Role of JNK and ERK1/2 MAPK signaling pathway in testicular injury of rats induced by di-N-butyl-phthalate (DBP)

Background Di-N-butyl-phthalate (DBP) is an endocrine disrupting substance. We investigated the adverse effect of DBP on testis of male rat and reveal its potential mechanism of MAPK signaling pathway involved this effect in vivo and in vitro. Gonadal hormone, sperm quality, morphological change and the activation status of JNK, ERK1/2 and p38 was determined in vivo. Primary Sertoli cell was established and cultivated with JNK, ERK1/2 inhibitors, then determine the cell viability, apoptosis and the expression of p-JNK, p-ERK1/2. Data in this study were presented as mean ± SD and determined by one-way analysis of variance (ANOVA) followed by Bonferroni’s test. Difference was considered statistically significant at P < 0.05. Results In vivo experiment, DBP impaired the normal structure of testicular tissue, reduced testosterone levels in blood serum, decreased sperm count and increased sperm abnormality, p-ERK1/2 and p-JNK in rat testicular tissue increased in a dose-dependent manner. In vitro studies, DBP could decrease the viability of Sertoli cells and increase p-ERK1/2 and p-JNK. Cell apoptosis in SP600125 + DBP group was significantly lower than in DBP group (P < 0.05). p-JNK was not significantly decreased in SP600125 + DBP group, while p-ERK1/2 was significantly decreased in U0126 + DBP group. Conclusions These results suggest that DBP can lead to testicular damage and the activation of ERK1/2 and JNK pathways, the JNK signaling pathway may be primarily associated with its effect.


Background
Mounting evidence has implicated that Phthalic acid esters (PAEs), as a widely used synthetic compound, may be related to carcinogenesis, inflammation, metabolic disorder and especially reproductive and developmental disease [1]. Dibutyl phthalate (DBP), one of the most used PAEs, has been proved to be an endocrine disrupting chemical (EDC) which displays estrogenic or anti-androgenic activity in male reproductive system, leading to testicular atrophy, seminiferous tubule degeneration, germ cell loss and infertility [2]. In 1983, animal experiments conducted by Oishi S have shown that di-2-ethylhexyl phthalate (DEHP) can cause testicular atrophy in young male rats [3]. In vivo, DBP acts by reducing cell proliferation and impairing differentiation through reducing expression levels of Pou5f1 and Mki67 in prepubertal and pubertal testes [4]. In compare to other EDCs including other Phthalates and the mixture of EDCs, the main effect of DBP was decrease intratesticular testosterone, and steroid hormone enzymes [5]. It can be seen from the above research results that the association of DBP exposure with male fertility problems is the concerning problems of this and others toxicologicals research in this field.
Testis injury induced by DBP is characterized with testis atrophy and seminiferous epithelium degeneration [6]. It was reported that DBP could penetrate into testis despite the existence of blood-testis barrier (BTB) which is one of the tightest physiological barriers in mammals [7]. Sertoli cells which form the BTB provide the germ cells with nutrition, structure support and protective shield [8]. Studies showed the distribution of vimentin cytoskeleton and intercellular junction proteins in Sertoli cells were altered by DBP, inducing spermatogenic cells to detach from Sertoli cells and then undergo apoptosis [9]. These studies may indicate that Sertoli cell could be the primary target of DBP in testis. However, the properties of Sertoli cells are modulated by various substances such as steroid hormone, cytokine, and protein kinase. Therefore elucidating the mechanisms underlying the impair effect of DBP to Sertoli cells would give hints to the prevention of EDCs induced male reproductive dysfunction.
MAPK signaling pathway is one of the important signal transduction systems, involved in cell proliferation, differentiation, apoptosis and response to environmental stimuli [10]. In mammalian testis MAPK can regulate cell proliferation, differentiation and apoptosis, is considered one of the important determinants of sperm development. MAPK can indirectly affect the development of animal germ cells by influencing the function of Sertoli cells [11]. There are three MAPK units in the mammalian cells, namely, c-Jun N-terminal kinase (JNK), p38, extracellular signal regulated kinase (ERK) subfamily [12]. Sertoli cell proliferation and differentiation are mainly regulated by follicle stimulating hormone (FSH), whereas FSH activity is inseparable from ERK signaling cascade [13]. Cells respond to many reproductive toxicants by activating the MAPK pathway, for example, bisphenol A induces apoptosis by activating ERK and JNK signaling pathways [14], 1-3-dinitrobenzene can induce apoptosis in TM4 mouse Sertoli cells by JNK-MAPK pathway [15]. 4-nonylphenol isomers can induce apoptosis of mouse Sertoli TM4 cells by activating mitogen-activated protein kinase pathway [16]. Therefore, we speculate that the effect of DBP on Sertoli cells may also be related to the MAPK signaling pathway.

DBP decreases testosterone level in blood serum
As revealed in this study (Table 1), the level of testosterone in blood serum decreased whereas FSH and LH increased in the DBP treated groups. Compared with the solvent control group, the level of serum FSH in middle and high dose DBP group increased, and the level of serum LH in high dose DBP group was significantly higher (P < 0. 05). The serum levels of testosterone in middle and high dose DBP group were significantly lower than those in solvent control group (P < 0.05).

DBP disrupts spermatogenesis
DBP can reduce the sperm count and sperm viability of rats and increase the Malformation rate (see Table 2). Compared with the solvent control group and the lowdose group, the sperm count and sperm viability of the rats in the high dose DBP group were significantly lower (P < 0.05). The total abnormal rate of spermatozoa in the middle and high dose DBP group was significantly higher than that in the solvent control group (P < 0.05). There were statistically significant on the rat sperm count and total sperm abnormality rate between the medium and high DBP dose group (P < 0.05). The dose response relationship is shown in the sperm malformation rate.

DBP induces seminiferous tubules degeneration
In the solvent control group, the testicular seminiferous tubules were arranged and the structure was complete. No cells were shed in the lumen, and the number and structure of the Sertoli cells were normal (Fig. 1a). Compared with the control group, the testis tissue structure of the rats in the low dose DBP group was not changed obviously (Fig. 1b). In the middle dose DBP group, the testicular seminiferous tubules arranged in the rule, but the diameter became smaller, the interstitial widened, the level of spermatogenic epithelium decreased, and the spermatogenic cell shedding phenomenon was seen (Fig. 1c). High-dose DBP group testicular seminiferous tubules arranged irregularly, spermatogenic epithelial cells severely damaged, Sertoli cells dropped,and showed a vacuolar change (Fig. 1d).

DBP induces activation of JNK and ERK1/2 signaling pathway in the testes
Western blot results showed that DBP can induce the activation of ERK1/2 and JNK in the MAPK signaling pathway in testicular tissue (see Fig. 2). The ratio of the optical density of the phosphorylated protein to the corresponding total protein of the MAPK signaling pathway in the rat testis was seen in Table 3. There was no statistical difference on p-P38/P38 in the testes between DBP groups and the control group. The ratio p-ERK/ERK and p-JNK/JNK in the testes of middle and high dose DBP group was significantly increased than those in control group and low-dose DBP group (P < 0.05) (see Fig. 2).

Effects of DBP on Sertoli cell viability
The results of MTT showed that DBP could significantly reduce the proliferation of Sertoli cells (see Fig. 3   The testis tissue structure of the rats in the low dose DBP group was not changed obviously. c The middle dose DBP group, the testicular seminiferous tubules arranged in the rule, but the diameter became smaller, the interstitial widened, the level of spermatogenic epithelium decreased, and the spermatogenic cell shedding phenomenon was seen. d High-dose DBP group testicular seminiferous tubules arranged irregularly, spermatogenic epithelial cells severely damaged, sertoli cells dropped, and showed a vacuolar change

Effects of DBP on Sertoli cell apoptosis rate
The results of flow cytometry ( Fig. 4) showed that compared with the control group (the apoptotic rate of the cells was 4.32 ± 0.98), DBP significantly induced the apoptosis of the Sertoli cells, and the apoptotic rate was 17.5 ± 1.21. After the pretreatment of the cells with ERK1/2 inhibitor (U0126) and JNK inhibitor (SP600125), cell apoptosis rate decreased. The apoptosis rates of U0126 + DBP and SP600125 + DBP cells were 13.4 ± 3.21 and 6.23 ± 1.08, respectively. Compared with DBP group, the apoptotic rate decrease in JNK inhibitor (SP600125) + DBP group was statistically significant (P < 0.05).

DBP induces activation of JNK and ERK1/2 signaling pathway in the Sertoli cells
Pretreatment with U0126 and SP600125, respectively to primary Sertoli cells for 2 h, then add 100 μg/mL DBP, Western blot (Figs. 5,6) showed that compared with the DBP group alone, the phosphorylated JNK was not significantly decreased in the JNK inhibitor (SP600125) + DBP group and the phosphorylated ERK1/2 expression was significantly decreased in the ERK1/2 inhibitor (U0126) + DBP group. The ratio of the optical density of the phosphorylated protein to the corresponding total protein in Sertoli cell was seen in Table 4. Compared with the solvent control group, the ratio of p-ERK/ERK and p-JNK/JNK in DBP group increased, the difference was statistically significant (P < 0.05). ERK inhibitors (U0126) and JNK inhibitors (SP600125) reduced the expression of phosphorylated ERK and JNK. Compared with the DBP group, the ratio of p-JNK/JNK was not significantly decreased in the JNK inhibitor (SP600125) + DBP group, while the ratio of p-ERK/ERK was significantly decreased (P < 0.05). These findings indicated that DBP mainly activates the phosphorylation of JNK and participates in the cell damage.

Discussion
As an environmental endocrine disruptor, DBP has certain male reproductive toxicity, can cause male rodents testicular atrophy, weight loss, decreased testicular activity of the enzyme, seminiferous tubules atrophy, spermatogenic cell loss, genital malformations, etc. [17]. In this vivo study of testicular pathology showed that DBP lead to testicular tissue structure damage, manifested as spermatogenic tubule disorders, Sertoli cell vacuolization, germ cell shedding, and so on. Sperm    we analyzed that the difference results is related to DBP dose, the time of exposure, the type, age of animal and other factors. But these suggested that DBP indirect damage to the testis through endocrine disruption, but also that Sertoli cells may be the direct target of DBP toxic effects [21]. Sertoli cells present in the testicular spermatogenic epithelium, the structure and function integrity of Sertoli cells is critical to the proliferation and maturation of spermatogenic cells. In this study, we used MTT assay to detect the inhibitory effect of DBP on the proliferation of Sertoli cells. It was found that DBP significantly inhibited cell proliferation compared with the control group. Flow cytometry showed that DBP-treated cell apoptotic rate was significantly higher than that the control group. The results confirm that DBP induces cytotoxicity in Sertoli cells causing apoptosis in Sertoli cells cultured in vitro. Many studies have found that male reproductive health have a relationship between MAPKs pathway. MAPKs involved in spermatogenesis [22], germ cell development and maturation [23], germ cell apoptosis [24]. We examined the phosphorylation of ERK1/2, JNK, p38 by Western blot to confirm whether DBP will interfere with MAPKs signaling pathway. In the vivo experiment study, the ratio of p-ERK/ERK and p-JNK/JNK in MAPKsrelated proteins increased compared with the solvent control group, the difference was statistically significant (P < 0.05), while the changes of p-P38/P38 were not significant, indicating that JNK, ERK phosphorylation level was significantly increased, and P38 phosphorylation level was not significant. These suggests that the JNK and ERK pathways in the MAPKs signal are involved in testicular damage. This result is not completely consistent with the relevant research reports. Qi et al. believe that JNKs/p38 MPAK is involved in the apoptosis of Sertoli cells [25]. Song et al. believe that p38 MPAK mainly plays a major role in Sertoli cell injury [26], Choi et al. believe that ERK pathway plays a major role in Sertoli cell damage [27]. This difference is due to the different reproductive chemical toxicants studied by the researchers, and different animal species and cell lines used in vivo and in vitro studies.
In addition, in order to further confirm the mechanism of JNK and ERK-MAPKs signaling pathway on testicular injury, we used testicular primary Sertoli in vitro experiments. The results showed that compared with the solvent control group, DBP could increase the phosphorylation of MAPKs-related proteins ERK and JNK, and the ratio of p-ERK/ERK and p-JNK/ERK increased, the difference was statistically significant (P < 0.05), indicating that DBP can activate the JNK and ERK-MAPKs signaling pathway of testicular Sertoli cells. To further confirm whether the phosphorylation of JNK and ERK1/2 is involved in apoptosis and whether the two effects are equal or which dominates, we used ERK1/2 inhibitors (U0126) and JNK inhibitors (SP600125) pretreatment primary Sertoli cells 2 h, and then incubated with 100 μg/mL of DBP. The results showed that ERK1/2 inhibitors (U0126) and JNK inhibitors (SP600125) reduced the expression of phosphorylated ERK1/2 and JNK, compared with the DBP group, the apoptosis rate of U0126 + DBP group and SP600125 + DBP group decreased, the cell proliferation rate increased, the ratio of p-ERK/ERK and p-JNK/ERK decreased, indicating that the inhibitors of JNK and ERK were all can weaken DBP-induced cell apoptosis, increase cell survival, reduce ERK1/2 and JNK phosphorylation. Furthermore, it was found that cell viability rate increase and the apoptotic rate decrease in JNK inhibitor (SP600125) + DBP group was more obvious, the difference was statistically significant (P < 0.05), indicating that the repress role of apoptosis by JNK inhibitors is more prominent. Western blot showed that compared with DBP group, the ratio of p-JNK/ERK was not significantly decreased in JNK inhibitor (SP600125) + DBP group, but in ERK1/2 inhibitor (U0126) + DBP group, the ratio of p-ERK/ ERK was significantly decreased. These findings illustrated that SP600125, a selective inhibitor of JNK, was shown to repress the DBP-induced JNK phosphorylation/activation in Sertoli cells, which indicated that DBP mainly activates JNK phosphorylation. So collectively, in vivo and in vitro study results, indicate that DBP mediates its disruptive effects at the Sertoli cell via the JNK-MAPK signaling pathway. These findings provide insightful information regarding a therapeutic approach to DBP-induced male infertility, such as via the use of specific JNK-MAPK inhibitor.
In summary, the results of this experiment indicate that the activation of MAPKs signaling pathway, especially JNK, may participate in the damage of DBP to testicular Sertoli cells. In addition, our previous in vitro results showed that the PTEN/PI3 K/AKT/mTOR signaling pathway plays an important role in DBP-induced apoptosis of testicular Sertoli cells [28]. These suggested that MAPK and Akt pathways both can mediate support cell death caused by reproductive toxicants which coincides with that nonylphenol-induced apoptosis in mouse Sertoli cell line TM4 cells can be mediated by MAPK and Akt pathways [29]. As noted herein, multiple pathways such as both Akt and MAPK signal pathways are involved in chemical toxicant-induced testicular injury, and research is needed to delineate the molecular mechanism(s) that regulates crosstalk between these signal pathways, which will be helpful in gaining insightful information to intervene toxicant induced testicular injury.

Conclusions
In conclusion, DBP can lead to testicular toxicity: decreased testosterone in blood serum, leaded to sperm reduction and malformation and even damaged the normal structure of seminiferous tubules. The activation of MAPKs signaling pathway, especially JNK, may participate in the damage of DBP to testicular Sertoli cells. We need to study more deeply such as the molecular mechanism(s) about signal pathways, which will be helpful in gaining insightful information to intervene the reproductive toxicity of DBP.

Animals and treatments
Male clean Sprague-Dawley rats (4 weeks old) were obtained from the Laboratory Animal Center of Jilin University (Jilin, China). All experimental protocols were conducted in accordance with the principles and procedures outlined in the "Guide for Care and Use of Laboratory animals" and approved by the Ethics Committee for the Use of Experimental Animals of Beihua University.
Rats were housed under a 12:12 h light-dark cycle with well ventilation and constant temperature (26 ± 1 °C). Animals were adapted to laboratory lighting and feeding condition for 1 week before experiment. Rats were allowed free access to food and drinking water. After adaptation, male SD rats were assigned randomly to four group (n = 8) and administered corn oil (vehicle control) or DBP (analytical grade, purity 99.5%) (Sigma, USA) at doses of 50, 500 and 1000 mg/kg/day by gavage for 35 days. Animals were sacrificed by decapitation after the last treatment and the blood, testes and epididymides were isolated immediately for the following analyses.

Measurement of reproductive hormone
The blood samples were centrifuged at 2000 rpm, 4 °C for 10 min and testosterone (T), follicle-stimulating hormone (FSH) and luteinizing hormone (LH) in serum were detected using ELISA kits according to the manufacturer's instructions (Shanghai Jiang Lai biological company, China).

Sperm analysis
The fresh epididymides were weighted then cut longitudinally and put in 2 mL 0.9% sodium chloride solution for 10 min at 35 °C to release sperms into the media. The suspension was filtered using nylon mesh and adjusted to an adequate concentration. Sperm count, viability rate and malformation rate were determined using WLJY-9000 color sperm quality detection system (Beijing Weili Inc., China).

Testis histological examination
Hematoxylin-eosin (HE) staining was applied to testes. Tissues were immersed in Bouin's solution (picric acidaqueous solution: formaldehyde:glacial acetic acid, 15:5:1) for 24 h at room temperature, embedded in paraffin wax and sectioned into 5 μm thick slices. After dewaxed in xylol, dehydrated in ethanol series and washed in water, slices were stained with hematoxylin and eosin, following the standard HE staining procedures. Images were taken by a digital camera (DP20, Olympus, Tokyo, Japan) to show the extent of testes injury.

Isolation of Sertoli cells
Primary Sertoli cells were isolated from 18-day-old male rats. Briefly, animals were euthanized by CO 2 asphyxiation, and testes were isolated, decapsulated, and cut into small pieces. After washed twice in DMEM-F12 (Hyclone, USA), fragments were digested with 0.1% (w/v) trypsin (Difco, USA) for 30 min then centrifuged twice at 800 rpm for 2 min. Cell debris was resuspended in 0.05% (w/v) collagenase I (Sigma, USA) with gentle pipetting using Pasteur pipette and digested for about 10 min, until seminiferous tubules were nearly invisible. Suspension was filtered through nylon mesh and centrifuged for 5 times. Resuspend cells with DMEM-F12 containing 15% fetal bovine serum (Hangzhou Sijiqing, China) and plate cells on 100 mm dishes at a density of 0.5 × 10 5 cells/cm 2 . High purity Sertoli cells were obtained after incubated for 36 h at 35 °C in 5% CO 2 followed by treated with 20 mM Tris-HCl buffer (pH 7.4) for 2.5 min to remove residual germ cells. The purity of Sertoli cells was routinely more than 90% [30]. On the 4th day of in vitro culture, Sertoli cells were ready for the subsequent treatments.

MTT assay
Sertoli cells were transferred into a 96-well plate at a density of 1 × 10 5 cells/mL. Cell viability was estimated by MTT assay after 24 h treatment. Cells were incubated in serum-free media containing 20 μL MTT (5 mg/ mL) for 4 h. 150 μL DMSO was added after discarding culture media. Shake for 10 min, and the absorbance were acquired at 490 nm by microplate reader (Tecan, Switzerland).

Sertoli apoptosis rate detection
After treatment for 24 h, the cells were digested and trypsinized, then harvested. The cells were treated according to the Annexin v-FITC/PI kit instructions (Biovision, USA). The cells were mixed with 400 μL binding buffer and then 4 μL PI and 4 μL Annesxin v were added. The cells were incubated at room temperature for 15-20 min at in dark room. FACS420 flow cytometer (Becton-Dickinson, USA) was used to detect cell apoptosis.

Western blot analysis
In vivo experiments, testicular tissue of each group rats was removed and quickly placed in liquid nitrogen to be stored for inspection. The sample was placed in 4 °C precooling lysis buffer, 4 °C ultrasonic mixing (6 s × 6 times), 4 °C incubated for 30 min, centrifuged 25,000 rpm, 10 min × 3 times, the supernatant sub-assembly; The content of protein was determined by Bradford method, and the protein was separated by 10% SDS-PAGE using standard bovine serum albumin. Each well was loaded with 60 μg of protein and electrophoresis was performed at a constant voltage of 160 V until the bottom of the gel was transplanted. After blocked with 5% non-fat dry milk for 2 h, 1: 100 rabbit anti-rat ERK1/2, p-ERK1/2, JNK, p-JNK, P38, p-P38 and tubulin monoclonal antibody (Beijing Solarbio, China) were added, shaken at 37 °C for 1 h, Washed three times with phosphate buffer solution-Tween 20 for 10 min. The conjugate horseradish peroxidase-labeled secondary antibody (1: 300) was added, shaken at 37 °C for 1 h, washed in PBST for 3 times and irradiated with chemiluminescence agent.
In vitro experiments, Sertoli cells were homogenized in lysis buffer on ice for 30 min and the homogenate was collected followed by centrifugation at 1000 rpm for 10 min at 4 °C. The protein concentration of supernatant was measured. Equal amounts of proteins (40 μg) were loaded on 10% polyacrylamide gel with 4% stacking gel to apply SDS-PAGE and then transferred to nitrocellulose membranes. After blocked with 5% nonfat milk for 1 h at room temperature, the membranes were incubated with primary antibodies (JNK, p-JNK, ERK1/2, p-ERK1/2, and tubulin, 1:1000 dilution) overnight at 4 °C. Protein blots were revealed by horseradish peroxidase-conjugated secondary antibody (1:3000 dilution) and visualized by enhanced chemiluminescent kit.
Proteins were quantified by densitometry with the ImageJ software (National Institutes of Health, USA). Data were normalized against tubulin in each group.

Statistical analysis
Data in this study were presented as mean ± SD and determined by one-way analysis of variance (ANOVA) followed by Bonferroni's test. Difference was considered statistically significant at P < 0.05.

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