Caveolin-1 is critical in the proliferative effect of leptin on osteoblasts through the activation of Akt.

Osteoblasts are critical in bone remodeling and the repair of bone fractures. Leptin is involved in bone metabolism and osteoblast survival through the downstream signaling pathway, however, the exact mechanism of the effect of leptin on osteoblasts remains to be fully elucidated. In the present study, hFOB 1.19 cells were used to observe the effects of leptin on cell proliferation and apoptosis, and to investigate the underlying mechanism. The results confirmed that treatment of hFOB 1.19 cells with leptin significantly induced cell proliferation. Western blot analysis showed that the expression of caveolin‑1 and the activation of Akt in the cells treated with leptin were significantly increased, compared with the control cells. Additionally, inhibiting Akt activation eliminated the effects on cell proliferation induced by leptin. The rates of cell apoptosis and cell cycle distribution were examined using flow cytometry, which revealed a decrease in the apoptotic rate and an increase in the proportion of cells in the S phase. This indicated that leptin was capable of inducing cell proliferation by inhibiting apoptosis and stimulating cell progression to the S phase. Transfection of the cells with caveolin‑1 small interfering RNA showed that the activation of Akt induced by leptin was significantly inhibited. Furthermore, caveolin‑1 knockdown and inhibiting Akt activation eliminated the increased proliferation, increased proportion of cells in the S phase and increased anti‑apoptotic effects induced by leptin. Taken together, the data obtained in the present study demonstrated that caveolin‑1 was critical in the proliferative effect of leptin on osteoblasts via the activation of Akt.

Introduction

Leptin, an adipocytokine, is a 16-kDa plasma protein primarily secreted by adipocytes (1,2). It is also produced by oesteoblasts, placental syncytiotrophoblasts and gastric epithelium (3–6). A previous study demonstrated that leptin contributes to body weight homeostasis as a signal to affect food intake and energy expenditure (7). In addition to its physiological actions on lipid metabolism, angiogenesis, fertility and hematopoiesis, leptin has a pathological role in certain bone diseases, including osteoporosis, osteoarthritis, rheumatic arthritis, bone tumors and fractures (8–11).

It is well known that leptin is an important regulator of bone metabolism through peripheral and central signaling pathways. It has been suggested that the peripheral pathway is direct and involved in a stimulatory effect on bone formation, whereas the central pathway is indirect and exerts an inhibitory effect on bone growth, which is supported by observations of bone loss resulting from the intracerebrovesicular administration of leptin (12). By contrast, a previous study showed that the intracerebrovesicular injection of leptin enhances bone formation (13). Osteoblasts are major cells in the bone, and are responsible for mineralization during bone formation and later bone remodeling. As such, osteoblasts are critical in normal skeletal physiology and are involved in several pathological conditions, including osteoporosis, osteopetrosis and bone cancer (14). It has been shown that leptin can affect bone formation by mediating the activity of osteoblasts (15). However, the mechanisms underlying the effect of leptin on osteoblasts remain to be fully elucidated.

Caveolin-1 is an essential and signature protein of caveolae, and is found to be expressed at high levels in osteoblasts and endothelial cells (16). The removal of caveolin-1 has been demonstrated to prevent the formation of caveolae in these cells (16). Numerous studies have shown the importance of caveolae in vesicular trafficking, cell adhesion, apoptosis and senescence (17,18). Although the predominant focus of interest has been centered on the role of caveolin-1 in cancer, there is substantial data providing evidence that it is also involved in bone metabolism (19,20). It has also been demonstrated that caveolin-1 appears to be a key regulator of osteoblast differentiation and function, including mineralization and matrix protein deposition (16).

In the present study, it was confirmed that leptin promoted the proliferation of osteoblasts in vitro, and demonstrated for the first time, to the best of our knowledge, that caveolin-1 critically contributed to the proliferative effect of leptin on osteoblasts, and this was mediated by the activation of Akt The results may aid in the development of therapeutics for leptin-induced bone diseases.

Materials and methods

Cell culture and reagents

An osteoblastic cell line derived from the bone of human fetal osteoblasts (hFOB 1.19), was purchased from American Type Culture Collection (Manassas, VA, USA). In culture conditions of 37°C with 5% CO2, the cells were grown in Dulbecco's modified Eagle's medium (DMEM; Sigma-Aldrich, St. Louis, MO, USA) at pH 7.4, supplemented with 3.7 g/l NaHCO3, 4.77 g/l HEPES, 10% fetal bovine serum (FBS; Invitrogen; Thermo Fisher Scientific, Waltham, MA, USA) and 0.5% penicillin/streptomycin (50 U/ml penicillin and 50 µg/ml streptomycin; Sigma-Aldrich). Every 2–3 days, the medium was replaced. When the cell culture reached ~85% confluence, subculture was performed. Cells at the third or fourth passage were used in the subsequent experiments.

Cell proliferation assay

Using an MTT assay, cell viability was evaluated. The cells were seeded in 96-well plates at a density of 3×103 cells per well. Following incubation overnight, the cells were exposed to leptin (Sigma-Aldrich); for 24–96 h Following incubation overnight, the cells were exposed to different concentration of leptin (0, 0.01, 0.05, 0.1, 0.5, 1, 5 and 10 µg/ml) for 24 h or the cells were exposed to 0.5 µg/ml leptin for 24–96 h. Fresh complete medium (0.2 ml) supplemented with 20 µl MTT dye [(5 mg/ml in phosphate-buffered saline (PBS)] was added to each well. Following incubation at 37°C for 4 h, each well was washed thoroughly with PBS. Subsequently, dimethyl sulfoxide (Sigma-Aldrich) was added to each well to terminate the MTT reaction and dissolve the formazan crystals. Following agitation at room temperature for ~10 min, the optical density (OD) of each well was measured at 450 nm. The viability of the control cells were considered as 100%, and the results were calculated as follows: (ODtreated cells − ODcontrol cells) / (ODcontrol cells − ODblank) × 100%.

Analysis of cell apoptosis

In 6-well plates, 2×105 cells/well were seeded and cultured overnight. Following treatment with 0.5 µg/ml leptin for 24 h, the cells were trypsinized and washed with PBS. The cells were suspended in 0.3 ml binding buffer, following by the addition of 2 µl Annexin V (Beyotime Institute of Biotechnology, Haimen, China) and careful pipetting of the mixture. Following the addition of 5 µl propidium iodide (PI; Beyotime Institute of Biotechnology), the mixture was incubated for ~10 min at room temperature. The rates of apoptosis were detected using a FACSCSalibur flow cytometer (Becton-Dickinson; BD Biosciences, San Diego, CA, USA).

Cell cycle analysis

In 6-well plates, 2×105 cells were seeded per well. Following 12 h starvation, the cells were treated with 0.5 µg/ml leptin for 24 h for 48 h. Following trypsinization and washing with PBS, the cells were resuspended with 500 µl medium containing 1 mg/ml RNase A and 100 µg/ml PI (Beyotime Institute of Biotechnology). Following incubation for 20 min at room temperature, in the dark, the DNA contents of the cells were measured using a FACSCalibur flow cytometer (Becton-Dickinson; BD Biosciences).

Small interfering (si)RNA knockdown

siRNA was used to knock down the gene expression of caveolin-1. A total of 5×104 cells/well were seeded in 24-well tissue culture plates. Following incubation for 24 h at 37°C, the medium was replaced. Using 6 µl transfection reagent (Qiagen), transfections were performed using siRNA (Santa Cruz Biotechnology, Inc., Dallas, TX, USA) at a final concentration of 30 nM. Based on the half-life of 5 h for caveolin-1 protein (21), the cells in the wells were exposed to the transfection mixture for 24 h at 37°C prior to cell harvest.

Reverse transcription-quantitative polymerase chain reaction (RT-qPCR)

Using TRIzol reagent (Takara Bio, Inc., Otsu, Japan), total RNA was extracted from the cells. A 200 ng quantity of total RNA was used to synthesize cDNA using M-MLV Reverse Transcriptase (Promega Corporation, Madison, WI, USA). Based on the previously published primers (22), qPCR was performed to measure the mRNA levels of caveolin-1. The primers were as follows: caveolin-1, forward 5′-TCA ACC GCG ACC CTA AAC ACC-3′ and reverse 5-′TGA AAT AGC TCA GAA GAG ACA T-3′; β-actin, forward 5′-GGA GCA ATG ATC TTG ATC TT-3′ and reverse 5′-CCT TCC TGG GCA TGG AGT CCT-3′. The conditions for qPCR were as follows: Enzyme activation at 95°C for 10 min, 40 cycles of amplification and each of them consisted of denaturation at 95°C for 15 sec, annealing at 60°C for 60 sec, and extension at 60°C for 60 sec. The results were calculated with the comparative quantification cycle (Cq) method. RT-qPCR was performed using the Applied Biosystems 7500 Sequence Detection system (Thermo Fisher Scientific, Inc.). The expression of caveolin-1 was normalized to β-actin. The conditions for qPCR were as follows: Enzyme activation at 95°C for 10 min, followed by 40 cycles of amplification, each consisting of denaturation at 95°C for 15 sec, annealing at 60°C for 60 sec and extension at 60°C for 60 sec. The results were calculated using the quantification cycle (Cq) method (23), and the expression of caveolin-1 was normalzed with β-actin.

Western blot analysis

Using lysis buffer (Beyotime Institute of Biotechnology), the cell lysates were prepared immediately following treatment. Protein concentrations were measured using the Bradford method (Bio-Rad Laboratories, Inc., Hercules, CA, USA). Equal quantities (100 µg) of proteins were loaded and separated on 8% SDS-polyacrylamide gels. The proteins were then transferred onto PVDF membranes (EMD Millipore, Bedford, MA, USA). Following blocking in TBST buffer containing 5% skim milk at room temperature for 2 h, the blots were incubated at 4°C overnight with the following primary antibodies: Rabbit anti-calveolin-1 (cat. no. 3267), rabbit anti-p473-Akt (cat. no. 4060), rabbit anti-GAPDH (cat. no. 5174) and rabbit anti-Akt (cat. no. 4691) (Cell Signaling Technology, Inc. Danvers, MA, USA). The blots were then washed in TBST and incubated with the horseradish peroxidase-conjugated Chicken anti-rabbit IgG secondary antibodies (cat. no. sc-516087; Santa Cruz Biotechnology, Inc.) at room temperature for 1 h. Following washing in TBST, the immunoreactive bands were visualized by enhancement using a chemiluminescence kit (Pierce Biotechnology, Rockford, IL, USA). The immunoreactive bands of GAPDH were used as an internal control.

Statistical analysis

Experiments were performed three times. Data are presented as the mean ± standard deviation. Statistical differences were analyzed using the Student's two-sided t-test or one way analysis of variance using SPSS 21.0 software (IBM SPSS, Armonk, NY, USA). P≤0.05 was considered to indicate a statistically significant difference.

Results

Leptin promotes cell proliferation

To determine the effect of leptin on the growth of hFOB 1.19 cells, an MTT assay was performed. The cells were exposed to leptin at the doses of 0, 0.01, 0.05, 0.1, 0.5, 1, 5 and 10 µg/ml for 24 h. As shown in Fig. 1A, the cell viabilities at the doses ranging between 0.01 and 1 µg/ml were comparable with the control, whereas the cell viabilities at 5 and 10 µg/ml were marginally decreased, but not significantly, compared with that of the control.

Figure 1

Leptin promotes the proliferation of hFOB 1.19 cells. The effect of leptin on cell viability was determined using an MTT assay. (A) Cell viabilities of hFOB 1.19 cells treated with a gradient of doses of leptin for 24 h and (B) treated with 0.5 µg/ml leptin for 24, 48, 72 and 96 h. *P≤0.05, compared with the hFOB group at the same time point. Data are presented as the mean ± standard deviation. OD, optical density.

Subsequently, time-response assessment was performed (Fig. 1B). The cells were incubated with 0.5 µg/ml leptin for 24, 48, 72 and 96 h. Between 24 and 72 h, a time-dependent increase in cell viability induced by leptin was observed. Although 96-h treatment with 0.5 µg/ml leptin resulted in a cell viability comparable with that of 72-h treatment, the cell viability was significantly increased, compared with that in the control group at 96 h. Taken together, these findings indicated that leptin induced hFOB 1.19 cell proliferation.

Leptin induces the expression of caveolin-1

To observe the effect of lepin on the expression of caveolin-1, the cells were exposed to leptin at the gradient doses of 0, 0.01, 0.05, 0.1, 0.5, 1, 5 and 10 µg/ml for 24 h. The mRNA and protein expression levels of caveolin-1 showed a significant dose-dependent increase between doses of 0.05 and 5 µg/ml, whereas 0.01 µg/ml leptin had no effect on the expression levels (Fig. 2A and B). Unexpectedly, the expression of caveolin-1 at 10 µg/ml was comparable to that at 5 µg/ml. Subsequently, time-response assessment of the effect of leptin on the expression of caveolin-1 was performed. The cells were incubated with 0.5 µg/ml leptin for 12, 24, 36 and 48 h. A time-dependent increase in the expression of caveolin-1 was observed between 12 and 36 h, whereas no increase in the expression of caveolin-1 was observed at 48 h, compared with that at 36 h (Fig. 2C and D). Taken together, these results indicated that leptin induced the expression of caveolin-1.

Figure 2

Exposure to leptin enhances the expression of caeolin-1. Following treatment with leptin at concentrations between 0.01 and 10 mg/ml for 24 h, the expression levels of caveolin-1 in the cells were measured using (A) western blot analysis and (B) reverse transcription-quantitative polymerase chain reaction analysis. (C) Protein and (D) mRNA expression levels of caveolin-1 were measured in the cells following treatment with leptin (0.5 mg/ml) for 12, 24, 36 and 48 h. Data are presented as the mean ± standard deviation. Different letters (a–f) represent significant differences between treatment groups (P≤0.05).

Caveolin-1 konckdown decreases leptin-induced Akt activation

It has been reported that leptin can activate the phosphoinositide 3-kinase (PI3K) signaling pathway in a variety of cells, including vascular smooth muscle, nucleus pulposus and leukemic cells (24–26). Therefore, the present study evaluated the effect of caveolin-1 knockdown on the activation of the signaling pathway by leptin. As Akt is the immediate downstream kinase activated by PI3K, the level of p-Akt was measured in the present study. As shown in Fig. 3, the level of p-Akt was markedly increased in the hFOB 1.19 cells exposed to 0.5 µg/ml leptin, whereas no significant change in the level of Akt was noted. Furthermore, the present study evaluated the effect of caveolin-1 on the activation of Akt by leptin. Caveolin-1 was knocked down by siRNA, and a marked decrease in the level of p-Akt was noted, indicating that caveolin-1 may functionally contribute to leptin-induced Akt activation. Additionally, the effect of Akt activation on the expression of caveolin-1 was evaluated. Following exposure to Akt inhibitor IV, the increased expression of caveolin-1 was significantly inhibited (Fig. 3).

Figure 3

Knockdown of caveolin-1 decreases the activation of Akt by leptin. (A) The effect of caveolin-1 on the activation of Akt by leptin was determined using western blot analysis following caveolin-1 knockdown. (B) Quantification of caveolin 1, pATK and AKT protein expression levels. *P<0.05 vs. the NC-siRNA group. #P<0.05 vs. the Leptin+NC-siRNA group. siRNA, small interfering RNA; NC, negative control; p-, phosphorylated.

Effect of caveolin-1 and p-Akt on leptin-induced cell proliferation

To evaluate the involvement of caveolin-1 and p-Akt in leptin-induced cell proliferation, the present study examined the effects of caveolin-1 knockdown and the inhibition of Akt activation on 0.5 µg/ml leptin-induced cell proliferation at 24, 48, 72 and 96 h. As shown in Fig. 4, leptin treatment significantly increased cell viability, compared with the control group. As expected, the cell viabilities in the groups of cells with caveolin-1 knockdown and Akt inhibition were significantly suppressed, compared with leptin-treated group. Taken together, these results indicated that caeolin-1 knockdown and Akt inhibition individually counteracted the proliferative function of leptin.

Figure 4

Knockdown of caveolin-1 and inhibition of Akt activation reverses the proliferation effect of leptin. The roles of caveolin-1 and p-Akt in the proliferative effect of leptin were determined using an MTT assay following exposure to leptin for 24, 48, 72 and 96 h. Data are presented as the mean ± standard deviation. *P≤0.05, compared with the control group at the same time point. OD, optical density; siRNA, small interfering RNA; NC, negative control.

Effect of caveolin-1 knockdown and Akt activation inhibition on the cell cycle distribution of cells exposed to leptin

The cell cycle distribution of the hFOB 1.19 cells was examined using flow cytometry. As shown in Fig. 5, exposure of the cells to leptin at 0.5 µg/ml for 24 h significantly decreased the proportion of cells in the G0/G1 phase and increased the proportion of cells in the S phase, compared with the control group, indicating that leptin promoted the cell cycle towards the S phase. Compared with the decreased proportion of cells in the G01/G1 phase and increased proportion of cells in the S phase in the cells treated with leptin, caveolin-1 knockdown and the inhibition of Akt activation significantly increased the proportion of cells in the G0/G1 phase and decreased the proportion of cells in the S phase, compared with control group. Furthermore, the proportions of cells in the G0/G1 and S phases following Akt inhibition were significantly higher and lower, respectively, compared with those following cavelin-1 knockdown. These results revealed that caveolin-1 knockdown and the inhibition of Akt activation arrested hFOB 1.19 cell proliferation via inducing cell cycle arrest at the G0/G1 phase.

Figure 5

Cell cycle distribution of hFOB 1.19 cells, analyzed using flow cytometry. (A) Cell cycle distribution of hFOB 1.19 cells in the indicated groups following treatment for 48 h. (B) Results of flow cytometry data, based on the cell cycle phase for the indicated groups. Data are presented as the mean ± standard deviation Different letters (a–d) indicate significant differences between treatment groups (P≤0.05). siRNA, small interfering RNA; NC, negative control.

Effect of caveolin-1 knockdown and Akt activation inhibition on the apoptosis of cells exposed to leptin

To evaluate whether caveolin-1 knockdown and Akt inhibition induced cell apoptosis following treatment with 0.5 µg/ml leptin, the rates of apoptosis at the early and late stages were detected. As shown in Fig. 6, treatment with letpin marginally, but significantly, decreased the rate of cell apoptosis at each stage, compared with the control group. By contrast, caveolin-1 knockdown and Akt inhibition resulted in A higher apoptotic rate, compared with th econtrol group. These results revealed that caveolin-1 and p-Akt were critical in the anti-apoptotic effect of leptin on the cells.

Figure 6

Knockdown of caveolin-1 and inhibition of Akt activation reverses the anti-apoptotic effect of leptin. (A) Dot plots of hFOB 1.19 cells exposed to NC-siRNA, leptin+NC-siRNA, leptin+siNRA or leptin+Akt inhibitor IV for 72 h. (B) Results of flow cytometry data based on the apoptotic rates of the indicated groups. Data are presented as the mean ± standard deviation Different letters (a–d) indicate significant differences between treatment groups (P≤0.05). siRNA, small interfering RNA; NC, negative control; p-, phosphorylated; FITC, fluorescein isothiocyanate; PI, propidium iodide.

Discussion

It is evident that leptin is important in bone formation (15), however, it remains controversial whether the effects of leptin on bone formation are positive or negative. Osteoblasts, or bone-forming cells, are one of three distinct cell types in bone. It is well known that osteoblasts are positively associated with bone mass and bone density (27). In the present study, it was confirmed that leptin directly enhanced the proliferation of osteoblasts and revealed that this effect was critically mediated by caveolin-1 through the activation of Akt.

Leptin functions as a growth factor in a variety of cell types, including human prostate cancer cells and mouse tracheal epithelial cells (28,29). Gordeladze et al (30) showed that leptin promotes human osteoblast proliferation. Consistently, it was observed that leptin increased the proliferation of the hFOB 1.19 cells in the present study. Additionally, the results of the present study showed that leptin suppressed the apoptosis of hFOB 1.19 cells. This supported the results of a previous report, which found that leptin can protect osteoblasts against apoptosis throughout the entire incubation period via enhancing the expression of B cell lymphoma-2 (Bcl-2)-associated X protein-α and Bcl-2 (30). Leptin receptors are present in osteoblasts (4,31), indicating that leptin exerts a proliferative effect on hFOB 1.19 cells by directly binding to its receptor. This further supports the hypothesis that peripheral leptin may protect against bone loss.

As the major structural protein in caveolae, caveolin-1 can be regulated by various cytokines, and is considered to functionally contribute to certain intracellular signaling pathways (32). According to the results of the present study, the expression of caveolin-1 was markedly elevated by leptin. This is consistent with the results of a previous study, which demonstrated that leptin increases the protein expression of caveolin-1 in vascular endothelial cells (33). In the present study, it was demonstrated that caveolin-1 and p-Akt were critical in the proliferative effect of leptin. Furthermore, it was observed that, in the cells with caveolin-1 knockdown, the activation of Akt by leptin was significantly decreased, however, it was significantly higher than that in the control group (Fig. 3), suggesting that caveolin-1 enhanced the activation of Akt by leptin. Taken together, these results indicated that caveolin-1 may be a positive regulator for the proliferative signaling mechanism of leptin. However, this differed from the results of a previous study, which reported that caveolin-1 shares a functional similarity to the suppressor of cytokine signalling proteins, which are involved in the classical negative feedback signaling mechanism (34). Additionally, it has been shown that increased expression of caveolin-1 impairs the activation of extracellular signal-regulated kinase (ERK) induced by exposure to 100 ng/ml leptin for 0–30 min in vascular endothelial cells, and may have implications for the development of leptin resistance in the endothelium (33). Caveolin-1 is found to be expressed at high levels in osteoblasts (16). In caveolin-1, there is a scaffolding domain, which can interact with various signal transduction molecules, including src family tyrosine kinases, receptor tyrosine kinases and protein kinase C (35). Zeidan et al (17) demonstrated that caveolin-1 colocalizes with leptin receptors, and suggested that caveolae are important, and may have a primary role in leptin-induced activation of ERK1/2 in vascular smooth muscle cells. This difference between the positive role of leptin in the present study and the negative role in the above mentioned studies may be due to different treatment methods and cell lines.

The present study confirmed the proliferative role of leptin in osteoblasts and demonstrated that caveolin-1 was critical in leptin-induced osteoblast proliferation. However, the present study involved in vitro experiments. Further investigations are required to further elucidate the mechanism of leptin signaling in osteoblasts. These data may assist in the development of therapeutics for leptin-induced bone diseases.