Abstract
The objective of this investigation was to examine alterations in PTEN expression within ovarian tissue in a rat model of polycystic ovary syndrome (PCOS). The analysis also encompassed the examination of PTEN alterations in the ovarian tissue throughout the process of folliculogenesis in rats with normal ovulatory cycles. The study involved 12 adult female Sprague‒Dawley rats randomly assigned to the letrozole-induced polycystic ovary syndrome (PCOS) group as part of an animal-based research endeavour. The sections derived from the ovaries were subjected to immunohistochemical staining for PTEN. The evaluation of PTEN staining levels in ovarian tissues was conducted using electron microscopy. Follicle counts, as well as hormonal and biochemical analyses (serum luteinising hormone (LH), follicle-stimulating hormone (FSH), anti-Müllerian hormone (AMH), testosterone, oestradiol levels and serum glucose, triglyceride, HDL and LDL-cholesterol levels), were conducted to provide evidence of the manifestation of polycystic ovary syndrome (PCOS) in rats. The number of primordial and Graafian follicles in the PCOS group decreased significantly, and the number of primary, secondary and antral follicles increased significantly. PTEN expression was found to be significantly higher in the PCOS group than in the control group in the primordial follicle oocyte cytoplasm, primordial follicle granulosa cells, primary follicle oocyte cytoplasm, primary follicle granulosa cells, antral follicle oocyte cytoplasm, antral follicle granulosa cells, and corpus luteum (p = 0.007, p = 0.001, p = 0.001, p = 0.001, p = 0.001, p = 0.002, and p = 0.018, respectively). In the non-PCOS group, a time-dependent comparison of the amount of oocyte cytoplasm and PTEN staining in granulosa cells of the oocytes at different stages of development was performed. While the follicles were developing from the primordial follicle to the primary and antral follicle, the amount of PTEN staining in the oocyte cytoplasm decreased, whereas the PTEN activity in the granulosa cells increased as the oocyte developed (p = 0.001 and p = 0.001, respectively). The current investigation demonstrated changes in PTEN expression in ovarian tissue throughout the course of normal folliculogenesis, as well as in instances of disrupted folliculogenesis, with a focus on rats with PCOS.
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Introduction
PCOS, a prevalent endocrine condition affecting women of reproductive age1, is a complex disorder with various clinical manifestations and associated morbidities2. The prevalence varies across different regions, with rates ranging from 6 to 21%, according to the ESHRE/ASRM 2003 criteria3. Despite extensive research, the precise molecular pathways involved in PCOS pathogenesis remain unexplored, highlighting the need for further analyses and treatments4.
PCOS affects the development of a mature oocyte, which is a crucial part of human follicle development5. Primordial follicles, grouped together as a cohort, are recruited for ovulation of a mature oocyte6. The intrafollicular hormonal environment is dynamic, and effective communication between granulosa cells and oocytes determines the oocyte’s developmental competence. Granulosa cells surrounding the oocyte play a crucial role in supplying nutrients and growth factors for oocyte development7. In PCOS, although there are more follicles in the ovary than in that without PCOS, a mature oocyte is challenging to form due to impaired follicle developmental stages8. Granulosa cells that surround oocytes in PCOS exhibit abnormal patterns of proliferation and apoptosis, which can be attributed to processes such as atresia, degeneration, and hypertrophy9.
PTEN (phosphatase and tensin homologue) is a tumour suppressor gene that plays a crucial role in regulating cell growth and division10. PTEN regulates the Akt/PKB signalling pathway, affecting phosphoinositol triphosphate levels, which are essential for cell development and cell survival11. The PI3K/AKT signalling pathway can affect ovarian granulosa cells, and the PI3K catalytic subunit p110d has been shown to be an important component of the PI3K pathway for follicular development stimulated by both follicle-stimulating hormone and oestradiol in ovarian granulosa cells12,13. PTEN deletion on the tenth chromosome dephosphorylates PIP3 to PI and P2, inhibiting the PI3K/AKT pathway and slowing biological processes, including proliferation, growth and motility14.
The impairment of PTEN function can result in detrimental consequences for the intricate hormonal signalling equilibrium within the ovaries, specifically with regards to folliculogenesis in PCOS. This phenomenon can be attributed to the involvement of PTEN in the regulation of ovarian follicle growth and oocyte maturation15. The PTEN protein, acting as a regulatory factor, exerts a substantial influence on both the proliferation and differentiation of granulosa cells and plays a critical role in the maturation of oocytes, facilitating the coordination of essential events needed for successful and optimal ovulation16.
In this study, PTEN expression in ovarian tissue was compared in a PCOS rat model and normo-ovulatory rats. PTEN tissue changes in a time-dependent manner during folliculogenesis in normo-ovulatory rats were also shown.
Materials and methods
Animals and experimental design
For the purpose of our research, a total of 12 female adult Sprague‒Dawley rats weighing 160–180 g were acquired from Harlan Laboratories located in the Netherlands. These rats were subjected to a 12-h light and dark cycle and had unrestricted access to a standard rat diet sourced from Korkuteli Food Industry in Turkey. The female rats, which exhibited regular oestrous cycles as confirmed by vaginal cytologic examination, were randomly allocated into two distinct groups. Aromatase inhibitor (Femara tablet; letrozole 2.5 mg, Novartis) dissolved in 1% carboxymethyl cellulose (CMC) (2 ml/kg) was administered daily through oral gavage at 1 mg/kg/day to Group 1 consisting of 6 rats for 21 days (the PCOS group), and 1% CMC (2 ml/kg) solution was administered daily through oral gavage to Group 2 (the control group) for 21 days. The methodology and dosage of the drug were established based on prior studies documented in the literature, wherein PCOS was induced in rats using letrozole17,18,19.
The sexual cycle was determined by microscopic analysis of the predominant cell type in vaginal smears obtained daily until the end of the experiment. All control rats had a normal oestrous cycle of 4.5 days, whereas letrozole-treated rats were completely acyclic, and vaginal smears showed leukocytes, the predominant cell type of the diestrus phase. Hormonal and histological changes in the ovary and uterus in both the control group and the letrozole group were evaluated in line with the data obtained as a result of vaginal cytological examination. All rats in the control group were sacrificed in the proestrus phase of the oestrous cycle.
All procedures that used animals were approved by the Gazi University Animal Experiments Local Ethics Committee in Turkey and were performed at the Laboratory Animal Breeding and Experimental Research Center of the same university. All animals were sacrificed with ketamine (45 mg/kg, i.m.) and xylazine (5 mg/kg, i.m.) anaesthesia. Female reproductive tissues (uterus and ovaries) were excised, and the dry weights of the ovaries were determined with a precision digital scale sensitive to 0.01 g. Tissues were first fixed for 72 h in a 10% neutral formaldehyde solution for light microscopic examination, and paraffin blocks were provided using routine procedures.
Blood samples were drawn intracardially into plain tubes without heparin on the 22nd day of administration for endocrine and biochemical analyses, and serum was separated by centrifugation at 3000 rpm for 10 min and stored at − 80 °C until analysis.
Hormonal and biochemical analysis
Serum luteinising hormone (LH), follicle-stimulating hormone (FSH), anti-Mullerian hormone (AMH), testosterone and oestradiol levels were estimated by enzyme-linked immunosorbent assays. FSH and LH analyses were performed using an ELISA kit (SunRed; SunRed Biotechnology Company Shanghai China), AMH analyses were performed with an ELISA kit (Ansh Labs, AL-113), and testosterone and oestradiol levels were determined by an ELISA kit (Oxford; Serotec, Ltd., UK). Serum glucose, triglyceride, HDL and LDL-cholesterol levels were measured by enzymatic methods using autoanalysers.
Histology
The right ovary of all rats was bisected longitudinally. Fixation of the ovarian tissues was carried out in 10% formalin solution, followed by routine tissue processing. Sections were obtained with a thickness of 5 μm and placed on glass slides. Sampling of consecutive sections was chosen systematically and randomly. These sections were stained with haematoxylin and eosin and then photographed using a Leica DCM 4000 microscope and an HD digital camera. Finally, stereological and histopathological investigations were carried out on micrographs.
Haematoxylin and eosin staining
Sections obtained from the ovaries were maintained in an incubator at 37 °C overnight. The paraffin sections were deparaffinized in xylene and rehydrated. Then, the specimens underwent a dehydration process with a graded series of ethanol (EtOH). The sections were then incubated in haematoxylin solution for 10 min and washed again under running water for 10 min. Next, the sections were dipped 2–3 times in a mixture of 70% alcohol plus three drops of glacial acetic acid, washed in running water for 10 min and stained with eosin solution for 5 min. Finally, the sections were washed in running water for 10 min, passed through 3 changes of 95% EtOH and 2 changes of 100% EtOH for 1 min each and cleared in 3 changes of xylene for 1 min each20. Coverslipped images were taken and evaluated on a Leica DCM 4000 computer-aided imaging system.
Stereology (follicle counting)
Physical disector and Cavalieri methods were used to estimate the number of ovarian follicles and mean volume of regions of interest in ovarian tissues21. The mean ovarian tissue volume was determined by multiplying the area of a point interval by the sum of the number of points that intersect the region of interest in each section. The mean volumes of the regions of interest were calculated using the following formula: Volume (V1) = t × A, where “t” represents the thickness and interval of each section, and “A” is the total area of the regions of interest. The sampling and counting methodology was devised based on a preliminary pilot study, and particles were enumerated using the ImageJ software program. The numerical density of follicles was determined using the following formula: Nv = ∑Q − ∑V disector. The morphological classification of follicles in the ovary was confirmed through the validation of the coefficient of error and coefficient of variation.
The morphological classification of follicles in the ovary was as follows: primordial follicle, unilaminar primary follicle, multilaminar primary follicle, antral follicle, Graafian follicle and corpus luteum22.
Immunohistochemistry (IHC) staining for PTEN
Sections obtained from the ovaries were maintained in an incubator at 37 °C overnight. The study involved deparaffinization of ovarian tissues using various methods. First, the sections were left in xylol for 5 min and then dehydrated in a graded alcohol series for 3 min each. The sections were then fixed in EDTA buffer in a microwave for 10 min to remove formaldehyde. After cooling to 25 °C, tissues were circled with a Pap pen, washed with PBS three times, treated with 3% H2O2, and treated with Ultra-V block. The tissues were then subjected to PTEN primary antibody at 4 °C overnight, followed by treatment with a biotinylated secondary antibody and streptavidin peroxidase for 20 min. Nuclear staining was achieved using 4′,6-diamino-2-phenolindole (DAPI), and background staining was performed with haematoxylin. The slides were closed using Entellan, and image analysis was performed using the Leica DCM 4000 computer-aided imaging system.
Evaluation of PTEN expression in ovarian sections
PTEN expression was scored using an immunoreactive scoring scale and evaluated by two researchers who did not have any prior knowledge of the groups of rats. Accordingly, six zones (one central and five peripheral) were selected from ovarian tissue sections (5 μm thickness) and subjected to IHC staining with anti-PTEN antibodies. The HSCORE, defined below, was used to evaluate the immunoreactive density in these zones. The HSCORE was determined by the following formula: HSCORE ¼ Pi (i + 1), where ‘i’ was the intensity of labelling with a value of 0, 1, 2 or 3 (none, weak, moderate or strong) and Pi the percentage of labelled cells for each intensity, within a range of 0–100%18. The rate of positive cells was scored by the extent of immunostaining and was assigned to one of the following categories: 0 (0%, no positive cells), 1 (≤ 30% positive cells), 2 (30–60% positive cells) and 3 (> 60% positive cells)18.
Statistical analysis
For the data analysis, the SPSS 11.5 program was used. Mean ± standard deviation and median (minimum–maximum) were used as descriptors for quantitative variables, and number (percentage) was used for qualitative variables. If normal distribution assumptions were provided, Student’s t test was used to determine whether there was a difference between the qualitative variable categories and the two quantitative variable categories; the Mann‒Whitney U test was used if they were not. Repeated measures ANOVA was used to determine whether there was a statistically significant difference between quantitative repeated measurements. The Tukey test was used as the post hoc test. The statistical significance level was taken as 0.05.
Ethical approval
This study was carried out in compliance with the ARRIVE guidelines and all methods were carried out in accordance with relevant guidelines and regulations.
Results
Rats administered letrozole for the induction of PCOS showed significant increases in ovarian size, and the mean ovarian weight in the PCOS group was found to be approximately twice that of the control group (p < 0.001) (Table 1).
Histopathological findings
The follicle numbers of the control and PCOS groups in different developmental stages were compared after H&E staining. Table 1 summarises the comparisons between the control and PCOS groups for follicle numbers. The PCOS group had significantly lower primordial follicle and Graaf follicle counts than the control group (p < 0.001). Furthermore, the PCOS group had significantly higher unilaminar primary follicle, multilaminar primary follicle, and antral follicle numbers than the control group (p < 0.001) (Table 1).
Hormones and biochemical findings
Comparisons between the control and PCOS groups for hormones and biochemical findings are summarised in Table 2. LH, FSH, and oestrogen levels in the PCOS group were found to be significantly lower than those in the control group (p = 0.012, p < 0.001, and p = 0.001, respectively). Furthermore, AMH, testosterone, triglyceride, glucose, and LDL levels in the PCOS group were found to be significantly higher than those in the control group (p = 0.003, p < 0.001, p = 0.015, p = 0.001, and p = 0.002, respectively).
Immunohistochemical findings for the ovary
As a result of IHC staining, PTEN primary antibody immunoreactivity was detected at every stage of follicular development. PTEN expression was observed in oocyte cytoplasm, granulosa cells, theca cells and the corpus luteum of follicles belonging to the control group (Figs. 1, 2, 3) and PCOS group (Figs. 4, 5).
PTEN expression was strong in the oocyte cytoplasm of primordial follicles but weak in granulosa cells (Fig. 1 and a). Similarly, PTEN immunoreactivity was moderate in the granulosa cells surrounding the oocyte in unilaminar primary follicles, but it was significantly strong in the granulosa cells belonging to multilaminary primary follicles and antral follicles (Fig. 2 and a). In the control group, during the transition from the primordial follicle to the primary follicle, PTEN immunoreactivity was observed to be strong in the primordial follicle cytoplasm, weak in the squamous granulosa cell surrounding the oocyte, and varying from weak to moderate in the oocyte cytoplasm with cubic granulosa cells (Fig. 3, a and b).
In the PCOS group, moderate PTEN immunoreactivity was observed in the oocyte cytoplasm of the antral and Graafian follicles, but this expression was strong in the granulosa cells of these oocytes. PTEN immunoreactivity was also strong in the cystic structures and in the corpus luteum (Fig. 4 and a). The PTEN immunoreactivity of the primordial and primary follicles was quite strong compared to that in the control (Fig. 5, a and b).
PTEN expression in the control and PCOS groups is presented in Table 3. PTEN staining levels were found to be significantly higher in the PCOS group than in the control group in the primordial follicle oocyte cytoplasm, primordial follicle granulosa cells, primary follicle oocyte cytoplasm, primary follicle granulosa cells, antral follicle oocyte cytoplasm, antral follicle granulosa cells, and corpus luteum (p = 0.007, p = 0.001, p = 0.001, p = 0.001, p = 0.001, p = 0.002, and p = 0.018, respectively).
In the final section of the study, PTEN staining levels in the primordial follicle, primary follicle, and antral follicle stages were compared to demonstrate the change in PTEN immunoreactivity in the follicular developmental stages in the control group. These findings are shown in Table 4. A time-dependent comparison of the amount of PTEN staining in the oocyte cytoplasm and granulosa cells of the follicles at different stages of development was made. While the follicles were developing from the primordial follicle to the primary and antral follicle, the amount of PTEN staining in the oocyte cytoplasm decreased, whereas the PTEN activity in the granulosa cells increased as the oocyte developed (p = 0.001 and p = 0.001, respectively).
Discussion
In this study, PCOS was modelled with letrozole in adult female Sprague‒Dawley rats, and PTEN expression in ovarian tissues was compared between the PCOS group and the normo-ovulatory (control) group. The results of our study indicate that there was a significant rise in PTEN staining levels in the oocytes of the PCOS group compared to the control group. This study additionally examined the alterations in PTEN expression within the ovary across various stages of folliculogenesis. The study revealed that PTEN expression became more prominent in granulosa cells as the follicles developed, whereas its presence in the oocyte cytoplasm decreased.
Hormonal and biochemical assessments, as well as follicle counting sections, were incorporated into the study to provide additional support for the development of the PCOS model. The utilisation of letrozole-induced rat models for the study of PCOS is widely favoured in the academic literature due to the notable matching of ovarian morphology and hormonal profiles to those observed in human PCOS17,18,19. The hormonal, biochemical, and histopathological analyses of the PCOS group in our study were comparable to those of human PCOS. In the PCOS group of the study, the observed reduction in primordial follicles, along with an elevation in primary and secondary follicles, may suggest atypical premature activation and commencement of development in primordial follicles. Alternatively, it is plausible that these findings could be attributed to potential discrepancies in the methodology employed for follicle quantification.
The histopathological analyses revealed a decrease in the number of granulosa cells within the follicles of individuals with polycystic ovary syndrome (PCOS) compared to that of the control group. Additionally, the arrangement of these cells appeared to be more loosely organised. The data presented in this study demonstrate a correlation between decreased ovulation and impaired granulosa cell function, despite an observed increase in the number of antral follicles. Furthermore, the ovaries of the PCOS group had many cystic forms and the absence of corpus luteum structures, which can be attributed to anovulation.
Based on the existing scientific evidence, the mechanism governing the proliferation of granulosa cells is highly intricate and is acknowledged to be intricately linked to numerous elements23. A growing body of literature has demonstrated that PTEN exerts regulatory control over the differentiation process in granulosa cells and is important in the aberrant proliferation of granulosa cells in polycystic ovaries24,25. In a study conducted by Yeung et al., the researchers examined the impact of PCOS on women by investigating PTEN expression in rat ovaries. The findings revealed a decrease in PTEN expression in PCOS-affected ovaries, leading to the hypothesis that PTEN may play a role in diminishing the proliferative potential of granulosa cells in polycystic ovaries. Consequently, this mechanism may contribute to the progression of follicular apoptosis and follicular atresia26,27. In the investigation conducted by Andreas et al.28, it was proposed that the decrease in PTEN expression leads to an augmentation in the proliferation of bovine granulosa cells. The variations observed in the outcomes of studies documented in the literature can be ascribed to the diverse origins of the granulosa cells utilised. Additionally, disparities may arise from the evaluation of distinct stages of cell development. Notably, the sources of these cells encompass rats, cattle, and female subjects, while the stages of follicle development examined encompass the primordial, primary, and antral stages. Hence, we conducted an investigation to analyse the fluctuation of PTEN expression during various developmental stages, with a focus on temporal dynamics. Our work revealed the presence of variation in PTEN expression inside both cytoplasmic and granulosa cells. Our study provides insights into the literature in this regard.
The primary constraint of our study is the limited sample size of rats employed in the research. The limited number of rats used in each study group was permitted by our ethics committee. A further constraint of this work pertains to the exclusive demonstration of time-dependent alterations in PTEN expression within follicular developmental stages solely in the control group. This particular aspect of the study was not conducted because the PCOS group did not have oestrous cycles and was deemed to be unable to ovulate.
There has been an emerging trend in recent years in the literature on PCOS and PTEN, wherein researchers have begun to challenge the plausibility of regulating PTEN expression. Researchers conducted a study to examine the fundamental mechanisms that contribute to the excessive proliferation observed in granulosa cells affected by PCOS. In this study, He et al., presented evidence indicating that miR-200b and miR-200c exert inhibitory effects on the proliferation of KGN cells through the targeting of PTEN. These findings contribute to the existing knowledge on the aberrant proliferation of granulosa cells in PCOS15. Zhou et al., investigated whether microRNA (miR)-18b-5p is one of the miRs that could functionally mediate PCOS progression via PTEN in rats that developed PCOS with letrozole, as in our study. miR-18b-5p targeted PTEN, reduced PTEN expression and activated the PI3K/Akt/mTOR signalling pathway to improve PCOS. As a result of this study, it was shown that circulating miR-18b-5p levels can contribute to the progression of PCOS complications29.
The objective of ongoing investigations on the PI3K/AKT/PTEN signalling system in polycystic ovary syndrome (PCOS) is to ascertain the viability of a pharmacological intervention capable of effectively addressing ovarian dysfunction30. Onal et al.31 conducted a recent study to determine whether PCOS treatment agents alter PTEN expression in the polycystic ovary, and the study highlighted the importance of PTEN pathway studies for PCOS treatment research groups.
Ongoing research is being conducted to investigate the importance of PTEN expression in polycystic ovary syndrome. Additionally, there is a parallel focus on examining the various elements that exert an influence on PTEN activity. The findings from these studies have paved the way for potential future therapies that can effectively modulate the mechanisms behind follicle and oocyte growth in patients with PCOS. The ability to modulate uncontrolled follicular development in patients with PCOS or the atretic process during follicular developmental stages holds great potential for minimising difficulties associated with PCOS and may have substantial implications, particularly in the field of assisted reproductive techniques.
Our research is anticipated to have a major impact on the existing body of literature, as it uncovers alterations in PTEN expression during the process of normal oocyte development, as well as diminished ovarian functions observed in those with PCOS.
Conclusion
The present study investigated the alterations in PTEN ovarian tissue expression during the process of normal folliculogenesis as well as in cases of impaired folliculogenesis, with a specific focus on rats with PCOS. The results of our study will provide a basis for further research on the relationship between PTEN and the processes of folliculogenesis, both in normal and disturbed contexts, particularly in PCOS.
Data availability
The datasets utilised in this investigation may be obtained from the corresponding author upon a reasonable request.
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M.N.K. and E.A. wrote the manuscript text. Z.K. edited the text. P.S. prepared tables and figures. C.E. and C.Y. carried out laboratory works. B.B. made statistically analysis.
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Namlı Kalem, M., Anadol, E., Kalem, Z. et al. A rat study on the PTEN expression in ovarian tissue in PCOS and folliculogenesis. Sci Rep 13, 20774 (2023). https://doi.org/10.1038/s41598-023-47809-y
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DOI: https://doi.org/10.1038/s41598-023-47809-y
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