{"paper_id":"8a9c324a-71f6-4b50-ae75-9ec58a28bf40","body_text":"MicroRNAs (miRNAs) are single-stranded RNA molecules approximately 22 nucleotides long.  \n 1 \n \nThese molecules play a significant and crucial role in gene expression through partial complementarity with the 3’ untranslated region (3’UTR).  \n 2 \n \nSeveral miRNAs have been identified in humans, and research has shown their importance in biological processes, including cell cycle regulation, differentiation, metabolism, proliferation, apoptosis, gametogenesis (both male and female), and embryo development.  \n 3\nOver the past decade, studies have indicated the ubiquitous presence of miRNAs across all human tissues, including the reproductive system.  \n 4 \n,  5 \n \nThe identification of miRNAs in various reproductive organs and tissues, such as the testis, ovary, uterus, epididymis, spermatozoa, oocytes, seminal plasma, and extracellular vesicles, coupled with their known regulatory functions, suggested that miRNA dysregulation might impair spermatogenesis, disrupt oocyte maturation, and contribute to various types of infertility.  \n 6\nThis study aimed to systematically review high-quality published studies to investigate the association between miRNAs and reproductive functions in both sexes, with particular focus on their role in infertility. While the available studies demonstrated considerable heterogeneity, a comprehensive synthesis of this evidence could help consolidate findings, resolve existing inconsistencies, and provide guidance for future research.\nThe growing urgency for rapid infertility diagnostics and treatments highlighted the potential of innovative approaches, such as liquid biopsy, which offers faster and less invasive alternatives to conventional approaches. Given their established role in gene expression regulation and demonstrated associations with various infertility-related factors, miRNAs represent promising candidates for diagnostic biomarker development.\nEpigenetics refers to changes in gene activity that do not involve changes in the underlying DNA sequence. These changes can be modulated by various environmental factors, such as diet status, psychological stress, and exposure to environmental toxins. Importantly, such epigenetic changes can significantly influence the expression of genes involved in reproductive health, which can affect fertility.\nResearch indicated that epigenetic modifications could contribute to both male and female infertility. In men, abnormal DNA methylation patterns in spermatozoa could affect sperm quality and motility and lead to problems with conception. In women, epigenetic alterations in ovarian or endometrial tissues might disrupt folliculogenesis, hormonal regulation, and embryo implantation success.\nIn addition, epigenetic changes can also be passed from one generation to another, potentially affecting the offspring’s fertility through mechanisms collectively termed transgenerational epigenetic inheritance.  \n 7 \n,  8 \n \nThis phenomenon underscores the critical need to elucidate epigenetic contributions to infertility. Among epigenetic regulators, miRNAs are known to exert epigenetic effects, altering gene expression and production of specific proteins.  \n 9 \n \nMiRNAs affect fertility by regulating various cellular processes, such as sperm production in men and the ovarian cycle in women.  \n 10 \n,  11 \n \nConsequently, changes in miRNA levels can affect these processes, potentially leading to infertility.\nBy studying the epigenetic mechanisms involved in infertility, researchers hope to develop novel diagnostic modalities and targeted therapeutic strategies to enhance fertility outcomes for couples trying to conceive. The identification and modulation of epigenetic contributors to infertility could enable more precise, personalized treatment approaches. In addition, improved understanding of epigenetic influences on fertility might also lead to lifestyle modifications to optimize outcomes in assisted reproductive technologies (ART).\nPolycystic ovary syndrome (PCOS) affects approximately 5-10% of reproductive-aged women, representing one of the most prevalent endocrine disorders in this population.  \n 12 \n \nThe diagnostic triad of PCOS includes chronic anovulation, polycystic ovarian morphology, and clinical and/or biochemical hyperandrogenism.  \n 13 \n,  14 \n \nImportantly, PCOS demonstrates strong associations with metabolic disorders, such as type 2 diabetes (T2D), insulin resistance, and obesity.  \n 13 \n,  14 \n \nWhile the precise etiology of PCOS remains unclear, current research implicates multifactorial influences including genetic predisposition, environmental factors, and iatrogenic effects such as chemotherapy exposure.  \n 15 \n \nRecent studies revealed distinct miRNA expression profiles in women with PCOS compared to healthy women, suggesting potential involvement of miRNAs in PCOS pathogenesis.  \n 16 \n \nThis section aimed to evaluate the research in this area and discuss probable associations between miRNA dysregulation in PCOS, with particular focus on establishing mechanistic links that may inform novel therapeutic strategies. According to a study, PCOS patients had significantly higher levels of miRNAs, including miR-21, miR-155, miR-103, and miR-27b, than healthy women ( table 1 ),  \n 17 \n \nwhich further supported the potential role of miRNAs in PCOS development and progression. Multiple studies demonstrated significant alterations in circulating miRNA profiles in women with PCOS. Specifically, serum levels of miR-16, miR-222, miR-106b, miR-19a, miR-146a, miR-30c, miR-186, and miR-24 were consistently increased in women with PCOS, while miR-320 was reduced compared to healthy controls ( table 1 ).  \n 18 \n,  19 \n \nTherefore, miR-146a and miR-30c exhibited particularly strong diagnostic potential for PCOS.  \n 20 \n \nIncreased expression of miR-222 was associated with type 2 diabetes and gestational diabetes pathogenesis.  \n 21\nDifferential expressions of miRNAs in polycystic ovary syndrome and endometriosis\nPCOS: Polycystic ovary syndrome\nAdditional studies revealed significant dysregulation of specific miRNAs in PCOS patients, with five miRNAs (let-7i-3 pm, miR-5706, miR-4463, miR-3665, and miR-638) showing increased expression and four miRNAs (miR-124-3p, miR-128, miR-29a-3p, and let-7c) demonstrating decreased expression\ncompared to controls ( table 1 ).  \n 22 \n \nBioinformatics analyses of these altered miRNAs suggested that they participate in multiple pathological mechanisms underlying PCOS, including metabolic dysfunction, inflammatory responses, programmed cell death (apoptosis), vascular development (angiogenesis), immune system function, cellular energy metabolism (ATP binding), MAPK signaling cascades, and p53 pathways.  \n 16 \n,  23 \n \nThese consistent findings suggested that changes in miRNA levels might contribute to the PCOS development and progression.\nResearch has also explored the relationship between abnormal androgen production in PCOS and miRNA. In PCOS patients, free testosterone levels were strongly associated with miRNA levels, such as miR-21, miR-103, and miR-155, suggesting that aberrant miRNA expression might contribute to PCOS characteristics.  \n 24\nWhile miRNA research has advanced considerably, the precise mechanisms by which miRNAs contribute to PCOS pathophysiology remain under investigation. Profiling miRNAs can provide new insights into these molecular changes, offering therapeutic and prognostic information.  \n 25 \n \nHowever, considerable controversy persists regarding optimal clinical strategies for symptom management, fertility improvement, and prevention of long-term PCOS complications.  \n 26 \n \nA better understanding of these relationships and underlying processes could ultimately lead to more effective interventions and improved outcomes for individuals with PCOS.\nEndometriosis is a gynecological disorder characterized by the growth of endometrial tissue outside the uterine cavity. Emerging evidence suggested that miRNAs might serve as natural post-transcriptional regulators involved in the development of endometriotic lesions.  \n 27 \n \nThe current gold standard for definitive endometriosis diagnosis remains laparoscopic surgical evaluation, an invasive procedure with inherent patient risks.  \n 28 \n \nTherefore, developing new non-invasive biomarkers to diagnose endometriosis in the early stages is an urgent need.  \n 29 \n \nA previous study identified serum miRNAs as promising diagnostic biomarkers,  \n 26 \n \nwith 14 upregulted miRNAs (miR-145, miR-143, miR-99a, miR-99b, miR-126, miR100, miR125-b, miR-150, miR-125a, miR-223, miR-194, miR-365, miR-29c, and miR-1) and eight downregulated miRNAs (miR-200a, miR-141, miR-200b, miR-142-3p, miR-424, miR-34c, miR-20a,\nand miR-196b) identified ( table 1 ).  \n 30 \n \nIn another study, researchers showed that in patients with endometriosis, the miR-9 and miR-34 families had abnormalities in the atopic endometrium.  \n 31 \n \nFor example, studies showed elevated miR-20a levels in endometriosis lesions.  \n 32 \n \nThe researchers suggested that dysregulation of these miRNAs and their target genes could contribute to the proliferative phenotype observed during the early secretory phase of the menstrual cycle in affected women.  \n 33 \n \nAs a result, many miRNAs have been identified as regulators of gene expression involved in inflammatory responses, local estrogen biosynthesis, progesterone resistance, cell invasion, extracellular matrix regeneration, and angiogenesis in endometriosis.  \n 34 \n \nSix miRNAs (i.e., miR-134-5p, miR-197-5p, miR-22-3p, miR-320a, miR-494-3p, and miR-939-5p) were selected as biomarkers of endometriosis and validated using qRT-PCR ( table 1 ).  \n 35 \n \nAmong these, miR-22-3p and miR-320a exhibited significantly increased expression in the serum exosomes of patients with endometriosis ( table 1 ).  \n 36 \n \nConsidering that endometriosis diagnosis and treatment are frequently delayed due to nonspecific symptoms and the lack of reliable biomarkers, with laparoscopic surgery remaining the diagnostic gold standard, there remains a critical need to identify effective non-invasive indicators for early stages of the disease.\nMale infertility represents a multifactorial reproductive disorder accounting for over 50% of couples’ infertility cases.  \n 37 \n \nThis condition may arise from diverse etiologies, including genital tract infections, hormonal disorders, genitourinary tract infections, genetic mutations, and testicular hyperthermia. The latter may occur in clinical contexts such as varicocele or behavioral patterns including prolonged driving with a vehicle, or habitual laptop use on the lap, a documented risk factor for elevated scrotal temperature.  \n 38 \n \nCurrently, semen analysis serves as the standard diagnostic tool for male infertility. However, this method has some limitations and fails to identify the cause of infertility in approximately 40% of cases, highlighting the need for more effective diagnostic tools. Biomarkers represent one of the most promising emerging diagnostic tools. These molecules, detectable in body fluids, can indicate disease states such as infertility through abnormal expression patterns. Thus, miRNAs have emerged as potential biomarkers for different types of male infertility, including azoospermia, oligospermia, asthenospermia, and teratozoospermia.  \n 38 \n \nIn related research, scientists developed a transgenic mouse model in which the downregulation of miR-382-3p was prevented by overexpression in mature Sertoli cells ( table 2 ).  \n 39\nDifferential expressions of miRNAs in male infertility\nAzoospermia, the most serious type of male infertility, affects 15-20% of infertile men and is classified into two main types: obstructive azoospermia (OA) and non-obstructive azoospermia (NOA).  \n 40 \n \nNOA, resulting from impaired spermatogenesis, represents approximately 60% of azoospermia cases. In contrast, OA accounts for the remaining 40% and occurs when normally produced sperm cannot reach the ejaculate due to genital tract obstructions.  \n 41 \n \nNOA specifically refers to testicular failure to produce sperm and accounts for approximately 0.6% of all men, 10% of infertile men, and 60% of men with azoospermia.  \n 41 \n \nIn recent years, the misplaced expression of miRNAs has been shown to affect several biological processes and was associated with certain reproductive disorders in men, particularly those affecting spermatogenesis. Given the crucial role of miRNAs in all stages of spermatogenesis, their dysregulation logically contributes to numerous male infertility issues.  \n 41 \n \nA study showed decreased levels of miR-383 and miR-520d-3p and increased expression of miR-302a and miR-491-3p in NOA patients. It also reported that the expression of miR-17-92 and miR-371 was regulated in\nthe testes of NOA patients ( table 1 ).  \n 42 \n \nAnother study found that decreased levels of miR-34b and miR-34c were associated with reduced male fertility, NOA, defective meiosis, impaired sperm maturation,\nand spermatogenesis disorders ( table 2 ).  \n 43\nA similar study showed that dysregulation of miR-449 was associated with male infertility characterized by impaired sperm motility.  \n 44 \n \nComparative analysis of seminal plasma from fertile and infertile men revealed significantly reduced levels of seven miRNAs, including miR-34c-5p, miR-122, miR-146b-5p, miR-181a, miR-374b, miR-509-5p, and miR-513a-5p in\nazoospermic patients ( table 2 ).  \n 45 \n \nAnother study found that miR-122-5p was upregulated in OA patients compared to NOA patients.  \n 46 \n-  48 \n \nThese miRNAs could be used as diagnostic biomarkers for idiopathic male infertility and could inform the development of targeted therapies. Their irregularity could be the key to developing new and advanced diagnostic and prognostic approaches in male infertility. To take full advantage of their potential, further investigation is required to identify additional miRNAs involved in reproductive pathologies, the mechanism by which they work, and how their expression modulation might improve clinical outcomes. Collectively, these findings substantiate the regulatory role of miRNAs in male germ and somatic cells, where expression alterations could lead to reproductive disorders.\nAn ideal biomarker should be target-specific, stable, non-invasive, sensitive to detection, and easily accessible from accessible biological sources.  \n 49 \n \nIn clinical practice, serum proteins have conventionally served as biomarkers for disease detection and prognosis.  \n 50 \n \nHowever, proteins as biomarkers have limitations, such as reduced diagnostic value due to inadequate specificity and sensitivity. On the other hand, miRNAs emerge earlier in both intracellular and extracellular environments and can be detected with greater precision, enabling earlier disease identification. MiRNAs are typically expressed during specific biological phases.  \n 50 \n,  51 \n \nAdditionally, miRNAs are often observed as homogeneous populations, while proteins often undergo post-translational modifications and create heterogeneous forms.  \n 52\nVarious diagnostic approaches have been developed for infertility assessment in both sexes, with biomarker-based methods representing the most recent advancement. Biomarkers can be utilized to detect diseases prior to clinical symptom manifestation. Among potential biomarkers, miRNAs are considered particularly promising due to their unique properties. Circulating (serum) miRNAs were initially employed as biomarkers for diagnosing B-cell lymphoma.  \n 53 \n \nIn another study, a decrease in miR-122, miR-181a, and miR-34c was observed in the serum of patients with oligoasthenospermia.  \n 54 \n,  55 \n \nSeveral studies published in recent years demonstrated that miRNAs could be suitable biomarkers for diagnostic purposes.  \n 52 \n,  56 \n,  57\nProtein factors, DNA methylation, and non-coding RNAs are all present in the sperm and egg genomes.  \n 58 \n \nDuring spermatogenesis and oogenesis in mammals, mRNAs undergo post-transcriptional and post-translational regulation in differentiated germ cells, enabling observation of miRNAs during both spermatogenesis and oocyte maturation.\nThe modification and manipulation of miRNA activity in the body is of great interest due to their abnormal expression and role in the pathogenesis of human diseases.  \n 59 \n \nThe use of anti-miRNA oligonucleotides to target disease-related miRNAs is the most widely used approach for understanding their  in vivo  function and shows promise for developing new miRNA-based therapies.  \n 60 \n,  61 \n \nIn addition to their potential use as biomarkers, miRNAs can be considered for therapeutic purposes in a personalized medical field related to male and female infertility.  \n 62 \n \nResearchers are exploring different methods to modulate miRNA levels for therapeutic purposes, including supplementation with microRNA mimics to either reduce or upregulate their expression, and using lab-engineered molecules called anti-miRNAs for conditions involving miRNA overexpression.  \n 62\nThe therapeutic potential of miRNAs, along with advances in nanomedicine, could lead to the development of novel fertility treatments for both male and female infertility.  \n 63 \n,  64 \n \nWith advances in genomics, researchers demonstrated that these small non-coding RNA molecules are essential for mammalian ovarian function. The most recent microRNA-based therapeutic strategies for infertility focus on addressing gonadal damage through multi-pathway targeting agents. Given existing treatment limitations, an integrated approach combining preventive measures with microRNA therapy represents both a practical and desirable clinical option.\n\nUnderstanding the mechanisms that lead to infertility in both men and women is essential. Despite careful and expensive clinical examinations, including invasive techniques such as testicular biopsy, infertility sometimes remains undiagnosed. Current research has provided conclusive evidence on the role of miRNAs in regulating infertility. When combined with traditional diagnostic techniques, miRNAs have significantly improved infertility diagnosis. MiRNAs are affordable, readily available, and can be easily extracted from blood and semen, making them clinically practical. This diagnostic simplification may enable more effective treatment strategies after symptom and goal identification. To establish miRNAs as diagnostic biomarkers for various infertility types, developing standardized protocols and accurate diagnostic validation techniques would be essential.","source_license":"public-domain-us","license_restricted":false}