The antiangiogenic activities of ethanolic crude extracts of four Salvia species

Background Angiogenesis is one of cancer hallmarks that are required for both cancer progression and metastasis. In this study we examined the antiangiogenic properties of the ethanolic crude extracts of four Salvia species grown in Jordan. Methods The direct antiangiogenic activity was evaluated using various models: ex vivo rat aortic ring assay, in vitro assessment of HUVEC proliferation and migration, and in vivo CAM assay, while we used the changes in the expression of HIF-1α and VEGF in breast cancer cells (MCF 7) as an indicative for the indirect antiangiogenic activity. Results All four crude extracts showed a potential antiangiogenic activity in the rat aortic assay, however two species were found to be cytotoxic against Fibroblast cell line (PLF); the finding that caused the exclusion of these two extracts from further studies. Of the two remaining extracts, S. triloba showed very promising direct and indirect antiangiogenic activities. S. triloba inhibited the HUVEC proliferation with an IC50 of 90 μg/mL and HUVEC migration by 82% at 150 μg/mL. Furthermore, the in vivo CAM assay also illustrated the high impact of S. triloba against the newly formed vessel in the chicken embryonic membrane. Interestingly, the S. triloba inhibited the expression of VEGF at the mRNA and protein and the HIF-1α mRNA in the MCF 7 breast cancer cells under both normoxic and hypoxic conditions. Conclusions Taken together, all these findings of the direct and indirect angiogenic investigations nominated S. triloba as a highly potent antiangiogenic plant that may have chemotherapeutic and/or chemoprevention potentials.


Background
Angiogenesis is the formation of new blood vessels. Cancer is angiogenesis dependent; any significant increment in tumour size must be in synchrony with increment in the blood supply. The new blood vessels supply the tumour cells with extra amount of oxygen and nutrients, and most importantly they facilitate cancer cell metastasis to other localities [1]. All solid tumours are dependent on the angiogenesis for tumour growth and metastasise [2]. Breast cancer is the most common cancer in women counting for approximately 27% of all new cancers [3]. It is characterized by a distinct metastatic pattern [4].
Cancer cells within the tumour use the newly formed blood vessels as a port to metastasize to other localities [5]. Although less than 0.05% of circulating tumour cells has a potential to become stable metastases [6], the vast majority of breast cancer-related deaths result from metastatic tumours [7]. Angiogenesis, one of cancer hallmarks is involved in the progression and metastasis of breast cancer [8]. The process is tightly controlled through a balance of positive and negative regulatory factors and is triggered by pro-angiogenic growth factors [9]. Vascular endothelial growth factor (VEGF) is a major mediator of angiogenesis in cancer [10]. VEGF expression is induced under hypoxic conditions; a multistage process, in which the alpha subunit of hypoxia inducible factor-1 (HIF-1α) plays an important role [10]. Under normoxic condition, HIF-1α rapidly decreases since it is bound to the tumour suppressor Von Hippel-Lindau (VHL) protein, which in turn results in HIF-1α ubiquitynation and becomes a target for the proteosome. However, the low blood supplies toward the tumour mass drives the tumour tissue into hypoxia, which may induce transcriptional activation of VEGF expression through HIF-1α stabilization [11]. Since angiogenesis plays a prominent role in tumour growth and metastasis, inhibition of angiogenesis is considered as an important strategy for cancer therapy [12]. Furthermore, inhibiting angiogenesis before it starts, which known as angioprevention, has the potential to block the expansion of hyperplastic foci and subsequent tumour development at the premalignant stage [13]. Angioprevention compounds work through diverse pathways, amongst those is the interference with expression of the VEGF and HIF-1α, which stand out among the diverse factors that drive angiogenesis [13].
The genus Salvia is the largest and the most important genus of the family Lamiaceae. This genus has about 900 species, widespread throughout the world, and includes several ornamental, culinary and medicinal species [14]. Nineteen species of Salvia are reported to occur in the flora of Jordan [15]. Published data indicated that many Salvia species exert diverse biological activities, and have been used in many parts of the world as part of the local traditional medicines to treat various conditions. Examples of pharmacological properties are antioxidant [16], antimicrobial [17], anti-inflammatory, analgesic [18], antipyretic, hemostatic [19], hypoglycemic [20] and anti-tumour [21] activities. S. miltiorrhiza Bunge, commonly used in traditional Chinese herbal medicine to treat cardiovascular and hepatic disorders, has been shown recently to have significant antitumour and anti-angiogenesis properties [22]. Interestingly, the same plant, S. miltiorrhiza, has demonstrated some proantiangiogenic activity. Another recent publication has also reported antiangiogenic activity for S. officinalis [23].
Encouraged from the promising results of S. officinalis, the current study was designed to evaluate the antiangiogenic activity of four Salvia species grown in Jordan. Ethanolic crude extracts of the leaves of S. dominica, S. syriaca, S. triloba and S. hormium were prepared and their direct antiangiogenic properties were investigated using rat aortic ring assay. Plant extracts that exhibited direct antiangiogenic activities, were further explored for their direct activity in human umbilical endothelial cells (HUVEC) cytotoxicity assay, migration assay and chicken embryo chorioallantoic membrane (CAM) assay. Moreover, to test the extracts' indirect antiangiogenic activity, the effect on the expression of the VEGF protein and expression of both, VEGF and HIF-1α mRNA was examined using MCF 7 breast cancer cell line. All extracts were phytochemically screened using thin layer chromatography (TLC) and the presence of detected classes of secondary metabolites was reported. The effects of the extracts on normal cells were tested using periodontal fibroblast cell line (PLF).

Plant samples collection and extraction
Plant samples were collected during early flowering period (spring/summer 2009) from different areas in Jordan and have been identified by Prof. Dr. Barakat Abu Iremaileh (Faculty of Agriculture, The University of Jordan). Voucher specimens were deposited at the Department of Pharmaceutical Sciences, Faculty of Pharmacy, The University of Jordan. Plant samples were cleaned from extraneous material and dried at room temperature. Each 2.5 g of coarsely powdered plant material was extracted by refluxing with 25 mL 70% ethanol for 30 min and kept overnight at room temperature before filtration. After filtration, ethanol was evaporated until dryness and the crude extracts were weighed. The crude extracts were dissolved in dimethyl sulphoxide (DMSO) to a final stock concentration of 10 mg/mL. All extracts were kept at 4°C until the time of experiment.

Cell lines and cell culture
The human breast adenocarcinoma (MCF 7) was purchased from the European Collection of Animal Cell Culture (ECACC). Fibroblast cell line provided kindly from the Faculty of Dentistry, Jordan University of Science and Technology. Human umbilical vein endothelial cell line (HUVEC) was purchased from American Type Cell Culture Collection (ATCC). The MCF 7 and fibroblast cell lines were cultured in DMEM/F12 and DMEM medium (Gibco, Invitrogen, USA), respectively. Media were supplemented with 10% fetal bovine serum (FBS) (Gibco, Invitrogen, USA), 1% of 2 mM L-glutamine, 50 IU/mL penicillin and 50 μg/mL streptomycin (Lonza, Belgium). HUVECs were cultured in F12K medium (Gibco, Invitrogen, USA) supplemented with 0.1 g/mL Heparin (Sigma, USA) and 1% EGFR (Sigma, USA) 10% FBS, 1% of 2 mM L-glutamine, 50 IU/mL penicillin and 50 μg/mL streptomycin. HUVECs from passages 2 through 4 were used through this study. All cells were maintained at 37°C, 5% CO 2 in a humidified incubator.

Rat aortic ring assay
The rat aortic ring assay experiment was conducted after the experimental procedures were revised and approved by the Animal Ethics Committee of The University of Jordan. The assay was performed according to the standard protocol of Brown et al. [24], with minor modifications. Twelve to fourteen weeks old Sprague Dawley male rats were obtained from the animal house facility of the Faculty of medicine, The University of Jordan (UJ). The animals were humanely sacrificed via cervical dislocation under anesthesia with diethyl ether. Thoracic aorta was excised, rinsed with serum free media, cleaned from the fibroadipose tissue and was cross sectioned into thin rings of 1 mm thickness. M199 basal medium (Gibco, Invitrogen, USA) was used for the lower layer after adding fibrinogen and aprotinin (Sigma, USA) at 3 mg/mL and 5 μg/mL, respectively. A 300 μl of M199 medium was loaded in each 48-well plate and one aortic ring was seeded in each well. To each well, 10 μl of thrombin (Sigma, USA); prepared at 50 NIH U/mL in 0.15 M NaCl: bovine serum albumin (1%); was added and then was allowed to solidify at 37°C in 5% CO 2 for 60-90 min. The top layer medium was prepared by adding the following to M199 basal medium: 20% of heat inactivated fetal bovine serum (HIFBS) (Gibco, Invitrogen, USA), 1% Lglutamine (Lonza, Belgium), 0.1% aminocaproic acid (Sigma, USA), 1% amphotericin B (Lonza, Belgium) and 0.6% gentamicin (Lonza, Belgium). Plant extracts were added to the top layer medium at concentration of 100 μg/mL. The tissue rings were incubated at 37°C, 5% CO 2 in a humidified incubator. On day 4, the top layer medium was changed with fresh medium prepared as previously mentioned. The DMSO (1% v/v) and Suramin (100 μg/mL) were used as negative and positive controls respectively. The results examined microscopically at appropriate magnification and the magnitude of blood vessel outgrowth was quantified using Leica Quin software package [25], according to the technique developed by Nicosia et al. [26]. The results are presented as mean percent inhibition to the negative control ± SD, (n = 3).

In vitro cytotoxicity assay
Plant extracts were tested for cytotoxicity against fibroblast cell line. Cells were seeded at density of 10,000 cells/ well in 96-well plates. Afterwards, the cells were treated with two concentrations; 50 and 100 μg/mL in quadricate. Control wells contained DMSO at same concentrations. After 72 h incubation, cell viability was determined by MTT assay according to cell proliferation assay kit (Promega, USA). Absorbance (OD) was measured at 570 nm with background subtraction at 630 nm.

Antiproliferative activity
HUVECs were seeded at a density of 10 × 10 3 cells/well in 96-well plates and allowed to attach overnight. Plant extracts that showed antiangiogenic activity with aortic ring assay were screened on HUVECs for their IC 50 . Cells were treated with different concentrations (1.5-100 μg/mL) in quadricate. After 72 h treatment, MTT assay was performed according to cell proliferation assay kit (Promega, USA). Absorbance (OD) was measured at 570 nm with background subtraction at 630 nm. The calculation of IC 50 was performed using a sigmoidal plotting function provided in the GraphPad Prism software. DMSO was used as a negative control.

Wound healing migration assay
The migration assay was carried out as described previously [27]. Briefly, HUVECs were seeded at 5 × 10 5 /well in 6-well plates and allowed to form a confluent monolayer. The layer of cells was then scraped with a 20-200 μl micropipette tip to create a wound of~1 mm width. Cells were then washed twice with PBS and replaced with medium containing 100 AND 150 μg/mL of the plant extracts. The wounds were photographed at 0, 12 and 18 h, and the number of migrated cells was counted. Ten readings per well were taken. The results are presented as mean percentage of migration inhibition to the control ± SD, (n = 3).

In vivo CAM assay
Antiangiogenic effect of the plant extracts was investigated in vivo using CAM assay as mentioned previously [28]. Five day-old fertilized eggs were obtained from local hatchery. 5 mL of albumin was aspirated and the eggs were incubated horizontally to allow the CAM to detach from the shell. Chosen extracts were prepared in 1.2% agarose discs at concentration of 100 μg/disc. Discs containing the vehicle only (DMSO) were used as negative control. A small window opening was made in the shell, and the discs were directly applied onto the CAM. The square opening was covered with sterilized surgical tape and the embryos were incubated for 48 h at 37°C. The CAMs were photographed under a dissecting microscope and blood vessels in each CAM were counted. The results are presented as a mean percentage of inhibition to the control ± SD, (n = 3).
Expression of VEGF and HIF-1α MCF 7 cells treatment MCF 7 cells were seeded at a concentration of 3 × 10 6 cells in T75 Flask on the day before treatment. Then, the medium was replaced with a new medium, containing three concentrations of plant extract 100, 200 and 300 μg/mL. The cells were incubated at 37°C, 5% CO 2 for 16 h, under two conditions; hypoxic (0.1% O 2 ) and normoxic conditions (20% O 2 ). However, before cells were exposed to the hypoxic condition, they were treated under normoxic condition for 1 h then maintained under hypoxic conditions for 16 h. Hypoxic condition was performed by incubating the cells in GasPak Pouch (Becton Dickinson, Sparks, Md., USA). DMSO with the same concentrations as the extracts were then used as negative controls. Then, cells were harvested for RNA extraction.

RNA extraction and cDNA synthesis
Total RNA was extracted using Trizol, LS (Invitrogen, USA). The RNA quality was assessed by spectrophotometric method (A 260 /A 280 ). RNA samples were stored at −80°C until used. Complementary DNA (cDNA) was synthesized from 1.0 μg total RNA using RT-PCR Kit (Promega, USA) in a final volume of 20 μl using random primers according to the manufacturer's instructions.

Quantitative real-time PCR (Q-PCR)
Q-PCR was carried out in IQ4 real time PCR (BioRad, USA). The reaction mixture consisted of 1X GoTaq qPCR Master Mix (12.5 μl) (Promega, USA), 2.5 μl primers and 1.0 μl of cDNA in a total volume of 25 μl. VEGF and HIF-1α QuantiTect Sybr green primers were purchased from Qiagen, Germany. GAPDH was used as internal reference control. GAPDH primers (Invitrogen, USA) sequences used in this study were as previously mentioned [29]. The PCR condition for GAPDH, VEGF and HIF-1α comprised of first incubation at 95°C for 15 min, 40 cycles of denaturation at 95°C for 15 sec, annealing at 55°C for 30 sec, extension at 72°C for 30 sec. Fluorescence was recorded at the end of extension. A negative control without cDNA template was run simultaneously with every assay. To generate a standard curve, template cDNA from untreated-control MCF 7 cells was used. Quantification of gene expression was calculated by the standard curve and cycle threshold of each sample. The results of genes expression were normalized to reference gene expression and the fold exchange was determined in comparing with untreated cell control. Two replicates of this experiment were carried out, in which every gene had a duplicated reading. A melt curve analysis was done after QPCR to ensure the specificity of PCR product.
Determination of VEGF protein level MCF 7 cells were seeded in a 96-well plate at a density of 1 × 10 5 cells/well and incubated overnight. Cells were cultured in a serum free medium for 2 h and then replaced with 10% FBS medium in presence of various doses of plant extracts at 100, 200, 300 μg/mL concentrations for 48 h under normoxic and hypoxic conditions. control wells were treated with DMSO Hypoxic condition were performed by incubating the cells in GasPak Pouch (Becton Dickinson, Sparks, Md., USA). Each concentration was prepared in triplicates. The negative control used was DMSO, with the same concentrations of the extracts. Media from each well was collected and stored at −20°C until tested. VEGF concentrations in the conditioned media were quantified by Quantikine Human VEGF ELISA kit (R&D Systems, Minneapolis, USA) according to the manufacturer's protocol. MTT assay was used for correcting the amount of VEGF produced to the number of viable cells.

Statistical analysis
Results were presented as means ± SD. The differences between groups were compared by the one way ANOVA followed by Tukey Post-hoc test and considered significant at P < 0.05. The statistical analysis was carried out by using SSPS edition 16.0.

Rat aortic ring assay
In order to evaluate the antiangiogenic properties of the plant extracts, we performed the rat aortic ring assay at two concentrations: 50 and 100 μg/mL (Figure 1). All of the 4 Salvia ethanolic extracts exhibited high inhibitory activity when tested at 100 μg/mL; they resulted in more than 70% of the mean percent inhibition to the vehicle (P < 0.05) ( Table 1). Interestingly, at 50 μg/mL, the four extracts demonstrated different behavior. S. dominica and S. syriaca continued to show the highest inhibitory effects ( Table 1 and Figure 1). While, S. hormium failed to keep any inhibitory activity at this concentration (P > 0.05) ( Table 1 and Figure 1). S. triloba succeed in keeping its inhibitory activity and scored 77.67 ± 5.97% vessel outgrowth inhibition (P < 0.05) ( Table 1 and Figure 1).

In vitro cytotoxicity assay
To assess the cytotoxicity effects of the four Salvia extracts on normal cells, we tested the effect of those extracts at 100 μg/mL on the proliferation of periodontal ligament fibroblasts cells (PLF) in culture. As indicated in Table 1, S. dominica and S. syriaca exhibited clear cytotoxic effects by reducing the cells viability to less than 25% (P < 0.05). On the other hand, S. triloba and S. hormium showed no or negligible inhibitory effect on PLF cell proliferation (P > 0.05).

Antiproliferative activity against HUVECs
In order to confirm the direct antiangiogenic activity which is demonstrated in the rat aortic assay, the effects of the non-toxic extracts on PLF cells on two of HUVEC functions (proliferation and migration) were evaluated. In HUVEC proliferation assay, S. triloba and S. hormium exhibited IC 50 of 90.0 ± 0.4 and 121.0 ± 3.5 μg/mL, respectively. The antiproliferative effect of these plant extracts on HUVECs did not result from a cytotoxic effect, because 90, 111% of the endothelial cells were alive at 50 μg/mL concentration after 72 h treatment, respectively.

In vivo CAM assay
In vivo antiangiogenic effect of S. triloba and S. hormium were also tested using CAM assay as an in vivo model at a dose of 100 μg/mL. As shown in Figure 3, a clear inhibitory activity for the S. triloba extract with 49.1 ± 4.1% (P = 0.001) inhibition was observed, while S. hormium extract showed insignificant inhibition 20 ± 5.3% (P >0.005).

Q-PCR for VEGF and HIF-1α expression after S. triloba treatment
Two steps RT-QPCR were used to evaluate VEGF and HIF-1α mRNA expression in MCF 7 cells after the treatment with S. triloba extract. As shown in Figure 4, the S. triloba extract showed a significant down-regulatory effect on the expression of HIF-1α mRNA at the 3 concentrations (100 μg/mL, 200 μg/mL and 300 μg/mL) under normoxic and at 200 and 300 μg/mL under hypoxic conditions (P < 0.05). This inhibitory activity reached the maximum at the 300 μg/mL (P = 0.00), where the HIF-1α mRNA expressions were down-regulated approximately 4 and 2.5 fold at the normoxic and hypoxic conditions, respectively. On the VEGF side, the inhibition of the expression was only observed at the 300 μg/mL under both the normoxic and the hypoxic conditions (P < 0.05).

Thin layer chromatography (TLC) of the extracts
All four plants showed the presence of terpenoids and flavonoids. Using preparative TLC techniques and in   comparison with the reference substances, the main volatile oils components identified were alpha terpineol and 1,8-cineol and the major flavonoid traced was quercetin.

Discussion
Angiogenesis is an essential step in solid tumour development, invasion, and metastasis. The antiangiogenesis strategy has been postulated for prevention and treatment of breast cancers [30]. There are two accepted ways to modulate angiogenesis, namely direct and indirect pathways. The direct way depends on modulating the vascular endothelial cells ability to proliferate, migrate and respond to angiogenic proteins such as VEGF. The indirect way is based on the ability to alter the expression as well as to change the activity of angiogenic proteins that activate angiogenesis. This also includes regulating the expression of the receptors on endothelial cells [31].
In the present study, the angiogenic activity of the crude ethanol extracts of four Salvia species grown in Jordan (S. dominica, S. syriaca, S. triloba and S. hormium) has been investigated.
Starting from the direct angiogenic findings, all four extracts have significantly inhibited the formation of new blood vessels in the rat aortic assay at 100 μg/mL. Interestingly, the reduction in the concentration to 50 μg/mL for the four extracts revealed different behavior. S. dominica, S. syriaca, S. triloba extracts continued to show a significant inhibitory activity (P < 0.05), while S. hormium failed to show any inhibitory activity (P > 0.05). To test whether this activity is a selective antiangiogenic or a result of a direct cytotoxic activity, the anti-PLF proliferative test at 100 μg/mL was performed. The results indicated that S. dominica and S. syriaca have significant cytotoxic effects (P = 0.000). These observations clearly point out that the strong inhibitory activity of S. dominica and S. syriaca belongs to their strong cytotoxic effects rather than their selective antiangiogenic actions. Based on these findings, these two extracts were excluded from further experiments and emphasis was given on the non-toxic extracts, S. triloba and S. hormium.
The direct antiangiogenic activity of the two extracts of S. triloba and S. hormium were tested further on two HUVEC functions, namely: endothelial cell proliferation and endothelial cell migration. These two assays represent two major steps in angiogenesis process. The anti-HUVEC proliferation results showed that the IC 50 value of S. triloba and S. hormium are 90 ± 0.36 and 121 ± 3.47 μg/mL, respectively. The obtained IC 50 indicated that the two extracts do possess a direct anti-proliferation activity against the HUVECs. The values also point out that the two extracts do not have a direct cytotoxic activity against HUVECs as the two IC 50 values are far from the 20 μg/mL; the IC 50 that has been chosen as an indication of a direct toxic activity of the plant extracts [32]. Interestingly, the results of migration assay of both extracts illustrated that S. triloba inhibits significantly HUVEC migration in concentration-dependent manner, while S. hormium showed significant inhibitory activity only at the highest concentrations (P = 0.000). The final step in the direct angiogenesis investigation was to test for antiangiogenic activity in vivo. The vascularization in chick embryo was chosen as an in vivo model. Again, the highly significant ability of inhibiting the formation of new blood vessels by S. triloba were obvious (P = 0.001), the finding that enforced the in vitro observation and voted for the high potential of S. triloba as inhibitor of many crucial steps of the angiogenesis process.
As to the indirect angiogenic activity, the investigation was limited to S. triloba, where we assessed the effect of ethanolic extracts of S. triloba on VEGF and HIF-1α mRNA and VEGF protein expression under normoxic and hypoxic conditions. The protein expression measurement was limited on the VEGF because it is the principle mediator of tumour angiogenesis [33]. The mRNA and protein expression measurements were conducted at two conditions, the normoxic and hypoxic conditions. The hypoxic environment was adapted to resemble the in vivo tumour conditions, in which the VEGF expression is known to be elevated [34,35]. Interestingly, S. triloba demonstrated a significant inhibitory activity on expression of the VEGF and HIF-1 α mRNA, and also on the protein expression of VEGF under normoxic and hypoxic conditions (P < 0.05). Interestingly, in comparison with normoxic condition, the hypoxic condition up-regulate the VEGF protein expression 1.5 times, and S. triloba illustrated a high potency in reversing this over-expression. Combining these indirect angiogenic findings with the fact that VEGF is one of the major HIF-1 targeted genes, specifically in recruiting the endothelial cells into hypoxic and vascular areas does point that the alteration in expression the of VEGF mRNA and protein by S. triloba may resulted from modulating the HIF-1 expression [10].
Taken the direct and indirect antiangiogenic investigations on crude ethanol extracts of four Salvia species, S. triloba can be nominated as a potent antiangiogenic plant that may have chemotherapeutic and/or chemoprevention potentials. Chemoprevention potentials are summarized by its direct antiangiogenic ability via the inhibition of the endothelial cell proliferation and its indirect antiangiogenic ability through inhibiting the VEGF expression. Since VEGF ligand may affect tumour vasculature in early tumour development through the recruitment of bonemarrow-derived progenitor cells that form the building blocks of a new vascular network [35], it is tempting to speculate that the antiangiogenic mechanisms described here might contribute to its angiopreventive effect. VEGF also work throughout tumour development, in which it helps existing vasculature survive, hence permitting tumours to sustain their requirements over their entire life cycle. Furthermore, the chemotherapeutic potential of S. triloba was noticed through significant inhibitory activity of this plant against HIF-1α mRNA expression, which is a master transcription factor related to cell proliferation/ survival and resistance to chemotherapy and radiation [34]. Importantly, HIF-1α antisense therapy demonstrated a synergistic anti-tumour effect with immunotherapy [36]. Moreover, the angioprevention activity can also be speculated building on the significant inhibitory activity of S. triloba against HIF-1α mRNA expression. HIF-1α is one of the most important transcription factors that operate to sense environmental clues that drives angiogenesis [13]. Importantly, Hao et al. (2011) showed that RNAi targeting HIF-1α is effectively inhibiting the progression of oral squamous cell carcinoma and concluded that it may be used as a potent and specific therapy for oral cancer, especially in inhibiting and preventing cancer cell angiogenesis and survival [37].
On the other hand, the chemoprevention values perhaps will be more convincing by knowing that this plant is very popular in the Middle East, especially in the Arabic countries such as Jordan and Palestine [38,39], where people consume S. triloba on daily basis, either by drinking it alone or using it as a flavoring agent to black tea. Further studies are needed to include S. triloba to the list of dietary phytochemicals for which chemopreventive activities by interfering with multiple signaling pathways aberrant in cancer have been demonstrated [40][41][42][43].

Conclusion
Out of the four crude ethanol extracts of four Salvia species grown in Jordan (S. dominica, S. syriaca, S. triloba and S. hormium). S. triloba has shown a potent direct and indirect antiangiogenic activity that may have chemotherapeutic and/or chemoprevention potentials. The direct antiangiogenic activity were proven using the rat aortic assay, The anti-HUVEC proliferation, migration assay and CAM assay. The indirect antiangiogenic activity were proven through assessing the effect on VEGF and HIF-1α mRNA and VEGF protein expression under normoxic and hypoxic conditions.