The Application of Dehydroepiandrosterone on Improving Mitochondrial Function and Reducing Apoptosis of Cumulus Cells in Poor Ovarian Responders.

Poor ovarian responders (PORs) pose a great challenge for in vitro fertilization (IVF). Previous studies have suggested that dehydroepiandrosterone (DHEA) may improve IVF outcomes in PORs. The current study attempted to investigate the clinical benefits of DHEA in PORs and the possible mechanisms of DHEA on cumulus cells (CCs). This was a prospective study performed at one tertiary center from January 2015 to March 2016. A total of 131 women who underwent IVF treatment participated, including 59 normal ovarian responders (NORs) and 72 PORs. PORs were assigned to receive DHEA supplementation or not before the IVF cycle. For all patients, CCs were obtained after oocyte retrieval. In the CCs, mRNA expression of apoptosis-related genes and mitochondrial transcription factor A (TFAM) gene, terminal deoxynucleotidyl transferase dUTP nick end labeling assay, mitochondrial dehydrogenase activity and mitochondrial mass were measured. The results indicated that PORs with DHEA supplementation produces a great number of top-quality embryos at day 3 and increased the number of transferred embryos and fertilization rate compared with those without DHEA supplementation. Additionally, supplementation with DHEA in PORs decreased DNA damage and apoptosis in CCs while enhancing the mitochondrial mass, mitochondrial dehydrogenase activity and TFAM expression in CCs. In conclusion, our results showed that the benefits of DHEA supplementation on IVF outcomes in PORs were significant, and the effects may be partially mediated by improving mitochondrial function and reducing apoptosis in CCs.

Introduction

Poor ovarian responders (PORs), characterized by a poor response to controlled ovarian stimulation (COS), pose a great obstacle for in vitro fertilization (IVF). PORs yield poor oocyte quality and ovarian reserve, leading to extremely low live birth rates 1, 2. Several strategies, including variety of COS protocols 3 and various adjuvant supplements 4-6, were proposed as an attempt to improve the reproductive outcomes in PORs. Regarding adjuvant supplements, dehydroepiandrosterone (DHEA) was considered a potential agent to better clinical outcomes in PORs 7, 8. DHEA, an endogenous steroid produced by the zona reticularis of the adrenal glands and by ovarian theca cells, is a precursor to estradiol and testosterone 9. The dehydroepiandrosterone sulfate level in follicular fluid has been reported to be a predictor of oocyte maturation, fertilization, embryo development and live birth in women undergoing IVF cycles 10. The Cochrane review concluded that pre-treatment with DHEA may be associated with improved live birth rates in PORs undergoing IVF cycles 11. However, the possible mechanisms of improved IVF outcomes in PORs following DHEA treatment are not fully known.

Oocytes were protected and nurtured from surrounding somatic cells, including cumulus cells (CCs) and granulosa cells 12. CCs and oocytes form cumulus-oocyte complex (COC), which communicate with each other through specialized gap junctions 12, 13. Numerous studies indicate that gene expression in CCs can serve as biomarkers for oocyte or embryo quality and pregnancy outcomes 14-16. Our previous self-controlled studies demonstrated the potential anti-apoptotic effect on CCs following DHEA treatment 17, 18. Apoptosis plays a critical role on oogenesis, folliculogenesis, oocyte loss, selection, atresia and luteogenesis 19. Several studies showed that the apoptosis of CCs was associated with impaired oocyte maturation, fertilization, embryo growth and pregnancy outcomes 20-23.

Mitochondria plays an important role on the intrinsic apoptosis pathway mediated by the BCL2 family 24. When stress stimuli are transduced to mitochondria, BAX and BAK, pro-apoptotic members of the BCL2 family, increase the mitochondrial membrane permeability to proteins such as cytochrome c, leading to caspase cascade activation 25. Our previous self-controlled study revealed that mitochondrial dehydrogenase activity of CCs significantly increased in PORs after DHEA supplementation. Mitochondria are involved in oocyte growth and embryo development; interference with mitochondrial function contributes to arrest of oocyte maturation, impaired fertilization and compromised embryo development 26-28.

Based on our previous studies 17, 18 and the numerous studies discussed thus far, we hypothesized that DHEA may improve reproductive outcomes in PORs through increasing mitochondrial function and decreasing apoptosis in CCs. To verify this hypothesis, we compared the IVF outcomes of normal ovarian responders (NORs), PORs with or without DHEA supplementation and collected their CCs for researches. In fact, this study was a further research of our previous work 18 by enrolling more patients, adding control groups and performing more experiments.

Materials and Methods

Patients and design

This prospective study was performed at the Reproductive Center of the Kaohsiung Veterans General Hospital between January 2015 and March 2016. The study enrolled NORs and PORs. The inclusive criteria for NORs included the following: (1) antral follicle counts (AFC) ≥ 5 or anti-Müllerian hormone (AMH) ≥ 1 ng/mL and (2) the number of retrieved oocytes was between 5 and 15. PORs met the Bologna criteria 29, having at least two of the three following features: (1) advanced maternal age (≥ 40 years) or any other risk factor for POR, (2) a previous POR (≤ 3 oocytes with a conventional stimulation protocol), and (3) an abnormal ovarian reserve test. An abnormal ovarian reserve test was defined as AFC < 5 or AMH < 1 ng/mL in this study. Moreover, two episodes of a previous POR after maximal stimulation alone would be sufficient to define a patient as a POR. PORs were divided into 2 groups in this study. In the POR group, patients directly underwent an IVF cycle without DHEA pre-treatment. In the POR/DHEA group, patients received DHEA supplementation (CPH; Formulation Technology, Oakdale, CA, USA) of 90 mg per day at least 2 months (8 to 16 weeks, mean 12.6 weeks) before entering an IVF cycle.

Ethical approval

All procedures performed in studies involving human participants were in accordance with the ethical standards of the institutional and/or national research committee and with the 1964 Helsinki declaration and its later amendments or comparable ethical standard. The institutional review board at Kaohsiung Veterans General Hospital approved all study procedures. The study was performed in accordance with approved guidelines. Informed consent was obtained from all individual participants included in the study.

Treatment protocol

All participants underwent a gonadotropin-releasing hormone (GnRH) antagonist protocol, as previously described 18. Briefly, ovarian stimulation occurred on day 2 of the menstrual cycle with daily recombinant follicle-stimulating hormone (rFSH) ± recombinant luteinizing hormone (rLH), including Gonal-F (rFSH, Merck KGaA, Darmstadt, Germany), Pergovaris (rFSH + rLH, Merck Serono, Aubonne, Switzerland) or Merional (rFSH + rLH, Institut Biochimique SA, Lamone, Switzerland). A GnRH antagonist (Cetrotide 0.25 mg; Merck Serono, Idron, France) was administered when the leading follicle reached a diameter of 12-14 mm. Recombinant human chorionic gonadotropin (Ovidrel, Merck Serono, Modugno, Italy) was administered until at least three dominant follicles reached ≥17 mm in diameter in the NORs or at least one dominant follicle reached ≥17 mm in diameter in the PORs. Transvaginal oocyte retrieval was performed 34-36 h later. Intracytoplasmic sperm injection (ICSI) was conducted in all PORs to reduce the possibility of fertilization failure. NORs underwent ICSI in the cases of poor sperm quality. Embryos were assessed and scored according to the criteria established by the Istanbul consensus workshop 30. Embryo transfer was done under transabdominal sonographic guidance on day 3 after oocyte retrieval in the PORs and on day 3 or day 5 after oocyte retrieval, depending on the embryo status in the NORs.

Luteal phase support was started on the day of oocyte retrieval. Daily progesterone, including Crinone 8% gel (Merck Serono, Hertfordshire, UK) and Duphaston 4 mg (Abbott, Olst, The Newtherlands) were given routinely. A pregnancy test was performed 14 days later. Once a positive pregnancy test was observed, progesterone was continued for an additional 6 weeks. Clinical pregnancy was established if visualization of a fetal heart beat was found in an intrauterine gestational sac by transvaginal ultrasound. Ongoing pregnancy was determined by the presence of a fetal heart beat beyond 20 weeks of gestation. Live birth was defined as delivery of a live fetus after 20 completed weeks of gestation.

Cumulus-oocyte complex grade and cumulus cell collection

After oocyte retrieval, COCs were collected, washed, and visually classified into one of three groups based on the degree of oocyte and cumulus expansion, as previously described 31. COCs were incubated in the IVF medium covered with paraffin oil until denudation. 2 h later, COCs were denuded individually using hyaluronidase (SynVitro™ Hyadase, Origo, Målov Denmark, Knardrupvej) for 30 s at most. CCs were isolated, pooled per patient, and transferred to a 15-mL centrifugation tube containing 4 mL of Histopaque 1077 (Sigma Chemical, St. Louis, MO, USA). CCs were separated from red blood cells by centrifugation at 600g for 10 min. CCs formed a thin layer between the Histopaque and the medium. Cells were removed and placed in a new centrifugation tube and washed using IVF medium, with centrifugation at 600g for 10 minutes. The supernatant was discharged and the CCs were placed at -80°C for further study.

RNA isolation and quantitative real-time polymerase chain reaction (Q-PCR)

The method for Q-PCR was as described previously 17. Total RNA was extracted from tissue specimens using the acid-phenol guanidium method. Briefly, TRIzol was added to the CCs. The mixture was pipetted to mix and allowed to sit for 5 min at room temperature. Chloroform was added, mixed, and allowed to incubate at room temperature for 10 min. The mixture was centrifuged at 12,000 g for 20 min, and the supernatant was transferred to a fresh tube. Isopropanol was added, mixed, and incubated for 10 min at room temperature. The solution was centrifuged at 12,000 g for 30 min, and the RNA was purified as above. The pellet was washed twice with 70% ethanol, re-suspended in diethylpyrocarbonate (DEPC)-treated water, and stored at -80°C. All Q-PCRs were performed using an ABI Prism 7700 Sequence Detection System (Perkin-Elmer Applied Biosystems, Foster City, CA, USA). PCR was performed using the SYBR Green PCR Core Reagents kit (Perkin-Elmer Applied Biosystems). The thermal cycling conditions included an initial denaturation step at 95°C for 10 min, and 40 cycles at 95°C for 15 s, and 60°C for 1 min. Specific PCR amplification products were detected by the fluorescent double-stranded DNA-binding dye, SYBR Green. Experiments were performed with triplicates for each data point. All samples with a coefficient of variation for Ct value > 1% were retested. The primers used for Q-PCR analysis are shown in supplemental Table S1.

Terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) analysis

After oocyte denudation, CCs were isolated and washed with phosphate-buffered saline (PBS) and fixed with 4% formaldehyde in PBS (pH 7.4) for 20 min at 4 °C. TUNEL analysis with fluorescein was performed with the ApopTag Fluorescein Direct In Situ Apoptosis Detection Kit (Millipore Co.). Slides were counterstained with 4',6-diamidino-2-phenylindole (DAPI) for 10 min, dehydrated, cleared, and cover-slipped.

Mitochondrial dehydrogenase activity assay

Mitochondrial dehydrogenase activity was analyzed using the cell counting kit-8 (CCK-8, Enzo Life Sciences Inc., NY, USA) that detected the metabolic activity of the cells. CCK-8 reagent (10 μL) was added to each well, and the cells were then incubated at 37°C for 4 h. Absorbance was recorded using an enzyme-linked immunosorbent assay microplate reader at 450 nm.

Mitochondrial mass measurement

The collected CCs were washed twice in PBS by centrifugation to avoid blood contamination, and the pellet was resuspended in PBS for analysis using an image flow cytometer. For the image cytometry assay, the cell pellet was gently and thoroughly re-suspended in the remaining 20 μL of media, and 20 μL was transferred to the disposable counting slide. Bright-field and fluorescent images of the sample were captured using the filter optics module VB-535-402 for MitoTracker green detection at an exposure time of 1 s with a size cut-off of 0.1 μm.

Statistical analysis

Standard statistical procedures were carried out using the Statistical Package for Social Sciences (SPSS) version 20.0. Normality of quantitative variables was revealed by Kolmogorov-Smirnov test. One-way analysis of variance (ANOVA) was used in comparing quantitative variables and Bonferroni's test was applied for post-hot test. The categorical variables were compared using the chi-square test. Data are presented as the mean ± the standard deviation (SD) of three biological replicates. Comparisons with a p value < 0.05 were considered significant.

Results

Basic characteristics of patients undergoing IVF cycles

The basic characteristics among the NOR, POR and POR/DHEA groups are presented in Table 1. A total of 131 women who underwent IVF treatment were enrolled, including 59 NORs and 72 PORs. Among the PORs, 34 women were treated with DHEA (POR/DHEA group) and 38 women were not (POR group). The mean age was significantly lower in the NOR group (35.9 years) than in the POR (39.4 years) and POR/DHEA groups (39.3 years). However, there were no significant differences among the three groups regarding body mass index or the percentage of primary infertility and secondary infertility. Infertility duration was significantly longer in the POR group (6.3 years) than in the NOR group (3.6 years). Furthermore, women in the POR/DHEA group had a higher percentage of multiple previous failed IVF cycles (≥ 3 times) than those in the NOR group (47.1% in the POR/DHEA group vs. 8.5% in the NOR group, p < 0.05).

Table 1

Basic characteristics of patients in the NOR, POR and POR/DHEA groups

Parameters	NOR (n=59)	POR (n=38)	POR/DHEA (n=34)
Age (years)	35.9 ± 3.9	39.4 ± 3.5a	39.3 ± 2.4a
Body mass index (kg/m2)	22.0 ± 3.6	21.1 ± 3.8	21.1 ± 2.0
Infertility duration (year)	3.6 ± 3.0	6.3 ± 5.2a	5.4 ± 3.9
Types of infertility n (%)
Primary infertility	22 (37.3)	19 (50.0)	16 (47.1)
Secondary infertility	37 (62.7)	19 (50.0)	18 (52.9)
Basal FSH (IU/l)	4.3 ± 1.8	7.1 ± 5.4a	6.4 ± 2.8a
Antral follicle counts (n)	10.7 ± 3.4	3.5 ± 1.4a	3.3 ± 1.1a
Anti-Müllerian hormone (ng/ml)	3.7 ± 2.0	1.0 ± 0.6a	1.0 ± 1.2a
Previous IVF failure n (%)
0	34 (57.6)	14 (36.8)	8 (23.5)a
1-2	20 (33.9)	14 (36.8)	10 (29.4)
≥ 3	5 (8.5)	10 (26.3)	16 (47.1)a

NOR: normal ovarian responder; POR: poor ovarian responder; DHEA: dehydroepiandrosterone; FSH: follicle stimulation hormone; IVF: in vitro fertilization

aSignificant difference compare with NOR group, p < 0.05.

As expected, the mean number of AFC and serum AMH levels were markedly higher in the NOR group than in the POR and POR/DHEA groups. Moreover, the mean FSH level was significantly lower in the NOR group than in the POR and POR/DHEA groups.

Cycle characteristics and pregnancy outcome of patients undergoing IVF cycles

The cycle characteristics and pregnancy outcome among the NOR, POR and POR/DHEA groups are shown in Table 2. There were no significant differences among the three groups in terms of stimulation duration and gonadotropin dose. However, the number of retrieved oocytes, metaphase II oocytes, top-quality embryos at day 3 and transferred embryos were significantly higher in the NOR group than those in the POR and POR/DHEA groups. Similarly, the clinical pregnancy rate, ongoing pregnancy rate and live birth rate were markedly greater in the NOR group than in the POR and POR/DHEA groups.

Table 2

Cycle characteristics and pregnancy outcome in the NOR, POR and POR/DHEA groups

Parameters	NOR (n=59)	POR (n=38)	POR/DHEA (n=34)
Stimulation duration (days)	11.0 ± 2.3	10.2 ± 2.2	10.6 ± 1.8
HMG/FSH dose (IU)	3152.1 ± 778.8	2967.5 ± 831.5	3097.0 ± 574.3
No. of oocytes retrieved (n)	9.5 ± 3.6	2.3 ± 1.2a	3.5 ± 2.0a
No. of metaphase II oocytes (n)	5.4 ± 2.6	1.1 ± 0.9a	2.2 ± 1.6a
No. of top-quality D3 embryos (n)	2.4 ± 1.8	0.3 ± 0.6a	1.2 ± 1.1a, b
No. of embryos transfer (n)	2.8 ± 0.8	1.1 ± 1.0a	2.1 ± 0.9a, b
Fertilization rate (%)	69.0	58.8	75.9b
Clinical pregnancy rate % (n)	55.1 (27/49)	5.2a (2/38)	18.7a (6/32)
Ongoing pregnancy rate % (n)	46.9 (23/49)	2.6a (1/38)	15.6a (5/32)
Live birth rate % (n)	43.7 (21/48)	2.6a (1/38)	12.9a (4/31)

NOR: normal ovarian responder; POR: poor ovarian responder; DHEA: dehydroepiandrosterone; HMG: human menopausal gonadotrophin; FSH: follicle stimulation hormone; D: day

aSignificant difference compare with NOR group, p < 0.05.

bSignificant difference compare with POR group, p < 0.05.

When comparing the POR/DHEA group with the POR group, the number of top-quality embryos at day 3 (1.2 ± 1.1 vs. 0.3 ± 0.6, respectively, p < 0.05), transferred embryos (2.1 ± 0.9 vs. 1.1 ± 1, respectively, p < 0.05) and fertilization rate (75.9% vs. 58.8%, respectively, p < 0.05) were significantly greater. Moreover, the POR/DHEA group was associated with a potentially greater number of retrieved oocytes (3.5 ± 2 vs. 2.3 ± 1.2, respectively) and metaphase II oocytes (2.2 ± 1.6 vs. 1.1 ± 0.9, respectively) compared with the POR group, but these differences were not significant. Similarly, the POR/DHEA group displayed higher clinical pregnancy rate (18.7% vs. 5.2%, respectively), ongoing pregnancy rate (15.6% vs. 2.6%, respectively) and live birth rate (12.9% vs. 2.6%, respectively) than the POR group. However, the difference was not statistical significant.

Effects of DHEA supplementation on cumulus-oocyte complex grade

As shown in Fig. 1A, DHEA supplementation ameliorated oocyte maturation and cumulus expansion. The CCs from the POR/DHEA group significantly increased proportion of grade 3 COC compared to those from the POR group (58.6% vs. 28.4%, respectively, p < 0.001) (Fig. 1B). In addition, the mean COC grade was significantly greater in the POR/DHEA group than that in the POR group (2.51 ± 0.64 vs. 1.97 ± 0.78, respectively, p < 0.001) (Fig. 1C).

Figure 1

DHEA supplementation ameliorated cumulus-oocyte complex grade in poor ovarian responders. (A) Representative cumulus-oocyte complexes (COCs) from different groups of normal ovarian responder (NOR), poor ovarian responder (POR) and POR/DHEA were shown. (B) The COC grade was assessed among the three groups. The proportion of COC grade in each group was shown. (C) The mean COC grade was compared among the three groups. Scale bar = 25 μm. Data represented the mean ± standard deviation. *** p < 0.001.

DHEA supplementation suppressed apoptosis in cumulus cells

The mRNA levels of BAX, BAD, caspase-3, caspase-9 and cytochrome c significantly decreased in the CCs from the POR/DHEA group compared with those from the POR group (Fig. 2A). Furthermore, BCL2 mRNA was greater in the CCs from the POR/DHEA group than those from the POR group (Fig. 2A). To further confirm the anti-apoptotic effect of DHEA, TUNEL staining was performed to directly assess the percentage of apoptotic cells in the presence or absence of DHEA in the PORs. The POR/DHEA group was associated with a significantly lower percentage of apoptotic cells when compared to the POR group (9.7% vs. 85.7%, respectively, p < 0.001) (Fig. 2B). Consistent with the results observed using Q-PCR, the addition of DHEA significantly reduced apoptosis of CCs.

Figure 2

DHEA supplementation reduced apoptosis of cumulus cells in poor ovarian responders. (A) Quantitative real-time polymerase chain reaction analysis for mRNA expression of apoptosis-related genes of cumulus cells (CCs) among the normal ovarian responder (NOR), poor ovarian responder (POR) and POR/DHEA groups. (B) Representative confocal microscopy images of DNA fragmentation in CCs were shown. DNA fragmentation, detected by terminal deoxynucleotidyl transferase dUTP nick end labeling, was depicted by green fluorescence, and all cell nuclei, stained with 4',6-diamidino-2-phenylindole (DAPI), were depicted by blue fluorescence. Quantitative analysis of apoptotic cells in CCs among the three groups was performed. Scare bar = 20 μm. Data represented the mean ± standard deviation of three independent experiments. * p < 0.05, *** p < 0.001; ns, non-significant.

Effects of DHEA supplementation on the mitochondria in cumulus cells

As shown in Fig. 3, compared to the CCs from the NOR group, the CCs from the POR group exhibited markedly lower expression of mitochondrial transcription factor A (TFAM) gene and reduced mitochondrial dehydrogenase activity. However, DHEA supplementation significantly increased the TFAM gene expression and enhanced mitochondrial dehydrogenase activity in CCs from the POR (Fig. 3A and 3B). To further assess whether supplementation with DHEA was sufficient to improve mitochondrial function, we analyzed the mitochondrial mass using real-time image cytometry. By visualizing the mitochondria with fluorescent MitoTracker green, lower mitochondrial mass was observed in the CCs from the POR group than those from the NOR group. However, mitochondrial mass in CCs from the POR remarkably increased following DHEA supplementation (Fig. 3C).

Figure 3

DHEA supplementation improved mitochondrial function of cumulus cells in poor ovarian responders. (A) Quantitative real-time polymerase chain reaction analysis for mRNA expression of TFAM gene of cumulus cells (CCs) among the normal ovarian responder (NOR), poor ovarian responder (POR) and POR/DHEA groups. (B) Mitochondrial dehydrogenase activity was assessed among the three groups. (C) CCs were stained with MitoTracker green, and the mitochondrial mass was measured by real-time image cytometry. The relative mean of fluorescent intensity (MFI) was calculated among the three groups. Data represented the mean ± standard deviation of three independent experiments. * p < 0.05, ** p < 0.01, *** p < 0.001.

Discussion

This prospective cohort study demonstrated that PORs following DHEA supplementation significantly improved the proportion of grade 3 COC and mean COC grade and markedly increased the number of top-quality embryos at day 3, transferred embryos and fertilization rate compared to PORs without DHEA supplementation. Additionally, PORs with DHEA pretreatment displayed a tendency of higher clinical pregnancy rate, ongoing pregnancy rate and live birth rate than PORs without DHEA pretreatment. These results supported the beneficial effects of DHEA on IVF outcomes in the previous studies 7, 8. A total of three meta-analyses have revealed that pretreatment with DHEA was associated with increased pregnancy rates or live birth rates in PORs undergoing IVF cycles 11, 32, 33. Moreover, an updated randomized controlled trial demonstrated that supplementation with DHEA in PORs significantly increased the number of retrieved oocytes, fertilized oocytes, high-quality embryos, fertilization rate and pregnancy rates 34. Therefore, DHEA, widely used as an adjuvant to IVF cycles in PORs worldwide, has been regarded as a potential intervention to improve reproductive outcomes in PORs. However, more large-scale, well-designed randomized controlled trials are needed to verify the results.

In the current study, supplementation with DHEA significantly decreased expressions of the pro-apoptotic genes (BAX, BAD) and caspase activation (cytochrome c, caspase-9 and caspase-3) and markedly increased expression of the anti-apoptotic gene (BCL2) in CCs (Fig. 2A). However, in our previous study, both BAX and BCL2 genes expressions in CCs were declined after DHEA supplementation 17. One possible explanation for the different gene expression of BCL2 was that BAX gene expression in CCs was severely suppressed and down to nearly zero after DHEA supplementation in our previous study 17, which might induce compensatory mechanisms to inhibit anti-apoptosis, resulting in decreased gene expression of BCL2 because apoptosis is important for normal ovarian physiology 19. Furthermore, a significantly lower percentage of apoptotic cells were observed in the CCs from the POR/DHEA group than those form the POR group (Fig. 2B). These results suggested the anti-apoptotic effect of DHEA on the CCs and several studies using cell culture also supported that DHEA could defend against apoptosis 35-38. The study conducted by Alexaki et al. exhibited a protective effect of DHEA in human keratinocytes against apoptosis through altered balance of BCL2 proteins 35. In the study of Liu et al., DHEA protected vascular endothelial cells against apoptosis by activating the Galphai-PI3K/Akt pathway and regulating antiapoptotic BCL2 expression 36. Furthermore, Ding et al. demonstrated that DHEA inhibited H2O2-induced apoptosis in the Leydig cells through activation of PI3K/Akt signaling pathways 38.

In fact, numerous studies have showed that the apoptosis of CCs was involved in oocyte maturity, fertilization, embryo development and pregnancy outcome 20-23. Host et al. observed that apoptosis in CCs was highly correlated with retarded nuclear development or atresia of the oocyte, which impaired the maturity and fertilization of the oocyte 20. The study conducted by Corn et al. demonstrated that a high degree of apoptosis in CCs impaired blastocyst development and quality 21. In the study of Lee et al., the incidence of CCs apoptosis was negatively associated with the number of retrieved oocytes, the embryo grade, and the pregnancy outcomes in the IVF cycles 22. In addition, Diaz-Fontdevila et al. demonstrated that patients with lower apoptotic rates in CCs had higher good-quality embryos and a tendency of higher pregnancy rates 23.

The present study showed that the expression of TFAM gene, mitochondrial dehydrogenase activity and mitochondrial mass were higher in the CCs from the POR/DHEA group than those from the POR group. TFAM is an essential protein that binds mitochondrial DNA (mtDNA) to regulate mitochondrial transcription initiation and is also a key regulator of mtDNA copy number 39. The abundance of mtDNA generally reflects TFAM levels 39. The results suggested that DHEA supplementation had the positive effects on the mitochondrial function in CCs; several studies using cell culture or an animal model also supported the beneficial effects of DHEA treatment on the mitochondrial function 35, 38, 40, 41. In a study using human keratinocytes, DHEA reversed serum deprivation-induced reduction of mitochondrial membrane potential to basal levels and conserved mitochondrial membrane integrity 35. Furthermore, DHEA significantly increased the activities of superoxide dismutase, catalase and peroxidase, and decreased the loss of mitochondrial membrane potential and the level of reactive oxygen species in the Leydig cells 38. Patel et al. indicated that DHEA treatment can improve oxidative energy metabolism by promoting ATPase activity and mitochondrial dehydrogenases activities in the mitochondria of rats 40, 41.

Mitochondria in oocytes or CCs participated in oocyte maturation, fertilization, embryo development and pregnancy outcomes 26, 42-44. Increased abnormal mitochondrial structure and decreased expression of mitochondrial genes were observed in human unfertilized oocytes 45, 46. The mtDNA content in oocytes was pivotal to fertilization and served as a predictor for oocyte quality 26, 27. Moreover, Boucret et al. concluded that mitochondrial biogenesis of the CCs may be a major determinant of oocyte competence 42. The study conducted by Ogino et al. demonstrated that mtDNA copy number in CCs can be used to predict embryo quality 43. In the study of Tsai et al., the mitochondria DNA 4977-bp deletion in CCs was negatively correlated with pregnancy rate during IVF cycles 44.

Taken together, DHEA treatment may ameliorate IVF outcomes partially though improving mitochondrial function and reducing apoptosis in CCs. The results of this study confirmed and strengthened the conclusions of our previous work 18 by stricter study design and further experiments. However, there were still some limitations in this study. First, the population size remained small. Thus, clinical pregnancy rate, ongoing pregnancy rate and live birth rate potentially increased following DHEA supplementation in PORs. However, the difference did not reach statistical significance. Second, this study was not a randomized controlled trial. Further randomized controlled trials are required to clarify the effect of DHEA treatment. Third, the participants enrolled based on Bologna criteria might be heterogeneous.

In conclusion, the benefits of DHEA supplementation on IVF outcomes in PORs were significant, and the DHEA effects may be partially mediated by improving mitochondrial function and reducing apoptosis of CCs. Our observations may provide a reasonable rationale for clinical uses of DHEA supplementation in PORs undergoing IVF cycles to improve clinical outcomes.

Supplemental Table S1.

Click here for additional data file.