sixth nitrogen at adenosine, which is transferred from the Sadenosylmethionine moiety of the RNA chain resulting in N6-methyladenosine (m6a) [63].This modification is enabled by a complex of methyltransferases known as 'writers', such as the METTL3/14 complex (Fig. 3) [64], and associated fractions including WTAP [65], KIA1429 [66], RBM15 [67], ZCH13 [68,69], and METTL16 [70].Excessive methylation is associated with excessive silencing of gene expression, so demethylases termed 'erasers' remain in close correlation with the methyltransferase complex [71].Prominent among these are the obesity-related protein (FTO) [72] and ALKBH5 (Fig. 3) [73,74].Recently described important regulatory sites of the m6a formation, are the YTH domaincontaining binding proteins [75], and the IGF2 mRNA binding protein subfamily [76].Interestingly, abnormalities in the expression of the METTL3 gene, the so-called m6a subunit, are associated with high fetal mortality and impaired oocyte development.Inactivation of the METTL3 gene leads to early embryonic lethality, with all embryos being lost in the METTL-cKO group and 232 being born in the F1 generation of the control group [77], confirming the previous studies [78].Interestingly, deletion of the METTL3 gene had no effect on the follicles of 6-week-old murine pups; however, a decreased number of follicles was observed when growing old [77].METTL3 has been reported to maintain high activity in terminal follicles, thus sustaining oocyte development by stabilizing functional maternal mRNA.Previous research provided evidence that there is an essential link between Intersectin1, which has a crucial function in microtubule formation and normal meiosis [79], and IGF2BP3, a cofactor that maintains levels of Itsn1 in terminal follicles.Interestingly, as the gene for METTL3 was knocked out, impaired meiotic maturation in oocytes was present, suggesting the disruption of the before-mentioned link between Itsn1 and IGF2BP3.Similar conclusions have been drawn by Zhang et al. [80], who reported high levels of double-stranded DNA breaks after METTL3 gene knockout.Among the components of the m6a heterodimer (Figure 3), KIA1429 has been identified as a maternal gene [81].Although its function remains elusive, previous studies have provided insight into its essential interaction in the deposition of m6a onto maternal mRNA during activation of the zygotic genome [82].Another important regulator of proper mRNA methylation is FTO [83].It is known to be a key control of early embryonic development and is essential for normal adipogenesis [84].A recent study by Wei et al. [85] reported the important role of FTO in maintaining proper methylation of chromatin-associated RNA in embryonic stem cells.The induced inactivation of the FTO gene revealed significant defects in oocytes with regard to the hypermethylation of RNA transcriptomes, particularly in the long interacting element 1 (LINE1), which is an important regulator of global chromatin availability in developing early embryos [86].Given that most mRNA modifications are regulated by m6a, this complex has attracted particular interest among researchers in recent years, since its critical role in embryonic development has been demonstrated.Previous research provided strong evidence that the m6a complex is a critical regulator of maternal mRNA expression and ovarian follicle growth [80,82].Deletions of key factors for normal mRNA methylation caused severe mRNA methylation disruption leading to oocyte growth inhibition, impaired oocyte development and the occurrence of early embryonic lethality [87].As obesity induces serious problems related to global DNA methylation of growing oocytes and pre-implantation embryos [18,55], future studies regarding obesity and its effects on the m6a complex may provide further insights into infertility problems in obese women.

Impact of obesity and metabolic changes on oocyte development
Nowadays, obesity among women is becoming a more and more serious problem globally [88].It is a wellknown fact that obesity significantly affects women's health leading among others to polycystic ovary syndrome, premature menopause, or impairment to maintain pregnancy [89].Besides, it leads to in-utero abnormalities of the developing fetus, leading to macrosomia, stillbirth, or intensive care of the newborn [88].Obesity negatively affects the microenvironment of ovarian follicles and the oocyte itself through energy deficiencies of the oocyte, or disorganization and misalignment of chromosomes [90][91][92].Obesity-related mechanisms by which the oocyte developmental competence is disrupted are for instance chronic inflammation, oxidative stress, or energy imbalances.
Triglyceride accumulation in adipocytes leads to their hypertrophy and consequent necrosis which stimulates macrophages and T lymphocytes to produce proinflammatory cytokines i.e., IL-1, IL-6, and TNF-alpha.Thus, latent chronic inflammation negatively affects all tissues of the body, including ovarian tissue and, consequently, oocytes [93].This is confirmed by a study by Nteeb et al. [94] who postulated that mice fed a highfat diet showed a high immune activity within the ovary which negatively affected its function.Remodeling of the intestinal microbiota leads to increased permeability for enterocytes, allowing the release of lipopolysaccharides into the bloodstream.Furthermore, the binding to toll-like receptor 4 induces a cascade leading to the activation of the pathway for NFκB phosphorylation p65 and another pathway for the synthesis of pro-inflammatory cytokines namely TNF-alpha and IL-6.In addition, this pathway leads to the activation of reactive oxygen species in the form of O2-, which are then catalyzed to hydrogen peroxide due to the action of superoxide dismutase [90].Together, these mechanisms act in a positive feedback loop, establishing a state of chronic inflammation that does not necessarily produce clinical symptoms, but significantly affects a number of body systems, including the female reproductive system.
Energy supply and balance for proper oocyte maturation and spindle assembly are of paramount importance.During oocyte development, the number of mitochondria can reach up to 160,000 [95] due to the fact that they are essential for the formation of the karyokinetic spindle, the polarization of chromosomes and the ejection of first and second polar bodies [96].Hence, mice fed a high-fat diet experience a number of structural changes in mitochondria manifesting as changes in energy availability and thus oocyte incompetence [97].In addition to structural changes, abnormalities in the expression of specific proteins for the maintenance of energy homeostasis in the oocyte have also been observed.Sirtuin 3 (SIRT3) is involved in maintaining constant energy levels in maturing oocytes, thereby preventing DNA damage through ROS accumulation [98].Superoxide dismutase 2 (SOD2) has been shown to be closely related to SIRT3, where its activation and reduction of ROS occurs through SIRT3-regulated deacetylation [99].In HFD-fed mice, there is a decrease in SIRT3 expression, and consequently what raises SOD2K68 acetylation levels contributes to ROS accumulation in the oocyte [100].In addition, chromosome misalignment and disorganization of the karyokinetic spindle with dysfunction of the SIRT3-SOD2 axis has been observed in HFD mice [101].An important regulator of oocyte and non-oocyte energy metabolism is the TIGAR gene, involved in DNA repair and upregulation of reactive oxygen species [102].
Previous research indicates that reduced expression of the TIGAR gene in an obesity mouse model led to similar negative effects of a high-fat diet [103].However, the aforementioned work focused on the effect of SIRT3 expression in HFD mice on in vitro cells, but Iljas et al., [104] indicated that mice lacking SIRT3 did not show abnormalities in spindle assembly or chromosome alignment.More interestingly, these parameters in HFDfed mice as above remained unchanged, and elevated ROS levels did not degrade ATP levels in the oocyte.To what extent these results can be extrapolated to human clinical practice and which exact relevance the described mechanisms could have in women needs to be elucidated.

Fibrosis and ER stress in the aged ovary and their impact on the oocyte
Fibrosis occurs in numerous aging-related diseases and as we grow older, it is known to cause increased rigidity in the heart, lungs, liver, and also ovary upon an excess accumulation of the extracellular matrix [105].Recent research provided strong evidence that the stiffness of the ovarian tissue seems to be important for follicular development, growth, and ovulation in advanced-age mothers [106].As a logical consequence, it appears that the older the mother the lower the chances for an adequate follicular expansion during maturation due to the restricted softness of the ovarian tissue, and the lower the chances that the follicle ruptures at ovulation.However, the molecular and cellular pathways that are responsible for ovarian fibrosis are still not widely investigated.Another important factor that prompted the interest of aging researchers and reproductive medicine is ER stress.The latter-mentioned stress leads to an accumulation of unfolded or misfolded proteins in the ER [107], and in consequence, results in the activation of a specific signal transduction cascade, which is also known as the unfolded protein response (UPR) [107].Noteworthy, ER stress is activated in oocytes, granulosa cells of growing follicles, and in pre-implantation embryos [107].ER stress seems to be also relevant to the pathogenesis of the polycystic ovarian syndrome (PCOS) [108][109][110].
The folding of secretory proteins is mainly processed by a crucial organelle, the endoplasmic reticulum.Once the latter-mentioned process is disturbed, upon for instance inflammation or oxidative stress, and unfolded or misfolded proteins are accumulated, the so-called ER stress takes place [111][112][113].The UPR that is activated during ER stress, consists of three branches: the doublestranded RNA-activated protein kinase-like ER kinase (PERK), the inositol-requiring enzyme 1 (IRE1), and the activating transcription factor 6 (ATF6) [114] (Fig. 1).In general, the pathway of UPR aims to correct imbalances of homeostasis and supports in a certain way the survival of cells by three essential processes: 1) attenuation of protein translation, 2) ER chaperones synthesis activation, and 3) ER-associated degradation (ERAD) factors are recruited [107] (Fig. 4).Though the activation of UPR is not always successful to reduce or eliminate ER stress, the pathway of programmed cell death is induced.It is known that activated ER stress induces apoptosis in granulosa cells and cumulus-oocyte-complexes what diminishes the egg´s developmental competence and fertilization chances.
Furthermore, ER stress influences steroidogenesis, and therefore, reduces follicular health and luteal function [107].Interestingly, a moderate degree of ER stress in granulosa-or cumulus cells appears to be beneficial for oocyte maturation [107].Noteworthy, previous studies provided strong evidence that in granulosa cells of advanced-age women there is an accumulation of so-called advanced glycation end products (AGE).In consequence, an increase of AGE in ovarian follicles of aged women appears to decrease the developmental competence of the egg by triggering inflammation in the surrounding microenvironment [115].Although it is known that ER stress is linked to the elevation of pro-inflammatory and profibrotic cytokines in granulosa cells [115,116], it is still elusive if and how ER stress is responsible for changes in the ovarian stroma during maternal aging [117][118][119].Per se, fibrosis can be characterized as a pathological state or mechanism upon an aberrant inflammatory injury, or an enormous accumulation of fibrous connective tissue occurring in numerous human organs while growing old.Moreover, excessive or progressive fibrosis might lead to severe tissue architecture destruction and even organ failure [105].Interestingly, an elevated collagen accumulation reflecting symptoms of aging-related stromal fibrosis has been shown both in human, post-menopausal ovaries [118,120] as well as in reproductively aged animals [117,118,121].Although in other organs the cause of fibrosis is well described, the pathways leading to ovarian fibrosis remain in some parts elusive.Furthermore, the question if there is a correlation between the aging-related fertility drop and changing ovarian architecture needs further elucidation.It appears likely that a chronic accumulation of collagen in the ovarian microenvironment with advancing maternal age restricts a proper ovulation process.There is a clear consensus about the fact that a physiologic ovulation process necessitates the remodeling of the extracellular matrix in such a way that the ruptured ovarian follicle releases adequately the oocyte to the fallopian tube.Therefore, there is no doubt that excessive collagen in the ovary-in other words, a high tissue stiffness, works like a barrier.Interestingly, fibrosis has been also characterized as a premetastatic niche for cancer metastasis in models for lung fibrosis, and fibrosis in the mammary gland [122,123].However, the reason why these metastases are attached to the ovary remains unknown.How the level of fibrosis in the ovary can be diminished will be discussed in the following section.where it is cleaved by site 1 protease (S1P) and site protease 2 (S2P).The cytosolically active fragment of ATF6 migrates to the cell nucleus and activates transcription of UPR target genes involved in ER protein folding homeostasis; (middle branch) PERK phosphorylates the α-subunit of eukaryotic translation initiation factor 2 (eIF2α).Some selective mRNAs, for example, ATF4 mRNA, are preferentially translated when eIF2α is phosphorylated; (right branch) RNase IRE1α is able to cleave ER-bound mRNA or miRNA upon degradation via IRE1-dependent regulated cleavage (RIDD), affecting protein folding charge, cellular metabolism, and inflammatory signaling pathways.The cytosolic domain ofIRE1α may also provide a scaffold for the recruitment of adapter proteins, such as members of the tumor necrosis factor receptor-associated factor (TRAF) family.In addition, IRE1α RNase combines mRNA from XBP1, which encodes a potent transcription factor that activates the expression of UPR target genes involved in ER proteostasis and cellular pathophysiology.Notably, unfolded or misfolded proteins that accumulate in the lumen of the ER can be degraded by proteasome-based ER-associated protein degradation (ERAD).

ER stress and fibrosis as therapeutic targets to extend ovarian lifespan
So far, anti-fibrotic compounds such as pirfenidone and nintedanib have been approved and used for the treatment of pulmonary diseases, to slow down the fibrosis progression [124,125].Previous studies showed that (O-[3-piperidino-2-hydroxy-1-propyl]-nicotinic amidoxime) BGP-15 improves the mitochondrial function in several disease models [126,127].Besides, metformin appears to reduce fibrosis in different pre-clinical studies via the AMPK-mediated pathway [128,129].Interestingly, in a very recent mouse model, it has been shown that both antifibrosis compounds pirfenidone and BGP-15 are able to reduce the level of fibrotic collagen, and restored ovulation rate in aged females when compared to untreated counterparts [106].The BGP-15 treatment did also elevate the levels of extracellular matrix remodeling enzymes such as matrix metalloproteinase Mmp13, indicating its possible role in the process of collagen removal [106].Moreover, in the same study, authors have shown that BGP-15 reverses mitochondrial dysfunction, oxidative damage, and ER stress in aged mice what in consequence, has also positive effects on the oocyte [106].The use of metformin has been shown to prevent ovarian fibrosis related to maternal aging [120].Interestingly, in the latter-mentioned study, the authors postulate that ovarian fibrosis seems to correlate with immune and stromal properties which are known as a tumorpermissive niche [120].As a logical consequence, these findings could help to answer the question of why metastases of other primary tumors are localized in the ovary.Noteworthy, probiotics also appear to have a positive effect when used to treat cystic fibrosis, and reduce ER stress, too [130][131][132].In conclusion, abovementioned compounds have a certain potential to extend the ovarian life span via the modulation of ER stress and fibrotic collagen.

Future research directions and conclusions
Novel research data raised the question of whether the modulation of epigenetic reprogramming, for instance with the help of gene therapy (or DNA methylation editing), could support tissue repair in the ovary and could therefore enable a partial reversal of the aging-related quality decline in oocytes.Interestingly, in a recent study in mice, researchers have postulated that a reduction of ovulation cycles minimizes the risk of oocyte aneuploidy in advanced-age mothers; in other words, keeps their oocytes young [133].Aberrant chromosome segregation, such as the before-mentioned aneuploidy, can lead to miscarriage or birth defects.The elucidation of novel pathways crucial for mammalian oocyte spindle assembly, particularly in eggs from donors of advanced reproductive age, could lead to the development of adequate medical interventions.Noteworthy, a high degree of aneuploidy in human oocytes is a major cause of pregnancy loss and infertility in women [134].Especially, defects in spindle assembly have been associated with high levels of aneuploidy in human eggs [135].However, the mechanisms that facilitate spindle assembly in human oocytes remain elusive.Spindle microtubule nucleation after nuclear envelope disintegration (NEBD) is significantly delayed in human oocytes compared to mitotic cells, and human oocyte chromosomes undergo rapid movement after NEBD and before spindle assembly begins [135].Moreover, it has been reported that an error-prone chromosome-mediated spindle assembly favors chromosome segregation defects in oocytes of women [136].Worth mentioning, previous research provided strong evidence that the possibility of aneuploidy increases by more than 50% in parallel to increasing maternal age both in human and mouse oocytes [137].With regard to the process of chromosome segregation, it is important to know that kinesins hydrolyze approximately 125 ATP molecules for each microtubule binding event [13].This clearly demonstrates the enormous need for a continuous high energy supply in the oocyte during the spindle assembly which is provided by mitochondrial oxidative phosphorylation (OXPHOS) [13].However, the latter-mentioned supply of ATP by mitochondria decreases with advancing maternal age [13], and it has been shown that oxidative stress was accompanied by a significant reduction in mitochondrial ATP production and oocyte spindle assembly impairment [138].Interestingly, the entire meiotic apparatus appears to be negatively affected by decreased mitochondrial potential (ΔΨm) levels such as during mitochondrial dysfunction [139].Using in vitro models of murine oocyte maturation, metformin has been reported to improve chromosomal segregation accuracy once oxidative stress and mitochondrial dysfunction were reduced upon treatment, [140].In recent years, various mechanisms have been described that play a role in age-related maternal aneuploidy, which has been reviewed elsewhere [141].
Interestingly, the production line theory states that the best oocytes are released from follicles first at relatively young reproductive ages, while those with diminished quality are ovulated at a more advanced age.Lowering the frequency of ovulations and protecting youthful epigenetic marks could represent a novel strategy to postpone the effects of aging upon oocytes.This gives hope of future interventions to counteract the negative effects of epigenetic aging in oocytes, specifically in IVF of reproductively aged patients.In conclusion, the power of epigenetics did lay a cornerstone for a new era of research and medicine and opened new possibilities to decipher the molecular codes of oocyte longevity.The constantly increasing number of people with associated metabolic diseases is a difficult challenge for clinicians.Maternal age, DNA methylation, and obesity are factors, which have a significant impact on female mammalian gamete and embryonic development.Importantly though, attention should be paid to genes and proteins involved in the regulation of epigenetic mechanisms and the oocyte's development including Stella, TET3, UHRF1, SIRT3 as well as m6a, and components of its complex.As it turns out, disorders related to the functioning of the aforementioned structures lead to impaired oogenesis, early embryonic development, and epigenetic reprogramming mechanisms in the embryo.Taken together, elucidating the molecular mechanisms which take place in the oocytes under the influence of aging, obesity, and DNA methylation will help to implement adequate interventions which are able to reduce the negative effects of the before-mentioned factors.Furthermore, in our Review, we aimed to connect the recent findings of these factors, which are mainly made in animal models, and emphasize their relevance for the mammalian egg.To what extent these findings are translational for the human egg needs further elucidation.However, the animal results could be a first hint to identify therapeutic targets to improve oocyte health.
Therefore, this commentary aimed to stimulate new interesting research projects to decipher the code of the oocyte's healthand life span.The above-mentioned effects of pirfenidone, BGP-15, and other substances in animal models of ovarian aging have to be treated with caution since the used concentrations are often very high compared to the physiological levels.Compounds, like for instance senolytics, that are targeting not only agingrelated fibrosis, but also mitochondrial dysfunction could be an interesting therapeutic strategy to maintain ovarian function in women with premature ovarian aging or metabolic disorders.Noteworthy, the use of senolytics in different trials or models for aging-related pathologies needs further elucidation, before these compounds could be safely used to prevent, delay or reverse the aging phenotype and related diseases.However, research on senolytics is rapidly advancing, and rigorous pre-clinical and translational experiments, also with regard to the ovary, should be performed.Since the birth of the world's first IVF baby born in 1978, there is still a big need to assess the long-term consequences of assisted reproductive technologies, particularly on age-related phenotypes, in children conceived with the help of these techniques.Especially, the two cornerstones such as excessive body weight and aging are common symptoms in infertile or subfertile women.This still leads to a dilemma for doctors and specialists in human reproductive medicine of whether to encourage weight loss first or to start infertility treatment immediately.Despite their well-known effects on fertility, studies evaluating the combined effect of women's age and body mass index (BMI) on cumulative live birth rates are still rare and conflicting.According to a very recent study, an intervention to induce weight loss in women prior to ART appears to be beneficial, particularly in women younger than 35 years with a BMI ≥ 25 kg/m 2 .Therefore, for clinical practice, an individualized strategy that takes into account maternal age, patient's weight, diet, and lifestyle may be the best course of action [142].

Figure 1 .
Figure 1.DNA methylation in human eggs with regards to aging.(A) Scheme showing the mechanism of methylation and demethylation of cytosine.(B) Scheme showing the consequences of advanced maternal age (especially in women at the age of 35 years and above) and how an accelerated and a deaccelerated aging process could impact the DNA-methylation age of oocytes.The oocytes in ovarian follicles are arrested in Prophase of the first meiotic division, and with advancing maternal age, more errors are likely after the resumption of meiosis what could lead to aneuploidies in the offspring (e.g., Trisomy 21/Down-Syndrome).Abbreviations: AMH=Anti-Muellerian Hormone, DNMT= DNA methyltransferase, TDG= Thymine DNA glycosylase, TET= ten-eleven translocation.

Figure 2 .
Figure 2. Scheme showing potential outcomes in case of maternal obesity and Stella insufficiency.

Figure 3 .
Figure 3. Scheme showing the working mechanism of the so-called writers and erasers.Writers are the MTTL3-14 complex, and the so-called erasers, are FTO and ALKBH5, which are necessary for the transfer of methyl groups between adenosine (A)and N6-methyladenosine (m6A).

Figure 4 .
Figure 4. Scheme showing the three pathways of unfolded protein response (UPR) during ER stress.The branches of the UPR are characterized by: (left branch) ATF6 passes from the lumen of the ER into the cytosol in the Golgi apparatus, where it is cleaved by site 1 protease (S1P) and site protease 2 (S2P).The cytosolically active fragment of ATF6 migrates to the cell nucleus and activates transcription of UPR target genes involved in ER protein folding homeostasis; (middle branch) PERK phosphorylates the α-subunit of eukaryotic translation initiation factor 2 (eIF2α).Some selective mRNAs, for example, ATF4 mRNA, are preferentially translated when eIF2α is phosphorylated; (right branch) RNase IRE1α is able to cleave ER-bound mRNA or miRNA upon degradation via IRE1-dependent regulated cleavage (RIDD), affecting protein folding charge, cellular metabolism, and inflammatory signaling pathways.The cytosolic domain ofIRE1α may also provide a scaffold for the recruitment of adapter proteins, such as members of the tumor necrosis factor receptor-associated factor (TRAF) family.In addition, IRE1α RNase combines mRNA from XBP1, which encodes a potent transcription factor that activates the expression of UPR target genes involved in ER proteostasis and cellular pathophysiology.Notably, unfolded or misfolded proteins that accumulate in the lumen of the ER can be degraded by proteasome-based ER-associated protein degradation (ERAD).