Low expression of SEMA6C accelerates the primordial follicle activation in the neonatal mouse ovary

Abstract The primordial follicle assembly, activation and the subsequent development are critical processes for female reproduction. A limited number of primordial follicles are activated to enter the growing follicle pool each wave, and the primordial follicle pool progressively diminishes over a woman's life‐time. The number of remaining primordial follicles represents the ovarian reserve. Identification and functional investigation of the factors involved in follicular initial recruitment will be of great significance to the understanding of the female reproduction process and ovarian ageing. In this study, we aimed to study whether and how semaphorin 6C (Sema6c) regulated the primordial follicle activation in the neonatal mouse ovary. The attenuation of SEMA6C expression by SiRNA accelerated the primordial follicle activation in the in vitro ovary culture system. PI3K‐AKT‐rpS6 pathway was activated when SEMA6C expression was down‐regulated. And the LY294002 could reverse the effect of low SEMA6C expression on primordial follicle activation. Our findings revealed that Sema6c was involved in the activation of primordial follicles, and the down‐regulation of SEMA6C led to massive primordial follicle activation by interacting with the PI3K‐AKT‐rpS6 pathway, which might also provide valuable information for understanding premature ovarian failure and ovarian ageing.


Introduction
Once the primordial follicles are activated, these follicles are destined either to undergo atresia or to ovulate. Under physiological conditions, every cycle only a limited number of primordial follicles are activated to step into the growing follicle pool [1]. The female reproductive capability and ovarian lifespan are determined by the regulation of primordial follicle initial recruitment [2]. With the female ageing, the primordial follicle number declines, the size of small antral follicles decreases, and the oocyte quality deteriorates. The factors that regulate the activation of the primordial follicle are of great importance for female fertility as well as for ovarian ageing.
Under physiological conditions, some primordial follicles remain dormant, while others enter the growth phase. The activation of primordial follicles is a process of precise regulation. Numerous growth factors, cytokines and bidirectional signalling between oocytes and granulosa cells are important and necessary to this process [3][4][5][6]. Recent studies using genetically modified mouse models have revealed that the PTEN/PI3K/AKT/FOXO3A and TSC/mTOR1 signalling pathways are important for the regulation of primordial follicle activation [7][8][9][10][11][12][13].
Besides, another recent study demonstrated that Lhx8 regulates postnatal folliculogenesis and primordial follicle activation through interaction with PI3K-AKT pathway via regulating Lin28a expression. Conditional depletion of Lhx8 by Gdf9-Cre could lead to massive primordial follicle activation [14]. A recent study also revealed the role of LKB1 as an indispensable gatekeeper for the primordial follicle pool through elevated mTOR signalling by an AKT-independent LKB1-AMPK pathway [15]. Expression change of anyone of the above-mentioned key genes may lead to different fate of the primordial follicle pool and reproductive productivity. Excessive activation of primordial follicles or cell death may lead to premature ovarian failure. However, the mechanisms by which some primordial follicles are activated, while others stay in a quiescent state are little known up to now.
Semaphorins were initially described in the nervous system based on their role in repulsive axon guidance, but now they act as crucial regulators of homeostasis and morphogenesis on more organ systems [16,17]. The structures of semaphorins are well conserved in rodents and human. The diverse characteristics of semaphorin signalling and its implication in disease have attracted great attention on the study of biological effects of semaphorins [16][17][18]. Nowadays, more studies about semaphorins are performed in cancer, immune system, vascular system and organogenesis et al. [17,[19][20][21][22]. Several studies have demonstrated that semaphorin family participates in the regulation of follicle development. Sema-4D/Plexin-B1 system could influence the follicular growth as well as the steroidogenesis [23]. Semaphorins (Sema3a, Sema6a and Sema6d), as cell-to-cell communication genes, play an important role in the maturation of the oocyte cumulus complex [24]. SEMA3A is up-regulated in the GnRHa-triggered follicle compared with that in the hCG-triggered follicle, which suggests an impaired induction of angiogenesis in the GnRHa-triggered MGC (mural granulosa cells) as compared with the hCG-triggered MGC [25]. SEMA6C, a member of the semaphorin family, has been demonstrated to interact with PLEXIN A1, which can regulate the axon repulsion and has growth cone collapsing activity [21,22]. This study aimed to explore the role of Sema6c in the process of primordial follicle activation and its signalling regulation in the neonatal mouse ovary.

Animals
Healthy C57BL/6J female mice were purchased from the Center for Laboratory Animal Administration of the Center for Disease Control and Prevention of Hubei Province (Wuhan, China). They were bred with free access to food and water under a light/dark cycle (12 hrs/12 hrs) at the Center for Laboratory Animal Administration of Tongji Medical College, Huazhong University of Science and Technology (Wuhan). The 6-to 8-week-old female mice were mated with adult male mice in specific pathogen-free conditions. The 3-dayold neonatal mouse ovaries were used for the experiment. All these mice received humane care according to the Guide for the Care and Use of Laboratory Animals of the Chinese Academy of Sciences.

Immunohistochemistry
The ovaries of the neonatal mice (Day 3, Day 5 and Day 7) were fixed in 4% paraformaldehyde for 24 hrs, transferred to a graded series of ethanol to dehydrate, embedded in paraffin and serially sectioned (5 lm). The ovary sections were processed for immunohistochemical analysis using routine immunohistochemistry procedures. The antigen was retrieved by citric acid buffer (PH 6.0) microwave antigen retrieval method. The citric acid buffer was heated to boiling in a microwave oven (M1-L213B; Midea, Guangdong, China); tissue sections after dewaxing and hydration were placed into the boiling buffer; and then, the sections were heated in the microwave oven as following: medium fire (600 Watts) 8 min., ceasefire 8 min., low fire (500 Watts) 7 min. The ovary sections were incubated with anti-SEMA6C primary antibody (AF2108, 1:100, 2 lg/ml; R&D Systems, Minneapolis, MN, USA) overnight at 4°C. The next day, the ovary sections were incubated with a secondary antibody (HRP-labelled rabbit Anti-goat IgG (H + L), Servicebio, GB23204, 1:200) for 50 min. at 37°C. Subsequently the ovary sections were visualized with DAB-HRP chromogenic agent (K5007; DAKO, Glostrup, DK) at room temperature for 20 sec. As the negative control, normal goat IgG (BA1044, 2 lg/ml; BOSTER, Wuhan, China) instead of the primary antibodies was used to treat the sections. Microscopy was performed using microscope (version 1.8.1; Olympus, Japan), and the images were acquired with the cellSens Dimension software (version 1.8.1, Olympus, Japan).

In vitro ovary culture
On postnatal Day 3, the female mice were killed by decapitation. Ovaries were removed, and then, the oviduct and excess tissue were trimmed under the stereomicroscope. The ovaries were placed on a piece of Millicell-CM filter membrane (Millipore, Billerica, MA, USA) floating in 400 ll of alpha-modified Eagle's medium (Invitrogen, Carlsbad, CA, USA) containing 1 mg/ml Albumax (Invitrogen), 1 mg/ml BSA (Sigma-Aldrich, St. Louis, MO, USA), 50 lg/ml L-ascorbic acid (Sigma-Aldrich), 0.23 mmol/l Na pyruvate (Sigma-Aldrich), ITS (1.0 mg/ml insulin, 0.55 mg/ml human transferrin and 0.5 lg/ml sodium selenite) (Sigma-Aldrich), 5 U/ml penicillin and 5 lg/ml streptomycin, as the study described before [26]. The culture medium was changed every other day together with the intervention factor.

SiRNA transfection
Cultured ovaries were treated with 2 lM/4 lM cholesterol-conjugated negative control SiRNA (NC-SiRNA) (Ribobio, China, NControl_05815, siN05815122147) or cholesterol-conjugated Si-Sema6c RNA (Si-Sema6c-Chol) (Ribobio, China, siG0931383544) for 48 hrs to determine the optimal intervention concentration. Follow-up experiments were conducted with the best intervention concentration for 4 days. The SiRNA sequences used for silencing Sema6c (Gene ID: 20360) were designed and synthesized by Guangzhou Ribobio company (Ribobio, China). The sequences of Si-Sema6c-RNAs were as follows: 5 0 CCAGUGAUGCUGUAGUUUA dTdT 3 0 , 3 0 dTdT GGUCACUACGACAUCAAAU 5 0 . The SiRNAs were cholesterolconjugated and Cy3-labelled to better enter the cells and be observed conveniently. The cholesterol-conjugated SiRNA has been demonstrated effective to down-regulate the gene expression. The PI3K-specific inhibitor LY294002 purchased from Selleckchem (S1105; Selleckchem, Houston, TX, USA) was added to the 48 hrs transfected ovary for another 48 hrs. The concentration of LY294002 added to the medium was 20 lM.

Fluorescence microscopy
To determine whether the Si-Sema6c-Chol could enter the ovary, the transfected ovaries were placed under the fluorescence microscope to observe the CY3 fluorescence after 48-hrs transfection. Images were photographed using the program cellSens Dimension by fluorescence microscope (version 1.8.1, Olympus, Japan).

Histology and immunofluorescence analysis
Ovaries, following 4 days of in vitro culture, were fixed in 4% paraformaldehyde and then dehydrated, embedded in paraffin and serially sectioned 5 lm per section. Two of the largest cross sections were stained with  haematoxylin and eosin (HE). The MVH (mouse vasa homolog) is specifically expressed in the germ cell lineage [27,28] and could be used as a germ cell-specific marker to label the oocytes of all stage follicles in the mouse ovaries [29]. Zona pellucida glycoprotein 3 (ZP3) is expressed specific in the growing follicles when the primordial follicles are activated [30]. Therefore, ZP3 antibody (H-300) (sc-25802; Santa Cruz Biotechnology, Santa Cruz, CA, USA) was also used for immunofluorescence to count growing follicles more accurately. The sections right adjacent to the above sections chosen for HE staining were used for immunofluorescence analysis as the routine procedures. Sections were incubated with MVH antibody (ab13840, 1:200; Abcam, Cambridge, MA, USA) and ZP3 antibody (H-300) (sc-25802, 1:100; Santa Cruz) overnight at 4°C. The next day, the ovary sections were incubated with secondary antibodies (Alexa Fluo â 594 donkey anti-rabbit IgG (H + L), AntGene, ANT030, 1:200; Alexa Fluo â 488 donkey anti-rabbit IgG (H + L), AntGene, ANT024. 1:200) for 60 min. at 37°C. As the negative control, normal rabbit IgG was used here instead of primary antibody. Microscopy was performed using microscope (version 1.8.1, Olympus), and the images were acquired with the cellSens Dimension software. The immunofluorescence result was quantified via counting the follicle with MVH-positive staining and ZP3-positive staining.

Morphological analysis and follicle counting
Primordial follicles and growing follicles are counted in this study. Identification of follicle types was categorized in accordance with the protocol of previous studies [31,32]. Growing follicles are follicles which have been activated. Morphologically, they are characterized by oocyte diameter greater than 20 lm and transition of the flat epithelial layer to cuboidal granulosa cells. While the primordial follicles are composed of small oocytes (< 20 lm) and flat granulosa cells, the numbers of follicles at each developmental stage were counted and averaged in two largest cross serial sections of the ovary centre with HE staining [26,31]. Meanwhile, to further identify the different stage follicles, the adjacent ovarian sections were labelled with ZP3 and MVH. For each ovary, we used the above two methods to determine its follicle number. Three individual persons counted the follicles in this study. The oocyte diameter was measured by ImageJ software program (a free software developed by contributors worldwide).

Quantitative real-time PCR
After the ovaries were cultured for 48 hrs, the blocking effect of Si-Sema6c-Chol was detected using quantitative real-time PCR. While the rest ovaries were harvested after 4 days culture to detect the mRNA expression of Gdf9 (growth differentiation factor 9), Zp1 (zona pellucida glycoprotein 1), Zp2 (zona pellucida glycoprotein 2) and Zp3 (zona pellucida glycoprotein 3), primer sequences of Sema6c were designed by https://www.ncbi.nlm.nih.gov/tools/primer-blast/. Primer sequences of Gapdh, Gdf9, Zp1, Zp2 and Zp3 were obtained from Primer Bank. All the primer sequences of the above genes are listed in Table 1.
Statistical analysis SPSS 18.0 software program (IBM, NY, USA) was used for statistical analysis and data comparison. To evaluate the statistical significance of differences between different groups, unpaired Student t-tests were applied in our study. All the experiments were repeated three times or more. The average standard error of the mean (S.E.M.) is presented in the results. P < 0.05 was defined as statistically significant.

Results
The expression of SEMA6C in the neonatal mouse ovaries To evaluate the SEMA6C protein expression in mouse ovaries, we first performed immunohistochemistry analyses with neonatal mouse Table 1 The sequences of primers used for quantitative real-time PCR

Genes
Primers Forward Primer TTCCAGGCCAGTGATGCTGTAG ovaries. The ovaries of D3 (Day 3) female mice contained mainly primordial follicles (Fig. 1A_a-d). In the ovaries of D5 (Day 5) mice, some primary follicles began to form (Fig. 1A_e-h) and follicles further developed on Day 7, and more primary follicles and secondary follicles came into being (Fig. 1A_i-l) as that we previously reported [26]. The follicles were classified as follows: an oocyte surrounded by flattened pre-granulosa cells was regarded as a primordial follicle; the growing follicle consists of an enlarged oocyte and one layer or more cuboidal granulosa cells. The immunohistochemistry results revealed that SEMA6C protein was mainly expressed in the cytoplasm of oocytes in the neonatal mouse ovary, whereas the granulosa cells and interstitial cells exhibited relatively weaker staining (Fig. 1A). However, in different primordial follicles, the intensity of SEMA6C protein expression was not the same, as the red arrows show two primordial follicles in Figure 1A_d. The Western blot results showed that SEMA6C expression decreased on Day 7 compared with Day 3, Day 5 (*P < 0.05), whereas there was no significant difference in the SEMA6C expression between Day 3 and Day 5 ovaries (Fig. 1B-C).
The attenuation of SEMA6C promoted the primordial follicle activation Cholesterol-conjugated SiRNA can be used to inhibit gene expression in the small tissue culture system, as the cell absorption of SiRNA is promoted and the half-life of SiRNA is extended. Therefore, cholesterol-conjugated Si-Sema6c RNA (Si-Sema6c-Chol) was applied in this study to down-regulate SEMA6C expression. To test whether the Si-Sema6c-Chol could well transfuse into the neonatal ovaries, we used CY3-labelled-Si-Sema6c-Chol in the culture system. After 48hrs culture, the strong red fluorescence (CY3 labelling) could be easily observed by fluorescence microscope and red fluorescence at the concentration of 4 lM was significantly stronger than that of 2 lM (Fig. 2A). And after 48 hrs culture, the Sema6c mRNA levels showed accordant result: the Sema6c mRNA expression at the concentration of 4 lM was better blocked (68.3 AE 4.2%) than that of 2 lM (18.2 AE 3.4%) (Fig. 2B). Meanwhile, the SEMA6C protein expression could be strongly inhibited, decreased more than 50% compared to the Con group (*P < 0.05) (Fig. 2C,D), as the Western blotting results showed at the concentration of 4 lM. So, we used 4 lM Si-Sema6c-Chol to carry on the following experiments.
To investigate the function of Seme6c in early follicle development, 3-day-old neonatal mouse ovaries were cultured with 4 lM Sinegative-control (Si-NC) or 4 lM Si-Sema6c-Chol for 4 days. During the 4 days in vitro culture, the morphology of cultured ovaries was observed and photographed under the microscope every day. The ovaries in all the groups appeared healthy, without dark regions (Fig. 3A). After the 4-day culture, ovaries were harvested for paraffin sections. To determine the effect of low SEMA6C expression on the activation of primordial follicles, the above-mentioned methods were used to count the follicles in different stages. Two largest cross section consecutive sections were stained with haematoxylin and eosin (Fig. 3B); meanwhile, the adjacent sections were separately labelled with MVH and ZP3 (Fig. 3C,D). The follicle counting results according   to the above two methods are shown in Figure 3E.  (Fig. 3E). The two different methods for follicle counting showed no significant difference (P > 0.05). To evaluate the oocyte growth, we measured the oocyte diameters of different stage follicles by ImageJ in the above HE-stained sections. The mean oocyte diameter was significantly greater in the Si-Sema6c group than that in the Con group (primordial follicles: 11.53 AE 1.81 lm and 10.03 AE 1.75 lm, respectively (**P < 0.01); growing follicles: 29.78 AE 3.83 lm and 26.95 AE 4.10 lm, respectively) (**P < 0.01) (Fig. 3F). The mRNA expressions levels of Gdf9, Zp1, Zp2 and Zp3 genes, which were involved in primordial follicle activation and oocyte growth, were evaluated by quantitative real-time PCR, and they were all up-regulated in Si-Sema6c group. The mRNA expressions of Gdf9, Zp1, Zp2 and Zp3 in Si-Sema6c group were 1.50-, 1.63-, 1.46-, 1.47fold of the Con group, respectively. (*P < 0.05) (Fig. 3G).

The molecular mechanisms underlying the accelerated primordial follicle activation in Si-Sema6c-treated ovaries
The initial recruitment of follicles was regulated by multiple signalling pathways, and PI3K-AKT signal pathway has been proved to have interaction with semaphorin family members [16,17,33,34]. SEMA6C signal pathway has been demonstrated that it regulates the primordial follicle activation. Therefore, ovaries transfected with Si-Sema6c were also treated with LY294002, the inhibitor of PI3K-AKT pathway to investigate the molecular mechanisms regulating the accelerated primordial follicle activation with SEMA6C down-regulated. LY294002 (20 lM) was added into the culture media of the ovaries after 48 hrs treated with Si-Sema6c. The cultured ovaries were harvested for morphological and molecular analyses as above described after another 48 hrs. The ovary sections were stained with HE (haematoxylin-eosin) (Fig. 4A-C). The number of growing follicles of the Si-Sema6c-LY294002 group relatively decreased compared with that of the Si-Sema6c group without LY294002 treated and showed similar morphology with the Con group ( Fig. 4A-C). Then, we further evaluated the number of follicles in different stages using the above-mentioned methods (HE staining and MVH/ZP3 labelling). Figure 4D shows the number of follicles counted according to HE staining. The number of primordial follicles in Si-Sema6c-LY294002-treated ovaries (82.92 AE 21.32/section) was significantly increased compared with Si-Sema6c-treated ovaries (62.79.5 AE 17.17 (*P < 0.05), while closed to the Con ovaries (89.73 AE 27.15) (P > 0.05). The numbers of growing follicles in the three groups (Con, Si-Sema6c, Si-Sema6c-LY294002) were 28.55 AE 3.58, 40.18 AE 11.41, 24.67 AE 5.82 respectively, and the growing follicle number of Si-Sema6c group significantly increased compared with the other two groups (*P < 0.05). Moreover, numbers of total follicles of the three groups were 118.27 AE 29.00, 102.96 AE 19.07, 107.58 AE 21.53 respectively (P > 0.05) (Fig. 4D). The Figure 4E shows the number of follicles counted according to MVH/ZP3 labelling. The number of follicles in the Con, Si-Sema6c, Si-Sema6c-LY294002 groups was as follows: primordial follicles ( (Fig. 4E). This follicle counting results showed no significant differences compared with the HE-staining methods (P > 0.05).
To further understand the mechanism of Sema6c effect on primordial follicle activation, Western blot analyses were carried out to detect the AKT and rpS6 protein expression levels and the phosphorylated forms of them. Figure 4F shows the levels of AKT, p-AKT (S473), rpS6, p-rpS6 (S235/236) by Western blot analyses. Quantification of Western blotting indicated an enhanced phosphorylation of AKT at Ser473 and rpS6 at Ser235/236 in Si-Sema6c group compared with the Con group (2.5-fold AE 0.3-fold, 3.3-fold AE 0.4-fold, respectively) (**P < 0.01, n = 3 independent blots) (Fig. 4G). LY294002 reversed the increased phosphorylation of AKT and rpS6 caused by the Si-Sema6c (**P < 0.01). Thus, SEMA6C suppression induced by Fig. 3 The attenuation of SEMA6C signalling activated early primordial follicle growth. (A) ovaries were cultured at the concentration of 4 lM Si-Sema6c-Chol; the morphology of the cultured ovaries was observed under a stereomicroscope during the 4 days of culture. After 4 days of culture, the ovaries in both groups appeared healthy under the stereomicroscope, without obviously dark internal areas. B-D, HE staining (B) of ovaries cultured in vitro for 4 days. To identify oocytes and growing follicles more clearly, ovarian sections were immunofluorescence labelled with MVH (C) and oocyte-derived ZP3 (D). (E) The numbers of primordial, growing and total follicles were determined according to HE staining and MVH/ZP3 labelling. In the Si-Sema6c group, the number of primordial follicles was significantly reduced (*P < 0.05), and the number of growing follicles increased compared with the control group (*P < 0.05). No significant difference was observed in the total number of follicles (P > 0.05), although a slight reduction was observed in the Si-Sema6c group. (F) mean diameters of oocytes in Con and Si-Sema6c groups. The mean oocyte diameters of primordial follicles were 10.03 AE 1.75 lm in Con group and 11.53 AE 1.81 lm in Si-Sema6c group (**P < 0.01); the mean oocyte diameters of growing follicles in the Si-Sema6c group (29.78 AE 3.83 lm) were significantly greater compared with the Con group (26.95 AE 4.10 lm) (**P < 0.01). (G) The relative mRNA expressions of Gdf9, Zp1, Zp2 and Zp3 in the Si-Sema6c group were significantly higher than those of the Con group (*P < 0.05). The data presented in panels (E-G) correspond to mean AE S.E.M. from three independent experiments.   Si-Sema6c resulted in increased PI3K pathway activation, while LY294002 reversed the activation of PI3K pathway.

Discussion
The initial recruitment of the primordial follicle is a gonadotropinindependent process regulated by intrinsic ovarian growth factors [6]. Dynamic homeostasis present between these inhibitory and stimulatory factors is quite important to guarantee the number of primordial follicles each wave. Recently, several studies have demonstrated that several key factors could affect the initial recruitment process through multiple signalling pathways [10,35,36], and the exact mechanism by which primordial follicles are activated and recruited into the growing pool is still less clear and need to be further explored.
The current study indicated that SEMA6C signalling was involved in the regulation of early primordial follicle dormancy/activation. Low expression of SEMA6C accelerated the primordial follicle activation process in the neonatal mouse ovary through PI3K-AKT-rpS6 signalling pathway.
The semaphorin family is a group of proteins that regulate axonal growth cone guidance and cell migration. These proteins could either promote or inhibit cell growth in different cases. Up to now, the researches of semaphorins in the female reproductive system are still relatively few. It is reported that SEMA4D and its receptor PLEXIN-B1 participate in the mouse ovary follicular development [23]. The gene expression profile of human cumulus-oocyte complex demonstrated that semaphorins (SEMA3A, SEMA6A and SEMA6D) significantly overexpressed in cumulus cells relative to oocytes [24]. Semaphorin 3B, semaphorin 3F and semaphorin 4D are all demonstrated to be involved in ovarian cancer and associated with ovarian function [37,38]. We found that the expression level of SEMA6C protein in ovaries sharply decreased between D5 and Day 7 after birth, which is the first time when primordial follicle activation begun. This result suggested the potential role of SEMA6C in the maintenance of primordial follicle quiescence and regulation of primordial follicle activation. Low expression of SEMA6C may accelerate the activation of primordial follicles.
SEMA6C expression of neonatal mouse ovaries was down-regulated by SiRNA in the in vitro culture system to explore the role of SEMA6C in primordial follicle activation, because physiologically the primordial follicle activation was accompanied with the decreased expression of SEMA6C. We found that down-regulation of SEMA6C of neonatal mouse ovaries resulted in a markedly decrease in the primordial follicles' number and an increase in the growing follicles' number and also promoted the oocyte growth. The expression levels of Gdf9, Zp1, Zp2 and Zp3 were significantly increased in Si-Sema6c treated ovaries, which demonstrated the overactivation of primordial follicles. All these results suggested that down-regulation of SEMA6C accelerated primordial follicle activation and indicated that SEMA6C may act as a suppressor for primordial follicle activation. Down-regulation of SEMA6C led to a slight reduction in the total follicle number; however, it was not statistically significant. We assume this slight reduction can be probably due to the inter ovary variability and can also be attributed to the death of primordial follicles. However, in which way SEMA6C affects primordial follicle survival needs further study.
Previous studies have shown that PTEN/PI3K/AKT signalling is involved in follicle survival and primordial follicle activation [10,12,39,40]. The phosphorylation of S6K1/rpS6 in oocytes is essential for the oocyte growth. PTEN could inhibit the phosphorylation of S6K1/ rpS6 so as to keep the quiescence of primordial follicles [41]. More studies demonstrated that enhanced phosphorylation of S6K1/rpS6 signalling by TSC/mTOR could promote the follicular activation [7,42]. Disorders of these signalling pathways can lead to accelerated primordial follicle activation and premature ovarian failure (POF). The above signal pathways play important roles in cell growth and proliferation. In the present study, we explored whether and how the Sema6c interacted with them.
Several studies have demonstrated that semaphorins participate in the regulation of PI3K signal pathway. Up-regulation of SEMA3A leads to a marked decrease in AKT phosphorylation, indicating the PI3K activity was decreased [33]. SEMA4D/PLEXIN-B1 inactivates PI3K and dephosphorylates GSK-3b and AKT through R-Ras GAP activity [34]. Semaphorins have been demonstrated to be able to regulate the PI3K/AKT pathway in the previous study [16,17,43]. The effect of SEMA6C on endogenous AKT activity, a downstream target of PI3K, was examined in the ovary culture system. We found that SEMA6C suppression caused a marked increase in phosphorylation of AKT and rpS6. The S6K1-rpS6, a downstream signalling of PTEN/ PI3K/AKT and TSC/mTORC1, is also known to be involved in follicular dormancy and activation [41,42]. Treatment with LY294002 in Si-Sema6c-treated ovaries could reverse the accelerated primordial follicle activation, which indicated that SEMA6C may act on the upstream of PI3K and regulate the phosphorylation of AKT as well as the rpS6, Fig. 4 Effect of Si-Sema6c on the PI3K-AKT-rpS6 signal pathway. (A-C), the morphology of ovaries treated by NC-SiRNA, Si-Sema6c or Si-Sema6c with LY294002 after 4 days of culture. (D,E) The numbers of primordial follicles and growing follicles were determined according to HE staining and MVH/ZP3 labelling. In the Si-Sema6c group, the number of primordial follicles decreased and the number of growing follicles significantly increased (*P < 0.05). But when we added LY294002, the number of primordial follicles increased and the number of growing follicles significantly decreased compared with the Si-Sema6c group (*P < 0.05). The Si-Sema6c-LY294002 group showed similar follicle number with the Con group (P > 0.05). The two methods (HE staining versus MVH/ZP3 labelling) showed no significant difference (P > 0.05). (F) The levels of AKT, p-AKT (S473), rpS6, p-rpS6 (S235/236) were examined by Western blot analyses. (G) Quantification of Western blotting indicated an enhanced phosphorylation of AKT at Ser473 and rpS6 at Ser235/236 in Si-Sema6c group compared with the Con group (**P < 0.01). LY294002 reversed the increased phosphorylation of AKT and rpS6 caused by the Si-Sema6c (**P < 0.01). The data presented at panels (D, E, G) correspond to mean AE S.E.M. from three independent experiments. but the exact mechanism that how SEMA6C interacts with PI3K/AKT/ rpS6 pathway needs to be explored further. Our study is innovative to expound SEMA6C affects primordial follicle activation by regulating the PI3K/AKT/rpS6 pathway.
In summary, we found that low SEMA6C expression could promote primordial follicle activation in the neonatal mouse ovaries by activating the PI3K-AKT-rpS6 signalling pathway. We could speculate that relatively high expression of SEMA6C may help to keep the primordial follicle dormancy so as to control exhausting rate of primordial follicle pool and extend the reproductive lifespan in mammals. It should be noted that the limitation of this study is that we only examined the effect of low SEMA6C expression on primordial follicle activation. We did not investigate the effect of SEMA6C overexpression in mouse ovaries, as SEMA6C protein was strongly expressed in the 3day-old mouse ovaries. More work will be carried out on this subject in further research.