Ahpatinins C, E, and G were prepared at a concentration of 50 mM using dimethyl sulfoxide (DMSO). In all experiments, the negative control groups were treated with equal volumes of DMSO. Fetal bovine serum (FBS) and minimum essential medium (MEM) were purchased from Invitrogen (Thermo Fisher Scientific, Inc.), and endothelial growth medium-2 (EGM-2) and antibiotics were obtained from Lonza Group, Ltd. Recombinant human VEGF, Matrigel, gelatin, and Transwell chamber systems were obtained from Koma Biotech, BD Biosciences, Sigma-Aldrich (Merck KGaA), and Corning Costar, Inc., respectively. Antibodies against VEGFR2 (230 kDa; cat. no. 2479), phospho-VEGFR2 (Tyr1175, 230 kDa; cat. no. 2478), AKT (60 kDa; cat. no. 9272), phospho-AKT (Ser473, 60 kDa; cat. no. 9271), ERK1/2 (42, 44 kDa; cat. no. 9102), phospho-ERK1/2 (Thr202/Tyr204, 42, 44 kDa; cat. no. 9101), JNK (46 kDa; cat. no. 9252), phospho-JNK (Thr183/Tyr185, 46 kDa; cat. no. 9251), p38 (43 kDa; cat. no. 9212), phospho-p38 (Thr180/Tyr182, 43 kDa; cat. no. 9211), NF-κB (65 kDa; cat. no. 3034), phospho-NF-κB (Ser536, 65 kDa; cat. no. 3033), MMP-2 (64, 72 kDa; cat. no. 4022), MMP-9 (84, 92 kDa; cat. no. 3852), HIF-1α (120 kDa; cat. no. 79233), β-actin (42 kDa; cat. no. 4967), rabbit IgG (cat. no. 7074), and mouse IgG (cat. no. 7076) were purchased from Cell Signaling Technology, Inc.

Streptomyces sp. 15JA150 was cultured in a 250-ml Erlenmeyer flask containing 50 ml of seed culture medium for 3 days at 28°C on a rotary shaker with agitation at 125 rpm. For a large culture, 1% of the preculture broth was inoculated into 40×1,000 ml baffled Erlenmeyer flasks containing 250 ml of modified YMG broth (glucose 1%, soluble starch 2%, malt extract 0.5%, yeast extract 0.5%, and CaCO₃ 0.05%) and cultured for 7 days at 28°C on a rotary shaker with agitation at 125 rpm. The residue was partitioned with EtOAc three times and evaporated to remove the EtOAc. The crude extract was fractionated by reversed phase C₁₈ vacuum column chromatography with a stepwise solvent system of MeOH:H₂O (20:80-100:0, each × 1 l). The 70% fraction was further separated by RP-HPLC with CH₃CN:H₂O (70:30) to yield ahpatinins C, E, and G.

HUVECs (ATCC^® CRL- 1730™) and human glioblastoma U87MG cells (Korean Cell Line Bank No. 30014; glioblastoma of unknown origin) were grown in EGM-2 and MEM supplemented with 10% FBS, respectively. The identity of the U87MG cell line was confirmed by STR profiling (D3S1358: 16,17; vWA: 15,17; FGA: 18,24; Amelogenin: X,Y; TH01: 9.3; TPOX: 8; CSF1PO: 10,11; D5S818: 11,12; D13S317: 8,11; D7S820: 8,9). All cells were maintained at 37°C in a humidified 5% CO₂ incubator. For hypoxic conditions, the cells were incubated in a hypoxic chamber (Forma Scientific) under 5% CO₂ and 1% O₂ balanced with N₂.

HUVECs (1×10⁵ cells/well) were seeded in a 12-well culture plate. Ahpatinins C, E, and G (1–25 µM) were added to each well, and the cells were incubated for 72 h. After 72 h, the cells were stained with trypan blue and counted by a hemocytometer using an optical microscope (Olympus Corporation) at an ×200 magnification.

HUVECs were seeded at a density of 3×10³ cells/well in a 96-well culture plate and then treated with various concentrations (1–25 µM) of ahpatinins C, E, and G in the presence of VEGF (30 ng/ml) for 72 h. The cell proliferation was measured using a 3-(4,5-dimethylthiazol- 2-yl)-2,5-diphenyltetrazolium bromide (MTT) colorimetric assay.

The invasiveness of HUVECs was examined using a Transwell chamber system with polycarbonate filter inserts with a pore size of 8.0 µm. The lower surface of the filter was coated with 10 µl of gelatin (1 mg/ml) for 1 h and the upper surface was coated with 10 µl of Matrigel (3 mg/ml) for 2 h. The serum-starved HUVECs (6×10⁴ cells) were seeded in the upper chamber of the filter, and ahpatinins C, E, and G (10 and 20 µM) were added to the lower chamber in the presence of VEGF (30 ng/ml). The chamber was incubated at 37°C for 6 h, and then the cells were fixed with 70% methanol at room temperature for 5 min and stained with hematoxylin and eosin (H&E) at room temperature for 5 min, respectively. The total number of cells that invaded the lower chamber of the filter was observed and counted using an optical microscope at an ×400 magnification.

The cell-matrix adhesion assay was performed in a 24-well culture plate coated with gelatin overnight at 4°C. The HUVECs (5×10⁴ cells/well) were cultured in each well in EGM-2 containing 1% FBS and treated with ahpatinins C, E, and G (10 and 20 µM) in the presence of VEGF (30 ng/ml). After 3 h, the unbound cells were carefully removed, and the attached cells were observed and counted under an optical microscope at an ×200 magnification.

The serum-starved HUVECs (8×10⁴ cells) were placed on a surface containing Matrigel (10 mg/ml) from an angiogenesis kit (Ibidi GmbH) and incubated with ahpatinins C, E, and G (10 and 20 µM) for 8 h in the presence of VEGF (30 ng/ml). The morphological changes of the cells and tube formation were visualized under an optical microscope and photographed at an ×200 magnification.

The fertilized chick eggs were incubated in a humidified incubator at 37°C and 50% humidity for 3 days. Approximately 6–8 ml of egg albumin was removed with a hypodermic needle, enabling the CAM and yolk sac to drop away from the shell membrane. After 2 days, the shell was punched out and peeled away. Thermanox coverslips (Nalge Nunc International) with or without ahpatinin E (10 µg/egg) were air-dried and applied to the CAM surface. Two days later, 2 ml of 10% fat emulsion (Sigma-Aldrich; Merck KGaA) was injected into the chorioallantois and the vascular images were observed by an optical microscope at an ×200 magnification.

A tumor cell-induced chemoinvasion assay was performed using an in vitro co-culture system based on the chemoinvasion assay. The U87MG cells were plated on the lower chamber and treated with ahpatinins C, E, and G (10 and 20 µM) for 24 h. The medium in each lower chamber was then replaced with fresh medium without ahpatinins C, E, and G, and serum-starved HUVECs (1×10⁵ cells) were placed in the upper chamber. The chamber was incubated at 37°C for 20 h, and the HUVECs that invaded the lower chamber of the filter were analyzed using the same procedure as described in the chemoinvasion assay.

To assess the effects of ahpatinins C, E, and G on tumor cell-induced capillary tube formation, a conditioned medium was obtained from the U87MG cells and used as the angiogenic stimulus for the tube formation of HUVECs. Briefly, the U87MG cells were treated with ahpatinins C, E, and G (10 and 20 µM) for 24 h, and then the medium was replaced with fresh medium without ahpatinins C, E, and G. The conditioned medium was used in the in vitro tube formation assay.

Cells were lysed using RIPA buffer (Sigma-Aldrich; Merck KGaA) supplemented with a protease inhibitor cocktail (Roche Diagnostics) on ice. Protein concentrations of the extracts were determined using a BCA Protein Assay kit (Pierce; Thermo Fisher Scientific, Inc.). Equal amounts of cell lysate (40 µg/lane) were separated by 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), and the separated proteins were transferred to polyvinylidene difluoride (PVDF) membranes (EMD Millipore) using standard electroblotting procedures. The blots were blocked in Tris-buffered saline with Tween-20 (TBST) containing 5% skim milk at room temperature for 1 h and immunolabeled with primary antibodies against phospho-VEGFR2 (dilution 1:2,000), VEGFR2 (dilution 1:2,000), phospho-AKT (dilution 1:2,000), AKT (dilution 1:2,000), phospho-ERK1/2 (dilution 1:2,000), ERK1/2 (dilution 1:2,000), phospho-JNK (dilution 1:2,000), JNK (dilution 1:2,000), phospho-p38 (dilution 1:2,000), p38 (dilution 1:2,000), phospho-NF-κB (dilution 1:2,000), NF-κB (dilution 1:2,000), MMP-2 (dilution 1:2,000), MMP-9 (dilution 1:2,000), HIF-1α (dilution 1:2,000), and β-actin (dilution 1:2,000) overnight at 4°C. After washing with TBST three times, the membranes were incubated with horseradish peroxidase-conjugated anti-rabbit (dilution 1:3,000) or anti-mouse (dilution 1:3,000) secondary antibody for 1 h at room temperature. Immunolabeling was detected with an enhanced chemiluminescence (ECL) kit (Bio-Rad Laboratories, Inc.) according to the manufacturer's instructions. The band density was analyzed using ImageJ software (version 1.5; NIH).

VEGF concentration in the media containing cells treated with ahpatinins C, E, and G (5, 10 µM) was detected using a VEGF immunoassay kit (R&D Systems, Inc.) according to the manufacturer's instructions. The results were expressed as the concentration of VEGF relative to the total amount of protein obtained from each well.

The data were presented as the mean ± standard error (SE) of three independent experiments. Differences among groups were analyzed using the analysis of variance (ANOVA) with SPSS statistics package (SPSS 9.0; SPSS Inc.). Post hoc analysis was carried out by Tukey's test. A P-value of <0.05 was considered to indicate a statistically significant difference.

Prior to assessing the antiangiogenic activities of ahpatinins C, E, and G, the cytotoxic effects of ahpatinins C, E, and G on HUVECs were first investigated using the trypan blue exclusion method. As revealed in Fig. 2A, treatment with 1–25 µM of ahpatinins C, E, and G did not affect the viability of HUVECs. Thus, the effects of ahpatinins C, E, and G on in vitro angiogenesis at sub-toxic doses were evaluated. To assess the endothelial cell growth inhibitory activities of ahpatinins C, E, and G, the proliferation assay was performed using the MTT colorimetric method. Treatment with VEGF (30 ng/ml) increased the proliferation of HUVECs up to 121.3%, whereas ahpatinins C, E, and G inhibited the VEGF-induced proliferation of HUVECs with different sensitivity to growth inhibition (Fig. 2B). Ahpatinin C inhibited cell growth at 5–25 µM, and ahpatinin G exhibited a relatively weak proliferation inhibitory activity. Among them, ahpatinin E most effectively inhibited the growth of HUVECs at all the treated concentrations (1–25 µM). These results indicated that ahpatinins C, E, and G suppressed the growth of HUVECs induced by VEGF without cytotoxicity.

The effects of ahpatinins C, E, and G on the key angiogenic phenotypes such as endothelial cell invasion, adhesion, and tube formation, were next determined (20). Serum-starved HUVECs were stimulated by VEGF with or without ahpatinins C, E, and G (10 and 20 µM), and their inhibitory activities on VEGF-induced angiogenesis were observed through chemoinvasion, adhesion, and tube formation assays. As revealed in Fig. 3A-C, ahpatinins C, E, and G dose-dependently decreased the invasiveness, adhesion, and tube forming ability of HUVECs stimulated by VEGF. Among them, ahpatinin E exhibited the greatest antiangiogenic activity. These results demonstrated that ahpatinins C, E, and G significantly inhibited angiogenesis without exhibiting cytotoxicity on endothelial cells in vitro.

To further assess the maximum inhibitory effects of ahpatinin E on in vitro and in vivo angiogenesis, a CAM assay was employed. Coverslips containing vehicle alone or ahpatinin E were located on the CAM surface, and the neovascularized zones were observed under a microscope. The ahpatinin E-treated CAMs had avascular zones as compared to the vehicle-treated ones (Fig. 4). The antiangiogenic response was calculated as the percentage of inhibited eggs relative to the total number of live eggs tested. The inhibition of neovascularization on the control coverslips was 6% (n=15), whereas ahpatinin E potently suppressed the angiogenesis of the CAMs (75% at 10 µg/egg, n=12), without any rupture of the preexisting vascular tubes. In conclusion, these results demonstrated that ahpatinin E significantly inhibited angiogenesis both in vitro and in vivo without exhibiting cytotoxicity against endothelial cells.

VEGF binding to VEGFR2 at the surface of endothelial cells leads to dimerization and autophosphorylation of specific tyrosine residues in the cytoplasmic domain of VEGFR2 resulting in the subsequent activation of multiple downstream signaling mediators, such as AKT, MAPKs, and NF-κB that promote angiogenesis (13–20). Thus, it was investigated whether the antiangiogenic activities of ahpatinins C, E, and G are associated with the suppression of VEGFR2-mediated signaling pathways. As revealed in Fig. 5, ahpatinins C, E, and G effectively suppressed the phosphorylation of VEGFR2, AKT, ERK1/2, JNK, p38, and NF-κB induced by VEGF, without affecting the total protein levels. Collectively, these data indicated that ahpatinins C, E, and G may exert antiangiogenic activities by inhibiting VEGFR2-mediated downstream signaling cascades in HUVECs.

MMPs degrade various ECM proteins present in the blood vessel basement membrane during angiogenesis (33). Therefore, the effects of ahpatinins C, E, and G on the expression of MMP-2/-9 stimulated by VEGF were examined. As revealed in Fig. 6, ahpatinins C, E, and G significantly decreased the expression levels of MMP-2 and MMP-9 in HUVECs, indicating that the antiangiogenic effects of ahpatinins C, E, and G may be associated with the downregulation of MMP-2/-9 expression.

Since tumor angiogenesis is a critical hallmark of tumor growth and metastasis, blocking tumor-induced angiogenesis is a promising strategy in limiting cancer progression (34,35). To evaluate whether ahpatinins C, E, and G inhibit tumor cell-induced angiogenesis, the effects of ahpatinins C, E, and G on the invasion and tube formation of HUVECs stimulated by U87MG glioblastoma cells were examined. As revealed in Fig. 7A, the HUVECs co-cultured with U87MG cells exhibited significant invasion compared to HUVECs alone. In contrast, when U87MG cells were treated with 20 µM of ahpatinins C, E, and G, the induced invasion of HUVECs was completely inhibited. In addition, the tube formation of HUVECs was increased by the conditioned medium obtained from U87MG cells compared to the control (medium only), whereas conditioned medium obtained from the U87MG cells treated with ahpatinins C, E, and G, effectively prevented the induced tube formation of HUVECs (Fig. 7B). These data revealed that ahpatinins C, E, and G could inhibit tumor cell-induced angiogenesis.

Activation of HIF-1α in the hypoxic tumor cells results in an increased expression of proangiogenic growth factors such as VEGF (36,37). To confirm the role of HIF-1α in mediating the antiangiogenic effects of ahpatinins C, E, and G, the inhibitory activities of ahpatinins C, E, and G on the HIF-1α expression of U87MG glioblastoma cells were determined. As revealed in Fig. 8A, treatment with 10 and 20 µM of ahpatinins C, E, and G decreased the hypoxia-induced accumulation of HIF-1α protein in U87MG cells. Furthermore, the effects of ahpatinins C, E, and G on the expression of VEGF induced by hypoxia were investigated. Ahpatinins C, E, and G (10 µM) also reduced VEGF production by U87MG cells under hypoxic conditions (Fig. 8B). These results indicated that ahpatinins C, E, and G could suppress tumor angiogenesis through the downregulation of HIF-1α and its downstream target gene, VEGF.