Ginkgolic acid inhibits the growth of renal cell carcinoma cells via inactivation of the EGFR signaling pathway.

Renal cell carcinoma (RCC) is one of the most common urological malignancies occurring in adult human kidneys worldwide. Recent research on antitumor drugs has focused on plant extracts, a class of compounds that play critical roles in cancer treatment. The present study aimed to investigate the potential antitumor effect of ginkgolic acid (GA) in RCC. Transwell invasion assay, cell counting kit-8 assay and flow cytometry were used to measure cell migration, cell viability and apoptosis, respectively. A network pharmacology approach was applied to identify pathway information, combining molecular docking techniques to screen for key target information. In the present study, GA inhibited the viability and proliferation of RCC cells (786-O and A498), both in vitro and in vivo, via G1 arrest. GA also reduced RCC cell invasion and migration. In addition, the epidermal growth factor receptor (EGFR) was identified as a critical target protein of GA, which significantly inactivated EGFR signaling in RCC (P<0.05). Collectively, the present study provided evidence that GA exerts its anticancer function by directly targeting the EGFR signaling pathway, revealing the potential of GA therapy for RCC. Copyright: © Zhu et al.

Introduction

Renal cell carcinoma (RCC), the most common urogenital neoplasm, accounts for ~5% of human adult malignancies worldwide (1). It is estimated that 64,000 new cases and 14,000 deaths occurred as a result of RCC in the United States in 2017(1). Additionally, the worldwide incidence and mortality rates of RCC are steadily increasing (1). To date, metastatic lesions are present in ~30% of patients at initial presentation due to an absence of symptoms at the early stages (2). Despite advances in therapeutic approaches, the prognosis of patients with RCC remains poor and <40% of patients survive ≥5 years post diagnosis, as therapeutic options are limited (3). Moreover, RCC recurrence is primarily due to the lack of routine adjuvant therapy in the clinic, as RCC is both chemotherapy and radiotherapy resistant (4,5). Therefore, it is necessary to screen new compounds and develop novel targeted therapies for RCC.

The leaves and seeds of Ginkgo biloba L., an ancient gymnosperm species, have a long history of use in traditional Chinese medicine (6,7). GA, which is characterized by a mixture of components containing 13-19 side chain carbon atoms at site 6 and 0-3 side chain double bonds, can be extracted from ginkgo fruit, exotesta and leaves (8-10). GA has been reported to display a wide range of bioactive properties, including antimicrobial, antivirus and molluscicidal activities (11). Accumulating evidence has demonstrated that several monomer structures of GA (C13:0, C15:0 and C17:1) exert antitumor activity in a number of human malignancies, including hepatocellular carcinoma as well as colon, breast and lung cancer (12-15). However, to the best of our knowledge, no previous study has been conducted to investigate the pharmacological effect of GA in RCC.

Network pharmacology, a novel systems pharmacology model, was established to explore the therapeutic mechanism of individual drugs on the basis of pharmacokinetics synthesis screening, target identification and network analysis (16,17). A network pharmacology-based approach has displayed potential for investigating the therapeutic mechanism of natural agents in a number of malignancies, including lung cancer, breast cancer and hepatocellular carcinoma (18,19). The identification of the therapeutic mechanism of GA could facilitate more precise GA application in malignant cancer treatment. Therefore, the present study utilized a network pharmacology-based approach to explore the key target of GA. Subsequently, molecular docking, a theoretical simulation method, was used to analyze the interaction between molecules and to predict the binding site and affinity of GA to ensure the accuracy and effectiveness of the network analysis.

Materials and methods

Cell culture and chemicals

The human RCC cell lines 786-O and A498 were purchased from the Cell Bank of Type Culture Collection of the Chinese Academy of Sciences. Cells were grown in RPMI 1640 medium (Sigma-Aldrich; Merck KGaA) supplemented with 10% fetal bovine serum (HyClone; GE Healthcare Life Sciences) and 100 µg/ml penicillin/streptomycin at 37˚C in a humidified incubator with 5% CO2. GA (C17:1; C24H38O3; Tauto Biotech Co., Ltd.; Fig. 1A) was dissolved in DMSO (Sigma-Aldrich; Merck KGaA) to make a 20 mM stock solution. For cell treatment, 10 and 20 µM GA (diluted in RPMI 1640 medium) were used.

Figure 1

Effect of GA on RCC cell proliferation. 786-O and A498 cells were pre-treated with or without 10 or 20 µM GA, as indicated. (A) Chemical structure of GA (C17:1; C24H38O3). (B) Representative images and quantification of cell viability (magnification, x200). Cell viability analysis was performed 72 h after treatment using an MTT assay. (C) Representative cell cycle plots and quantification 2 days after GA treatment (red, G0/G1 phase; green, S phase and purple, G0/M phase). Assessment of cell phase percentage was conducted using flow cytometry. (D) Representative images and quantification of subcutaneous xenograft tumors derived from mice in the GA and DMSO groups. Scale bar, 1 cm. Tumor weight was measured 6 weeks after injection. (E) Representative image and quantification of immunohistochemical staining for Ki-67 (magnification, x200). n=5. *P<0.05. GA, ginkgolic acid; RCC, renal cell carcinoma.

Cell viability assay

786-O and A498 cells were seeded at a density of 1x103 cells per well in 96-well plates. After culture for 12 h at 37˚C, the medium was replaced with maintenance medium containing the desired concentrations (10 and 20 µM) of GA or DMSO. Cell viability was assessed after 72 h incubation at 37˚C using an MTT assay kit (Nanjing KeyGen Biotech Co., Ltd.) according to the manufacturer's protocols. DMSO was used to dissolve formazan crystals and absorbance was measured in each well at 450 nm using a 318C microplate reader (Shanghai Peiou Analytical Instruments Co., Ltd.).

Transwell invasion assay

To determine c ell invasion, invasion assays were performed using 24-well Matrigel-coated invasion chambers (8-µm pore size; Corning Inc.). RCC cells were pre-treated with GA for 24 h, seeded into the upper chamber of the Transwell insert and incubated for 24 h at 37˚C. Subsequently, cells on the upper side of the membrane were wiped off and invading cells were fixed in 100% cold methanol at 4˚C for 20 min and stained with 0.2% crystal violet at room temperature for 30 min (Sigma-Aldrich; Merck KGaA). The stained cells were quantified under a light microscope, from five randomly selected fields of view (magnification, x400).

Wound healing assay

RCC cells were pre-treated with 10 and 20 µM GA for 24 h at 37˚C and allowed to grow to 90-95% confluence without serum. The cell monolayers were scratched with a sterile 200-µl pipette tip. Subsequently, the cells were washed with RPMI 1640 medium to remove cell debris and fresh cell culture medium (RPMI 1640 medium supplemented with 10% FBS) was added. Images of the scratches were obtained at 0 and 24 h using a light microscope (magnification, x200). Migratory ability was measured as the percentage of wound closure with the initial wound width defined as 1.

Cell cycle and early apoptosis assay

Cell cycle distribution and apoptosis were analyzed using the Annexin V-FITC Apoptosis kit (Solarbio Life Sciences) according to the manufacturer's protocols. Briefly, RCC cells were cultured in RPMI 1640 medium in 6-well plates at a density of 1x106 cells for 12 h at 37˚C. Then, the medium was replaced with RPMI 1640 medium containing 20 µM GA. Cells were stained with Annexin V-FITC and propidium iodide buffer at room temperature for 15 min followed by the addition of Annexin V binding buffer. Cell cycle and apoptosis assays were performed on a BD Accuri C6 (BD Biosciences) flow cytometer and BD Accuri C6 software Version 1.0 (Becton, Dickinson and Company) was used to analyze the data.

Xenograft implantation

Animal experiments were approved by The Animal Care and Use Committee of the Second Military Medical University (approval no. NMU20181032). Animals had free access to autoclaved chow diet and water in a pathogen-free state, at 22±1˚C with 45±10% humidity and 12-h light/dark cycles. The health and behaviour of the mice were monitored every 12 h. Moribund mice (exhibiting anorexia, immobility or an unkempt coat) would be euthanized by CO2 at the rate of 3.5 l/min displacing 20% of the cage volume per minute. Death was verified by monitoring cessation of breathing. To detect the effect of GA on tumorigenicity in nude mice, 6-8-week-old male BALB/c mice (n=10; weight, 20-30 g; Second Military Medical University) were injected subcutaneously with 786-O or A498 cells (1x107 dissolved in PBS per site; one tumor burden per mouse) on the right flank. Mice were randomly divided into two groups (n=5 per group) that either received an intragastric administration of GA (10 mg/kg) or 0.9% saline twice per week (13). At 6 weeks after GA injection, mice were euthanized by decapitation. The tumor volumes and weight were measured. Prior to 6 weeks after GA injection, no mice were euthanized or found dead.

Protein-protein interaction (PPI) network construction and analysis

The Online Mendelian Inheritance in Man (OMIM) Database (version 1.0; www.ncbi.nlm.nih.gov/omim), from which the original data used in the present study was obtained, is a central-level database covering relevant information and literature on human genetic diseases and gene loci. Data were input into the Search Tool for the Retrieval of Interacting Genes/Proteins (version 11.0; string-db.org) database for further network construction. The obtained PPI networks were then visualized using Cytoscape software (version 3.6.1; https://cytoscape.org). Topology analysis (CentiScaPe plug-in; version 2.2; http://apps.cytoscape.org/download/stats/centiscape/) was used to identify key targets in the network. Degrees of betweenness were assessed using the key hubs of centrality, namely betweenness (the number between nodes) and closeness (the distance between nodes).

Molecular docking

The docking between GA and key targets of RCC was implemented using Sybyl X software (version 2.1.1; https://en.freedownloadmanager.org/Windows-PC/SYBYL-X.html). The conformation of GA was downloaded from the Traditional Chinese Medicine Systems Pharmacology Database (version 1.0; https://tcmspw.com/tcmsp.php). The mol2 format file was further transformed and extracted by Openbabel software (release date, 2017-02-22; https://sourceforge.net/projects/openbabel/). The X-ray crystal structures of key targets were obtained from the RCSB Protein Data Bank (version 1.0; www.rcsb.org). Prior to docking, targets were structurally optimized by adding hydrogen atoms and removing water molecules, and the representative protein activity docking pockets were subsequently generated. Molecular docking was implemented based on the Docking Suite module (release date, 2013-04-08; https://sourceforge.net/projects/wpfdocking/) and hydrogen bond stability and domain structure similarity were used to evaluate the reliability of results. The criteria of binding scoring: 0-3, Poor; 4-6, moderate; and 7-10, good.

Immunohistochemistry and immunoblotting assay

Cells were pre-treated with 10 ng/ml epidermal growth factor (EGF; PeproTech, Inc.) for 12 h at 37˚C. Immunohistochemical assays of xenografts were conducted using Ki-67 (cat. no. ab15580; 1:50; Abcam) and EGF receptor (EGFR; cat. no. ab52894; 1:50; Abcam) monoclonal antibodies, as previously described (20). The expression level was analyzed from images obtained using a light microscope (magnification, x200) from five random fields of view. Immunoblot assays were performed as previously described (20). Primary antibodies included those targeted against phosphorylated (p)-EGFR (cat. no. 4370; 1:1,000; Cell Signaling Technology, Inc.), EGFR (cat. no. 2085; 1:1,000; Cell Signaling Technology, Inc.), p-Akt (Ser473; cat. no. 4060; 1:1,000; Cell Signaling Technology, Inc.), Akt (cat. no. 4691; 1:1,000; Cell Signaling Technology, Inc.), p-ERK (Thr202/Tyr204; cat. no. 4370; 1:1,000; Cell Signaling Technology, Inc.) and ERK (cat. no. 4370; 1:1,000; Cell Signaling Technology, Inc.). Horseradish peroxidase-conjugated secondary antibody (1:2,000; cat. no. ab6112; Abcam) was used. β-actin antibody (cat. no. ab8226; 1:5,000; Abcam) was used as a control. Relative protein expression and staining intensity was calculated based on the densitometric analysis by Image Lab software Version 3.0 (Bio-Rad Laboratories, Inc.).

Statistical analysis

All data are presented as the mean ± SD. SPSS software (version 18.0; SPSS Inc.) was used for statistical analysis. The statistical significance between two groups was analyzed using an unpaired Student's t-test. One-way ANOVA followed by a Dunnett's post hoc test was performed to compare data among ≥3 groups. P<0.05 was considered to indicate a statistically significant difference.

Results

GA inhibits RCC cell proliferation in vitro and in vivo

To investigate the role of GA in RCC, human RCC cells (786-O and A498) were incubated with different concentrations of GA. An MTT assay was performed 72 h after treatment and a dose-dependent decrease in cell viability was observed (Fig. 1B). In addition, GA increased the proportion of cells in the G0/G1 phase and decreased the proportion of cells in the S phase (Fig. 1C). However, GA treatment did not significantly affect RCC cell apoptosis (Fig. S1). Based on in vitro data, xenograft implantation in BALB/c nude mice was performed to clarify the effect of GA on RCC in vivo. RCC cell suspensions (1x107) were subcutaneously injected into nude mice. The tumor volumes and weights of the group treated with GA were significantly lower compared with those of the group treated with 0.9% saline (P<0.05; Figs. 1D and S2A). In the present study, the maximum diameter of a single tumor was 1.8 cm. However, no significant difference in body weight loss was observed between the two groups (Fig. S2C). Additionally, immunohistochemical staining revealed that GA significantly reduced Ki-67 expression in the xenograft (P<0.05; Fig. 1E).

GA inhibits RCC cell invasion and migration

The effect of GA on the invasion and migration of RCC cells was evaluated using Transwell invasion and wound healing assays, respectively. Transwell invasion assays showed that GA reduced the number of invading RCC cells in a dose-dependent manner (Fig. 2A). Consistent with this result, wound healing assays also showed that GA inhibited RCC cell migration in a dose-dependent manner (Fig. 2B).

Figure 2

GA inhibits the migration and invasion ability of RCC cells. (A) Matrigel-coated invasion chamber following treatment with DMSO or GA (10 or 20 µM) and quantification of the number of invading cells in each chamber (magnification, x400). (B) Wound healing assays were performed in RCC cells treated with DMSO or GA (10 or 20 µM). Representative images were obtained at 0 and 24 h (magnification, x100). Quantification of migratory distance. Scale bar, 100 µm. n=5. *P<0.05, as indicated. GA, ginkgolic acid; RCC, renal cell carcinoma.

PPI network and topology analysis

The interaction network was constructed based on OMIM original data and is depicted in Fig. 3, and included 549 nodes and 11,836 edges. Larger areas and deeper colours represent higher node connectivity, which likely indicates greater importance of the node in the network. The results displayed the scale-free property of the network, meaning the number of nodes decreases as the number of edges in the network increases. Betweenness degree was used to distinguish these highly connected key nodes from other nodes in the network (Fig. 4). Finally, 15 key targets were selected: Tumor protein p53, 284 points; albumin, 267 points; AKT1, 251 points; vascular endothelial growth factor A, 243 points; insulin, 230 points; interleukin 6, 223 points; JUN, 215 points; tumor necrosis factor, 213 points; MYC, 211 points; phosphatidylinositol-4,5-bisphosphate 3-kinase catalytic subunit-α, 208 points; EGFR, 198 points; mitogen-activated protein kinase 1, 186 points; transforming growth factor β1, 185 points; BCL2, 179 points; and STAT3, 173 points.

Figure 3

Protein-protein interaction network including 549 nodes and 11,836 edges. Larger areas and deeper colours represent higher node connectivity.

Figure 4

Topological analysis. The higher the degree of the node, the more important the node is in the network. unDir, undirected index.

GA inactivates the EGFR pathway in RCC

Molecular docking, a tool for studying the interaction strength between molecules, was used to explore the accuracy and effectiveness of the PPI network. To assess the reliability of the aforementioned drug-target interactions and to further investigate binding mode and affinity, molecular docking models were constructed for GA and the 15 key targets. Analysis of the binding data indicated stable conformational binding and good scoring (>7 points) of EGFR to GA (9.4558 points; Fig. 5A). Immunohistochemical staining displayed lower EGFR expression in the xenograft after GA treatment compared to before treatment (Fig. 5B). The immunoblotting assay demonstrated that EGFR, p-Akt and p-Erk (downstream of the EGFR signaling pathway) were significantly downregulated after GA treatment in xenografts, as well as in vitro (P<0.05; Fig. 5C).

Figure 5

GA exerts its function via suppressing the EGFR pathway. (A) Binding interaction model of EGFR and GA. (B) Mice were injected subcutaneously with 786-O cells (1x107 cells) followed by intragastric administration of GA (10 mg/kg) or 0.9% saline twice per week. Representative image and quantification of immunohistochemical staining for EGFR in the xenograft (magnification, x200). (C) 786-O cells were pre-treated with 10 ng/ml EGF for 12 h at 37˚C followed by DMSO or GA for 48 h at 37˚C. The expression of p-EGFR, EGFR, p-Akt, Akt, p-Erk1/2 and Erk1/2 was analyzed by immunoblotting. β-actin was used as an internal control. n=5. *P<0.05, as indicated. GA, ginkgolic acid; EGFR, epidermal growth factor receptor; EGF, epidermal growth factor; p, phosphorylated.

Discussion

Despite great advances in cancer therapy, major limitations still exist in the management of RCC (21). Moreover, patients with metastatic RCC have a short life expectancy (median overall survival, 22.5 months) (22). Extracts from natural plants are becoming an increasingly popular strategy to identify novel antitumor compounds (23,24). Recently, several studies have reported that GA displays promising antitumor activities (12-15). Therefore, identification of the regulatory mechanism of GA in tumorigenesis would provide valuable insight for the treatment of malignancies. Collectively, the results of the present study indicated that GA suppressed the development of RCC. These results were consistent with previous studies demonstrating that GA plays an inhibitory biological role in cancer (12-15,25). However, the biological effect of GA on RCC was observed at high concentrations of GA in vitro and it is uncertain whether this concentration would be possible in vivo. Therefore, further in vivo investigation (pharmacokinetics and toxicology analysis) is required.

GA suppresses tumor growth and invasion via various signaling pathways, including the hepatocyte growth factor/c-Met signaling pathway in hepatocellular carcinoma (12), the protein kinase AMP-activated catalytic subunit α2 signaling pathway in colon cancer (13), the NF-κB signaling pathway in breast cancer (14) and the PI3K/Akt/mTOR signaling pathway in lung cancer (15). A number of studies have reported that, in addition to inducing cell cycle arrest, GA also increases apoptosis in colon cancer and hepatocellular carcinoma (26,27). Therefore, it is difficult to clarify the antitumor mechanism of GA in RCC. Network pharmacology provides a strategy to investigate complex mechanisms of drug action and to identify potential drug targets (28). In a network pharmacology system, therapy response can be taken into account based on the robustness of complex disease networks in dealing with node attacks (node linking degree) due to inherent diversity and redundant compensation signaling pathways (12,19). The result of network pharmacology is a highly resilient network system with topological interaction (19,29). Therefore, computational prediction with a PPI network and topology analyses reveals the potential interactions among compounds and multiple signaling transduction molecules underlying a disease phenotype (30). According to the algorithm value, 15 key targets associated with RCC were identified in the current study. Furthermore, analysis of the molecular docking model demonstrated a stable conformational affinity between EGFR and GA. EGFR was validated as a direct target for GA both in vitro and in vivo. Furthermore, GA negatively modulated p-Akt and p-Erk expression via the EGFR/Akt/Erk signaling pathway in RCC cells. However, the mechanism of EGFR protein degradation (autophagy and ubiquitination) requires further investigation.

EGFR belongs to the ErbB family of receptor tyrosine kinases, which can be activated by several ligands, including EGF, transforming growth factor-α, amphiregulin, heparin-binding EGF, β-cellulin and epiregulin (31-34). In humans, EGFR is upregulated and/or activated in various malignancies and suppression of EGFR activation is considered a valid strategy for tumor treatment (34,35). Akt and Erk are downstream signaling molecules of EGFR, and the aberrant activation of either triggers a cascade of proliferative responses (36). Akt and Erk phosphorylation are increased when EGFR is activated in RCC (37,38). Previous studies have provided direct evidence that the EGFR signaling pathway is highly activated in RCC progression and EGFR expression is associated with prognosis in patients with clear cell RCC (38-40). Furthermore, inactivation of the EGFR signaling pathway inhibited RCC cell migration and invasion in vitro (41). These data imply that activation of the EGFR signaling pathway may be an important event that occurs during RCC development. The present study demonstrated that GA, which acts as a suppressor of EGFR, exhibited a biological effect in RCC cells via the EGFR/Akt/Erk signaling pathway.

The present study investigated the molecular mechanism by which GA exerts its negative effects on proliferation, invasion and migration in human RCC cells. GA significantly inhibited the EGFR signaling pathway by directly binding to EGFR. The downstream targets of EGFR, including p-Akt and p-Erk, were also downregulated following GA treatment. EGFR, as a novel target of GA, may be a promising therapeutic agent for human RCC.