Phytochemical Characterization and Evaluation of Biological Activities of Egyptian Carob Pods (Ceratonia siliqua L.) Aqueous Extract: In Vitro Study

Ceratonia siliqua (Carob) is an evergreen Mediterranean tree, and carob pods are potentially nutritive and have medicinal value. The present study was carried out to estimate the possible biological activities of phytochemical-characterized carob pod aqueous extract (CPAE). The phytochemical contents of CPAE were determined by using colorimetric methods and HPLC. In addition, the free radical scavenging properties and anti-diabetic, anti-hemolytic, and antimicrobial activities were estimated by using standardized in vitro protocols. The phytochemical analysis revealed that CPAE was rich in polyphenols, flavonoids, and alkaloids, where it contained a significant amount of gallic acid, catechin, and protocatechuic acid. Furthermore, CPAE exhibited strong antioxidant activity where it prevented the formation of 2, 2-Diphenyl-1-picryl hydrazyl, hydroxyl, and nitric oxide free radicals. Additionally, it had a potent inhibitory effect against digestive enzymes (amylase, maltase, sucrase, and lactase). Moreover, CPAE exhibited anti-Staph aureus, anti-Escherichia coli, anti-Candida albicans, and anti-herpes simplex type I virus (HSV-I). Finally, CPAE protected the erythrocyte membrane from hypotonic solution-induced hemolysis. Altogether, CPAE could be regarded as an interesting source of biologically active antioxidant, anti-diabetic, and antimicrobial preparation for a potential application in pharmaceutical and food supplement fields.


Introduction
Plants are of great interest in drug discovery and are the main source of our modern medicine. About 25% of modern medicines are derived from a plant origin and only 5-15% of plants are being investigated for their medicinal use [1]. Today, medicinal herbs and functional foods are being widely studied resulting in lucrative therapeutic potentials [2]. Where the secondary metabolites, which possessed antioxidant properties can fight several pathological disorders such as cancer, heart disease, hypertension, dementia, and stroke [3]. However, chemotherapies have many adverse effects; several anti-diabetic drugs such as Rosiglitazone and Alogliptin can have severe complications. Therefore, scientists have The mature carob pods were collected from the farms of the City of Scientific Research and Technological Applications (SRTA-City), New Borg El-Arab City, Alexandria, Egypt. The pods were washed with distilled water to remove debris and dried. The seeds were removed from the pods. Then, the pods were ground to a fine powder with a grinder. Two hundred grams of fine dry powder were soaked in one liter of distilled water and boiled for one hour after that the mixture was incubated for 24 h in a shaker incubator. Then, the mixture was filtrated by gauze to remove fiber and insoluble particles. After that, the filtrate was lyophilized to obtain a fine powder (30 g) that was stored at −20 until used.

Phytochemical Analysis of the Carob Extracts 2.2.1. Quantification of the Total Flavonoid Content
The total flavonoid content was determined by using the aluminum chloride colorimetric method [15]. Briefly; 0.1 mL of the CPAE (1 mg/mL in water) or each rutin concentration (2,4,6,8, and 10 mg/mL in distilled water) was mixed with 1.5 mL of distilled water and 750 µL of sodium nitrite solution, and incubated for 6 min at room temperature. Then, a volume of 150 µL of aluminum chloride solution was added, mixed well, and the absorbance was measured immediately at 510 nm using an optima spectrophotometer. The test was carried out in triplicate. The levels of total flavonoid contents were determined as milligram rutin equivalents per g lyophilized powder, and then the data were converted into milligram rutin equivalents 100 mg CPAE.

Quantification of the Total Phenolic Content
Total phenolic content was determined by using Folin-Ciocalteu colorimetric method described by Taga et al. (1984) [16]. Folin-Ciocalteau reagent (100 µL) and 2 mL sodium carbonate were added and mixed well with 100 µL of CPAE (1 mg/1 mL) or each gallic acid (GA) standard; each mixture was incubated at 25 • C for 2 h. The absorbance of the resulting blue color solution was measured at 750 nm using an optima spectrophotometer. The test was carried out in triplicate. The data were converted to milligram gallic acid equivalents (GAE)/100 mg CPAE.

Quantification of the Total Alkaloid Content
Total alkaloid content was determined by using the method developed by Ayoola et al. (2008) [17] which is based on the reaction between alkaloid with bromocresol green (BCG), resulting in a yellow-colored product. This method has the benefits of sensitivity and stability. In brief, 0.1 mL of CPAE was mixed with 2 N HCl, and one milliliter of this solution was transferred to a separatory funnel and washed (three times) using 10 mL chloroform. The pH of this solution was adjusted to neutral with 0.1 N NaOH. Then 5 mL of BCG solution and 5 mL of phosphate buffer were added to this solution. After that, the mixture was shaken and the complex formed was extracted with 1, 2, 3, and 4 mL chloroform using vigorous shaking. The extracts were collected in a 10 mL volumetric flask and diluted to volume with chloroform. The absorbance of the complex in chloroform was measured at 470 nm. Alkaloids (mg/mL) = (Abs − 0.048)/0.021.

High-Performance Liquid Chromatography (HPLC) Analysis of CPAE
A sample (1 g) of CPAE was placed in a quick-fit conical flask, 20 mL of 2M NaOH was added, the flasks were flushed with N2, and the stopper was replaced. The samples were shacked for 4 h at room temperature. The pH was adjusted to 2, with 6 M HCl. The samples were centrifuged at 5000 rpm for 10 min and the supernatant was collected. Phenolic compounds were extracted twice with 50 mL ethyl ether and ethyl acetate 1:1. The organic phase was separated and evaporated at 45 • C and the samples were redissolved in 2 mL of methanol. HPLC analysis was carried out using Agilent Technologies 1100 series liquid chromatograph equipped with an autosampler and a diode-array detector. The analytical column was an Eclipse XDB-C18 (150 × 4.6 µm; 5 µm) with a C18 guard column (Phenomenex, Torrance, CA). The mobile phase consisted of acetonitrile (solvent A) and 2% acetic acid in water (v/v) (solvent B). The flow rate was kept at 0.8 mL/min for a total run time of 70 min and the gradient program was as follows: 100% B to 85% B in 30 min, 85% B to 50% B in 20 min, 50% B to 0% B in 5 min, and 0% B to 100% B in 5 min. The injection volume was 50 µL and peaks were monitored simultaneously at 280 and 320 nm for the benzoic acid and cinnamic acid derivatives, respectively. All samples were filtered through a 0.45 µm Acrodisc syringe filter, Pall Corporation, USA, (Gelman Laboratory, MI) before injection. Peaks were identified by congruent retention times and UV spectra and compared with those of the standards [18].

Quantification of the Total Carbohydrate Content
The total carbohydrate content was determined using anthrone reagent (Hedge and Hofreiter, 1962) [19]. Briefly; 0.1 mL of the CPAE was hydrolyzed by keeping it for three hours in a boiling water bath with 5 mL of 2.5 N HCl. The solution was neutralized by adding sodium carbonate until effervescence ceased, the volume was completed to 100 mL with distilled water then centrifuged for 5 min and the supernatants were used for analysis. Different aliquots of standard glucose were used (0, 0.2, 0.4, 0.6, 0.8, and 1 mL). The volumes were completed to 1 mL with distilled water, and then 4 mL of anthrone reagent were added and the solutions were heated for eight minutes in a boiling water bath.
The green to dark green color was read at 630 nm. The content of carbohydrate present in 0.1 mL of the sample = (mg of glucose/volume of the test sample) × 100.

Quantification of the Total Amino Acid Content
The total amino acids content was determined according to Moor and Stein (1957) [20]. Briefly; 0.1 mL of the CPAE was taken in a 20 mL test tube and then 1 mL of ninhydrin solution was added to it. The tubes were heated for 20 min in a boiling water bath. Then they were cooled, and 5 mL of the ethanol were mixed and incubated at room temperature for 15 min. The optical density was read at 570 nm using a spectrophotometer. The concentration of unknown was calculated from the standard curve. A volume of 20 µL amylase (1:100 w/v) was mixed with 5 µL (10 mg/100 mL) of CPAE and 100 µL phosphate buffer (pH = 6.9); then, the mixture was incubated for 45 min at room temperature. After incubation, 20 µL of soluble starch (1:100 w/v) was added and the mixture was incubated for 20 min. Then, 100 µL of glucose detection reagent was added to the previous mixture and incubated at room temperature for 20 min. Absorbance was measured at 490 nm wavelength. Specific α-Amylase activity is reported as U = µmol of glucose min −1 [21].

Determination of Maltase, Sucrase and Lactase Activities
The activities of the disaccharidases enzymes were determined as previously described by Dahlqvist, et al. (1974) [22]. A volume of 10 µL of pancreatin (0.1 g/10 mL H 2 O containing drops of NaOH) was mixed with 5 µL of CPAE (10 mg/100 mL) and 50 µL phosphate buffer (pH 7.4), and the mixture was incubated for 45 min at room temperature, then 10 µL of maltose, sucrose, or lactose (1 g%) as substrate was added and the mixture was left for 20 min at room temperature. The reaction was stopped by thermal denaturation, and 100 µL of glucose detection reagent was added to the previous mixture and incubated for 20 min at room temperature. Absorbance was measured at 450 nm wavelength. The specific activity of the enzyme was reported as U = µmol of glucose min −1 .

Determination of 2,2-Diphenyl-1-picryl hydrazyl (DPPH) Radical Scavenging Activity
The DPPH radical scavenging activity was determined according to the method described by Blios, (1958) [23]. Briefly, 100 µL of DPPH was mixed with 100 µL of different concentrations of CPAE, 100 µL standard (Ascorbic acid) or 100 µL DEMSO (control). The reaction mixture was thoroughly vortexed and left in the dark at room temperature for 30 min. The absorbance of the mixture was measured spectrophotometrically at 517 nm. The ability of CPAE to scavenge DPPH radical was calculated by the equation:

. Determination of Hydroxyl Radical Scavenging Activity
This assayed as described by Elizabeth and Rao (1990). The assay is based on the degradation of 2-deoxy ribose by hydroxyl radical generated by the Fe 3+ Ascorbate -EDTA -H 2 O 2 system (Fenton reaction). The degradable 2-deoxy ribose was condensed with thiobarbituric acid (TBA) and then measured as TBARS.

Determination of Ferric Reducing Antioxidant Power (FRAP)
One milliliter of CPAE with different concentrations (100, 75, 50, 12.5, and 6.25 mg/mL) was mixed with 1 mL of sodium phosphate buffer (pH 6.6) and 1 mL of potassium ferricyanide. The mixtures were incubated for 20 min at 50 • C, followed by the addition of 1 mL of trichloroacetic acid (TCA 10%), then centrifuged for 10 min at 2000 rpm. One mililiter of the supernatant was added to 1 mL of deionized water and 200 µL of FeCl 3 . The blank was prepared in the same manner as the sample, except that potassium ferricyanide was replaced by distilled water, and the mixture was incubated for 30 min at room temperature. The absorbance of the reaction mixture was measured at 700 nm wavelength (Sutharsingh, et al., 2011) [24].

Determination of Nitric Oxide (NO) Radical Scavenging Activity
Briefly, 400 µL of sodium nitroprusside and 100 µL of phosphate buffer were mixed with 100 µL of CPAE, standard, or DMSO (control). This reaction mixture was incubated for 2.5 h in a dark place at 25 • C. After incubation, 20 µL of Griess reagent was added to the previous mixture and allowed to stand for 30 min at room temperature. The absorbance was measured at 540 nm wavelength (Garratt, 1964) [25].

Hemolytic Activity Assay
The test was performed according to the method described by Farias et al. (2013) [11], with some modifications. Firstly, a serial dilution of CPAE was prepared with 0.9% NaCl ranging from1000 to 1.9 µg·mL −1 and reserved. Then, 100 µL of a 1% red blood cell (A, B, and O human blood types) suspension was added to a new microtube containing 900 µL of CPAE dilution, then incubated at 37•C for 1h. After that, the tubes were centrifuged at 3000× g for 5min. The supernatant (200 µL) was placed in a 96-well plate and read at 540 nm using a microplate reader. The cell suspensions of each human blood type (100 µL) were mixed with distilled water or 0.9% NaCl (900 µL) to obtain the absorbance for 100 and 0% of cell lysis, respectively. The percentage of hemolysis was calculated as follows: % hemolysis = Abs test/Abs pc × 100, where Abs test = Abs540 of the 1% cell suspension treated with sample test and Abs pc = Abs540 of the 1% cell suspension treated with distilled water.

Antibacterial and Antifungal Method
The antimicrobial activities of the CPAE were studied on Mueller-Hinton agar plates by Agar diffusion technique against Gram-positive (Bacillus subtilis (ATCC 6051) and Staphylococcus aureus (ATCC 6538) and Gram-negative (Escherichia coli (ATCC 8739) and Pseudomonas aeruginosa (ATCC 90274)) pathogenic bacterial strains beside fungi (Aspergillus falvus (ATCC 9643) as well as yeast Candida albicans (ATCC 10221). Gentamicin (10 mg/mL) was used standardly as a positive control. Mueller-Hinton agar plates seeded with 1.8 × 10 8 cfu/mL (0.5 OD 600 ) of the test bacteria. Following 24 h of incubation at 37 • C, plates were examined for the presence of inhibition zones. The inhibition zones surrounding the wells were measured (mm) [26].

Evaluation of the Maximum Non-Toxic Concentration (MNTC) of CPAE on Vero Cells
This assay was selected to show the maximum non-toxic concentration of CPAE in susceptible mammalian cells (Hu, et al. 2008). The Vero cells (ATC CCL-88) were propagated in a growth medium (Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% heat-inactivated fetal bovine serum (FBS), 1% L-glutamine, HEPES buffer, and 50 mg/mL gentamicin). All cells were maintained at 37 • C in a humidified atmosphere with 5% CO 2 . Growth medium was decanted from 96-well microtiter plates after the formation of the confluent sheet of Vero cell, and the cell monolayer was washed twice with wash media PBS. Different concentrations of CPAE were prepared in DMEM. A volume of 100 µL of each dilution and 100 µL of culture medium (DMEM supplemented with 2% FBS, 1% L-glutamine, HEPES buffer, and 50 mg/mL gentamicin) were added to cells then the plate was incubated at 37 • C for 48 h. After that, 20 µL of MTT solution (5 mg/mL in PBS) (Bio Basic Canada Inc, Toronto, Canada) was added to each well, then the plate was incubated at (37 • C, 5% CO 2 ) for 4 h. The media was discarded and the formed formazan (MTT metabolic product) was suspended in 200 µL DMSO. The optical density was read at 560 nm wavelength using an ELISA reader (TECAN Inc., Chapel Hill, NC, USA) and the background was subtracted at 620 nm wavelength [27].
Evaluation of the Antiviral Activity of CPAE Using MNTC In brief, a monolayer of 1 × 10 4 (Vero cells/well) was placed in a 96-well plate. The plate was incubated at (37 • C, 5% CO 2 ) overnight. Then, 100 µL herpes simplex type I virus (HSV-I)/CPAE suspension which was incubated for one hour was added to cells and incubated for 24 h at (37 • C, 5% CO 2 ). Then, the cell viability was determined by MTT assay.

Statistical Analysis
All tests were analyzed in triplicate of three independent measurements and the results were expressed as mean values ± standard deviation (SD). The statistical difference was measured with a t-test when it was applicable, at p < 0.05, by using SPSS v. 18.0 software.

The Phytochemical Ingredients of the CPAE
The phytochemical analysis revealed that CPAE contained many active compounds including total phenolics, flavonoids, carbohydrates, amino, acids, and alkaloids (Table 1). Moreover, HPLC analyses showed that CPAE contained a high content of gallic acid followed by catechin, protocatechuic acid, and cinnamic acid, while it also contained a low concentration of p-coumaric acid, rutin, gentisic acid, p-hydroxybenzoic acid, vanillic acid, and ferulic ( Figure 1 and Table 2).

The Antioxidant Effect of CPAE
The antioxidant effect of CPAE was measured in vitro. The scavenging activity of the CPAE was often evaluated according to its IC50; the lowest IC50 value corresponds to the highest free radical scavenging activity. It is obvious that CPAE had DPPH, NO, FRAP, and OH free radical scavenging activities. The CPAE antioxidants properties were lower than those of ascorbic acid which was used as a positive control, at p < 0.05 (Table 3). In each raw, CPAE mean with * was significantly difference compared to that of the ascorbic acid mean, at p < 0.05.

Anti-Digestive Enzymes Effect of CPAE
The results in Figure 2 revealed that Amylase, Maltase, Sucrase, and Lactase activities were strongly inhibited by CPAE in a concentration-dependent manner.

The Hemolytic Effect of CPAE
Hemolytic activity of CPAE was screened against normal human erythrocytes. Figure 3 showed that the hemolytic percent was increased from 0.7 to 3.2% when the concentration of CPAE increased in the range from 10 mg/mL to 100 mg/mL. The calculated hemolytic IC50 was 1562.5 mg/mL.    Table 4 shows that the CPAE had a significant antibacterial property against Bacillus subtilis, Staph. aureus, and Escherichia coli. However, CPAE did not show any activity against Gramnegative bacteria Pseudomonas aeruginosa. Moreover, it exhibited a potent antibacterial effect compared to that of gentamicin (positive control antibiotic) in the case of Staphylococcus aureus and Escherichia coli with ZOI (25 and 24 mm, respectively). In addition, the extract exhibited an antifungal effect against Candida albicans, while it did not show any activity against Aspergillus falvus Table 4.  Table 5 indicated that the CPAE was considered safe for Vero cells until 5000 µg/mL where cell viability was 96.5%. Moreover, our results showed that CPAE inhibited HSV-1 in a concentration-dependent manner ( Table 6). The value expressed mean ± SE. Means with different superscript letters were significantly different at p < 0.05. Mean with letter (a) was the lowest one while mean with letter (c) was the highest one. Value expressed mean ± SE. Means with different superscript letters were significantly different at p < 0.05. Mean with letter (a) was the lowest one while mean with letter (c) was the highest one.

Discussion
The phytochemical investigation of CPAE in the current study revealed the presence of flavonoids, total polyphenols, alkaloids, carbohydrates, and amino acids. The presence of these phytochemicals marked it understandable why carob pods are a prominent medicinal plant for the treatment of various diseases. In agreement with this finding, Ayache et al. (2020) demonstrated that carob pulp contains a significant amount of phenolic compounds and flavonoids (1.8 EAG/100 gDW, 0.6 EC/100 gDW) respectively [28]. In addition, Nawel et al. (2018) found that carob pods contain high content of alkaloids 56.51 ± 1.02 mg/100 g [29]. Moreover, there are many reports demonstrating the presence of alkaloids in carob [30,31] which can explain the traditional therapeutic uses of carob. Moreover, the high content of amino acids increases the nutritional value of carob; according to the World Health Organization (WHO), carob has all the essential amino acids [32]. In addition, the HPLC analysis revealed that CPAE contained a high content of gallic acid, catechin, and protocatechuic acid, respectively, and gallic acid is the most abundant phenolic compound in CPAE. These results were in agreement with previous reports, which revealed that gallic acid was the major phenolic acid present in carob pods [30,33].
Many studies have demonstrated that these molecules are well known for their antioxidant and anticancer properties [32,34]. There are several data about the component of carob performed by HPLC, Ritib et al. 2015 found that the main components of CPAE are pyrogallol 48.0% and catechin 19.1%, and the gallic acid is present in a small content 3.1% [35]. In addition, the study by Ghanemi et al. (2017) showed that m-coumaric acid and gallic acid are the major polyphenols present in carob (2192.3 and 1445.3 µg/g DW, respectively) [36]. Moreover, Goulas and Georgiou found that the main components of water carob pod extract are myricetin 94.5%, gallic acid 80%, epicatechin 77.3%, and rutin 67% [37]. Another study by Al-Olayan et al. (2016) found that carob pods contain high content of polyphenols 68.3 ± 5.8 mg gallic acid equivalent/g dried pod of polyphenols and a relatively low amount of flavonoids 9.8 ± 2.2 mg quercetin equivalent/g dried pod. The main components of CPAE are kaempferol (53.53%) and gallic acid (11.19%) [30]. This variation in phenolic content depends on many factors such as genetic, geographical, environmental, physiological, and cultural conditions, preparation of samples, extraction, and method of analysis [38]. Due to the complex nature of phytochemicals present in carob pods, we used multiple assays to provide preliminary evidence about the antioxidant activity of the Egyptian carob pods. Firstly, our results of in vitro antioxidant activity indicated that the CPAE had a strong ability to inhibit DPPH, and this activity is due to the presence of active constituents in carob pods which have the ability to donate hydrogen to a free radical in order to remove the odd electron which is responsible for the radical's reactivity. Our results were in agreement with previous findings, which recorded that carob had a strong DPPH scavenging activity [28,34,39]. Further, the reducing power of CPAE was evaluated with its ability to transform Fe 3+ to Fe 2+ through electron transferability, which acts as a significant indicator of its antioxidant activity. Hence, iron participates in many cellular functions, and any excess iron can generate reactive oxygen species through the Fenton reaction. The iron-chelating capacity would prevent transition metals from participating within the commencement of oxidative stress [40]. Here, the Fe 2+ chelating activity of the CPAE was increased with increasing concentration, reaching a level of 92.79% at high concentrations (1 g/mL). These results were in agreement with many other studies that reported the ability of carob to reduce Fe3+ to Fe2+could be due to the presence of polyphenols [28,39]. In agreement with these findings, Goulas and Georgiou found that ceratonia siliqua extract has a good antioxidant activity as evidenced by the DPPH IC50 (1.9 mg/mL) and FRAP (339.7 mg FeSO4 100 g −1 ) [37]. In another study by Abidar et al. (2020) found that carob has a strong antioxidant activity with a DPPH IC50 = 0.116 mg/mL and a high FRAP with an EC50 = 0.123 mg/mL [41].
In addition, the results of this study indicated that CPAE was an effective hydroxyl radical scavenger with IC50 = 7.07 mg/mL, and the result was in line with the findings of Nadia Amessis et al. (2016), who reported that ceratonia siliqua had a hydroxyl radical scavenging activity of 38% [42]. The hydroxyl radicals are formed as a result of the reduction of oxygen to water and are considered the major active oxygen species implicated in lipid peroxidation and many biological damages leading to many diseases such as atherosclerosis, cancer, and neurological disorders, and can be prevented by the action of non-reducing substances [43]. Additionally, nitric oxide plays a significant role in the pathogenesis of various diseases associated with inflammation [44]. As shown in our results, CPAE produced significant antioxidant effects against nitric oxide production at serial dilutions; this result is consistent with Rico et al. (2019) who reported that carob pods significantly inhibit NO production [45]. These observations give an indication of the strong antioxidant potential of the CPAE, which is confirmed with its action on DPPH, FRAP, OH, and NO.
Phenolic compounds as depicted in carob pods are good electron donors and could terminate the radical chain reaction by converting free radicals into more stable products [28]. The antioxidant activity of phenolics depends on the number and substitution of the hydroxyl group. As such, carob's antioxidant activity can thus be attributed to the presence of gallic acid, protocatechuic, catechin, p-hydroxybenzoic, and vanillic acid [46].
There are several methods to control blood glucose level; one of them is the control of postprandial hyperglycemia via delaying the absorption of carbohydrates after food intake [47]. This could be done through the inhibition of α-amylase and α-glucosidase enzymes (maltase, lactase, and sucrase) present in the gastrointestinal tract [48]. Inhibitors of these enzymes slow down the digestion of carbohydrates, causing a decrease in glucose absorption rate, thereby reducing the increase in blood sugar after a meal [49]. Although carob contains a high content of carbohydrates, it exhibited a significant antidiabetic effect, which gave carob great importance as a natural sweetener for diabetics. As presented in Figure 1, our results indicated that CPAE had a potent inhibitory effect against all digestive enzymes. These findings were in agreement with Custódio et al. (2014) who confirmed that the leaves and stem bark of the carob tree has a high inhibitory effect on the activity of α-amylase, α-glucosidase, and also display significant antioxidant activity [50]. Many studies have reported that polyphenols, mainly flavonoids, phenolic acids, and tannins, have a significant benefit in inhibiting α-glucosidase and α-amylase, which are the two critical enzymes involved in the conversion of dietary carbohydrates to glucose. [51].
The results of this study also showed that CPAE had a significant antibacterial effect against pathogenic gram-positive and gram-negative bacteria (Bacillus subtilis, Staphylococcus aureus, and Escherichia coli). These results were in agreement with Hsouna et al. (2015), who reported that carob ethyl acetate extract showed antimicrobial activity against many pathogenic bacteria [52]. The antibacterial activity of CPAE could be explained by the presence of biologically active compounds such as phenolic acids and flavonoids that impact the growth and metabolism of microorganisms. The phenols and flavonoids contribute significantly to the antibacterial activity and can form complexes with the cell wall and also disrupt bacterial envelopes [53]. Further, Tassou et al. (1997) reported that carob had an inhibitory effect against many pathogenic bacteria [54]. CPAE is very rich in gallic acid, which can inhibit the motility, adherence, and biofilm formation of many pathogenic bacteria [55]. Gallic acid can also disrupt the integrity of the cell membrane in Gram-positive and Gram-negative bacteria and change the charge, hydrophobicity, and permeability of the membrane surface [56]. Furthermore, protocatechuic has broad-spectrum antibacterial activity against a wide range of bacterial species [57].
In addition, The CPAE exhibited a significant inhibitory effect on the growth of Candida albicans, suggesting that the studied CPAE are possibly a secure and natural source of antifungal agents. Hussein et al. (2011) reported that carob leaves had a significant antibacterial and fungal effect [58]. In addition, our results indicate that CPAE exhibited a safe effect on Vero cells and revealed a significant inhibitory effect against HSV-1. As a result of the highest content of gallic acid in CPAE, which explains the antiviral effect of HSV-1, Kratz et al. (2008) reported that gallic acid has the ability to inhibit the herpes simplex virus' (HSV-1 and HSV-2) attachment and penetration [59].

Conclusions
This study indicated that CPAE contained phenolic, flavonoid, alkaloid, and amino acids, and carbohydrates. Thus, CPAE possessed antioxidants activity. In addition, it had hypoglycemic effect via inhibiting the intestinal enzymes, maltase, sucrase, lactase, and amylase. Furthermore, it had strong antimicrobial activity against Staph. aureus, Escherichia coli, Escherichia coli and HSV-1. Therefore, this study suggested that CAPE can be used as a food supplement and supportive therapeutic agent for microbial and diabetic treatment.

Data Availability Statement:
The data presented in this study are available on request from the corresponding author.