Phytochemical Profiling, In Vitro Biological Activities, and In-Silico Studies of Ficus vasta Forssk.: An Unexplored Plant

Ficus vasta Forssk. (Moraceae family) is an important medicinal plant that has not been previously investigated for its phytochemical and biological potential. Phytochemical screening, total bioactive content, and GCMS analysis were used to determine its phytoconstituents profile. Antioxidant, antibacterial, antifungal, anti-viral, cytotoxicity, thrombolytic, and enzyme inhibition activities were examined for biological evaluation. The plant extract exhibited the maximum total phenolic (89.47 ± 3.21 mg GAE/g) and total flavonoid contents (129.2 ± 4.14 mg QE/g), which may be related to the higher antioxidant potential of the extract. The extract showed strong α-amylase (IC50 5 ± 0.21 µg/mL) and α-glucosidase inhibition activity (IC50 5 ± 0.32 µg/mL). Significant results were observed in the case of antibacterial, antifungal, and anti-viral activities. The F. vasta extract inhibited the growth of HepG2 cells in a dose-dependent manner. The GCMS analysis of the extract provided the preliminary identification of 28 phytocompounds. In addition, the compounds identified by GCMS were subjected to in silico molecular docking analysis in order to identify any interactions between the compounds and enzymes (α-amylase and α-glucosidase). After that, the best-docked compounds were subjected to ADMET studies which provide information on pharmacokinetics, drug-likeness, physicochemical properties, and toxicity. The present study highlighted that the ethanol extract of F. vasta has antidiabetic, antimicrobial, anti-viral, and anti-cancer potentials that can be further explored for novel drug development.


Introduction
Medicinal plants have played a major role as source of lead compounds that may be used for a variety of medicinal and pharmacological activities [1]. These plants are commonly used to treat various diseases including asthma, diabetes, respiratory, gastrointestinal diseases, skin disorders, urinary, cardiovascular, and hepatic diseases [2]. Recently, due to the wide variety of secondary metabolites identified in medicinal plants, there has been a greater focus on research which can help to obtain lead compounds from medicinal plants [3]. Some countries have started botanical drug research projects to investigate phyto-pharmaceuticals due to the enormous therapeutic potential of plants [4]. Diabetes is a metabolic disease that is caused by hyperglycemia due to the deficiency of insulin secretion or insulin action (or both in some cases) [5]. As the incidence of diabetes continues to rise, there is an increasing interest in plants with strong antidiabetic properties. These plants could provide a breakthrough in the fight against this disease [6]. There are many mechanisms by which antidiabetic drugs can help to regulate blood sugar levels. These include suppressing hepatic glucose production, improving the sensitivity of insulin receptors, stimulating insulin secretion, and increasing peripheral glucose uptake. In addition, antidiabetic drugs can also delay digestion and absorption of carbohydrates from the gut, helping to control post-meal blood sugar levels [7]. Recent research suggests that α-amylase and α-glucosidase inhibitors help to control blood sugar levels post-meal by delaying digestion [5]. α-Glucosidase and α-amylase inhibitors such as acarbose and miglitol inhibited the absorption of carbohydrates from the intestine [8]. The traditional medicinal plants are rich source of chemical constituents and phytotherapeutic preparations for the development of antidiabetic drugs [9].
Liver cancer is the second main cause of death globally [10]. Hepatocellular carcinoma causes around 90% of all primary liver cancers [11], and chemotherapy, radiation treatment, or both may be used to treat advanced liver cancer [12]. Many studies have shown that medicinal plants have compounds that can slow cancer progression [13]. Antioxidants are compounds that act as scavengers of free radicals created by the body's cells due to various metabolic reactions and external factors. These free radicals are unstable and one of the most common causes of cancer in the human body, they cause serious damage to the proteins, lipids, DNA, and RNA [12].
Infectious diseases are a main cause of death and illness in developing countries. They are a serious public health problem that can have a devastating impact on communities [14]. There are different types of pathogenic microbes that can cause illness, including fungi, bacteria, parasites, and viruses [15]. Scientists have been prompted to seek for novel compounds with antimicrobial activity from a wide range of sources, including medicinal plants, as a result of the increase cases of multidrug-resistant (MDR) infections [16]. Plant polyphenols are known to have medicinal qualities, including antibacterial, antifungal, and anti-viral activities. This is due to the fact they can induce damage to the bacterial cell membrane, either structurally or functionally. Different studies have revealed that polyphenol-rich plants have antioxidant and antibacterial activities [17]. To effectively combat fungal illnesses, new antifungals must be developed. In this regard, interest in alternative medicinal approaches is expanding, and the use of plant extracts as antimicrobial adjuvants has gotten much attention in recent years [18]. Polyphenols are a promising area in research for developing anti-viral medications. They work in various ways, including preventing virus entrance or affecting virus replication. Polyphenols are widely available and relatively inexpensive to produce, making them an attractive option for medication development [19].
Ficus is a genus that belongs to the Moraceae family of woody trees, shrubs, and vines that includes roughly 800 species and 2000 variations. Ficus plants have long been used in traditional medicine for their wide range of therapeutic properties. Recent studies have revealed that these plants possess various biological activities, including antioxidant, anti-inflammatory, anti-cancer, antidiabetic, anti-tumor, antiproliferative, antimicrobial, antihelminthic, and hepatoprotective effects [20]. These properties make Ficus a promising natural therapy for many different diseases and conditions. Ficus vasta Forssk. is a large tree that can grow over 25 m tall. Its leaves are alternate and spirally arranged with an uneven texture. They are almost circular in shape, with an entire margin and a rounded tip, though often with a blunt point. The leaves are usually glabrescent above and below, puberulous or hirsute [21]. These are widespread in dry, arid regions of Africa, such as Sudan, Uganda, Saudi Arabia, Tanzania, and Ethiopia. The leaves and bark can be used to prepare a poultice for tumors [22]. The leaves of F. vasta are traditionally used to treat rheumatic diseases, intestinal worms, and muscle pains. Preliminary phytochemical analysis showed that it consists of carbohydrates, flavonoids, tannins, coumarins, and triterpenes [23]. Some phytochemical constituents such as beta-sitosterol, lupeol, stigmasterol, and ursolic acid were isolated and identified from the ariel part of this plant [24]. Moreover, antioxidant and antibacterial activities are investigated in a hydro-methanolic extract of F. vasta leaves [25].
The literature review regarding F. vasta demonstrated that there are only few data in terms of phytochemical investigations and biological activities as compared to the other members of the genus Ficus. Therefore, the goal of this research was to explore the aerial parts of F. vasta for its phytochemical and biological activities. The therapeutic potential of F. vasta was assessed for the first time through its antioxidant, antibacterial, antifungal, anti-viral, cytotoxicity, and enzyme inhibitory activities. GCMS was used to identify the phytocompounds responsible for these activities. The major phytocompounds identified by GCMS in the ethanolic extract were further studied for in silico studies.

Total Bioactive Contents
The results of the total phenolic and flavonoid content of F. vasta are shown in Table 2. The TPC and TFC of F. vasta extract was carried out with the help of regression equation that was obtained from gallic acid and quercetin standard curve. The ethanolic extract of aerial parts of F. vasta showed total phenolic content of 89.47 ± 3.21mg GAE/g and total flavonoid contents of 129.2 ± 4.14mg QE/g.

Antioxidant Activities
In this study, the antioxidant activity of F. vasta extract was examined by the DPPH, ABTS, FRAP, and CUPRAC, and the results are shown in Table 2. In the case of radical scavenging activities, the DPPH result suggested that the ethanolic extract of aerial parts of F. vasta exhibited the highest activity with IC 50 1.75 mg/mL. In comparison, the ABTS result showed the activity with IC 50 1.63 mg/mL. According to the reducing power assays, the FRAP and CUPRAC results showed the highest activity with IC 50, i.e., 1.91 mg/mL, and 1.51 mg/mL, respectively. The results of FRAP and DPPH activities of the extract suggested a direct correlation with the polyphenol content.

Enzyme Inhibition Activities
This study used acarbose as a positive control to determine the enzyme inhibition activity. The α-glucosidase activity result showed that ethanolic extract of F. vasta exhibits the excellent α-glucosidase inhibitory effect with IC 50 5 ± 0.32 µg/mL compared to the standard acarbose with IC 50 2.59 ± 0.11 µg/mL. At the same time, the result of α-amylase activity showed that ethanolic extract of F. vasta showed an excellent α-amylase inhibitory effect with IC 50 5 ± 0.21 µg/mL compared to the standard acarbose with IC 50 41.10 ± 3.21 µg/mL. The results of α-glucosidase and α-amylase inhibition activities were shown in Figure 2.  standard acarbose with IC50 2.59 ± 0.11 µg/mL. At the same time, the result of α-amylase activity showed that ethanolic extract of F. vasta showed an excellent α-amylase inhibitory effect with IC50 5 ± 0.21 µg/mL compared to the standard acarbose with IC50 41.10 ± 3.21 µg/mL. The results of α-glucosidase and α-amylase inhibition activities were shown in Figure 2.

Antibacterial Activity
The antibacterial potential of F. vasta was evaluated using the agar well diffusion method against five positive strains include Bacillus subtilis, Bacillus pumilus, Staphylococcus epidermidis, Staphylococcus aureus, Micrococcus luteus, and two negative strains including Escherichia coli, and Bordetella bronchiseptica and results are shown in Table 4 and Figure  S3. This antibacterial potential was revealed by inhibition of growth of bacteria which was

Antibacterial Activity
The antibacterial potential of F. vasta was evaluated using the agar well diffusion method against five positive strains include Bacillus subtilis, Bacillus pumilus, Staphylococcus epidermidis, Staphylococcus aureus, Micrococcus luteus, and two negative strains including Escherichia coli, and Bordetella bronchiseptica and results are shown in Table 4 and Figure S3. This antibacterial potential was revealed by inhibition of growth of bacteria which was measeured as zone of inhibition. The results showed that plant extract has a dose-dependent effect on bacteria. Its activity against the bacteria is lowest at low concentrations (25 mg/mL). However, antibacterial activity was observed to be higher for S. aureus and E. coli, with 22 mm and 24 mm zones of inhibition, respectively, at a concentration of 100 mg/mL.  Table 5 presented the antifungal activity of F. vasta extract. The results of this activity showed the maximum antifungal activity of extract was observed against fungal strain F. avenaceum (54.94%) followed by F. brachygibbosum (48.51%) and A. niger (42%).

Anti-Viral Activity
The anti-viral potential against three strains (i.e., avian infectious bronchitis virus (IBV), influenza virus (H9), and Newcastle disease virus (NDV)) was carried out using a haemagglution test method, and the results are tabulated in Table 6. The ethanolic extract of F. vasta was more active against the avian infectious bronchitis virus and Newcastle disease virus (IBV and NDV titer 0) while less effective against the influenza virus and its H9 titer was 16.

Thrombolytic Activity
The results of thrombolytic activity of F. vasta and Streptokinase are described in Figure 3. The percentage clot lysis of ethanolic extract of F. vasta was 47.78 ± 4.21% while streptokinase showed 81.86 ± 6.37% clot lysis. The results of thrombolytic activity of F. vasta and Streptokinase are described in Figure  3. The percentage clot lysis of ethanolic extract of F. vasta was 47.78 ± 4.21% while streptokinase showed 81.86 ± 6.37% clot lysis.

Hemolytic Activity
Data shown in (Table 7) represented the hemolytic activity of ethanolic extract of F. vasta. The hemolytic % value of extract was 6.39 ± 0.45% while the value of standard was 92.27 ± 4.71%. The hemolysis activity of extract was less than 30%, so extract is nontoxic and safe as food. The hemolysis activity can be performed using a wide range of methods, which is one of its major challenges and limitations. This produces a wide range of absolute values in addition to complicates comparisons between studies [57]. Table 7. Hemolytic activity of F.vasta and standard Triton X-100.

Hemolytic Activity
Data shown in (Table 7) represented the hemolytic activity of ethanolic extract of F. vasta. The hemolytic % value of extract was 6.39 ± 0.45% while the value of standard was 92.27 ± 4.71%. The hemolysis activity of extract was less than 30%, so extract is nontoxic and safe as food. The hemolysis activity can be performed using a wide range of methods, Antibiotics 2022, 11, 1155 9 of 26 which is one of its major challenges and limitations. This produces a wide range of absolute values in addition to complicates comparisons between studies [57]. MTT activity was used to evaluate the effect of F. vasta extract on HepG2 cell growth. Treatment with F. vasta extract for 48 h inhibited the growth of cells in a dose-dependent manner. The IC 50 value for this assay was 0.563 µg/mL. The outcomes of the activity are represented in Figure 4.

Molecular Docking
Molecular docking studies were conducted against all compounds that were identified by the GCMS for both α-glucosidase and α-amylase. The docking results suggested that the binding affinity of 7 compounds was higher than the binding affinity of acarbose (standard) in α-glucosidase and α-amylase. Ursa-9(11),12-dien-3-ol was the most active of all of the tested compounds, with a binding affinity of −10.5, which interacted in the active site of α-amylase by forming one H-bond interaction with ASP 197 amino acid residue at a bond distance of 2.87 angstroms. From the 2D structures of ligands with α-amylase, it was clear that beta-amyrin, Campesterol, beta-Sitosterol, and Stigmasterol showed Hbond interactions. In contrast, Olean-12-en-3-ol, acetate, (3beta)-and 11-Oxours-12-en-3yl acetate did not show any H-bond interactions. The docking results of α-glucosidase showed that beta-amyrin exhibit the highest binding affinity of −8.4 by making H-bond interaction with GLU 113 amino acid residue with a bond distance of 2.78 angstroms. Olean-12-en-3-ol, acetate, (3beta)-, Stigmasterol, Campesterol, and beta-Sitosterol also showed H-bond interactions with binding affinity -8.1, -7.5, -6.9, and -6.9 respectively while Ursa-9(11),12-dien-3-ol and 11-Oxours-12-en-3-yl acetate didn't show any H-bond interactions. This demonstrates F. vasta's ability to inhibit α-glucosidase and α-amylase. Figures 5, 6 and S4, and Table 8 illustrate the docking results of the compounds with both receptors. The docking study was validated by superimposing the co-crystallized ligand (Acarbose) with extracted Acarbose and redocked to α-amylase (PDB: 1b2y) crystal structure and a low RMSD of 1.525 Å was observed. Similarly, an RMSD of 1.234 Å was observed with α-glucosidase (pdb id: 3TOP). The co-crystallized Acarbose (Yellow) and extracted Acarbose (Red) are shown in Figure S5.

Molecular Docking
Molecular docking studies were conducted against all compounds that were identified by the GCMS for both α-glucosidase and α-amylase. The docking results suggested that the binding affinity of 7 compounds was higher than the binding affinity of acarbose (standard) in α-glucosidase and α-amylase. Ursa-9(11),12-dien-3-ol was the most active of all of the tested compounds, with a binding affinity of −10.5, which interacted in the active site of α-amylase by forming one H-bond interaction with ASP 197 amino acid residue at a bond distance of 2.87 angstroms. From the 2D structures of ligands with α-amylase, it was clear that beta-amyrin, Campesterol, beta-Sitosterol, and Stigmasterol showed Hbond interactions. In contrast, Olean-12-en-3-ol, acetate, (3beta)-and 11-Oxours-12-en-3-yl acetate did not show any H-bond interactions. The docking results of α-glucosidase showed that beta-amyrin exhibit the highest binding affinity of −8.4 by making H-bond interaction with GLU 113 amino acid residue with a bond distance of 2.78 angstroms. Olean-12-en-3ol, acetate, (3beta)-, Stigmasterol, Campesterol, and beta-Sitosterol also showed H-bond interactions with binding affinity -8.1, -7.5, -6.9, and -6.9 respectively while Ursa-9(11),12dien-3-ol and 11-Oxours-12-en-3-yl acetate didn't show any H-bond interactions. This demonstrates F. vasta's ability to inhibit α-glucosidase and α-amylase. Figures 5, 6 and S4, and Table 8 illustrate the docking results of the compounds with both receptors. The docking study was validated by superimposing the co-crystallized ligand (Acarbose) with extracted Acarbose and redocked to α-amylase (PDB: 1b2y) crystal structure and a low RMSD of 1.525 Å was observed. Similarly, an RMSD of 1.234 Å was observed with αglucosidase (pdb id: 3TOP). The co-crystallized Acarbose (Yellow) and extracted Acarbose (Red) are shown in Figure

ADMET Analysis
The most promising docked compounds were further investigated by the SwissADME online tool, which provides information on pharmacokinetics, drug-likeness, and physicochemical properties. According to Lipinski's rule, all compounds violated the rule of lipophilicity while Olean-12-en-3-ol, acetate, (3beta)-and Stigmasterol violated the rule of molar refractivity. When a drug fails to meet two or more criteria, it is classified as a non-orally available drug. However, all of the compounds had one violation, indicating that they are orally available or bioavailable drugs. According to Lipinski's criteria, all of the compounds exhibited orally active likeness characteristics. All of the compounds had no Blood-brain barrier penetration and lowed GI absorption. However, this study does not determine whether a compound has a specific biological effect. Table 9 presents the properties of the best seven best-docked compounds, such as molecular weight, no. of hydrogen bond acceptor and doner, no. of rotateable bond, Lipinski rule, and lipophilicity, while Figure 7 presents the bioavailability radar of best-docked compounds. Table S1 tabulates the pharmacokinetic properties of best-docked compounds. Olean-12-en-3-ol, acetate, (3beta)-, and 11-Oxours-12-en-3-yl acetate were predicted to have carcinogenic and immunotoxic properties in ProTox-II. In this investigation, all compounds were predicted to have minimal toxicity, except beta-Amyrin, which was predicted to be non-toxic. Table S2 presents different compounds along with their predicted toxicity class and LD50 value.

Discussion
The phytochemicals profiling showed that the extract of F. vasta is a good source of carbohydrates, alkaloids, steroids, glycosides, flavonoids, phenols, tannins, and saponins. The antioxidant, antimicrobial, antifungal, antidiabetic, anti-inflammatory, anti-cancer, and antihypertensive effects are known to exist in these recognized phytochemical classes [58]. Some classes such as alkaloids have anti-viral, antifungal, antitumor, and antimicrobial activity [59]; flavonoids, phenols, and tannins have antioxidant and anti-cancer potential [60]; and saponins have antidiabetic, antibacterial, anti-inflammatory, and anti-cancer properties [61]. These phytochemicals in F. vasta extract may play a part in its therapeutic benefits. Ficus genus is medically important due to the presence of high value of total bioactive contents (TPC and TFC) [62]. Previously, some flavonoid compounds were identified in leaves of F. vasta [25]. The high value of total phenolic and flavonoid contents in plant extract correlates with the strong antioxidant activities [63].
According to the literature, the antioxidant activity of the ethanolic extract in aerial parts of F. vasta has not been reported, while the methanol extract of F. vasta leaves showed the antioxidant activity [25]. The results of the DPPH, ABTS, FRAP, and CUPRAC activities showed that there is a direct link of antioxidant activities and the polyphenol contents (i.e., high value of phenolic and flavonoid contents correlates with the strong antioxidant activity) [63].
The α-amylase initiates carbohydrate digestion by hydrolyzing 1,4-glycosidic bonds in polysaccharides to disaccharides, which is followed by α-glucosidase catalyzing the disaccharides to monosaccharides, resulting in postprandial hyperglycemia [64,65]. As a result, α-amylase and α-glucosidase inhibitors can control hyperglycemia by delaying carbohydrate digestion and lowering postprandial plasma glucose levels [66]. There is no data in the literature about the in vitro antidiabetic studies of F. vasta. Our results showed that ethanolic extract of Ficus vasta exhibits excellent α-glucosidase and α-amylase inhibitory effects. Such significant inhibition of α-amylase and α-glucosidase may be due to the presence of some phytocompounds which were identified by GCMS profiling, such as Ursa-9(11),12-dien-3-ol and beta-Amyrin which showed significant binding affinities with these enzymes, and due to presence of some other compounds in the extract. This suggests the potential of F. vasta for the management of diabeties.
The antibacterial ability of F. vasta was tested against five gram-positive strains and two gram-negative strains. Most of the bacteria employed in the assay showed a significant zone of inhibition (>9 mm) in the results. The antifungal ability of F. vasta was tested against three strains, including Aspergillus niger, Fusarium avenaceum, and Fusarium brachygibbosum. Most of the fungi employed in the test showed a significant zone of inhibition in the results. The anti-viral potential against three strains (i.e., avian infectious bronchitis virus (IBV), Influenza virus (H9), and Newcastle disease virus (NDV)) was carried out using a haemagglution test method. The ethanolic extract of F. vasta was effective and strongly active against the viral strains. The presence of phytochemical components such as alkaloids, phenolic and flavonoid compounds could be responsible for the antimicrobial activities [67]. Tentative identification of the ethanolic extract by GCMS revealed many compounds with antibacterial, antifungal, and antiviral activities, namely Methyl (Z)-5,11,14,17-eicosatetraenoate [4,8], Octadecanoic acid [45], 4-((1E)-3-Hydroxy-1-propenyl)-2-methoxyphenol [34], Nonanoic acid [31], Catechol [27], and Stigmasterol, 22,23-dihydro [54] etc. Methanolic extract obtained from leaves of F. vasta previously tested against E. coli, Pseudomonas aeruginosa, Streptococcus pneumonia, Salmonella typhimurium, and Staphylococcus epidermidis [25,68].
To the best of our knowledge, there is no information in the literature about the ethanolic extract of F. vasta thrombolytic activity. Plants containing flavonoids and polyphenols have been reported to possess thrombolytic activity and hence attracted researchers to explore more for better and safer drugs of plant origin [69]. The thrombolytic activity of F. vasta was significant. Microbial plasminogen activators such as staphylokinase and streptokinase function as co-factoring molecules to promote development [70].
Hemolysis is the breakdown or disruption of the integrity of the RBC membrane, which causes hemoglobin to be released from red blood cells [71]. Some traditional plants sometimes become harmful if used over an extended period. There are chemical elements in many plants that may have an anti-hemolytic or hemolytic effect on human erythrocytes. Plant extracts can disrupt red blood cell membranes, leading to serious side effects such hemolytic anemia [72]. Therefore, it is important to evaluate the possible hemolytic activity of a number of the frequently used herbs. When there is more than 30% hemolysis, the plant extracts are thought to be harmful to erythrocytes [73]. Table 7 displays the hemolytic activity of aerial parts of the entire F. vasta plant. Plant hemolysis was measured as a percentage of hemolysis. The results showed that extract had the hemolytic activity (6.39 ± 0.45%). Since the hemolysis activity of extract is less than 30%, they are all nontoxic and safe for human utilization. This is the first time that the F. vasta plant's hemolytic activity has been reported.
MTT activity was used to evaluate the effect of F. vasta extract on HepG2 cell growth. Treatment with F. vasta extract for 48 h inhibited the growth of cells in a dose-dependent manner. Our results found that F. vasta is rich in antioxidants which can act as scavengers for free radicals created by the body's cells as a result of a variety of metabolic reactions and external influences. These antioxidants are useful to cells since they help to prevent the growth of cancer [12].
In recent years, computer-based modeling techniques have been increasingly used to predict the interactions between small molecules and their biological targets. This approach can provide useful insights into the molecular basis of the biological activity of natural products and the possible mechanisms of action and binding modes of active compounds [74]. To understand the ability of the compounds to inhibit enzymes and to find a correlation between the in vitro enzyme inhibition results, all compounds from the GCMS analysis of ethanolic extract were docked against α-amylase and α-glucosidase enzymes, along with acarbose. According to the validation criteria, RMSD values less than 2.0 Å demonstrate that the docking protocol is capable of accurately predicting the cocrystallized ligand's binding orientation [75]. The hydrogen bond and other hydrophobic interactions, such as alkyl and pi-alkyl, plays an important protein-ligand interactions as well as ensuring the stable binding of ligands with proteins [76].
For further investigation, the best docked compounds were studied using online tool SwissADME which gave information about their pharmacokinetics, drug likeness, and physiochemical properties [77]. According to Lipinski, a chemical can exhibit drug-like behaviour if it meets all of the following criteria: (i) Molecular weight (<500); (ii) Hydrogen bond donor (≤5); (iii) hydrogen bond acceptor (less than and equal to 10); (iv) Lipophilicity (Log Po/w, <5); and (v) molar refractivity 40 to 130. Those compounds which followed the Lipinski rule were considered potential therapeutic candidates [78]. When a drug fails to meet two or more of Lipinski's criteria, it is classified as non-orally available drug. However, all of the compounds had 1 violation, indicating that they are bioavailable or orally available drugs. According to Lipinski's criteria, all of the best docked compounds exhibited orally active likeness characteristics. Compounds with lower lipophilicity, molecular weight, and hydrogen bond capacity are said to have good absorption, high permeability, and bioavailability [79,80]. All of the compounds had no blood-brain barrier penetration and low GI absorption. However, this study does not determine whether a compound has a specific biological effect. The colors in the bioavailability radar of best docked compounds represent the best physico-chemical space indicator for oral bioavailability, taking into account factors such as lipophilicity, saturation, size, flexibility, polarity, and solubility.
LogP is a measure of lipophilicity, can range from −0.7 to +5.0, molecular weight can range from 150 to 500 (g/mol). The TPSA, which is a measure of the size and polarity of a molecule, ranges from 20 to 130 A 2 . The logS (ESOL) insolubility, which measures the solubility of a molecule, ranges from 0 to 6. The number of rotatable bonds for a molecule is between 0 to 9, with an unsaturation fraction between 0.25 and 1.0. This indicates that the carbon atom fraction in sp3 hybridization cannot be less than 0.25 [81]. ProTox-II is a program that predicts toxicity based on the similarity of chemical structures and then compares them to other chemicals with known toxicities [82]. In silico toxicity analysis of seven phytocompounds showed that they all have low toxicity potential. However, beta-Amyrin was predicted to be non-toxic.
Overall, Ursa-9(11),12-dien-3-ol, Olean-12-en-3-ol, acetate, (3beta)-, beta-Amyrin, 11-Oxours-12-en-3-yl acetate, Campesterol, beta-Sitosterol, and Stigmasterol may have some potentials as inhibitors of important proteins (α-glucosidase and α-amylase) and might have contributed either singly or in synergy to the antidiabetic properties of F. vasta. However, further research is needed to explore the pharmacokinetic properties of these compounds and whether or not they are effective in both in vitro and in vivo models.

Materials and Reagents
Chemicals used in the study were of analytical grade purchased from Sigma Aldrich, Louis, MO 63103, USA. All of the standards were also purchased from Sigma.

Collection and Extraction of Plant
The aerial parts of F. vasta were collected in September 2020 from Jazan province, Fayfa Mountains, Saudi Arabia. A botanist identified the plant at the Science College, King Saud University, Saudi Arabia. A Voucher specimen No. 24557 was submitted to the herbarium of the Science College, King Saud University. The plant was air-dried and then subjected to crushing and grinding to form a coarse powder. Air-dried plant was macerated with 80% ethanol for 15 days. After maceration, it was filtered and then concentrated (40 • C) using a rotary evaporator (Heidolph, Germany), yielding a dark brown residue and further air dried to yield 98.5 g extract.

Total bioactive contents (TPC and TFC) TPC
The Folin-Ciocalteu method was used to determine the total phenolic content (TPC) as previously reported in the literature [84]. Different concentrations of Gallic acid (0.05-0.5 mg/mL) were used as a standard to establish a standard calibration curve ( Figure S1). The sample solution was prepared as 0.5 mg/mL, from which an aliquot of 0.1 mL was taken in a test tube, followed by adding Folin-Ciocalteu's reagent (0.1 mL). Then, 10% Na 2 CO 3 (2.8 mL) was combined with the resultant solution, and the solution was placed for 30 min in the dark. Absorbance was read at 765nm using a BioTek Synergy HT microplate reader. TPC was expressed in milligrams of Gallic acid equivalent per gram of dry extract.

TFC
The aluminum chloride colorimetric method was used to estimate the content of flavonoids [84]. In 96 % ethanol, standard quercetin solutions of 30, 40, 50, 60, 70, 80, 90, 100 µg/mL were prepared ( Figure S2). Firstly, the 1 mg/mL solution of extract and then  50 µL extract and standard solutions were added in 10 µL of aluminium chloride (10 %) solution, and then 150 µL of ethanol (96%) was added. At last, in 96 well plates, 10 µL of sodium acetate (1M) was added to the mixture. Ethanol was used as a blank, and then all reagents were mixed, and the mixture was then incubated for 40 min at room temperature in the dark. Finally, the absorbance was measured at 415 nm using a BioTek Synergy HT microplate reader. TFC was expressed in milligrams of quercetin equivalents per gram of dry extract.

Gass Chromatography-Mass Spectroscopy Analysis
The phytometabolites of ethanolic extract of F. vasta were determined by GCMS analysis using Agilent, 6890 series, and Hewlett Packard, 5973 mass selective detector. An HP-5MS column with a length of 30m, a diameter of 250 µL, and a film thickness of 0.25 µL were used to achieve the best possible separation. The volume of 1.0 µL of the extract was diluted with the appropriate solvent and injected at 250 • C in a splitless mode. Helium gas as a carrier was used at a constant flow rate of 1.02 mL/min., the temperature was increased gradually, starting at 50-150 • C and increasing by 3 • C per min, with a 10 min holding time at each temperature. The final temperature was set to 300 • C at 10 • C/min. The components were identified using their retention indices, and the mass spectrum was interpreted using the National Institute of Standards and Technology database (NIST) [85].

Biological Activities 4.4.1. Antioxidant Activities
The antioxidant activities of F. vasta included determining the free radical scavenging and reducing power activities. Ascorbic acid was used as a standard for all antioxidant activities. The DPPH, ABTS, FRAP, and CUPRAC activities were performed according to the literature with minor modifications [86].

DPPH Assay
A solution of 0.1 mM DPPH was prepared, and 90 µL of DPPH solution was added to a 96-well plate, followed by 10 µL of the substance being tested. The mixture is then incubated for 30 min, after which the absorbance is read at 517 nm using a BioTek Synergy HT microplate reader.

ABTS Assay
ABTS activity was carried out by the modified method in which 100 µL of sample solution was mixed with 200 µL of prepared ABTS solution. This mixture was incubated for 30 min at room temperature. The absorbance was recorded at 417 nm using a BioTek Synergy HT microplate reader.

FRAP Assay
For this activity, 100 µL of F. vasta extract (1mg/mL) was mixed with 2 mL of FRAP reagent and mixture was incubated for 30 min. The absorbance was measured at 593 nm using a BioTek Synergy HT microplate reader. Similarly, the blank sample was prepared without extract.

α-Glucosidase Inhibition Assay
The method described in previous literature was followed to determine the α-glucosidase inhibitory activity [87]. In this assay acarbose was used as a standard or positive control and methanol as a negative control. The volume of 10 µL of a plant extract, 70 µL of a 0.1 molar phosphate buffer (pH 6.8), and 10 µL of α-glucosidase was added to the wells of a 96 well plate and incubated for 15 min at 30 • C. In the end, 10 µL p-Nitrophenyl-α-D-glucopyranoside solution was added for the next 30 min and absorbance was read at 405 nm using a BioTek Synergy HT microplate reader.

α-Amylase Inhibition Assay
According to the previously reported method [88], the starch iodine test method was used to evaluate the inhibitory activity of α-amylase. 25 µL of 0.02 molar sodium phosphate buffer containing 6 millimolar NaCl, 20 µL of soluble starch (concentration 1% w/v), and 20 µL of plant extract/acarbose was incubated at 37 • C for 5 min. Acarbose was used as a standard. Then 15 µL of amylase solution were placed into each well and incubated at 37 • C for the next 10 min. After that, 20 µL of 1 molar was added to stop the reaction. Then, 100 µL of iodine reagent was added. The color change was observed, and absorbance was measured at 620 nm using a BioTek Synergy HT microplate reader. The color of the mixture changes based on the presence of starch. If there is an active inhibitor, the color will be dark blue. If there is no inhibitor, the color will be yellow. If the starch is partially degraded, the color will be brownish, indicating that the inhibitor is partially active.

Antibacterial Activity Strains of Bacteria
Antibacterial activity was performed against the five positive strains, including Bacillus subtilis, Bacillus pumilus, Staphylococcus epidermidis, Staphylococcus aureus, Micrococcus luteus, and two negative strains, including Escherichia coli, and Bordetella bronchiseptica. These bacterial strains were provided by the Microbiology lab of the Islamia University of Bahawalpur.

Agar Well Diffusion
The culture of bacteria was streaked on Mueller Hinton agar plates and placed in an incubator for 24 h at 37 • C. After 24 h, the colony was picked and inoculated into the saline solution and vortexed. In the end, turbidity was set to 0.5 McFarland standards. The plant extracts were prepared in DMSO at four concentrations 25, 50, 75, and 100 mg/mL. Mueller Hinton agar plates were inoculated with various strains of bacteria. The organisms were spread evenly over the surface of the agar, and four wells (6 mm in diameter) were punched into each plate. 100 µL of sample solution was added to each well, and the plates were incubated at 37 • C for 24 h. The diameter millimeter of a zone of inhibition was measured and ceftriaxone was used as standard in the activity [89].

Antifungal Activity Fungal Strains
Antifungal activity was performed against the three strains, including Aspergillus niger, Fusarium avenaceum, and Fusarium brachygibbosum. These fungal strains were provided by the Microbiology lab of the Islamia University of Bahawalpur.

Agar Tube Dilution
Antifungal activity was performed according to the previous method with little modifications [90]. The sample solutions were prepared in DMSO at 20 and 40 mg/mL concentrations. Agar was prepared, and the sample solution was added to melted agar. Then tubes were solidified at room temperature in a slanting position. After solidification, each slant was inoculated by 4 mm diameter piece of fungal strain. Terbinafine was used as standard and DMSO as the negative control in the activity. Tubes were incubated for 3 days at 27-29 • C. The percentage inhibition was measured with the following formula: Percentage inhibition = Linear growth in test tubes (mm) Linear growth in control (mm) × 100 (1)

Inoculation of Viruses in Chicken Embryonated Eggs
The reported procedure was performed for anti-viral activity in ethanolic extract of F. vasta [91]. Chicken eggs are used for preliminary growth of the viruses and formation of novel vaccines. Eggs are considered as one of the most used media due to excellent growth of viruses. The chicken eggs are easy to collect, easy to handle, aseptic conditions, cheep, and require little space for storage making them the best resource of viral inoculations studies. The viruses accumulate in the chorioallantoic membrane fluid during incubation period of the eggs and keep replicating. Viral strains were cultured in the 7 to 11 days old embryonated poultry eggs. Pathogen-free eggs were collected from Government Poultry Farm, Model Town a, Bahawalpur. Ethyl alcohol was used to sterilize the eggs, and a sterile needle was used to make holes in the egg. Viral strains were injected through the chorioallantoic route into the embryonated eggs with the help of a syringe (5 cc). After inoculation, the hole was closed with melted wax after the inoculation. The eggs were incubated at 37 • C for 48-72 h. Melted wax was then used to close the hole. The incubation period for the inoculated eggs was 48 to 72 h at 37 • C. Titer viruses were then assessed after collecting the allantoic fluid with the syringe in the Eppendorf at 4 • C for further processing. A 96-well microtiters round bottom plate was used for performing the Haemagglutination test.

Heamagglutination (HA) Test
The first step of the Haemagglutination test is to prepare 1% red blood cells (R.B.Cs.) Alsever solution was poured into a test tube, and fresh chicken blood (5 mL) was added. Blood (5 mL) was centrifuged for 5 min at 4000 rpm, and the supernatant was removed. For better results and more purification, the process was repeated three times. In the Eppendorf tubes, 10 µL packed R.B.Cs were mixed with 1 mL phosphate buffered saline solution at pH 7.4 to prepare a 1% R.B.Cs solution. To avoid precipitation, Eppendorf tubes were shaken gently. In each microtiter plate well, PBS (50 µL) was added. The samples (50 µL) were added in the first column. The diluted upto the 11th and 12th well was left as negative control only containing PBS. After that, 1% RBCs solution (50 µL) was added to all 12 wells, and the plate was incubated for 2 to 3 h at 37 • C. The uniform red color indicated positive results; however, red dots at the bottom of the well indicate negative results. 56 Haemagglutination Titer had the highest dilution number showing positive results. The test was used for testing the titer of Avian Infectious Bronchitis Virus (IBV), Newcastle disease virus (NDV), and Influenza virus (H9).

Thrombolytic Activity
The blood samples were taken in the incubated Eppendorf tubes for 45 min at 37 • C. Serum was removed from the blood sample without damaging the blood clot, and the Eppendorf tube was weighed again. In each pre-weighed Eppendorf tube with a blood clot, 1 mg/mL (100 µL) of plant extract was added. Streptokinase was used as a standard and negative non-thrombolytic control. Eppendorf tubes containing blood samples and plant fractions were incubated at 37 • C for 90 min. After 90 min, the thrombolytic activity was observed in these Eppendorf tubes. The fluid released in the Eppendorf tubes was removed and weighed again. The weight difference of Eppendorf tubes showed the antithrombotic activity of the extract or fractions against streptokinase [92]: Percentage o f clot lysis = Wr Wc × 100 (2) where: Wr = released clot weight; Wc = clot weight 4.4.7. Hemolytic Activity The hemolytic activity was performed according to the literature with some modifications [93]. A hemolytic activity on human erythrocytes was used to determine the preliminary toxicity of phytochemical compounds from plant extract. To prepare the erythrocyte suspension, blood (type O blood from Civil Hospital, Bahawalpur) was used. The volume of 50 µL of the erythrocyte suspension (pH 7.4) and 100 µL of the extract were mixed and incubated for 1 h at 37 • C. After that, 850 µL of phosphate-buffered saline (pH 7.4) was added in already prepared mixture, then centrifuged for 3 min at 3000 rpm. The supernatant was obtained, and the absorbance at 540 nm of the hemolysis was measured by using a BioTek Synergy HT microplate reader. A total of 0.1% Triton X-100 was used as a positive control while phosphate-buffered saline was used as a negative control: Hemolysis percentage = Absorbance of sample − Absorbance of negative control Absorbance of positive control × 100

Cytotoxicity
The human HepG2 liver cancer cells were grown in the Dulbecco's Modified Eagle's Medium (DMEM), with added 10% fetal bovine serum (FBS), 100 IU/mL penicillin, and 100 µg/mL streptomycin in a 75 cm 2 flask and maintained at 37 • C with 5% CO 2 incubator. Cells were treated with extracts dissolved in DMSO (0.05% concentration).

Determination of Cell Viability
Cell viability was determined by MTT activity as described in the literature with some modifications [94]. Firstly, HepG2 cells were treated with different concentrations from 10 to 100 ug/mL of extracts for 48 h. Following treatment, each well was introduced with a 10 µL MTT reagent and further incubated for 4 h. Then 150 µL of DMSO was subsequently introduced to dissolve formazan crystals, and absorbance was read at 490 nm. The % age of cell viability was calculated: Cell viability % = Absorbance of sample − Absorbance of blank Absorbance of control − Absorbance of blank × 100 (4)

Molecular Dockings
The interaction between the bioactive compounds discovered in F. vasta ethanolic extract, α-glucosidase (PDB: 5zcb), and α-amylase (PDB: 4w93) was assessed using PyRx software. The 3D shapes of proteins were taken from the RCSB Protein Data Bank (https://www.rcsb.org/ accessed on 30 May 2022). First, the proteins were prepared for docking using the Discovery studio by removing water and ligands, inserting polar hydrogen atoms, and saving them in PDB format. Then download the ligand in SDF format from PubChem (https://pubchem.ncbi.nlm.nih.gov accessed on 30 May 2022). The Open Babel software converted the ligands to PDB files. The prepared and optimized ligands were docked blindly in the protein's grid box to allow them to find any suitable binding location [95]. The docking studies were validated by superimposing the co-crystallized ligand (Acarbose) with extracted Acarbose from crystal structure and redocked to α-amylase and α-glucosidase crystal structures. The Ligplot software was used to visualize 2D structures of ligand-protein interactions [96].

Statistical Analysis
The findings were all presented as mean standard deviation (mean ± SD). The information obtained through quantitative analysis IBMSPSS (v20, Chicago, IL, USA) was used to perform a one-way analysis of variance (ANOVA) followed by post-hoc test on the phytochemicals. Significant values were defined as p values less than 0.05.

Conclusions
The results of the present study suggest that ethanolic extract of Ficus vasta Forssk. has identified bioactive phytochemicals responsible for therapeutic and pharmacological activities. F. vasta showed the good TPC, TFC, and antioxidant potential and had a good antidiabetic potential for α-amylase and α-glucosidase inhibition. The extract exhibited the good antibacterial, antifungal, and anti-viral potentials against the strains. F. vasta extract inhibited the growth of HepG2 cells in a dose-dependent manner. The GCMS analysis of ethanol extract indicated the tentative presence of important phytocompounds, which justified their biological activities. Hence, it is concluded that in vitro analysis of F. vasta showed the plant's medicinal potential with respect to antioxidant, antidiabetic, thrombolytic, enzyme inhibition, cytotoxicity, anti-viral, antifungal, and antibacterial potential. The in silico molecular docking studies further explained the enzyme inhibition activity. Based on in vitro and in silico docking studies, further investigation is required to evaluate its toxicity profile and clinical studies. Conclusively, the findings of this research could help researchers who are struggling continuously for the development of novel and effective drugs from natural products. The observed phytochemical and biological potential of this plant indicated that it might be valuable for further isolation of bioactive compounds.