Abstract
Previously, we found that the silencing of growth arrest-specific gene 6 (Gas6) expression in oocytes impairs cytoplasmic maturation through mitochondrial overactivation with concurrent failure of pronuclear formation after fertilization. In this study, we report that Gas6 regulates mitophagy and safeguards mitochondrial activity by regulating mitophagy-related genes essential to the complete competency of oocytes. Based on RNA-Seq and RT-PCR analysis, in Gas6-silenced MII oocytes, expressions of mitophagy-related genes were decreased in Gas6-silenced MII oocytes, while mitochondrial proteins and Ptpn11, the downstream target of Gas6, was increased. Interestingly, GAS6 depletion induced remarkable MTOR activation. Gas6-depleted MII oocytes exhibited mitochondrial accumulation and aggregation caused by mitophagy inhibition. Gas6-depleted MII oocytes had a markedly lower mtDNA copy number. Rapamycin treatment rescued mitophagy, blocked the increase in MTOR and phosphorylated-MTOR, and increased the mitophagy-related gene expression in Gas6-depleted MII oocytes. After treatment with Mdivi-1, a mitochondrial division/mitophagy inhibitor, all oocytes matured and these MII oocytes showed mitochondrial accumulation but reduced Gas6 expression and failure of fertilization, showing phenomena very similar to the direct targeting of Gas6 by RNAi. Taken together, we conclude that the Gas6 signaling plays a crucial role in control of oocytes cytoplasmic maturation by modulating the dynamics and activity of oocyte mitochondria.
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Introduction
Growth arrest-specific gene 6 (GAS6) is a ligand of receptor tyrosine kinases of the TAM (Tyro3, Axl, and Mertk) receptors, and its role as a potential therapeutic target in human cancer has been recently emphasized1. The expression of Gas6 is widespread in many tissues and cells, including immune cells, endothelial cells, vascular smooth muscle cells, bone marrow cells, adipocytes, platelets and various cancer cells1,2,3. GAS6 and TAM receptors activate a series of different downstream signaling cascades and regulate diverse functions, especially cell migration, adhesion, inflammation, cell growth, survival and other cell type-specific functions4,5,6.
To date, two studies support Gas6 involvement in reproduction7,8. We first found that Gas6 is expressed in mouse oocytes and is not involved in the completion of the meiotic division since Gas6-depleted oocytes mature to the metaphase II (MII) stage with extrusion of the first polar body7. However, depletion of Gas6 in oocytes results in failure of sperm chromatin remodeling and pronuclear formation through insufficient cytoplasmic maturation7. In a successive study, we found that the depletion of Gas6 in oocytes inhibited heparan sulfate biosynthesis and glutathione production via mitochondrial overactivation, characterized by increased ATP production and mitochondrial membrane potential8. Most importantly, Gas6 was a crucial factor for the completion of oocyte cytoplasmic maturation.
Mitochondria are important cellular organelles for energy production. They have important roles in ATP synthesis, metabolism, calcium homeostasis, fatty acid oxidation and apoptosis9. Mitochondria play pivotal roles in mammalian reproduction. Researchers have reported that, in mice, mitochondrial activity is important for oocyte maturation and subsequent embryo development but that an altered mtDNA copy number does not affect nuclear maturation9,10. In humans, mitochondrial function and mtDNA contents are also correlated with oocyte maturity and fertilizability11,12. Moreover, fertilization failure observed in oocytes with a low mtDNA number and mitochondrial dysfunction was resulted from defective oocyte cytoplasmic maturation and decreased oocyte quality. Thus, the mtDNA copy number in MII oocytes is being investigated as a marker of embryo viability13. It has been reported that an increase in the number of healthy mitochondria and/or improvement in mitochondrial function could provide a significant boost in fertility14,15. Recently, mitochondrial replacement therapy has resulted in the birth of healthy primate (including human) offspring16,17.
As females become older, maternal reproductive capacity decreases. The main reason for this decline is the decreased quality of oocytes and their mitochondria. In oocytes, ATP production and mtDNA copy number decrease and mitochondrial mutations increase with aging18. Transgenic mice with induced mtDNA mutations exhibit reduced fertility19. In mammalian cells, mitochondrial quality can be improved through the facilitation of mitophagy and selective autophagy of mitochondria20. The clearance of dysfunctional mitochondria via mitophagy screens the damaged mtDNA and prevents its transmission to the next generation21.
Mitophagy is essential for the mitochondrial quality and quantity control mechanism that eliminates damaged mitochondria22. Removal of damaged mitochondria through mitophagy requires five steps: initiation of phagophore formation, elongation, closure and autophagosome formation, autophagosome-lysosome fusion and lysosomal degradation23. Autophagosome formation is finely regulated by autophagy-related genes24. Among the numerous proteins involved in the regulation of autophagy, MTOR is a key component. MTOR inhibits autophagy as well as mitophagy by decreasing the expression of autophagy-related genes25. Several studies have examined the role of the MTOR-specific inhibitor rapamycin in rescuing the poor developmental capacity of aged pig oocytes26 and cloned mouse and pig embryos27,28.
In this study, we compared gene expression profiles using RNA-Seq between oocytes with or without Gas6 expression. Based on the data of the present study, we report for the first time that Gas6 regulates mitophagy via a MTOR-dependent pathway during in vitro maturation of mouse oocytes. Additionally, Gas6-silenced MII oocytes exhibited the accumulation and aggregation of mitochondria in the cytoplasm. We found that Gas6 depletion led to a greater suppression of mitophagy through MTOR signaling activation and a reduction in the mtDNA copy number and levels of mitochondria-encoded mRNA in oocytes, supporting a novel role of Gas6 in the maintenance of mitochondrial contents and activity during oocyte cytoplasmic maturation.
Results
Definition of the transcriptome in Gas6-silenced MII oocytes
Previously, we found that Gas6 depletion impairs cytoplasmic maturation and pronucleus (PN) formation7. We asked whether cytoplasmic maturity in oocytes is reflected at the level of transcription, and, if so, what patterns of gene expression are characteristic of GFP-dsRNA treated (control group) or Gas6-silenced MII oocytes. We performed transcriptome analysis with RNA-Seq. In this study, 18,666,312 to 41,440,784 raw reads were generated for each sample. Of these, 7,674 and 11,118 expressed genes were identified in GFP-dsRNA treated or Gas6-silenced MII oocytes, respectively. There were 2,238 commonly expressed genes between the two groups. A comparison of transcript abundances showed relatively few differentially abundant transcripts in MII oocytes between GFP RNAi and Gas6 RNAi. A total of 312 genes were changed more than two-fold in Gas6-depleted MII oocytes than in GFP dsRNA-injected MII oocytes. This analysis revealed that 210 genes were upregulated and 102 were downregulated. The top 20 differentially expressed genes are listed in Table S1.
Disruption of Gas6 causes changes in mitochondria-related gene expression
Previously, we reported that disruption of Gas6 resulted in insufficient oocyte cytoplasmic maturation via mitochondrial dysfunction such as mitochondrial overactivation and abnormal mitochondrial accumulation8. Based on the RNA-Seq analysis, we selected 2 genes related to mitochondrial functions (Phyhipl and Tomm7) and 3 for mitophagy (Atg2b, Binp3 and Esr2) and added Ptpn11, as a downstream target of Gas6 (Fig. 1A) for validation by quantitative real-time RT-PCR (qPCR). Genes associated with increased (Atg2b, Ptpn11, Phyhipl and Tomm7) or decreased (Esr2 and Bnip3) transcript levels were evaluated by qPCR to determine the transcript levels in MII oocytes after GFP RNAi or Gas6 RNAi. Five of the six genes analyzed demonstrated similarly significant changes in transcript levels between RNA-Seq and qPCR results, demonstrating the validity of RNA-Seq analysis; however, Atg2b showed an increase in transcript abundance in RNA-Seq but a decrease in expression by qPCR analysis (Fig. 1). Thus, transcript levels of mitochondrial proteins (Phyhipl and Tomm7) and Ptpn11 were significantly increased, whereas transcript levels of mitophagy-related genes (Atg2b, Binp3 and Esr2) were markedly reduced (Fig. 1B), suggesting that downregulation of the Atg2b, Binp3 and Esr2 genes may cause the accumulation of mitochondria as observed by us previously in Gas6-depleted oocytes.
Disruption of Gas6 induced the activation of MTOR signaling in oocytes
Based on RNA-Seq and qPCR results, we hypothesized that the mitochondrial dysfunction and inhibition of mitophagy through Gas6 silencing may have resulted in failure of PN formation. It has been reported that MTORC1 plays a pivotal role in autophagy and can be selectively inhibited by rapamycin29. MTORC1 consists of MTOR, RAPTOR, mLST8 (GβL) and PRAS4030. Among these, MTOR is an important regulator of mitophagy, with activated MTOR suppressing mitophagy, and negative regulation of MTOR promoting mitophagy25. Therefore, we performed Gas6 RNAi and then evaluated the changes in mitochondrial quality and quantity, expression of mitophagy-related genes, and MTOR activation in MII oocytes.
Previously, we found by using JC-1 staining that Gas6 depletion induces mitochondrial overactivation and accumulation in the cytoplasm8. We hypothesized that the abnormal mitochondrial accumulation in response to decreased Gas6 may be due to the activation of PTPN11 and MTOR as well as reduction of BNIP3, known as an inactivator of MTOR31. Thus, we next investigated the mechanism whereby Gas6 regulates mitophagy, by measuring Ptpn11, Bnip3 and Mtor in Gas6-silenced MII oocytes. The natural expression of Gas6 downstream target genes, Ptpn11, Bnip3 and Mtor was higher in GV than in MII oocytes (Fig. 2A). In Gas6-silenced MII oocytes, Ptpn11 expression increased, whereas Bnip3 expression was decreased (Fig. 2B). The expression of Mtor was not significantly altered (Fig. 2B). Interestingly, however, depletion of Gas6 induced a remarkably increased expression of proteins, for PTPN11, phosphorylated-PTPN11 (p-PTPN11), MTOR and phosphorylated-MTOR (p-MTOR; Fig. 2C). These data suggest that, as we hypothesized, Gas6 disruption leads MTOR activation probably through PTPN11 activation and BNIP3 suppression, which then may lead mitophagy inhibition.
Suppression of mitophagy was observed after Gas6 RNAi
As we illustrated in Fig. 2, Gas6 RNAi inhibited the expression of genes related to mitophagy as well as the activation of MTOR signaling in oocytes. To investigate whether loss of Gas6 promotes mitochondrial accumulation through mitophagy suppression and altered distribution in the cytoplasm; we stained mitochondria with MitoTracker. In the control GFP RNAi group, MII oocytes had evenly dispersed mitochondria in the cytoplasm, and some more-aggregated mitochondria around the spindles (Fig. 3Aa–b). Conversely, mitochondria were mainly accumulated and aggregated from the meiotic spindle to the cortex in the Gas6-silenced MII cytoplasm (Fig. 3Ac–d). To determine whether disruption of Gas6 attenuates mitophagy in oocytes via the regulation of autophagy-related genes, we measured the changes in the expression of seven genes related to mitophagy, i.e., Atg2b, Atg5, Atg7, Atg12, Becn1, Map1lc3a and Map1lc3b. Among these genes, Atg7 was not detected in oocytes (Fig. 3B). In Gas6-silenced MII oocytes, the expression levels of five autophagy-related genes, Atg2b, Atg5, Atg12, Becn1 and Map1lc3a, were slightly decreased, while the expression of Map1lc3b was not changed (Fig. 3B). We next determined the expression of LC3 in Gas6-silenced MII oocytes. The LC3 are known as the mitophagy regulator marker. Indeed, the initiation of mitophagy causes the conversion of LC3-I to LC3-II, which is associated with the formation of autophagosomes. We measured LC3-II protein levels by Western blotting, and as shown in Fig. 3C, the LC3-II levels were markedly decreased after Gas6 RNAi, suggesting decreased formation of autophagosomes. Taken together, these results suggest that Gas6 depletion induced mitochondrial accumulation and altered the mitochondrial distribution in the cytoplasm probably via suppression of mitophagy.
Gas6 RNAi resulted in a lower mtDNA copy number
Mitochondria play important roles in oocyte maturation9. We examined the expression of mRNAs associated with mitochondria during oocyte maturation. The expression of mtDNA-encoded genes, mt-Nd1, mt-Nd6 and mt-Atp6, were not significantly altered during oocyte maturation (Fig. 4A). After Gas6 RNAi, the expression of mt-Nd1 was increased in GV but reduced in MII oocytes (Fig. 4B), but no change in mt-Nd6 and mt-Atp6 expression was observed (Fig. 4C and D).
Oocyte quality is tightly linked to the oocyte mtDNA content in mice, humans and other species10,11,12,13. To determine whether there was a change in the mtDNA copy number during in vitro maturation, qPCR was performed on GV and MII oocytes. We found that the GV oocytes contained an average of 47,400 ± 3,010 mtDNA copies per oocyte, while the MII oocytes possessed an average of 99,380 ± 11,070 mtDNA copies (Fig. 4E). The mtDNA copy number was almost doubled with oocyte maturation. In contrast, in Fig. 4F, the average mtDNA copy number was markedly lower in Gas6-depleted MII oocytes (57,590 ± 2,890) than in Gas6-silenced GV oocytes (127,950 ± 3,610), suggesting that Gas6 disruption had opposite effects on the mtDNA content depending on the oocyte stage. Regarding the up-regulated mtDNA content in Gas6-silenced GV oocytes (Fig. 4F), we do not have substantial data for that specific phenomena at this moment. However, we guess the potential mechanism for that increase as follows. To allow Gas6 dsRNA to work for breakdown endogenous Gas6 transcripts at GV stage, we holding the GV membrane breakdown by treating oocytes with IBMX for 8 hours. It may be one of the potential points to check with. To hold the GV membrane intact against the natural breakdown force, oocytes may need more energy than normal maturation. That is the reason for increased mtDNA at GV stage after RNAi. However, more experiment is required for this issue.
Inhibition of MTOR rescued impaired mitophagy after Gas6 RNAi
Having shown that the reduction of Gas6 accumulates mitochondria in the cytoplasm via mitophagy suppression, we examined whether the MTOR-dependent regulatory pathway of mitophagy is related to this phenomenon in Gas6-silenced MII oocytes. To determine whether inhibition of the MTOR pathway would rescue impaired mitophagy by Gas6 silencing, we added rapamycin, a MTOR inhibitor, to the medium for in vitro maturation after Gas6 RNAi. Upon treatment, rapamycin-treated Gas6-silenced MII oocytes exhibited markedly reduced expression of MTOR and p-MTOR, indicating that rapamycin treatment blocked the MTOR activation caused by Gas6 silencing (Fig. 5A). In addition, as shown in Fig. 5B, the expression levels of five autophagy-related genes, Atg2b, Atg5, Atg12, Becn1 and Map1lc3a, were significantly upregulated in Gas6-depleted MII oocytes with rapamycin treatment. As expected, blocking MTOR signaling with rapamycin led a more even distribution of mitochondria throughout the cytoplasm with significantly reduced mitochondrial numbers (Fig. 5C; red staining). Importantly, rapamycin treatment rescued the mitophagy suppression caused by Gas6 depletion, and so it was reasonable to conclude that the oocytes exhibited blocked MTOR activation and increased expression of autophagy-related genes.
Gas6 is a reciprocal regulator of oocyte mitophagy
To address the effect of Mdivi-1, a mitochondrial division/mitophagy inhibitor, on oocyte nuclear maturation, mitochondrial quantity and expression of Gas6 in oocytes, we analyzed the mitochondrial content in oocytes after Mdivi-1 treatment. As shown in Fig. 6A, the number of mitochondria, stained red, was increased by Mdivi-1 stimulation in a dose-dependent manner in the cytoplasm of MII oocyte (Fig. 6A and B). Our results revealed that the mitochondria were aggregated more commonly in Gas6-silenced MII oocytes (Fig. 3A) but were not aggregated in MII oocytes with Mdivi-1 stimulation (Fig. 6A). To further elucidate the relationship between the mitophagy suppression and oocyte maturation, the oocyte maturation rate was observed after treatment with Mdivi-1. Despite the increase in Mdivi-1 treatment in a dose-independent manner, oocyte maturation rates were not changed (Fig. 6C and D). These results suggest that the inhibition of mitophagy is not involved in oocyte nuclear maturation. We also found that the expression levels of Gas6 in oocytes, which is implicated in the regulation of cytoplasmic maturation and mitochondrial function and/or content, was changed and decreased in a dose-dependent manner with Mdivi-1 treatment (Fig. 6E), suggesting that Gas6 and mitophagy are interconnected and reciprocally regulate each other in oocytes.
To verify the effect of mitophagy inhibition by Mdivi-1 on fertilization, we added Mdivi-1 in the medium during oocyte maturation and then performed in vitro fertilization. Following in vitro fertilization, control oocytes (vehicle, open bar) exhibited a substantial percentage of PN formation after sperm penetration (Fig. 6F). However, similar to the effects of directly targeting Gas6, all MII oocytes with Mdivi-1 at any dose (1~100 μM) failed to in vitro fertilization with no PN formation (Fig. 6F). Taken together, mitochondrial accumulation due to suppression of mitophagy resulted in the insufficient cytoplasmic maturation and consequently the failure of fertilization.
Discussion
In this study, we report a novel role for Gas6 associated with mitochondrial quality and quantity through MTOR-dependent mitophagy signaling during oocyte maturation, and the regulation of mitophagy and Gas6 expression are mutually interconnected. In Gas6-depleted MII oocytes, we observed an increased content of mitochondria and an aggregated and accumulated distribution of mitochondria from the meiotic spindle to the cortex. Disruption of Gas6 resulted in stimulated PTPN11 downstream of Gas6 and increased MTOR activity via reduction of BNIP3, autophagy-related genes and autophagosome formation-related genes, resulting in mitophagy suppression (Fig. 7). Interestingly, Gas6 depletion led a reduction in mitochondrial transcription and mtDNA copy number, suggesting that GAS6 functions to maintain both the quality and quantity of mitochondria in oocytes for sufficient cytoplasmic maturation.
Autophagy, a very intriguing pathway, is regulated by multiple proteins, such as PI3K III, MTOR, MAPK and BNIP332. During the past two decades, more than 30 autophagy-related genes involved in the regulation of the formation of autophagosome have been identified22. These proteins are also important for mitophagy. In the present study, we showed that mouse oocytes contain MTOR and BNIP3 proteins, the main regulators of mitophagy, and confirmed that those autophagy-related genes and LC3 are involved in autophagosome formation. Although each protein is essential for controlling mitophagy, the most commonly used marker for monitoring the mitophagic flux was the ratio of LC3-II/LC3-I33. Disruption of Gas6 induced a significant decrease in the ratio of LC3-II/LC3-I. Ultimately, increased, accumulated, and aggregated mitochondria were found in the oocyte cytoplasm after Gas6 RNAi. These results strongly indicate that GAS6 regulates mitochondrial distribution and quantity in oocytes via mitophagy.
Mitophagy, a selective form of autophagy, is responsible for eliminating dysfunctional or damaged mitochondria and maintaining the balance in mitochondria quality and quantity. MTOR is a key regulator of autophagy as well as mitophagy30. There is evidence that mitophagy requires the suppression of MTOR activity25,30. In the present study, we found that Gas6-depleted MII oocytes exhibit increased MTOR activity and, therefore, mitophagy inhibition. Upon rapamycin stimulation, the inhibition of MTOR activity in Gas6-silenced MII oocytes suppressed the downregulation of the autophagy-related genes and rescued the mitophagy caused by Gas6 RNAi, which did not induce mitochondrial aggregation in the cytoplasm. Therefore, we concluded that GAS6 regulates mitophagy through a MTOR-dependent pathway, thereby efficiently safeguarding mitochondria in oocytes.
The regulation of mitochondrial dynamics is important for oocyte maturation. Mitochondria redistribute during oocyte maturation into regions requiring high ATP concentrations due to high metabolic demands34. During the first meiotic division, mitochondria aggregate around the spindle, migrate to the oocyte cortex in association with the spindle and then distribute asymmetrically, causing almost all mitochondria to remain in the oocyte and very few mitochondria to remain in the polar body35. During the second meiotic division, mitochondria aggregate around the spindle and then distribute throughout the cytoplasm35,36. We showed in this study that the mitochondria in Gas6-depleted MII oocytes also markedly accumulate and aggregate around the meiotic spindle; however, the mitochondria aggregates remained when the spindle formation was completed. In addition, previously, we found that the disruption of Gas6 increases ATP production and the mitochondrial membrane potential8. However, Gas6 RNAi does not affect oocyte nuclear maturation7. Despite the abnormal mitochondrial distribution, it is possible that the formation and separation of the meiotic spindle during nuclear maturation progressed normally in oocytes after Gas6 RNAi because ATP was abundant in Gas6-depleted MII oocytes.
Oocyte maturation involves nuclear and cytoplasmic maturation, during which oocytes acquire fertilizability. Mitochondria play an important role in both processes since they provide the main supply of ATP10. It has been reported that mtDNA in oocytes is pivotal for healthy reproduction and that a lower mtDNA copy number can cause fertility problems37. Mouse oocytes containing as few as 50,000 copies of mtDNA can give rise to healthy embryos38. Prior to fertilization, the mtDNA copy number in oocytes needs to be amplified to sufficient levels. Mature oocytes contain at least 100,000 copies of mtDNA38,39, and we obtained the same results in this study. The mtDNA copy number in MII oocytes could be used as a marker of embryo developmental competence11,13. Moreover, studies have shown that a high mitochondrial content can increase the quality and competence of mature mammalian oocytes11,38. We did not determine how Gas6 RNAi induced a lower mtDNA copy number in Gas6-silenced MII oocytes in this study, but it was approximately 50% that of the control oocytes, and we assume that the defective cytoplasmic maturation caused by Gas6 silencing was due to this lower mtDNA copy number.
Mitochondrial dysfunction causes a decrease in oocyte quality and interferes with embryonic development, resulting in declining fertility. Recently, it has been reported that mitochondrial replacement therapy, a new gene-therapy technique, could lead to better fertility outcomes and a remarkable clinical amelioration of mitochondrial diseases40. The mitochondrial replacement therapy can be performed by three different processes, such as maternal spindle transfer16,41, polar body transfer42 and pronuclear transfer43. This technique in oocytes may safely prevent next-generation transmission of harmful mtDNA mutations44. The other method that improves mitochondrial function may be performed by using small molecules, such as resveratrol45, L-carnitine46 and coenzyme Q1047,48. In the present study, we also found that GAS6 is another avenue for safeguarding the mitochondrial quality and quantity in oocytes. Therefore, we propose that the discovery of Gas6-level regulation in oocytes may open a new method to improve oocyte mitochondrial function and its application in human IVF for oocyte competency. Although GAS6 seem to be appealing for improving fertility, well-designed clinical studies are necessary to test the therapeutic efficacy, safety and potential benefits, as well as its side effects for clinical application in IVF lab.
In conclusion, our findings clearly demonstrated that Gas6 regulates mitophagy and safeguards mitochondrial activity through regulating central mitophagy-related genes, such as MTOR, BNIP3, ATG family and LC3, thereby resulting in fully competent oocytes (Fig. 7). We previously reported that GAS6 regulates mitochondrial function for ATP production and mitochondrial membrane potential7. It is noteworthy that mitochondrial accumulation with impaired mitophagy may induce the overactivation of mitochondria and lead to insufficient cytoplasmic maturation, with a negative impact on the remodeling sperm nucleus and pronuclear formation after fertilization. Taking these results together, we suggest that control of the GAS6 signaling network in oocytes may improve the decreased fertilizability caused by the deterioration of mitochondrial functions and/or contents.
Methods
Animals
Imprinting control region (ICR) mice, exclusively provided by Koatech (Pyeoungtack, Korea), were mated to produce embryos in the breeding facility at the CHA Research Institute of CHA University. All procedures described herein were reviewed and approved by the Institutional Animal Care and Use Committee of CHA University and were performed in accordance with the Guiding Principles for the Care and Use of Laboratory Animals.
Reagents
Chemicals and reagents were obtained from Sigma-Aldrich (St. Louis, MO, USA) unless otherwise noted.
Oocyte isolation
To isolate germinal vesicle (GV) oocytes, three-week-old female ICR mice were injected with 5 IU pregnant mare serum gonadotropin and sacrificed 46 hours later. Isolated ovaries were punctured in M2 medium containing 0.2 mM 3-isobutyl-1-methyl-xanthine (IBMX), and cumulus-oocyte complexes (COCs) were collected. Cumulus cells were mechanically retrieved from oocytes by repeated pipetting via a fine-bore pipette. To obtain oocytes in other stages, GV oocytes were cultured in M16 medium without IBMX in 5% CO2 at 37 °C. Isolated oocytes were snap-frozen and stored at −80 °C prior to RNA isolation.
Microinjection and in vitro culture
For RNAi experiments, we prepared GFP and Gas6 dsRNA as previously described7. GV oocytes were microinjected with dsRNA in M2 medium containing 0.2 mM IBMX; 10 pl of dsRNA was microinjected into the oocyte cytoplasm using a constant flow system (Transjector; Eppendorf, Hamburg, Germany). The oocytes were cultured in M16 medium containing 0.2 mM IBMX for 8 hours, followed by culture in M16 alone for 16 hours in 5% CO2 at 37 °C. After the RNAi experiments were completed, in vitro maturation rates and morphological changes were recorded as previously described7.
Library preparation and RNA-Seq (QuantSeq)
Total RNA (300 MII oocytes) was isolated using a RNeasy mini kit (Qiagen, Inc., Valencia, CA, USA). RNA quality was assessed by an Agilent 2100 bioanalyzer using an RNA 6000 Nano Chip (Agilent Technologies, Amstelveen, Netherlands), and RNA quantification was performed using an ND-2000 Spectrophotometer (Thermo, Inc., Waltham, MA, USA). For control and test RNAs, the library construction was performed using a SENSE 3′ mRNA-Seq Library Prep Kit (Lexogen, Inc., Vienna, Austria) according to the manufacturer’s instructions. In brief, each 500 ng sample of total RNA was prepared, an oligo-dT primer containing an Illumina-compatible sequence at its 5′ end was hybridized to the RNA, and reverse transcription was performed. After degradation of the RNA template, second-strand synthesis was initiated by a random primer containing an Illumina-compatible linker sequence at its 5′ end. The double-stranded library was purified by using magnetic beads to remove all reaction components. The library was amplified to add the complete adapter sequences required for cluster generation. The finished library was purified from PCR components. High-throughput sequencing was performed as single-end 75 sequencing using NextSeq. 500 (Illumina, Inc., San Diego, CA, USA).
Data analysis
SENSE 3′ mRNA-Seq reads were aligned using Bowtie2 version 2.1.049. Bowtie2 indices were generated from either the genome assembly sequence or the representative transcript sequences for aligning to the genome and transcriptome. The alignment file was used for assembling transcripts, estimating their abundances and detecting the differential expression of genes. Differentially expressed genes were determined based on counts from unique and multiple alignments using EdgeR within R version 3.2.2 (R development Core Team, 2011) using Bioconductor version 3.050. The read count data were processed based on the global normalization method using the Genowiz™ version 4.0.5.6 (Ocimum Biosolutions, Hyderabad, India). We analyzed differentially expressed genes and generated a scatter plot to compare expression values (Fig. S1). Gene classification was based on searches performed in the DAVID (http://david.abcc.ncifcrf.gov/) and MEDLINE databases (http://www.ncbi.nlm.nih.gov/).
Rapamycin and Mdivi-1 treatment of oocytes
An experiment of rescued mitophagy in Gas6-depleted MII oocytes was performed in the presence or absence of rapamycin, a specific inhibitor of MTOR. After RNAi, oocytes were cultured in M16 medium containing 1 nM rapamycin, followed by staining of mitochondria (MitoTracker) and Western blot analysis of MTOR and p-MTOR.
For analysis of oocyte nuclear maturation by mitochondrial division/mitophagy inhibitor Mdivi-1, in vitro maturation rates and morphological changes were recorded after incubation with 1 μM, 10 μM, 50 μM and 100 μM Mdivi-1 for 16 hours. After treatment, the oocytes were washed thoroughly and prepared for qPCR. Oocytes in the vehicle group were treated with the same concentration of DMSO in M16 medium.
In vitro fertilization (IVF)
Sperm were collected from the caudal epididymides of 8-week-old male ICR mice (Koatech). The sperm were incubated in M16 medium for 1 hour to allow capacitation. After the zona pellucida (ZP) was removed using Tyrode’s solution (pH 2.5), ZP-free MII oocytes were then placed in a 200 μl droplet of M16 medium under mineral oil and inseminated with 2.5 × 104/ml sperm. After 2 hours, the oocytes were washed to remove unbound sperm and cultured in M16 medium for 5 hours (37 °C, 5% CO2) to observe PN formation.
Messenger RNA isolation
Oocyte mRNA was isolated using a Dynabeads mRNA DIRECT kit (Dynal Biotech ASA, Oslo, Norway) according to the manufacturer’s instructions. Briefly, oocytes were suspended with lysis/binding buffer and mixed with prewashed Dynabeads oligo dT25. After RNA binding, the beads were washed with buffer A twice, followed by buffer B, and mRNA was eluted with Tris-HCl by incubation at 72 °C. Purified mRNA was used as a template for reverse transcription with an oligo (dT) primer according to the MMLV protocol.
Quantitative real-time RT-PCR (qPCR)
qPCR was carried out with a single-oocyte-equivalent amount of cDNAs and gene specific primers (Table 1), as previously described7, using an iCycler iQ™ Detection System (Bio-Rad). The iQ SYBR Green Supermix PCR reagents (Bio-Rad) were used to monitor amplification, and the results were analyzed using iCycler iQ™ proprietary software. The melting curves were used to identify any nonspecific amplification products. H1foo was used as a control. The relative expression levels of the target genes were evaluated using the comparative CT method, and all experiments were repeated at least three times.
Measurement of the mitochondrial DNA copy number
Mitochondrial DNA extraction in 50 MII oocytes after GFP RNAi or Gas6 RNAi was performed using a mitochondrial DNA isolation kit (Abcam, Cambridge, MA, USA). For mtDNA content analysis in oocytes, we selected a region of the mouse mitochondrial Nd1 gene corresponding to bases 2929–3128 (Accession number NC_005089.1). The mtDNA copy number was determined by performing qPCR using an iCycler iQ™ Detection System with the primer set (5′-CAATACGCCCTTTAACAACC-3′ and 5′-TTTGGAGTTTGAGGCTCATC-3′) and iQ SYBR Green Supermix PCR reagents. The mtDNA content in a single oocyte was extrapolated from the standard curve and calculated according to the target PCR product length. A standard curve was generated for each run using 10-fold serial dilutions representing the copy number of the external standard. The external standard was the PCR product of the corresponding gene cloned into a vector using the Zero Blunt TOPO PCR cloning kit (Invitrogen, Carlsbad, CA, USA), and the PCR product was sequenced for confirmation before use. All samples were analyzed in triplicate.
Western blotting
To confirm protein expression, Western blotting was performed as previously described7. Briefly, a protein extract was separated using 6%, 10% or 15% SDS-PAGE and transferred onto a PVDF membrane (Amersham Biosciences, Piscataway, NJ). After blocking, the membrane was incubated with antibodies against GAS6 (1:1000), BNIP3 (1:1000; #3769, Cell Signaling Technology, Danvers, MA, USA), LC3 (1:1000; ab48394, Abcam), MTOR (1:1000; #2972, Cell Signaling Technology), p-MTOR (1:1000; #2971, Cell Signaling Technology), PTPN11 (1:1000; #3752, Cell Signaling Technology), p-PTPN11 (1:1000, #3751, Cell Signaling Technology), and α-TUBULIN (1:2000; sc-8035, Santa Cruz Biotechnology), followed by incubation with HRP-conjugated anti-goat IgG (1:2000; A5420), anti-rabbit IgG (1:5000; #7074, Cell Signaling Technology, Danvers, MA, USA) or anti-mouse IgG (1:2000; A2554). Bound antibodies were detected using an enhanced chemiluminescence detection system (Amersham Biosciences) according to the manufacturer’s instructions.
Staining of mitochondria
To evaluate the distribution of mitochondria, oocytes were stained using MitoTracker Orange CMTMRos (Molecular Probes). MitoTracker, which fluoresces orange, was used at a concentration of 300 nM in M16 supplemented with 0.3% BSA for 30 minutes at 37 °C in the dark. After washing, the oocytes were fixed and immunofluorescently stained with an anti-α-TUBULIN antibody and then counterstained with DAPI. The stained oocytes were stored below 4 °C until confocal microscopy was performed. The oocytes were examined using a laser scanning confocal microscope (LSCM; Leica, Wetzlar, Germany). A minimum of 30 oocytes per RNAi group was examined by an LSCM. For the fixed MitoTracker measurements, the signal intensities for each oocyte were calculated using Leica Application Suite Advanced Fluorescence (LAS AF) software. Data represent the average fold change from three experiments.
Immunofluorescence staining
Denuded oocytes were placed in PBS containing 0.1% polyvinyl alcohol (PBS-PVA), 4% paraformaldehyde, and 0.2% Triton X-100 and then fixed for 40 minutes at room temperature (RT). After the oocytes were washed in PBS-PVA, fixed oocytes were blocked with 3% BSA-PBS-PVA for 1 hour and then incubated with mouse anti-α-TUBULIN antibody (1:100) at 4 °C overnight. After the oocytes were washed, they were incubated with an Alexa Fluor 488-conjugated secondary antibody (Molecular Probes, Eugene, OR, USA) for 1 hour at RT.
Statistical analysis
Data were derived from at least three separate and independent experiments and expressed as the mean ± SEM. The p values were calculated based on a paired t-test of the means from the GFP RNAi group and the Gas6 RNAi group, and p < 0.05 was considered statistically significant.
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Acknowledgements
This research was supported by the Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Ministry of Education (NRF-2015R1D1A1A01056595) and the Korea government (MSIT; NRF-2019R1C1C1002454).
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K.-H.K. and K.-A.L. conceived and designed the experiments; K.-H.K. and E.-Y.K. performed the experiments; K.-H.K., J.-J.K. and K.-A.L. analyzed the data and acquired financial support; K.-H.K. and K.-A.L. wrote the manuscript.
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Kim, KH., Kim, EY., Ko, JJ. et al. Gas6 is a reciprocal regulator of mitophagy during mammalian oocyte maturation. Sci Rep 9, 10343 (2019). https://doi.org/10.1038/s41598-019-46459-3
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DOI: https://doi.org/10.1038/s41598-019-46459-3
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