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About the Authors:

Gildas Tetaping Mbemya

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Conceptualization, Data curation, Investigation, Methodology, Writing – original draft, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Jesus Cadenas

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Naiza Arcângela Ribeiro de Sá

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

ORCID logo http://orcid.org/0000-0003-4745-0108

Denise Damasceno Guerreiro

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Nathalie Jiatsa Donfack

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Luis Alberto Vieira

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

ORCID logo http://orcid.org/0000-0002-2419-1329

Francisca Geovania Canafístula de Sousa

Contributed equally to this work with: Gildas Tetaping Mbemya, Jesus Cadenas, Naiza Arcângela Ribeiro de Sá, Denise Damasceno Guerreiro, Nathalie Jiatsa Donfack, Luis Alberto Vieira, Francisca Geovania Canafístula de Sousa

Roles Conceptualization, Methodology, Writing – review & editing

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Benner Geraldo Alves

Roles Data curation, Formal analysis, Software, Writing – review & editing

Affiliation: Laboratory of Biology of Reproduction, Federal University of Uberlândia, Minas Gerais, Brazil

ORCID logo http://orcid.org/0000-0001-9465-8054

Carlos Henrique Lobo

Roles Data curation, Methodology, Writing – review & editing

Affiliation: Laboratory of Animal Physiology, Department of Animal Science, Federal University of Ceará, Fortaleza, CE, Brazil

Francielli Weber Santos

Roles Data curation, Writing – review & editing

Affiliation: Laboratory of Reproduction Biotechnology (Biotech), State of University of Pampa, Uruguaiana, Brazil

Francisco das Chagas Lima Pinto

Roles Methodology, Writing – review & editing

Affiliation: Laboratory of Phytochemical Analysis of Medicinal Plants (LAFIPLAN), Federal University of Ceará, Fortaleza, Brazil

ORCID logo http://orcid.org/0000-0003-1481-7970

Otília Deusdênia Loiola Pessoa

Roles Data curation, Writing – review & editing

¶‡ These authors also contributed equally to this work.

Affiliation: Laboratory of Phytochemical Analysis of Medicinal Plants (LAFIPLAN), Federal University of Ceará, Fortaleza, Brazil

Johan Smitz

Roles Conceptualization, Funding acquisition, Writing – review & editing

¶‡ These authors also contributed equally to this work.

Affiliation: Follicle Biology Laboratory, Center for Reproductive Medicine, UZ Brussel, Brussels, Belgium

Pierre Comizzoli

Roles Data curation, Supervision, Writing – review & editing

¶‡ These authors also contributed equally to this work.

Affiliation: Center for Species Survival, Smithsonian Conservation Biology Institute, Front Royal, VA, United States of America

José Ricardo Figueiredo

Roles Writing – review & editing

¶‡ These authors also contributed equally to this work.

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Ana Paula Ribeiro Rodrigues

Roles Conceptualization, Data curation, Funding acquisition, Project administration, Supervision, Validation, Writing – review & editing

* E-mail: [email protected]

Affiliation: Laboratory of Manipulation of Oocyte and Ovarian Preantral Follicles (LAMOFOPA), Faculty of Veterinary (FAVET), State University of Ceará, Fortaleza, Brazil

Introduction

The secondary follicles, the last category of preantral follicles (PF), according to Araújo et al. [1], is an excellent source of potentially fertilizable oocytes; however, the in vitro development of these follicles has been a great challenge to produce fully grown and competent oocytes. To date, live birth after the in vitro culture of PF has been reported only in mice [2–4]. In large mammals, on the other hand, results are still modest and may be summarized in the production of a variable number of embryos in buffaloes [5], sheep [6] and goats [7, 8].

Several variables may affect the outcome of in vitro follicle culture such as the culture base media composition [9, 10] and supplementation [11]; the animal model [8]; culture system [1, 12]; follicular category [13, 14] and reactive oxygen species (ROS) production [15], leading to oxidative stress. Many authors have shown that an increase of glutathione peroxidase (GPx) can represent a cellular transcriptional response to ROS [16], such as an activation or silencing of genes encoding antioxidant defense enzymes, growth and progression of meiosis [17]. To date it still is a challenge to reach a good balance between all components of the culture medium, getting the right concentrations and interaction that should exist between the components of the medium.

The addition of supplements (energy substrates, antioxidants, hormones and/or growth factors) to alpha modified minimal essential medium (α-MEM) is necessary to enable acceptable rates of follicular growth, oocyte viability and maturation [18] in caprine [19, 20] and ovine species [9, 21]. In an attempt to improve secondary follicles development, oocyte viability and maturation, natural supplements may be added to the culture media such as Amburana cearensis [22, 23], anethole [19] and rutin [24]. Although these studies have not involved investigation related to gene expression, it is known that GPx [25], kit ligand (KL—[13]), cyclin B1 (CCNB1 –[26]) and hyaluronan synthase 2 (HAS2 –[27] genes are expressed in mature oocytes. Therefore, the identification of these genes in oocytes may be a good indicator of an in vitro culture system's viability for secondary follicles.

Justicia insularis T. Anders (Acanthaceae) is an herbaceous and perennial plant of 30–75 cm high with opposite ascending branches, widely distributed in the tropical area of Africa [28]. Besides alkaloids, glycosides, polyphenols and triterpenoids, studies undertaken by Telefo et al. [29] and Goka et al. [28] revealed the presence of flavonoids in their leaves which acts as natural antioxidant and FSH-like compound. In fact, a literature survey showed that several studies performed with Justicia species have revealed the presence of the aforementioned secondary metabolites. It is worth mentioning that major part of these studies was done by phytochemical screening. In the Western region of Cameroon, J. insularis is used in association with the leaves of three others medicinal plants (Aloe buettneri, Hibiscus macranthus and Dicliptera verticillata), to treat dysmenorrhoea and some cases of women infertility. This aqueous extract mixture has also been proven, in a series of studies to induce ovarian steroidogenesis and folliculogenesis in female rats [29–31]. In a recent study performed by our team, the aqueous extract of J. insularis has successfully promoted beneficial effects on morphology, activation and growth of PF (primordial, intermediary, primary and secondary) enclosed in ovarian tissue cultured in vitro for 7 days [32]. To date, due to their widely distribution and cost compared to chemical product, there is an increase interest in natural products that prevent oxidative damages, promote follicular growth and oocyte maturation.

Considering the positive results of J. insularis on the reproductive function in vivo [33] and in vitro culture of ovarian tissue [32], previously reported, in a general way, the aim of this study was to investigate the effect of different concentrations of the aqueous extract of J. insularis on the behavior of secondary follicles after 18 days of in vitro culture. In addition, we evaluate the effect of the extract on in vitro maturation of oocytes from in vivo grown follicles. Therefore, were analyzed: a) follicular morphology; b) ability to grow and form the antral cavity; c) gene expression (GPx, KL, CCNB1 and HAS2) in the follicular wall; d) ROS levels in the follicles culture medium and finally, e) the viability and in vitro maturation of oocytes from in vitro and in vivo grown secondary follicles.

Materials and methods

This study was approved and performed according to the recommendations of the Committee of Animal Handling and Ethical Regulation from the State University of Ceará (N° 6004720/2015).

Chemicals and media

Unless mentioned otherwise, the culture media and other chemicals used in the present study were purchased from Sigma Chemical Co. (St. Louis, Mo, USA).

Plants materials and phytochemical investigation from leaves of J. insularis

The fresh leaves of J. insularis previously identified in the National Herbarium of Cameroon under voucher specimen code 34997 [29] were collected in Western Cameroon (Batoufam subdivision, Upper-Plateau division, 5° 21′ Nord 10° 24′ East, Altitude 1515 m). The fresh leaves were then dried at room temperature in the shade. Subsequently, the plant extract decoction was prepared according to the protocol described by Telefo et al. [33]; briefly, 100 g of powder was submerged in 1.5 L of boiling distilled water for 30 minutes. After cooling, the extract was filtered and dried in a ventilated oven at 45°C. Finally, the plant decoction was lyophilized and kept in the freezer at -20°C. 22.96 g of the lyophilized extract was then diluted in the distilled water to obtain the desired concentrations.

A phytochemical screening of J. insularis, was performed by thin layer chromatography (TLC), proton nuclear magnetic resonance (1H NMR) and liquid chromatography-mass spectrometry (LC-MS), reliable methods used for identification of secondary metabolites.

Firstly, 100 mg of aqueous extract was suspended in MeOH (2 x 10 mL), over sonication for 15 min. The MeOH soluble fraction was evaporation under reduced pressure to yield 1.8 mg of the MeOH fraction (F1), while the insoluble fraction, designed F2, afforded 98.2 mg. 1.0 mg of each fraction (F1 and F2) was solubilized in 1.0 mL of MeOH and H2O, respectively, and subsequently applied on silica gel (Merck) chromatography plates (6 x 2 cm) with fluorescence indicator (F254). The samples were applied to the plates with the aid of a capillary tube, and for its development a ternary mixture of n-BuOH/AcOH/H2O (6:2:2) was used as the elution system. The plates were immersed in suitable developers and heating to ~100°C, when necessary. Developers specific for each class of secondary metabolites were used: Drangendorffi reagent (A) to identify alkaloids; α-naphthol acid solution (B) for glycosylated compounds; cerium sulfate acid/EtOH (C) for flavonoids and terpenoids, and vanillin/EtOH/perchloric solution (D) and EtOH/H2SO4 solution (E) as universal developers [34, 35]. After this procedure, a sample of the aqueous extract was fractionated on sephadex LH-20 using MeOH/H2O 8:2 as solvent of elution to obtain four main fractions; whose 1H NMR and LC-MS spectra were obtained.

Source of ovaries and experimental design

Ovaries from 35 adults (1–3 years old) mixed-breed sheep (Ovis aries) were collected at a local abattoir (Guaiúba municipality, Ceará, Brazil) at different times. Immediately postmortem, pairs of ovaries were washed once in 70% alcohol and then twice in minimum essential medium (MEM) plus HEPES (MEM-HEPES). The ovaries were placed into tubes containing 15 mL of MEM-HEPES, supplemented with penicillin (100 μg/mL) and streptomycin (100 μg/mL) and then transported to the laboratory at 4°C within 1 h since they were collected [36]. A total of 342 secondary follicles obtained from those ovaries were randomly in vitro cultured for 18 days in five different treatments as described below.

Additionally, to ensure that oocytes respond to in vitro maturation (IVM), ovaries from others 40 (1–3 years old) mixed-breed sheep were obtained as previously described and transported at 34°C during 1–2 h. We performed three replicates to obtain a total of 328 complexes oocyte cumulus cells (COCs) from antral follicles which were randomly distributed into five different IVM protocols as described below.

Isolation, selection and in vitro culture of sheep secondary follicles

In the laboratory, ovarian cortical slices (1–2 mm thick) were cut using a surgical blade and placed in MEM-HEPES. Then, secondary follicles (approximately 150–250 μm in diameter) were visualized under a stereomicroscope (SMZ 645 Nikon, Tokyo, Japan) and manually dissected from the slices of ovarian cortex using 26-gauge needles. After isolation, only secondary follicles with a visible oocyte, surrounded by granulosa cells, an intact basement membrane and no antral cavity [36] were selected to in vitro culture in different media conditions, corresponding to five different treatments. Therefore, secondary follicles were cultured in α-MEM (M5650, pH 7.2–7.4), supplemented with 3 mg/mL of bovine serum albumin (BSA), ITS (10 μg/mL insulin, 5.5 μg/mL transferrin, 5 ng/mL selenium), 2 mM of glutamine, 2 mM of hypoxanthine, 50 ng/mL of Leukemia Inhibitory Factor (LIF) and 50 ng/mL of Kit Ligant (KL), referred as α-MEM+ [37], considered the Control. Others follicles were in vitro cultured in α-MEM+ supplemented with 100 ng/mL recombinant bovine follicle stimulating hormone (FSH) or 0.3, 1.25, or 2.5 mg/mL of J. insularis (JI0.3, JI1.25, and JI2.5, respectively). The concentration of recombinant bovine FSH and J. insularis were chosen based on previous studies performed in our laboratory [8, 32]. The secondary follicles were individually cultured in 100 μL drops of five different (α-MEM+, FSH, JI0.3, JI1.25, and JI2.5) culture medium on Petri dishes (60 ×15 mm; Corning, USA) under mineral oil for 18 days at 39°C in 5% CO2 in air. Fresh medium was prepared immediately before use and incubated for 2 h prior to use, with 60 μL medium being replaced in each drop every 2 days [24].

After in vitro culture, follicular development and ROS levels were analyzed. In addition, oocytes recovery from follicles at the end of the culture period were in vitro matured for evaluation of oocyte viability, meiotic stages, meiotic resumption, and genes expression on follicular walls.

Morphological and follicular development (diameter and antrum formation) evaluation.

Follicles were classified according to their morphology as intact (no rupture of basement membrane), extruded (follicles were those that underwent rupture of their basement membrane) or degenerated (follicles showed darkened oocyte and/or misshapen granulosa cells). The percentage of morphologically intact follicles and follicular diameter were calculated only in intact follicles. The percentage of extruded follicles was calculated taking into account the total of extruded follicles divided by the total of intact normal follicles. Follicular diameter was calculated as the mean of two perpendicular measures of each follicle every 6 days with the aid of an ocular micrometer attached to a stereomicroscope (SMZ 645 Nikon, Tokyo, Japan; 100 x magnification). The average follicular daily growth was calculated as follows: the diameter of morphologically intact follicles on the last day they were intact minus their diameter at day zero divided by the number of days they remained intact. Antral cavity formation was defined as a visible translucent cavity within the granulosa cell layers [37].

Categories of follicular growth velocity.

All follicles in each treatment (Control, FSH, JI0.3, JI1.25 and JI2.5) were divided into three categories according to their daily growth as described previously [38]: (1) null growth (–12.7–0.0 μm day –1), follicles that did not grow during the culture, (2) low growth (0.1–12.0 μm day–1), follicles that grew up to 12 μm daily and (3) fast growth (12.1–46.7 μm day–1), follicles that grew up to 46.7 μm daily.

Reactive oxygen species levels.

The ROS levels were determined in the conditioned media by a spectrofluorometric method [39], using 2’, 7’ dihydrodichlorofluorescein diacetate (DCHF-DA) assay. Sample aliquot (50 μL) of media collected was incubated with 5 μL of DCHF-DA (1 mM). The oxidation of DCHF-DA to fluorescent dichlorofluorescein was measured for the detection of ROS. The DCF fluorescence intensity emission was recorded at 520 nm (with 480 nm excitation) 2 h after the addition of DCHF-DA to the medium.

Quantitative RT-PCR.

For evaluation of GPx, KL, CCNB1, HAS2 and GAPDH mRNA expression, total RNA of three pools of 8–10 viable follicular walls (granulosa and theca cells) was extracted using the Trizol reagent method (Invitrogen, Carlsbad, CA, USA) according to the recommendations of the manufacturer and further purified with PureLink RNA Mini Kit (Anbion, Carlsbad, CA, USA). After extraction, RNA concentration was determined using the NanoDrop System (Thermo Scientific NanoDrop Products), performed with 2 μL of material. Before the cDNA synthesis, all samples were standardized with the same amount of RNA to minimize qPCR variability. cDNA synthesis was performed according to the instructions of SuperScript III RT-PCR (Invitrogen, Carlsbad, CA, USA) manual using random primers (Invitrogen, Carlsbad, CA, USA) from 1 ng of total RNA. The gene-specific primers used for the amplification of different transcripts are shown in Table 1. All primers set annealed at 60°C.

[Figure omitted. See PDF.]

Table 1. Oligonucleotide primers used for polymerase chain reaction analysis.

https://doi.org/10.1371/journal.pone.0208760.t001

The qPCR reaction was performed in quadruplet always using control without cDNA to avoid possible contamination. Evaluations were performed in IQ5 Real-Time PCR Detection System (Bio-Rad, Hercules, CA, USA) using analysis of relative quantification. Detection of PCR products was measured by monitoring the increase in fluorescence emitted by the marker Power SYBR Green PCR Master Mix (Applied Biosystems, Carlsbad, CA, USA). For all amplifications, one dissociation curve (melting curve) was done for the verification of unspecific amplifications arising from contamination was held. The qPCR thermal cycle was as follow: initial denaturation and activation of the polymerase for 15 min at 94°C, followed by 40 cycles of 15 s at 94°C, 30 s at 60°C and 45 s at 72°C. The final extension was for 10 min at 72°C. Quantification of the transcripts of target genes was calculated from the difference of the values of the Ct values (threshold cycle PCR) in relation to transcripts of the endogenous gene, glyceraldehyde 3-phosphate dehydrogenase (GAPDH). First, the mean Ct of each sample, both the target gene and the endogenous gene was determined. From each sample, the subtraction of the mean value of the Ctgene-target to Ctgene-endogene provided the ΔCt. Subsequently, one ΔCt corresponding to a calibrator was chosen, normalizing all values by subtracting the resulting ΔCt chosen, to obtain the ΔΔCt. Finally, the final value of relative quantification was given by 2-ΔΔCt, where the calibrator or standard sample chosen was equal to one [40].

In vitro maturation of oocytes from in vitro grown secondary follicles

At the end of the culture period (day 18), all morphologically intact and extruded secondary follicles were carefully opened with 26-G needles under a stereomicroscope for oocyte recovery. Only oocytes (≥110 μm) with homogeneous cytoplasm and surrounded by at least one compact layer of cumulus cells were selected for in vitro maturation (IVM). The recovery rate was calculated by dividing the number of oocytes (≥110 μm) by the sum of morphologically intact and extruded follicles at day 18 of culture, multiplied by 100. The selected cumulus oocyte complexes (COCs) were washed three times in maturation medium composed of TCM 199 supplemented with 1% BSA, 5 μg/mL LH, 0.5 μg/mL recombinant bovine FSH, 10 ng/mL epidermal growth factor (EGF), 50 ng/mL insulin like growth factor 1 (IGF-1), 1 mM pyruvate, 1 μg/mL estradiol (E2), 100 μM cysteamine and different concentrations of J. insularis (JI0.3, JI1.25, or JI2.5). After being washed, the COCs were transferred to 100-μL drops of IVM medium (approximately 10 COCs per drop) under mineral oil and then incubated for 40 h at 39°C with 5% CO2. At the end of the maturation period, oocytes were stained with 10 μM Hoechst 33342 (483 nm) for the assessment of chromatin configuration.

In vitro maturation of oocyte recovery from antral follicles

To evaluate the effect of J. insularis on viability and maturation of oocytes grown in vivo (from antral follicles), selected COCs which served as a control for IVM of oocytes from secondary follicles grown in vitro were recovered from sheep ovary by slicing. The recovered COCs were washed twice with TCM 199 buffered with 25 mM HEPES (TCM 199—HEPES) and antibiotics. Then, only oocytes with homogeneous cytoplasm and surrounded by at least one compact layer of cumulus cells were selected and randomly distributed into five maturation procedures as follows: TCM 199 (Control), TCM 199 supplemented with 0.5 μg/mL FSH or with 0.3, 1.25, or 2.5 mg/mL of J. insularis (JI0.3, JI1.25, and JI2.5, respectively). Furthermore, groups of 20–35 oocytes were cultured in 200–350 μL (10 μL per COCs) maturation medium, for 24 hours in the same conditions mentioned above. At the end of the maturation period, the oocyte viability, meiotic resumption, and meiotic stages were evaluated.

Assessment of oocyte viability and chromatin configuration.

After IVM, oocyte (grown in vitro or in vivo) chromatin configuration and viability were assessed by fluorescence microscopy (Nikon, Eclipse 80i, Tokyo, Japan; 400x magnification). Oocytes were mechanically denuded by repeated pipetting and incubated in 100 μl droplets of PBS with 4 μM calcein-AM, 2 μM ethidium homodimer-1 (Molecular Probes Live/dead Viability/Cytotoxicity Kit for mammalian cells L3224, Invitrogen, Karlsruhe, Germany), 10 μM Hoechst 33342, and 0.5% glutaraldehyde. The emitted fluorescent signals of calcein-AM and ethidium homodimer were collected at 488 and 568 nm, respectively. Whereas the first probe detected the intracellular esterase activity of viable cells, the later labeled the nucleic acids of non-viable cells after plasma membrane disruption. Oocyte chromatin was stained by Hoescht 33342 (emission at 483 nm), and classified as germinal vesicle (GV), germinal vesicle breakdown (GVBD), metaphase I (MI), metaphase II (MII), or degenerated (DEG). The oocytes were considered viable when cytoplasm stained with calcein-AM (green) did not show abnormal chromatin configuration and/or did not label with ethidium homodimer (red).

Statistical analysis

All statistical procedures were carried out with Sigma Plot version 11.0 (Systat Software Inc., USA). Normality and homogeneity of variance were evaluated by Shapiro-Wilk and Levene's tests, respectively. Comparisons of means was performed by Kruskal-Wallis or Wilcoxon-Mann-Whitney tests, when appropriate. The percentage variables were analyzed among treatments and days of culture by chi-square or Fisher’s exact tests. Odds ratio and confidence interval (95%) were calculated to evaluate the effect of follicular growth category on percentages of extrusion. The mRNA expression level was analyzed using the t-Tests. Data were presented as mean (± SEM) or percentage. Statistical significance was defined as P < 0.05 (two-sided).

Results

TLC, 1H NMR and LC-MS analysis

According to the TLC procedures (S1 Fig), 1H NMR and LC-MS data were detected alkaloids, phenol compounds and sugars in the aqueous extract of J. insularis, corroborating with previous phytochemical reports on the Justicia species [34, 35].

Influence of J. insularis extract on follicular morphology during in vitro culture

Over the 18 days of the culture period, a significant decrease (P < 0.05) in the percentage of intact follicles was observed in all treatments. However, JI0.3 led to a higher (P < 0.05) percentage (36.8%) of intact follicles than in control treatment (21.6%) at the end of the culture period (Fig 1).

[Figure omitted. See PDF.]

Fig 1. Percentage of morphological intact follicles at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

D: day, MEM+: Minimal essential medium supplemented, FSH: recombinant bovine follicle stimulating hormone, JI: J. insularis. A total of 342 secondary follicles were distributed in the different treatments (n = 6 replicates). a,b,c,d Different letters denote significant differences among time for a given treatment group (P < 0.05). A,B Different letters denote significant differences among treatment groups within the same time point (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g001

No degenerated follicles were observed at D0 and D6. Small proportions of follicles were degenerated at D12 across all treatments. At D18, only JI1.25 treatment significantly increased the percentage of degenerated follicles compared to D0 (Fig 2).

[Figure omitted. See PDF.]

Fig 2. Percentage of degenerated follicles at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

D: day, MEM+: Minimal essential medium supplemented, FSH: recombinant bovine follicle stimulating hormone, JI: J. insularis. A total of 342 secondary follicles were distributed in the different treatments (n = 6 replicates). a,b,c,d Different letters denote significant differences among time for a given treatment group (P < 0.05). A,B Different letters denote significant differences among treatment groups within the same time point (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g002

Influence of J. insularis extract on follicular growth and antral formation during in vitro culture

Overall, follicular diameters progressively increased (P < 0.05) in all treatments until D12, except for FSH and J0.3 treatments in which diameter remained unchanged from D6 onwards. At D18, JI1.25 treatment led to a larger (P < 0.05) follicular diameter compared to control, JI0.3 and JI2.5 (Fig 3).

[Figure omitted. See PDF.]

Fig 3. Follicles diameter at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

D: day, MEM+: Minimal essential medium supplemented, FSH: recombinant bovine follicle stimulating hormone, JI: J. insularis. A total of 342 secondary follicles were distributed in the different treatments (n = 6 replicates). a,b,c,d Different letters denote significant differences among time for a given treatment group (P < 0.05). A,B Different letters denote significant differences among treatment groups within the same time point (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g003

During the three intervals (D0—D6; D6—D12; D12—D18), growth rates reflected what we observed in Table 2 about the lack of differences between treatments until D12. The control, JI0.3 and JI1.25 treatments maintained growth rate until the second third of culture, although it dropped (P < 0.05) from the second (D6—D12) to the last third of culture (D12—D18). Comparing among treatments at D18, except JI0.3, all of them showed higher (P < 0.05) growth rate than control. Regarding the overall growth rate, none treatment differed from control. However, JI0.3 treatment showed a lower (P < 0.05) daily growth rate than all treatments, except the JI2.5 treatment.

[Figure omitted. See PDF.]

Table 2. Mean (± SEM) daily growth of morphologically intact secondary follicles at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

https://doi.org/10.1371/journal.pone.0208760.t002

Looking at the different follicular growth categories: non-growing, slow-growing and fast-growing follicles (Table 3), both treatments JI1.25 and JI2.5 presented, respectively, higher (P < 0.05) percentage of slow-growing follicles and lower (P < 0.05) percentage of fast-growing follicles than control.

[Figure omitted. See PDF.]

Table 3. Percentage of secondary follicles within a growth category at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

https://doi.org/10.1371/journal.pone.0208760.t003

All treatments induced a progressive increase (P < 0.05) in the percentage of antral cavity formation compared to D0. Interestingly, at D6, JI0.3 treatment presented higher (P < 0.05) percentage of antral cavity formation than in the other treatments. In addition, JI0.3 was the only treatment that showed a higher (P < 0.05) percentage of antrum formation than control at any evaluated time point, although did not differ from the other treatments at the end of the culture or at D18 (Fig 4A).

[Figure omitted. See PDF.]

Fig 4.

Percentage of antrum formation (A) at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively). (B): Normal sheep secondary follicle at D0 (i) or at D18 day in J. insularis 0.3 mg/mL (JI0.3) (ii). Note formation of antrum (a) on D18. Representative images of fluorescent metaphase II oocyte grown in vitro (iii) or in vivo (iv). Note presence of the first polar body (cp). D: day, MEM+: Minimal essential medium supplemented, FSH: recombinant bovine follicle stimulating hormone, JI: J. insularis. A total of 342 secondary follicles were distributed in the different treatments (n = 6 replicates. a,b,c,d Different letters denote significant differences among time for a given treatment group (P < 0.05). A,B Different letters denote significant differences among treatment groups within the same time point (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g004

Representative images of normal follicles, and metaphase II oocyte grown in vitro or in vivo are shown (Fig 4B).

Influence of J. insularis extract on follicular extrusion during in vitro culture

The percentage of extruded follicles increased (P < 0.05) in all treatments from D0 to D18. Moreover, at D12, a higher percentage (P < 0.05) of extruded follicles was observed in the control compared to all treatments, except JI2.5. On the other hand, at D18, the percentage of extruded follicles in the control was higher (P < 0.05) only than JI0.3 (Fig 5).

[Figure omitted. See PDF.]

Fig 5. Percentage of extrusion at different time point (D0, D6, D12, D18) in MEM+ (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

D: day, MEM+: Minimal essential medium supplemented, FSH: recombinant bovine follicle stimulating hormone, JI: J. insularis. A total of 342 secondary follicles were distributed in the different treatments (n = 6 replicates). a,b,c,d Different letters denote significant differences among time for a given treatment group (P < 0.05). A,B Different letters denote significant differences among treatment groups within the same time point (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g005

Dynamic of follicular growth and extrusion of secondary follicles.

Regardless the treatment, JI0.3 showed a fast-growing rate and a low percentage of extrusion compared to control. When comparing between follicle growth categories in different intervals of in vitro culture, the odds ratio (OR) analysis showed that this positive association was greater in fast-growing follicles compared to slow-growing follicles in the first two intervals of culture (D0—D6 and D6—D12) (P = 0.0001 and 0.0062, respectively) (Table 4).

[Figure omitted. See PDF.]

Table 4. Association analyses between follicular growth categories and percentage of extrusion in different intervals of in vitro follicle culture.

https://doi.org/10.1371/journal.pone.0208760.t004

Influence of J. insularis extract on levels of ROS during the in vitro culture of follicles

Differences among treatments were not found at D6. On the other hand, at D18 all treatments presented higher (P < 0.05) ROS concentration than the control. In addition, JI2.5 presented a higher (P < 0.05) levels of ROS than FSH, although did not differ from JI0.3 or JI1.25 (Table 5).

[Figure omitted. See PDF.]

Table 5. Level of ROS measured in the culture medium from secondary follicles before (D0) and during 18 days of in vitro culture (D6, D12, D18) in MEM+ (Control), FSH or in JI0.3, JI1.25 or JI2.5.

https://doi.org/10.1371/journal.pone.0208760.t005

Influence of J. insularis extract on gene expression in follicular walls during in vitro culture

The relative expression of GPX, KL, CCNB1, and HAS2 was measured in follicular walls. No differences were observed between control and all treatments in mRNA expression for GPX, KL, CCNB1 and HAS2 (Fig 6A, 6B, 6C and 6D respectively).

[Figure omitted. See PDF.]

Fig 6.

Relative mean (standard error of the mean) expression of mRNA of GPX (A), KL (B), CCNB1 (C), and HAS2 (D) before (D0) and during 18 days of in vitro culture (D6, D12, D18) in MEM+ (Control), FSH or in JI0.3, JI1.25 or JI2.5. A,B Different letters denote significant differences among treatments (P < 0.05).

https://doi.org/10.1371/journal.pone.0208760.g006

Influence of J. insularis extract on structure and function of oocytes resulting from follicle cultured in vitro

In the first experiment, the percentage of fully grown oocytes (≥110 μm), oocyte diameter, viability rate and meiotic stages after IVM are shown in Table 6. None treatment differed from control in any evaluated end point. However, the viability rate was significantly higher in JI0.3 compared to FSH treatment.

[Figure omitted. See PDF.]

Table 6. Percentage of fully grown oocytes, oocyte diameter, viability rate, percentage of meiotic resumption, and meiotic stages of oocytes matured in TCM 199 (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

https://doi.org/10.1371/journal.pone.0208760.t006

After IVM of oocytes originate from follicles grown in vivo (Control experiment), the percentage of oocyte viability and meiotic resumption (n/total) was significantly higher (P < 0.05) in JI1.25 compared to JI2.5. Regarding to the percentage of metaphase II oocytes, FSH showed a similar percentage than JI0.3. Moreover, only JI0.3 showed a significant higher (P < 0.05) percentage than control (Table 7).

[Figure omitted. See PDF.]

Table 7. Percentage of oocyte viability, meiotic resumption, and meiotic stages of oocytes recovery from antral follicles matured in TCM 199 (Control), FSH or in J. insularis 0.3, 1.25 or 2.5 mg/mL (JI0.3, JI1.25 or JI2.5 respectively).

https://doi.org/10.1371/journal.pone.0208760.t007

Discussion

To the best of our knowledge, this study constitutes the first report demonstrating the beneficial effects of the J. insularis extract on the in vitro culture and maturation of ovine isolated follicles. While FSH has been widely used to maintain follicle survival [41], promote the antrum formation [42] and stimulate follicular growth and oocyte maturation [11, 36], similar effects were obtained with 0.3 mg/mL of J. insularis. Addition of this natural substance in the culture or maturation medium represents an efficient alternative to FSH.

The phytochemical screening by TLC of the aqueous extract of J. insularis revealed alkaloids and flavonoids. In addition, a sample (1.0 g) of the aqueous extract was fractionated on sephadex LH-20 eluted with MeOH 8:2 to furnish four fractions which were analyzed by 1H NMR and LC-MS. Inspection of these techniques allowed to identify the alkaloid trigonelline [43] and phenol compounds as eucomic acid [44] and kaempferol glycosides derivatives [45] in agreement with TLC. As expected, sugars as sucrose, and the α- and β-glucose stereoisomers [46] were also identified. Although there are no studies on the isolation of the chemical constituents of J. insularis, a literature survey on Justicia species revealed the presence of those classes of compounds [29], corroborating with our findings (S2 Fig). In addition, according to the literature, plants of the genus Justicia are known as producers of bioactive compounds as alkaloids and flavonoids [47].

We should take into account that the seasonality of climatic elements such as temperature, relative humidity and solar radiation can alter the physiological behavior of plants and, consequently, their growth and development, as well as the chemical and biological composition of the soil [48]. Thus, for all the secondary metabolites identified from J. insularis, the variation of climatic elements can affect their concentrations in the plant [49]. Therefore, the environments in which the plant develops exert a direct influence on the chemical composition of the extracts.

In our study, percentages of morphologically intact follicles decreased at the end of the culture period regardless of the treatment. This expected result is common during in vitro culture of secondary follicles [12, 19]. Such effect could be due to the action of toxic metabolites and ROS. In excess, these metabolites can oxidize important molecules that induce the release of nucleases, proteases, and lipases from mitochondria [12], resulting in the disruption of the basal membrane [50]. This was observed in previous published articles using natural substances with the same culture period in ovine [22, 24] and goat species [19, 23]. Interestingly, J. insularis at 0.3 mg/mL showed a higher percentage of intact follicles than the control. This could be due to the action of the flavonoids 3’-Metoxy-kaempferol-arabinosyl-rhamnoside, and Kaempferol-arabinosyl-rhamnoside which are phenolic compounds identified in the extract and have the capacity to neutralize damage caused by oxidation. Choi, [51] has demonstrated that pretreatment with kaempferol prior to antimycin A exposure significantly reduced cell damage by preventing mitochondrial membrane potential dissipation and ROS production. Other authors showed that cellular reactive oxygen species levels distinctly diminished by trigonelline treatment of HT-29/Caco-2 cells [52].

Percentages of extrusion increased significantly during culture period in all treatments. Moreover, the JI0.3 showed lower percentage of extruded follicles compared to control. This may be due to the increased in the follicular growth. Indeed, analyses of the chances of extrusion in non, slow or fast-growing follicles within the first (D0—D6) and second (D6—D12) third of the culture in vitro showed that in the first third (D0—D6), fast-growing follicles were 3.3 times more likely to extrude than those with slow growth. Furthermore, in the second third (D6—D12), the same behavior occurred (fast-growing follicles were 2.6 times more likely to extrude than slow-growing follicles).

During the culture period, all treatments increased follicle diameter. Interestingly, FSH and JI0.3 treatments showed similar follicle diameter. FSH has a well-established role in modulating granulosa cell proliferation and antrum formation which contributed to an increase in follicular diameter [53]. Erickson et al. [54] reported that FSH interacts with several growth factors such as KL to induce follicular growth. Luz et al. [21] showed that culture medium of ovine secondary follicles supplemented with KL resulted in an increased rate of follicular diameter and antrum formation. The JI 0.3 response similar to FSH could be due to the action of the trigonelline which is a phytohormone that induced the proliferation of neuronal cells [55]. How trigonelline acts on the receptor of granulosa cells awaits further investigations.

All the treatments increased the antrum formation. Such effect could be due to the secondary metabolites of the plant. The TLC, 1H NMR and LC-MS analysis revealed the presence of alkaloid, flavonoids and glycosylated terpenoids. These metabolites are responsible for enhancing ovarian follicle growth and increasing in the number of corpus luteum in rats [33], and promoted the in vitro activation and survival of ovine preantral follicles enclosed in ovarian tissue [32]. Interestingly, at D6, JI0.3 showed a higher percentage of antrum formation. This finding is important because the ability to form an antrum is considered as a good marker of follicular functionality [56], as the mechanisms by which small cavities of fluid develop inside the follicle to form the antral cavity are related to the secretion of osmotically active molecules into small spaces between the granulosa cells [57]. Recently, a study using Amburana cearensis showed that its metabolite protocatechuic acid improves the antrum formation after 18 days of ovine preantral follicle culture in vitro [22].

In the current study, JI0.3 caused a fast-growing of secondary follicles, however, this treatment resulted in low percentage of extrusion compared to control. This means that there was an adequate response of the oocytes without membrane damages. Similar results were reported in sheep secondary follicles, grown for 6 days with the same culture medium [58]. This may be due to the interaction between flavonoids present in the plant extract and components of the culture medium. It is known that the flavonoids protect human vascular endothelial cells against oxidative damages [59] and have antimicrobial and antioxidant properties [60]. These flavonoids interact with membrane proteins, making them stable. Therefore, we believe that this increasing hardness can give follicular membrane firmness and prevent its rupture, consequently avoiding oocyte extrusion. On the other hand, other studies using androstenedione and FSH in the culture medium of isolated caprine secondary follicles found that higher percentage of fast-growing follicles was detrimental for efficiency of caprine secondary follicles cultured in vitro [38].

Recent studies have shown that J. insularis maintains the ROS level [32], however, in the current study at D18, all treatments presented higher ROS concentration than control. We believe that these results may be attributed to an excess of antioxidants in the culture medium. It is known that the balance between ROS and antioxidants within the oocytes is critical to cell functions, such as chromosome segregation [61], mitochondria activity [62], ATP level maintenance and DNA methylation [63]. Therefore, ROS may affect follicles and oocyte growth during the in vitro culture. Indeed, our basic culture medium is rich in supplements among which selenium (5.5 μg/mL) and transferrin (50 ng/ mL). These supplements in addition to J. insularis increases the ROS level. In this study, the increase of the ROS level was not detrimental for the follicles because no significant difference was observed on the GPx mRNA expression.

Several genes have been identified in follicular walls as biomarkers to understand the dynamics of follicular development. Among them GPx related to oxidative stress [64], KL indicative of follicular growth [65]; cyclin B1 and HAS2 indicative of progression of oocyte maturation [66]. We observed that after the IVM of COCs from secondary follicles, the follicular walls (granulosa and theca cells) expressed similar transcript levels. The gene expression similarity between J0.3 and FSH may support the use of this natural substance for the in vitro culture of ovine isolated secondary follicles.

Despite no effect was observed on the meiotic resumption of oocytes from in vitro growth secondary follicles, addition of JI0.3 on the maturation medium of oocyte from antral follicles showed similar percentage than FSH. In addition, this percentage was higher than the control. We believe that the presence of J. Insularis in the maturation medium could have improve the synthesis of the mitosis-promoting factor (MPF). In fact, during the meiosis resumption, the MPF, a protein complex composed of subunits cyclin B1 and p34cdc2 [67] is activated and regulate the germinal vesicle breakdown (GVBD) [68]. MPF activity is regulated by the CDK1 produced by the cells. The activity of MPF was described in many mammalian oocytes: it appears just before GVBD and increases until metaphase I stage, then its activity decreases in anaphase-telophase and increases again, reaching its maximum level in metaphase II in goat [69], sheep [70] and cow [71]. The oocyte (recovery from antral follicles) viability rate of was higher in JI1.25 compared to JI2.5. This could be due to an excess of toxic metabolites and reactive oxygen species present of the maturation medium. In fact, phytochemical analysis of the extract showed that it is constitute of secondary metabolites (flavonoids 3’-Metoxy-kaempferol-arabinosyl-rhamnoside, and Kaempferol-arabinosyl-rhamnoside, trigonelline among others) which have antioxidant activity as revealed by previous study (Bakuradze et al., 2010; Choi et al., 2011). In high concentration, those metabolite could acts as pro-oxidant and therefore increase the level of reactive oxygen species (free radical, hydrogen peroxide, hydroxyl ion…). As reported by Costa et al., 2011, although a critical amount of reactive oxygen species is essential for the physiological activities of follicles, excessive amount of them generates a contrary effect.

In summary, the present study showed for the first time that 0.3 mg/mL of J. insularis showed similar effect than FSH when added in the culture or maturation media of ovine isolated secondary follicles. It seems that when FSH is not available, Justicia iusularis could be used with the same benefits. Further studies are needed to isolate the metabolites present in J. insularis and assess the developmental competence of the oocytes after IVF.

Supporting information

[Figure omitted. See PDF.]

S1 Fig. Identification of secondary metabolites by thin layer chromatography (TLC).

The developers used are specific to each class of metabolite as described: (A) specific Drangendorffi reagent to identify alkaloids; (B) α-Naphthol acid solution for glycosylated compounds; (C) acid solution of vanillin; (D) solution of ethanol / sulfuric acid used as universal developers and (E) acid solution of cerium sulfate for flavonoids and terpenoids.

https://doi.org/10.1371/journal.pone.0208760.s001

(PDF)

S2 Fig. Metabolites of J. insularis identified by proton nuclear magnetic resonance (1H NMR) and liquid chromatography-mass spectrometry (LC-MS).

https://doi.org/10.1371/journal.pone.0208760.s002

(PDF)

Acknowledgments

The authors thank Dr. Phelix Bruno Telefo and Mr. Celestin Tchouanguep for providing the medicinal plants.

Citation: Mbemya GT, Cadenas J, Ribeiro de Sá NA, Damasceno Guerreiro D, Donfack NJ, Alberto Vieira L, et al. (2018) Supplementation of in vitro culture medium with FSH to grow follicles and mature oocytes can be replaced by extracts of Justicia insularis. PLoS ONE 13(12): e0208760. https://doi.org/10.1371/journal.pone.0208760

References

1. Araújo VR, Gastal MO, Figueiredo JR, Gastal EL. In vitro culture of bovine preantral follicles: a review. Reprod Biol Endocrinol 2014; 13:12–78. pmid:25117631

2. Dela Peña EC, Takahashi Y, Katagiri S, Atabay EC, Nagano M. Birth of pups after transfer of mouse embryos derived from vitrified preantral follicles. Reproduction 2002, 123:593–600. pmid:11914121

3. O’brien MJ, Pendola JK, Eppig JJ. A revised protocol for development of mouse oocyte from primordial follicles dramatically improves their development competence. Biol Reprod 2003; 68:1682–1686. pmid:12606400

4. Higuchi CM, Maeda Y, Horiuchi T, Yamazaki Y. A simplified method for three-dimensional (3-D) ovarian tissue culture yielding oocytes competent to produce full-term offspring in mice. PloS one 2015; 16:e0143114. pmid:26571501

5. Agarwal A, Durairajanayagam D, Du Plessis SS. Utility of antioxidants during assisted reproductive techniques: an evidence based review. Reprod Biol Endocrinol 2014; 12:112. pmid:25421286

6. Arunakumari G, Shanmugasundaram N, Rao VH. Development of morulae from the oocytes of cultured sheep preantral follicles. Theriogenology 2010; 74:884–894. pmid:20615540

7. Saraiva MVA., Rossetto R, Brito IR, Celestino JJH, Silva CMG, Faustino LR et al. Dynamic medium produces caprine embryo from preantral follicles grown in vitro. Reprod Sci 2010; 17:35–43. pmid:20926838

8. Magalhães DM, Fernandes DD, Mororó MB, Silva CM, Rodrigues GQ, Bruno JB, et al. Effect of the medium replacement interval on the viability, growth and in vitro maturation of isolated caprine and ovine pre-antral follicles. Reprod Domest Anim 2011; 46:134–140. pmid:20403127

9. McNatty KP, Reader K, Smith P, Heath DA, Juengel JL. Control of ovarian follicular development to the gonadotrophin-dependent phase: a 2006 perspective. Soc Reprod Fertil Suppl. 2007; 64:55–68. pmid:17491140

10. Santos J, Menezes VM, Barberino RS, Macedo TJS, Lins TLB, Gouveia BB, et al. Immunohistochemically localization of fibroblast growth factor-2 in the sheep ovary and its effects on pre-antral follicle apoptosis and development in vitro. Reprod Domest Anim 2014; 49:222–228. pmid:24750547

11. Ferreira ACA, Maside C, Sá NAR, Guerreiro DD, Correia HHV, Leiva-Revilla J, et al. Balance of insulin and FSH concentrations improves the in vitro development of isolated goat preantral follicles in medium containing GH. Anim Reprod Sci 2016; 165:1–10. pmid:26723481

12. Pessoa AFC, Rocha RMP, Brito IR, Silva GM, Chaves RN, Magalhães-Padilha DM, et al. Effect of morphological integrity, period, and type of culture system on the in vitro development of isolated caprine preantral follicles. Theriogenology 2014; 82:312–317. pmid:24839921

13. Joyce IM, Pendola FL, Wigglesworth K, Eppig JJ. Oocyte regulation of kit ligand expression in mouse ovarian follicles. Dev Biol 1999; 214:342–353. pmid:10525339

14. Magalhães-Padilha DM, Geisler-Lee J, Wischral A, Gastal MO, Fonseca GR, Eloy YRG, et al. Gene Expression During Early Folliculogenesis in Goats Using Microarray Analysis. Biol Reprod 2013; 89:1–12. pmid:23759311

15. Leiva-Revilla J, Cadenas J, Vieira AL, Campello CC, Celestino JJH, Pessoa ODL, et al. Toxicity effect of Auxemma oncocalyx fraction and its active principle oncocalyxone A on in vitro culture of caprine secondary follicles and in vitro oocyte maturation. Semin Cienc Agrar 2017; 38:1361–1374. https://doi.org/10.5433/1679-0359.2017v38n3p1361

16. Turpaev KT. Reactive Oxygen Species and Regulation of Gene Expression. Biochemistry (Moscow), Vol. 67, No. 3, 2002, pp. 281–292. https://doi.org/10.1023/A:1014819832003. pmid:11970728

17. Dalton TP, Shertzer HG, Puga A. Regulation of gene expression by reactive oxygen. Annu Rev Pharmacol Toxicol 1999; 39:67–101. pmid:10331077

18. Rossetto R, Saraiva MV, Dos Santos RR, Da Silva CM, Faustino LR, Chaves RN et al. Effect of medium composition on the in vitro culture of bovine pre-antral follicles: morphology and viability do not guarantee functionality. Zygote. 2013; 21:125–128. pmid:22717039

19. Sá NAR, Araújo VR, Correia HHV, Ferreira ACA, Guerreiro DD, Sampaio AM, et al. Anethole Improves the in vitro Development of Isolated Caprine Secondary Follicles. Theriogenology 2016; 89:226–234. pmid:28043356

20. Gouveia BB, Macedo TJS, Santos JMS, Barberino RS, Menezes VG, Müller MC, Almeida JRGS, et al. Supplemented base medium containing Amburana cearensis associated with FSH improves in vitro development of isolated goat preantral follicles. Theriogenology. 2016; 86:1275–1284. pmid:27287468

21. Luz VB, Araújo VR, Duarte ABG, Silva GM, Chaves RN, Brito IR, et al. Kit ligand and insulin-like growth factor I affect the in vitro development of ovine preantral follicles. Small Rumin Res 2013; 115:99–102. https://doi.org/10.1016/j.smallrumres.2013.09.003

22. Barberino RS, Barros VRP, Menezes VG, Santos LP, Araújo VR, Queiroz MAA, et al. Amburana cearensis Leaf Extract Maintains Survival and Promotes in vitro Development of Ovine Secondary Follicles. Zygote 2015:1–9. pmid:26083197

23. Gouveia BB, Macedo TJ, Santos JM, Barberino RS, Menezes VG, Müller MC, et al. Supplemented base medium containing Amburana cearensis associated with FSH improves in vitro development of isolated goat preantral follicles. Theriogenology 2016; 86:1275–1284. pmid:27287468

24. Lins TLBG, Cavalcante AYP, Santos JMS, Menezes VG, Barros VRP, Barberino RS, et al. Rutin can replace the use of three other antioxidants in the culture medium, maintaining the viability of sheep isolated secondary follicles. Theriogenology 2017; 89:263–270. pmid:28043362

25. Mishra A, Reddy IJ, Gupta PS, Mondal S. Expression of Apoptotic and Antioxidant Enzyme Genes in Sheep Oocytes and In vitro Produced Embryos. Anim Biotechnol 2017; 28:18–25. pmid:27379566

26. Kuroda T, Naito K, Sugiura K, Yamashita M, Takakura I, Tojo H. Analysis of the roles of cyclin B1 and cyclin B2 in porcine oocyte maturation by inhibiting synthesis with antisense RNA injection. Biol Reprod 2004; 70:154–159. pmid:12954723

27. Cadenas J, Leiva-Revilla J, Vieira LA, Apolloni LB, Aguiar FLN, Alves BG, et al. Caprine ovarian follicle requirements differ between preantral and early antral stages after IVC in medium supplemented with GH and VEGF alone or in combination. Theriogenology 2017; 87:321–332. pmid:27729112

28. Goka MSC, Telefo PB, Mbemya GT, Awouafack MD, Lienou LL, Yemele DM, et al. Potentialisation of Pregnant Mare Serum Gonadotropin Inducing Effect on Ovarian Follicles Growth by the Aqueous Extract of Aloe buettneri, Dicliptera verticillata, Hibiscus macranthus and Justicia insularis Leaves in Immature Rats. Pharmacolology 2016; 7:328–336.

29. Telefo PB, Moundipa PF, Tchana AN, Tchouanguep D, Mbiapo FT. Effects of an Aqueous Extract of Aloe buettneri, Justicia insularis, Hibiscus macranthus, Dicliptera verticillata on Some Physiological and Biochemical Parameters of Reproduction in Immature Female Rats. J Ethnopharmacol 1998; 63:193–200. pmid:10030723

30. Telefo PB, Moundipa PF, Tchouanguep FM. Oestrogenicity and effect on hepatic metabolism of the aqueous extract of the leaf mixture of Aloe buettneri, Dicliptera verticillata, Hibiscus macranthus and Justicia insularis. Fitoterapia. 2002; 73:472–478. pmid:12385869

31. Telefo PB, Moundipa PF, Tchouanguep FM. Inductive Effects of the Leaf Mixture Extract of Aloe buettneri, Justicia insularis, Dicliptera verticillata and Hibicus marcranthus on in vitro production of oestradiol. J Ethnopharmacol 2004; 91:225–230. pmid:15120443

32. Mbemya GT, Guerreiro DD, Donfack NJ, Silva LM, Vieira LA, Sousa GFC, et al. Justicia insularis Improves the in vitro Survival and Development of Ovine Preantral Follicles Enclosed in Ovarian Tissue. J Pharm Pharmacol 2017;5:668–680.

33. Telefo PB, Tagne SR, Koona OES, Yemele DM, Tchouanguep FM, Effect of the Aqueous Extract of Justicia Insularis T. Anders (Acanthaceae) on Ovarian Folliculogenesis and Fertility of Female Rats. Afr J Tradit Complement Altern Med 2012; 9:197–203. pmid:23983335

34. Da Silva NLA, Miranda FAA, Da Conceição GM. Phytochemical Screening of Cerrado Plants, from the Municipal Environmental Protection Area of Inhamum, Caxias, Maranhão, Scientia Plena 2010; 6:1–17.

35. Sherman J, Fried B. Handbook of Thin-Layer Chromatography. 3ª, 1991. Lafayette College. Easton, Pennsylvania, U.S.A. ISBN: 0-8247-0895-4

36. Lima LF, Rocha RM, Duarte AB, Brito IR, Silva GM, Rodrigues GQ, et al. Unexpected effect of the vehicle (grain ethanol) of homeopathic FSH on the in vitro survival and development of isolated ovine preantral follicles. Microsc Res Tech 2017; 4:406–418. pmid:27921341.

37. Luz VB, Araujo VR, Duarte AB, Celestino JJ, Silva TF, Magalhaes-Padilha DM, et al. Eight-cell parthenotes originated from in vitro grown sheep preantral follicles. Reprod Sci 2012; 19:1219–1225. pmid:22562971

38. Apolloni LB, Bruno JB, Alves BG, Ferreira ACA, Paes VM, Moreno JLRC, et al. Accelerated follicle growth during the culture of isolated caprine preantral follicles is detrimental to follicular survival and oocyte meiotic resumption. Theriogenology

39. Loetchutinat S, Kothan S, Dechsupa J, Meesungnoen J, Jay-Gerin SM. Spectrofluorometric Determination of Intracellular Levels of Reactive Oxygen Species in Drug-Sensitive and Drug-Resistant Cancer Cells Using the 2’,7’-Dichlorofluorescein Diacetate Assay. Radiat Phys Chem 2005; 72:323–331.

40. Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-time quantitative PCR and the 2 (Delta Delta C (T)) method. Methods 2001; 25:402–408. pmid:11846609

41. Costa SH, Santos RR, Rondina D, Andrade ER, Ohashi OM, Rodrigues AP, et al. Effects of IAA in combination with FSH on in vitro culture of ovine preantral follicles. Zygote 2010; 18:89–92. pmid:19586559

42. Barros VR, Cavalcante AY, Macedo TJ, Barberino RS, Lins TLB, Gouveia BB, et al. Immunolocalization of Melatonin and Follicle-Stimulating Hormone Receptors in Caprine Ovaries and their Effects During in vitro Development of Isolated Pre-Antral Follicles. Reprod Domest Anim 2014; 48:1025–1033. pmid:23981138

43. Farag MA, Porzel A, Wessjohann LA. Unraveling the active hypoglycemic agent trigonelline in Balanites aegyptiaca date fruit using metabolite fingerprinting by NMR. J Pharm Biomed Anal. 2015; 115:383–387. pmid:26275727

44. Chahdoura H, Barreira JC, Barros L, Santos-Buelga C, Ferreira IC, Achour L. Phytochemical characterization and antioxidant activity of the cladodes of Opuntia macrorhiza (Engelm.) and Opuntia microdasys (Lehm.). Food Funct. 2014; 9:2129–2136. pmid:25007233

45. Abu-Reidah IM, Arráez-Román D, Warad I, Fernández-Gutiérrez A, Segura-Carretero A. UHPLC/MS2-based approach for the comprehensive metabolite profiling of bean (Vicia faba L.) by-products: A promising source of bioactive constituents. Food Res Int. 2017; 93:87–96. pmid:28290284

46. Palama TL, Menard P, Fock I, Choi YH, Bourdon E, Govinden-Soulange J, et al. Shoot differentiation from protocorm callus cultures of Vanilla planifolia (Orchidaceae): proteomic and metabolic responses at early stage. BMC Plant Biol. 2010; 10:82. pmid:20444255

47. Corrêa GM, Alcântara AFDE. Chemical constituents and biological activities of species of Justicia—a review. Braz J Pharmacog 2017; 22:220–238.

48. Inderjit , Dakshini KMM. Hesperitin 3 rutinoside (hesperidin) and taxifolin 3-arabinoside as germination and growth inhibitors in soils associated with the weed Pluchealanceolata (DC.) C.B. Clarke (Asteraceae). J Chem Ecol. 1992; 17:1585–1591. pmid:24257882

49. Suarez S, Gil A, Lorenzo E. Aloysia citriodora: morphology and density of glandular trichomes, and its relationships with essential oil content. In: Simpósio Brasileiro de Óleos Essenciais, 2, 2003, Campinas, SP. Anais… Campinas: Instituto Agronômico. pp. 78.

50. Nijveldt RJ, Van Nood E, Van Hoorn DE, Boelens PG, Van Norren K, Van Leeuwen PA. Flavonoids: a review of probable mechanisms of action and potential applications. Am J Clin Nutr. 2001;74:418–425. pmid:11566638

51. Choi EM. Kaempferol protects MC3T3-E1 cells through antioxidant effect and regulation of mitochondrial function. Food Chem Toxicol. 2011; 49:1800–1805. pmid:21565246

52. Bakuradze T, Lang R, Hofmann T, Stiebitz H, Bytof G, Lantz I, et al. Baum M, Eisenbrand G, Janzowski C Antioxidant effectiveness of coffee extracts and selected constituents in cell-free systems and human colon cell lines. Mol Nutr Food Res. 2010;54:1734–1743. pmid:20589861

53. Richards JS, Russell DL, Ochsner S, Hsieh M, Doyle KH, Falender AE, et al. Novel signalling pathways that control ovarian follicular development, ovulation and luteinization. Rec Prog Horm Res 2002; 57:195–220. pmid:12017544

54. Erickson GF, Shimazak S, The spatiotemporal expression pattern of the bone morphogenetic protein family in rat ovary cell types during estrous cycle. Reprod Biol Endocrinol 2003; 5:1–9. pmid:12741959

55. Zhou J, Chan L, Zhou S. Trigonelline: a plant alkaloid with therapeutic potential for diabetes and central nervous system disease. Curr Med Chem. 2012;19:3523–3531. pmid:22680628

56. Rossetto R, Santos RR, Silva GM, Duarte ABG, Silva CMG, Campello CC, et al. Comparative study on the in vitro development of caprine and bovine preantral follicles. Small Rumin Res 2012; 113:167–170. https://doi.org/10.1016/j.smallrumres.2013.03.004

57. Rodgers RJ, Irving-Rodgers HF, Formation of the ovarian follicular antrum and follicular fluid. Biol Reprod 2010; 82:1021–1029. pmid:20164441

58. Lunardi FO, Chaves RN, Lima LF, Araújo VR, Brito IR, Souza CE, et al. Vitrified sheep isolated secondary follicles are able to grow and form antrum after a short period of in vitro culture. Cell Tissue Res 2015; 362:241–251. pmid:25948481

59. Ruijters EJB, Weseler AR, Kicken C, Haenen GRMM, Bast A, The flavanol (–)-epicatechin and its metabolites protect against oxidative stress in primary endothelial cells via a direct antioxidant effect. Eur J Pharmacol 2013; 715:147–153. pmid:23747595.

60. Tatsimo SJN, Tamokou JD, Havyarimana L, Csupor D, Forgo P, Hohmann J, et al. Antimicrobial and antioxidant activity of kaempferol rhamnoside derivatives from Bryophyllum pinnatum. BMC Res 2012; 5:158–163. pmid:22433844

61. Taylor CT. Antioxidants and reactive oxygen species in human fertility. Environ Toxicol Pharmacol 2001; 10:189–98. pmid:21782576

62. Costa RAP, Romagna CD, Pereira JL, Souza-pinto NC. The Role of Mitochondrial DNA Damage in the Citotoxicity of Reactive Oxygen Species. J Bioenerg Biomembr 2011; 43:25–29. pmid:21286795

63. Heinzmann J, Mattern F, Aldag P, Bernal-Ulloa SM, Schneider T, Haaf T, et al. Extended in vitro maturation affects gene expression and DNA methylation in bovine oocytes. Mol Hum Reprod 2015; 10:770–782. pmid:26155800

64. Sadeghipour M, Terreux R, Phipps J. Flavonoids and Tyrosine Nitration: Structure Activity Relationship Correlation with Enthalpy of Formation. Toxicology 2005; 19:155–65. pmid:15649628

65. Ribeiro RP, Portela AMLR, Silva AWB, Costa JJN, Passos JRS, Cunha EV, et al. Effects of jacalin and follicle-stimulating hormone on in vitro goat primordial follicle activation, survival and gene expression. Zygote 2014;23:537–549. pmid:24869637

66. Zhao G, Chen Y, Carey L, Futcher B. Cyclin-Dependent Kinase Co-Ordinates Carbohydrate Metabolism and Cell Cycle in S. cerevisiae Molecular Cell 2016; 62:546–557. pmid:27203179

67. Robert C, Hue I, McGraw S, Gagne D, Sirard MA. Quantification of Cyclin B1 and p34cdc2 in Bovine Cumulus-Oocyte Complexes and Expression Mapping of Genes Involved in the Cell Cycle by Complementary DNA Macroarrays. Biol Reprod 2002; 67:1456–464. pmid:12390876

68. Taieb R, Thibier C, Jessus C. On cyclins, oocytes, and eggs. Mol Reprod Dev 1997; 48:397–411. pmid:9322253

69. Anguita B, Paramio MT, Ana R, Macedo J, Morat R, Mogasb T, Izquierdo D. Total RNA and protein content, Cyclin B1 expression and developmental competence of prepubertal goat oocytes. Anim Reprod Sci 2008; 103:290303. pmid:17250980

70. Ledda S, Bogliolo L, Leoni G, Naitana S. Cell coupling and maturation-promoting factor activity in in vitro matured prepubertal and adult sheep oocytes. Biol Reprod 2001; 65:247–52. pmid:11420246

71. Mihm M, Baker PJ, Fleming LM, Monteiro AM, O’Shaughnessy AJ. Differentiation of the bovine dominant follicle from the cohort upregulates mRNA expression for new tissue development genes. Reproduction 2008; 135:253–265. pmid:18239053

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© 2018 Mbemya et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.

Abstract

The present study evaluated the effect of supplementing in vitro culture medium with J. insularis compared to FSH on isolated secondary follicles and in vitro maturation of oocytes from those follicles. Secondary follicles were isolated from sheep ovaries and individually cultured for 18 days in α-MEM+ (Control), α-MEM+ supplemented with 100 ng/mL recombinant bovine follicle stimulating hormone (FSH) or with 0.3, 1.25, or 2.5 mg/mL of J. insularis extract (JI0.3, JI1.25, and JI2.5, respectively). Culture medium collected every 2 days was used to measure ROS levels. At the end of the culture period, cumulus oocytes complex (COCs) were collected and matured in vitro. Follicular walls were used for mRNA quantitation. JI0.3 led to a higher (P < 0.05) percentages of intact follicles than other groups after 18 days of culture. While follicular diameter remained unchanged from Day 6 onwards with JI0.3 and FSH, percentages of antral cavity formation were higher (P < 0.05) with JI0.3 at Day 6 than in all other treatments. No differences were observed between controls and treatment groups regarding ROS levels and mRNA expression of genes. Viability of resulting oocytes was higher (P < 0.05) in JI0.3 compared to FSH. Interestingly, in control experiment, supplementation of maturation medium with JI0.3 led to higher (P < 0.05) percentages of metaphase II compared to controls. Although more validations will be needed, it seems that this natural extract could be used as a cheap and easily available alternative to commercial FSH.

Details

Title
Supplementation of in vitro culture medium with FSH to grow follicles and mature oocytes can be replaced by extracts of Justicia insularis
Author
Mbemya, Gildas Tetaping; Cadenas, Jesus; Naiza Arcângela Ribeiro de Sá; ⨯ Denise Damasceno Guerreiro; Donfack, Nathalie Jiatsa; Vieira, Luis Alberto; ⨯ Francisca Geovania Canafístula de Sousa; Benner, Geraldo Alves; ⨯ Carlos Henrique Lobo; Francielli Weber Santos; Francisco das Chagas Lima Pinto; ⨯ Otília Deusdênia Loiola Pessoa; Smitz, Johan; Comizzoli, Pierre; Figueiredo, José Ricardo; Ana Paula Ribeiro Rodrigues
First page
e0208760
Section
Research Article
Publication year
2018
Publication date
Dec 2018
Publisher
Public Library of Science
e-ISSN
19326203
Source type
Scholarly Journal
Language of publication
English
DOI
https://doi.org/10.1371/journal.pone.0208760
ProQuest document ID
2151747010
Copyright
© 2018 Mbemya et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.