1 - 17: In utero Androgen Excess: A Developmental Commonality Preceding Polycystic Ovary Syndrome? Free

With a staggering 10–20% prevalence among premenopausal women, polycystic ovary syndrome (PCOS) is the most common endocrine and metabolic women’s health disorder [1]. Its diagnosis on the basis of Rotterdam criteria requires at least 2 of the following 3 parameters: high testosterone (T) levels or hirsutism, intermittent or absent menstrual cycles, and ultrasonography-visualized polycystic ovaries, excluding endocrine mimics such as congenital adrenal hyperplasia [1]. Luteinizing hormone (LH) hypersecretion commonly accompanies hyperandrogenism [4] likely due to T-diminished, estradiol (E₂) induction of neural progesterone receptors in the mediobasal hypothalamus [2, 3], resulting in diminished E₂-progesterone negative feedback regulation of gonadotropin-releasing hormone (GnRH) episodic release from the medial basal hypothalamus. Elevated ovarian granulosa cell anti-Müllerian hormone (AMH) production commonly accompanies polycystic ovary morphology and provides an accurate biomarker for increased numbers of growing follicles [5].

Clinical sequelae for PCOS can include acne, infertility, endometrial hyperplasia and malignancy, obesity, type 2 diabetes (T2D), sleep apnea, cardiovascular disease, mood disorders, and sexual dysfunction [1, 6, 7]. PCOS is thus a uniquely challenging, multi-faceted disorder with several phenotypes, in which progressive obesity enhances severity of phenotype, and diminishes the well-being and quality of life [8]. Overt signs and symptoms of PCOS usually manifest at puberty.

While complex, PCOS is highly heritable and familial, and hyperandrogenism is its most heritable trait [1]. Pathogenic mechanisms, however, have remained elusive, hindering progress toward a cure. In this regard, in utero findings of hyperandrogenic origins for PCOS-like traits in nonhuman primates [9, 10], provided a novel, single pathogenic origin for PCOS that mimicked PCOS phenotypic diversity in women (hence PCOS-like traits). Subsequent (androgen-induced) epigenetic mechanisms may provide an amplification mechanism [11], effectively reprogramming diverse genetic backgrounds into PCOS-like individuals [12]. Confirmatory findings soon followed in sheep [13], mice [14], and rats [15], expanding into molecular insight of developmental pathogenesis [16-18]. While acceptance of in utero hyperandrogenic origins for PCOS is not universal [19], accumulating supportive evidence from human studies provides increasing evidence for pathogenic onset for PCOS during fetal life [1, 12, 20]. This brief review focuses on the current understanding emerging from human and animal model studies concerning in utero androgen excess contributing to PCOS and its potential pathogenic mechanisms, with an emphasis on nonhuman primate findings.

During early-to-mid gestation, ∼40% of fetal girls experience elevated circulating concentrations of unbound, bioavailable, testosterone (T) levels in the fetal male range [21]. This is relevant to PCOS, since comparable circulating T excursions into the fetal male range generate PCOS-like traits in gestational T-exposed female rhesus monkeys [22] and sheep [23], revealing the life-long impact on females of in utero androgen excess. In short-gestation rodents, late gestation, and the immediate postpartum period, provide a comparable developmentally vulnerable period for females [12]. Perhaps not surprisingly, therefore, amniotic fluid from daughters of women with PCOS exhibit male-similar T levels in mid-gestation, exceeding levels in mid-gestation daughters of women without PCOS [24]. As mid-gestation amniotic fluid T originates from the fetus [25], elevated T levels suggest hyperandrogenism in fetal daughters of women with PCOS during a crucial, developmental window when female nonhuman primates and sheep are vulnerable to PCOS-like reprogramming [12, 16]. Approximately 50% of daughters born to PCOS women develop signs and symptoms of PCOS by adolescence [26], indicating the substantial risk for PCOS phenotype accompanying female in utero androgen excess in humans [12].

Pregnant women with PCOS retain hyperandrogenism throughout pregnancy [27], together with elevated AMH levels [28] and reduced placental aromatase expression [29]. Despite population differences [30], ∼40% of PCOS women experience gestational diabetes [31] and other pregnancy complications [32], with maternal diabetes predisposing offspring to metabolic dysfunction in later life through fetal hyperinsulinemia [33]. A recent mouse model suggests that increasing AMH levels in pregnancy (as seen in PCOS women) can promote both LH-mediated T excess and reduced placental aromatization of maternal androgens [28], thereby contributing to fetal hyperandrogenism in their daughters (Fig. 1), although such a mechanism in humans remains to be confirmed.

Post-natal consequences of in utero androgen excess are found as early as the newborn for women with PCOS. Infant daughters not only exhibit transient facial sebum [34], a biomarker of prior T exposure, but also demonstrate an elongated anogenital distance [35], a reliable biomarker for early-to-mid gestation androgen excess [36]. Newborn daughters of women with PCOS also exhibit elevated AMH levels indicative of increased numbers of ovarian antral follicles, a PCOS trait. In adulthood, women with PCOS retain an elongated anogenital distance ([37, 38], typical of in utero, T-exposed, PCOS-like female monkeys [36] and sheep [23]. A diminished or exaggerated 2D:4D finger length ratio is also associated with both in utero androgen excess and PCOS, in women [39], their prepubertal daughters [24] and adult, early-to-mid gestation, T-exposed PCOS-like monkeys [36], since similar T- and E₂-regulated genes control differentiation of gonads, hands, and feet. Prepubertal daughters of women with PCOS also excrete increased concentrations of dihydrotestosterone (DHT) metabolites in their urine compared to prepubertal girls of women without PCOS [40], indicating increased 5-alpha reductase activity, and perhaps amplified target tissue androgen action, well before the onset of PCOS signs and symptoms at puberty.

Mixed umbilical cord blood androgen levels from human female fetuses at term, however, have yielded inconsistent results in support of late gestation fetal hyperandrogenism in daughters of PCOS women, regardless of whether or not “gold standard” liquid chromatography-tandem mass spectrometry assays are employed. Increased T or androstenedione levels are reported in two studies [41, 42], equivalent levels in one [43], and diminished levels in a further two studies [29, 44]. Labor onset and duration, together with increasing term gestational age, however, diminish umbilical cord androgen levels and likely often confound understanding of late gestation female androgenic state from this measure [45]. Moreover, no sex differences remain between circulating T levels in male and female human fetuses by late gestation [21], suggesting term birth is inauspicious for exploration of developmental hyperandrogenism.

Family-based and extensive genome-wide association studies have yielded 17 replicated PCOS risk genes, regulating gonadotropin secretion (FSHB), gonadotropin action and ovarian function (LHCGR, FSHR, DENND1A, RAB5/SUOX, HMGA2, C9orf3, YAP1, TOX3, RAD50, FBN3), and various metabolic functions (THADA, GATA4/NEIL2, ERBB4, SUMO1P1, INSR,and KRR1) [46-48]. Of the genes regulating gonadotropin and ovarian function, a substantial number have been proposed as enabling ovarian hyperandrogenism [46, 49]. A recent alternative approach, employing rare gene variant association testing, followed by targeted resequencing of AMH in a replication cohort, identified an additional 17 PCOS-specific, rare coding and splice-site variants in AMH that diminish AMH signaling [49]. Ovarian hyperandrogenism is a potential outcome of reduced ovarian AMH inhibition of CYP17A1 expression [49]. While progress toward understanding gene variant-based PCOS heritability has clearly advanced, a heritability gap between low incidence of PCOS risk genes (∼10%) and the high heritability of PCOS (∼70%) [50], indicates a pressing need to identify (1) more PCOS risk genes, as each may confer a small degree of disease risk, (2) rare gene variants, as each may confer unduly large degrees of PCOS risk, and/or (3) epigenetic mechanisms altering a wide range of gene expression that confer considerable risk for PCOS. Current thinking embraces a combination of polygenic, epigenetic, and developmental contributions to PCOS pathogenesis that are ameliorated or exaggerated by lifestyle [1, 47].

T and its biopotent metabolites are highly effective regulators of DNA methylation during fetal development. They enable the majority of phenotypic sexual differentiation in multiple organ systems and tissues, including the brain [51]. Increased or decreased DNA methylation can diminish or enhance, respectively, mRNA transcription of inherited gene variants [52]. Different patterns and degrees of DNA methylation at any single gene locus, however, are specific to each organ system or cell type in each individual. Unlike GWAS, therefore, there is less certainty as to how genome-wide methylation studies generalize beyond an organ system or cell type. DNA is differentially methylated in a variety of organ systems in women with PCOS [53, 54]. Gene-targeted DNA methylation studies of LHCGR have reported its hypomethylation in blood cells and subcutaneous (SC) adipose of women with PCOS, concurrent with increased LHCGR mRNA expression in these tissues [55-57]. If comparable DNA hypomethylation of LHCGR occurs in PCOS ovarian theca cells, it would likely increase androgenic responses to LH pulses, causing or amplifying ovarian hyperandrogenism. GWMS and bioinformatic pathway analyses have identified clusters of differentially methylated genes in PCOS women that may alter a variety of cellular functions, including immune response pathways (including autoimmunity), ovarian steroidogenic and metabolic functions, and cancer-related pathways [56, 58, 59]. Notably, there are commonalties between identified PCOS risk genes and differentially methylated genes in PCOS women, including LHCGR, RAB5/SUOX, AMH/AMHR2, and INSR, suggesting convergence of molecular pathogenic mechanisms around the same critical genes. Do similar mechanistic insights emerge from animal models of in utero female hyperandrogenism?

To induce fetal male levels of T in fetal female rhesus monkeys, monkey dams require daily SC injections of 10–15 mg T propionate to generate circulating T levels equivalent to nighttime adult male levels of T (∼20 ng/mL). Such high maternal levels are needed to exceed the primate liver’s ability to produce sex hormone-binding globulin, rendering >90% of circulating T non-bioavailable, as well as the primate placenta’s capacity to aromatize, conjugate, and metabolize T, thus delivering a small fraction (1–2%) of dam T concentrations to a female monkey fetus [22], as determined by liquid chromatography-tandem mass spectrometry. Why start with such a challenging animal model? When PCOS-like traits are reliably replicated in a nonhuman primate with >90% of its genome shared with humans, and with highly similar neuroendocrine, reproductive, metabolic, developmental, aging, and behavioral attributes to humans [60], translational application is likely.

As illustrated in Table 1, T exposure in monkeys during early-to-mid gestation is more effective at inducing reproductive and metabolic PCOS-like signs and symptoms in female offspring than T exposure during late gestation, reinforcing the concept of a particularly vulnerable, mid-gestation developmental window for in utero T reprogramming of females in long gestation species. Mid-gestation excessive maternal weight gain and transient hyperglycemia, accompanied by fetal hyperglycemia, are all T-induced metabolic sequelae contributing potential additional reprogramming to exposed female fetuses [61]. As late gestation T exposure-induced PCOS-like traits demonstrate, however, a degree of fetal female monkey vulnerability to T reprogramming (and its gestational metabolic sequelae) remains beyond mid-gestation (Table 1). Increased incidence of gestational diabetes, as well as increased or diminished birthweight [54], accompanying PCOS gestations, closely emulates metabolic compromise of hyperandrogenic gestation in monkeys. Importantly, metabolically compromised gestation, alone, including obese monkeys and women [62], and women with T2D, is insufficient to cause PCOS. Increased T in utero, however, may reprogram female neurocircuitry controlling energy balance and increase vulnerability to in utero metabolic compromise [62].

Phenotypic manifestation of early-to-mid gestation T reprogramming of female monkeys begins with mid-gestation increase in fetal head size, followed in late gestation by hypolipidemia and fetal LH hypersecretion [22, 61]. LH hypersecretion persists into early infancy, accompanied by modest hyperandrogenism [22], reflecting precocious development of insensitive negative feedback regulation of GnRH/LH in the absence of mature ovarian hormone levels providing homeostatic constraint. While birthweight is normal, accompanying metabolic dysfunctions includes newborn hypoglycemia, accelerated infant weight gain and relative hyperinsulinemia related to defective pancreatic beta cell compensation for insulin sensitivity and excessive beta-to-alpha cell ratio in infant pancreatic islets [61, 63]. Increased fetal growth, neonatal hypoglycemia, and subsequent accelerated postnatal growth are typical of human pregnancies encountering excessive maternal weight gain and hyperglycemia [64], and such gestations greatly increase the risk of developing T2D in adulthood.

During adolescence, menarche is delayed by ∼6 months in both early-to-mid and late gestation T-exposed female monkeys [65], but such pubertal delay is absent when lower amounts of T are administered to monkey dams [66]. Subsequent onset of menstrual cycles in early-to-mid gestation T-exposed monkeys is accompanied by a prolonged succession of luteal insufficiency [65], demonstrating adolescent origins of ovulatory cycle dysfunction, an attribute of adolescent girls presenting with PCOS [54].

By their reproductive years, early-to-mid gestation T-exposed female monkeys become comprehensive counterparts of women with PCOS. Ovarian and adrenal hyperandrogenism co-occur with intermittent and absent menstrual cycles, as well as large, polyfollicular ovaries [9, 22]. Elevated LH levels are omnipresent, driven by increased hypothalamic GnRH pulse frequency and increased pituitary gonadotrope response to GnRH, both likely resulting from diminished sensitivity to E₂- and progesterone-mediated negative feedback regulation [67], all neuroendocrine traits found in women with PCOS [68, 69]. Oocyte developmental competence is compromised in these monkeys [70], and may reflect contributions from increased adiposity that accompanies diminished oocyte quality in women with PCOS [71]. Circulating AMH levels in T-exposed monkeys, however, do not exceed those of controls, and exhibit premature, aging-related decline [72]. While the absence of AMH excess is not typical of women with PCOS, PCOS women over 30 years of age demonstrate a steeper decline in circulating AMH levels than their non-PCOS counterparts [73]. Early-to-mid gestation T reprogramming of ovarian follicle granulosa cells may therefore be less pronounced than ovarian theca, stroma, or oocytes, and a maternal source of fetal hyperandrogenism, alone, may be insufficient to reprogram granulosa cell AMH hypersecretion or increased follicle number and proliferation.

Accompanying metabolic dysfunction is just as pronounced in adult T-exposed monkeys as in PCOS women, despite the monkeys’ non-obesogenic diet. Monkey visceral fat accumulation is increased (“metabolic obesity”), likely arising from PCOS-like hyperandrogenic adipogenic constraint, limiting SC adipocyte maturation and safe lipid storage [74]. Such pro-lipotoxic traits may contribute to hyperlipidemia-associated insulin resistance, impaired pancreatic beta cell compensation and compromised islet size [63] enabling increased progression to T2D [12]. Consistent with gestational origins of PCOS-like metabolic dysfunction, increased postnatal weight gain is associated with increased risk of PCOS in women [54], as well as T2D [64]. Interestingly, DNA methylation array analysis of visceral adipose identifies transforming growth factor beta signaling as the most significantly altered pathway in adult, T-exposed female monkeys [11], implicating an influential signaling pathway regulating adipocyte catabolism (brown or beige adipose) and adipocyte accumulation of lipid (white adipose) that potentially enables positive energy balance [75, 76] favoring weight gain.

When T treatment of female monkeys begins peri-pubertally (renewable SC capsules generating circulating total T levels of ∼1.5 ng/mL), and 50% are additionally switched to a “western-style diet” (T+WSD), age at first pregnancy is later, blood flow in the primary lobe of the placenta is diminished by early gestation, and these pregnant, T-treated females demonstrate glucose intolerance, hyperinsulinemia, and insulin resistance, while female fetuses harvested during late gestation exhibit increased abdominal circumference suggestive of fetal adiposity [77]. Fetal female concentrations of T and other reproduction-related hormones, as well as postnatal phenotypes, are yet to be reported for female offspring of these T-treated female monkeys.

Sexual dysfunction [7] and depression [78] can occur with PCOS in women. In this regard, and in addition to reproductive and metabolic dysfunction, early-to-mid gestation T-exposure reprograms (“organizes”) prepubertal and adult female behavior. T-exposed female monkeys exhibit increased male-typical infant vocalizations, diminished intimate social grooming of mothers and interest in infants, increased mounting of peers, and diminished, but not absent, engagement in female-typical sexual interactions with males [79], all independent of circulating sex hormone levels. Such behavioral reprogramming is difficult to reconcile with traditional female gender roles in human societies, potentially leading to sexual dysfunction and depression. Recent reports from in utero androgen excess rodent models clearly demonstrate anxiety-like behavior in female offspring accompanied by the upregulation of amygdala gene expression, including corticotropin-releasing hormone [80], an identical neural site and neuropeptide system implicated in the pathogenesis of anxious phenotype in monkeys and humans [81], leading to depression.

Non-primate models of in utero androgen excess emulate many of the reproductive and metabolic traits found in PCOS women and T-exposed monkeys (Table 1). With their relative ease of manipulation, these models have generated a plethora of incisive pharmacological and molecular manipulations that provide additional insight into pathogenic mechanisms engaged by in utero androgen excess (recently reviewed by [16-18]). Differential gestational timing or duration of T exposure in female sheep (Table 1), illustrate the skew in gestational vulnerability to PCOS-like reprogramming of both reproductive and metabolic traits reported in female monkeys, and suggest that longer durations of T exposure commencing before mid-gestation induce a more pronounced PCOS-like phenotype. By late gestation, following cessation of maternal early-to-late T administration, increased ovarian theca cell expression of CYP17A1 and increased release of androstenedione are already present [82]. Postnatally, however, circulating androgen levels in such T-exposed sheep are not elevated, but ovarian androgen receptor expression is increased suggesting “functional hyperandrogenism” within an androgen target organ [83]. Early-to-late DHT exposure, while recapitulating T reprogramming of reproductive traits and insulin resistance, does not disrupt maturation of regular ovarian cycles or ovarian morphology (Table 1), suggesting limits to androgen receptor-mediated PCOS-like reprogramming in sheep. Maternal co-administration of the androgen receptor antagonist, flutamide, along with T during early-to-late gestation prevents early puberty, and likely LH hypersecretion, as well as onset of ovulatory dysfunction, PCOS-like ovarian morphology, and ovarian steroidogenic abnormalities [84]. Gestational flutamide co-treatment, however, fails to prevent metabolic phenotype, including insulin resistance, adipogenic constraint, hyperlipidemia, and fatty liver [16], again demonstrating limits to androgen receptor-mediated, PCOS-like reprogramming. In this regard, flutamide treatment of adult female mice previously exposed to fetal T reverses their acyclicity [14], and in some PCOS women, improves fertility, menstrual cyclicity, and LH levels [85], as well as normalizing progesterone negative feedback regulation of episodic GnRH/LH release [69].

Gestational co-administration of the peroxisome proliferator-activated receptor gamma or NR1C3, a nuclear transcription factor crucial for adipocyte maturation, along with T during early-to-late gestation, prevents insulin resistance and early puberty onset, and likely LH hypersecretion, in T-exposed female lambs, but does not prevent adipogenic dysfunction, hyperlipidemia and fatty liver [16]. In this regard, it is interesting that treatment of late gestation DHT-exposed female offspring as adults with the insulin sensitizer, metformin, restores normal cyclicity, as well as normalizes androgen and LH levels. Taken together, these findings suggest that while reprogramming of a variety of PCOS-like reproductive traits involves androgen receptor and/or insulin-mediated actions, adipogenic and lipogenic traits may involve additional reprogramming, perhaps engaging estrogenic T metabolites.

Mouse models have predominantly used the non-aromatizable androgen, DHT, to induce late gestation in utero androgen excess and PCOS-like reprogramming (e.g., [14, 17, 18]). Late gestation DHT administered to female GnRH-green fluorescent protein (GFP)-transgenic mouse dams (derived from CBB6/F1 strain) produces PCOS-like female offspring exhibiting hyperandrogenism, intermittent/absent cycles, aberrant ovarian follicle morphology, LH hypersecretion derived from accelerated episodic GnRH release, fatty liver, and enlarged adipocytes, without accompanying increased adiposity and insulin resistance (Table 1). The elegant use of genetic manipulation to globally delete androgen receptor (ARKO) protects fetal female mice (>98% C57BL/6J strain) from fetal DHT-induced, PCOS-like reprogramming, including absence of intermittent/absent cycles, aberrant follicle morphology, and enlarged adipocytes [86]. The wild type mice from which ARKO females are derived, nevertheless, do not exhibit fetal DHT-induced hyperandrogenism or LH hypersecretion, possibly reflecting GnRH-GFP and ARKO mouse strain differences in fetal female susceptibility to DHT fetal reprogramming. Neural androgen receptor expression may be particularly crucial for DHT-mediated, PCOS-like reprogramming since selective deletion of neuronal androgen receptor expression, NeuroARKO, provides the best protection against peri-pubertal onset, DHT induction of PCOS-like traits [87]. NeuroARKO mice, however, have not yet been challenged with late gestation DHT to ascertain if absence of neuronal androgen receptor abrogates in utero PCOS-like reprogramming. With less resemblance to in utero androgen excess in sheep, androgen receptors of in utero DHT-exposed female mice may mediate the majority of PCOS-like reprogramming.

GnRH-GFP transgenic mice have also enabled neuro-immunohistochemical delineation of hypothalamic changes that may underlie PCOS-like reprogramming of GnRH release and its negative feedback regulation. Late gestation DHT increases anatomical and functional gamma-aminobutyric acid (GABA) neuronal connectivity to GnRH neurons, generating increased firing rate of GnRH neurons, as well as LH hypersecretion, related to diminished progesterone negative feedback regulation [14, 88]. Such enhanced GABA excitatory connectivity, originating at least in part from the hypothalamic arcuate nucleus, is established before puberty, when circulating androgen levels are low [88]. Since GABA, but not GnRH, neurons express detectable levels of progesterone, estrogen, and androgen receptors, aberrant GABA excitatory connectivity may mediate diminished progesterone (and E₂) negative feedback regulation demonstrated by in utero androgen excess female mice, and potentially rats, sheep and monkeys.

Unexpectedly, long-term administration of flutamide to adult, prenatally DHT-treated female mice normalizes neuronal connectivity between GABA and GnRH neurons, as well as circulating LH levels, negative feedback regulation of GnRH/LH, ovarian cyclicity and follicle morphology [88], suggesting that extant, extra-ovarian androgen excess is crucial to maintain neuronal reprogramming and its PCOS-like sequelae. Figure 2 illustrates hypothetical sites, implicated by animal models, for specific, androgen receptor-mediated, in utero programming of PCOS-like traits. The implication, emphasized by sheep and transgenic mouse studies, is that abrogation of androgen production and action in specific organ systems may effectively normalize PCOS traits.

Naturally occurring high levels of T confer athletic advantage in women [89] and accompany female behavioral dominance in some, but not all, nonhuman primates [90, 91]. About 15–25% of women in their reproductive years exhibit androgen excess, but most have PCOS [92]. Naturally occurring, hyperandrogenic (high T) female macaque monkeys emulate PCOS women in the co-occurrence of PCOS-like traits [93, 94]. In a multi-Primate Research Center study, adult female macaques with average BMI and in prime reproductive years were identified with high levels of T, 1SD above each population mean. Naturally occurring high T levels were observed in 3 separate laboratory populations of macaques. In the Wisconsin rhesus monkey population [94], PCOS-like traits of high T females exhibited generalized hyperandrogenism and increased steroidogenesis, including elevated circulating levels of unbound, “free” testosterone (unpublished results), hypersecretion of both LH and AMH, as well as uterine endometrial hyperplasia and infertility (Table 1). Intriguingly, a predominance of infertility and insulin resistance is found among high T monkeys with the most extreme elevations of T, 2SD above the monkey population mean (unpublished results), and equivalent to hyperandrogenic criteria required for peer-reviewed clinical studies of PCOS [95].

High T, in and of itself, may not impair either fertility or metabolic function. Subtle changes in anatomical biomarkers of prior T exposure suggest fetal origins for naturally hyperandrogenic female rhesus monkeys [94], analogous to findings in behaviorally dominant female Malagasy lemurs [91], a more ancient branch of nonhuman primates. Interestingly, mild-to-moderate PCOS-like phenotypes were typically those identified among naturally hyperandrogenic female monkeys, emulating PCOS phenotype prevalence in studies of women recruited from local populations, and not from clinical referrals (Table 2). The contrast of predominantly mild-to-moderate phenotypes in naturally occurring PCOS-like monkeys and PCOS women recruited from local human populations to the predominantly severe and classic phenotypes of early-to-mid gestation T-exposed monkeys and clinically referred PCOS women suggests commonality in PCOS phenotype may include duration or degree of gestational T exposure, age, and BMI (younger age and normal BMI with more mild-to-moderate phenotype). Naturally occurring PCOS-like phenotypes beyond humans certainly support increasing speculation of survival and reproductive advantages from hyperandrogenic, energy-conserving, insulin resistant, delayed fecundity, female phenotypes [1, 96].

Mounting evidence from human and animal studies repeatedly implicates appropriately timed in utero androgen excess, from either maternal and/or fetal sources, as high risk for PCOS emerging at adolescence. Figure 1 provides a diagrammatic representation of maternal and fetal sources of gestational androgen excess, taken together with relevant PCOS risk genes, may programme for ovarian androgen excess. Figure 2 illustrates hypothetical sites for female reprogramming mediated by androgen receptor, as identified by genetically manipulated mouse studies [17, 18]. Such a unified hypothetical model is compatible with postnatal androgen-activated reprogrammed functions, such that anti-androgens or androgen-diminishing consequences of weight loss interventions, including lifestyle, diet, bariatric surgery, and insulin-sensitizing treatments, ameliorate PCOS traits in adulthood. Increasing sophistication of bioinformatics to assess risk for functional outcome of genomic and epigenomic variants vulnerable to in utero androgen excess, hold promise for identification of PCOS risk in newborn, enabling early intervention.

We thank Suzanne M. Moenter, PhD, for her comments on an earlier draft of this manuscript.

This work was funded, in part, by NIH grants P50 HD028934 (PI: Marshall), P50 HD044405 (PI: Dunaif), and P50 HD071836 (PI: Stouffer).

The authors declare that they have no potential conflicts of interest to disclose.