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Pakistan Journal of Biological Sciences

Year: 2022 | Volume: 25 | Issue: 10 | Page No.: 875-884
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Research Article

Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro

Elsayed K. Bakhiet, Hosni A.M. Hussien Hosni A.M. Hussien's LiveDNA and Mohamed Elshehaby

ABSTRACT

Background and Objective: Bacterial and fungal infections are major public health problems. Emerging of drug-resistant microbial strains urges the need for the development of alternative untraditional antimicrobial agents. Bee venom is a rich source of secondary metabolites and antimicrobial agents. In this study, the antimicrobial and antifungal potential of Apis mellifera BV (AmBV) against some medically important bacterial and fungal pathogens was investigated. Materials and Methods: Broth microdilution method and Colony Forming Unit (CFU) assay were used to screen the antibacterial potential of AmBV. Similarly, the antifungal activity of AmBV was evaluated using the agar-well diffusion assay. Moreover, the minimum inhibitory concentration (MIC) values of AmBV against tested microorganisms were determined. Results: AmBV significantly inhibited bacterial and fungal growth. The MIC values of AmBV were 15.625, 31.25, 7.8, 7.8 μg mL1 against Escherichia coli ATCC 8739, Staphylococcus aureus ATCC 6538P, Serratia marcescens AUH 98 and Streptococcus mutans ATCC 25175, respectively. Similarly, AmBV at concentrations of 300 and 600 μg mL1 significantly inhibited the growth of Aspergillus niger ATCC 16404, Alternaria alternata MLBM09, Fusarium oxysporum MLBM212 and Aspergillus flavus. Conclusion: These results indicated that AmBV could be used in future preclinical and clinical studies to develop cost-effective and efficient antibacterial and antifungal agents. Moreover, this study presents AmBV as an efficient alternative antimicrobial agent against medically important pathogens.
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INTRODUCTION

Bee’s venom (BV) has been used in traditional medicine applications to treat a variety of diseases1. There are many pharmacologically and biologically active components in BV, including there are many pharmacologically and biologically active components in BV including melittin, adolapin, apamin, hyaluronidase, phospholipase A2, histamine, epinephrine, lipids, carbohydrates and minerals2,3. The BV is released by the poison glands of honeybee workers as a defence mechanism4.

Natural products such as BV are bioactive compound-rich products and have been shown to mediate a wide range of effects against several diseases5,6. Although BV is poisonous to bee predators, it has been developed as a medicinal tool by humans through time. The use of BV for therapeutic purposes dates back to Ancient Egypt (4000 BC), Hippocrates, Aristotle and Galen used it during the Greek and Roman periods7,8. Inflammatory disorders such as rheumatoid arthritis, tendinitis, fibrosis, lupus and multiple sclerosis were treated with BV in traditional Chinese medicine and other historical traditions8,9. Melittin is the main active polypeptide in BV and has anti-cancer, anti-inflammatory, antibacterial and antiviral properties10,11. In their study, Yu et al.12 demonstrated that BV has potent antifungal properties against Trichophyton mentagrophytes and Trichophyton rubrum, which are far more potent than fluconazole, a commercial antifungal used to treat superficial and systemic fungal infections.

Multidrug-resistant bacteria (MDRB) like Escherichia coli (E. coli ) are becoming more common globally, this in part owing to the expansion of bacterial mobile resistant genetic components like plasmids13. Similarly, MDRB strains of S. marcescens cause a wide spectrum of clinical features including pneumonia, meningitis, conjunctivitis, sepsis, urinary tract infections and surgical wound infections14. S. aureus is one of the major opportunistic human pathogens. S. aureus evades the immune system and causes a variety of human illnesses ranging from minor skin irritations to life-threatening sepsis15,16. Streptococcus mutans (S. mutans) colonize the oral cavity and are responsible for dental caries and periodontal diseases. The antimicrobial resistance of many bacterial and fungal strains has limited the efficacy of available commercial antimicrobial agents. Thus, new untraditional antimicrobial agents are highly in need to control infection of MDRB. The current study aimed to evaluate the antimicrobial activity of Apis mellifera BV (AmBV) against some important bacterial and fungal pathogens.

MATERIALS AND METHODS

Study area: This study was conducted in 2021 at the Botany and Microbiology Department, Faculty of Science, Al-Azhar University, Assiut Governorate, Egypt.

Microbial strains: For this study, the American Type Culture Collection (ATCC) reference strains (Streptococcus mutans ATCC 25175 (S. mutans ATCC 25175), Staphylococcus aureus ATCC 6538P (S. aureus ATCC 6538P), Escherichia coli ATCC 8739 (E. coli ATCC8739) and Aspergillus niger ATCC 16404 (A. niger ATCC 16404) and clinical isolates (Serratia marcescens AUH 98 (S. marcescens AUH 98), Alternaria alternata MLBM09 (A. alternata MLBM09), Fusarium oxysporum MLBM212 (F. oxysporum MLBM212) and Aspergillus flavus (A. flavus)) were used17. Bacterial strains were grown on Mueller Hinton Broth (MHB) at 37°C, while the fungal strains were grown in potato dextrose agar (PDA) medium and incubated at 28°C. Bacterial suspensions were freshly prepared before each experiment and adjusted to the turbidity of 0.5 McFarland standards (OD630 ~ 0.08 in MHB). Bacterial suspensions were used within 30 min of preparation.

Collection of Apis mellifera Bee Venom (AmBV): The venom of Apis mellifera forager honeybees descended from naturally mated queens was used to study its antimicrobial activity as previously described by Surendra et al.18. These bees were derived from a colony pool and collected from the Department of Bees, The Institute of Plant Protection, the Center for Agriculture and the Ministry of Agriculture Egypt. They were rendered immobile by rapid freezing at -20°C. The stinging apparatuses of honeybees were dissected at 4°C and the venom reservoirs were extracted and stored at -20°C till used in subsequent assays. Venom sacs were resuspended in Milli-Q water and whole bee venom (WBV) was extracted by disrupting the reservoir using a glass rod under rapid defrosting and light pressure. Extracted venom samples were centrifuged at 10,000 g for 5 minutes at 4°C and the supernatants were used as protein and enzyme sources before being lyophilized. Lyophilized Bee venom was dissolved in Milli-Q water and filtered through a 0.22 m syringe filter before using it in further experiments.

Determination of the antibacterial activity of AmBV
Broth microdilution method: Serially diluted AmBV was transferred into wells of 96-well plate in 90 μL volume. The final concentrations of AmBV in wells were 7.6-4000 μg mL1. Next, 10 μL of bacterial suspension was added to each well. The plate was incubated at 37°C for 24 hrs before reading the optical density (OD) at 630 nm using a microplate reader19. Untreated (UT) bacterial suspension was used as a growth control.

Colony Forming Unit (CFU) assay: Antibacterial activity of AmBV was assessed by counting Colony Forming Units (CFUs)20-22. Briefly, 1 mL of serially diluted AmBV (250 to 4000 μg mL1) was inoculated with 10 μL of bacterial suspension and incubated at 37°C for 6 hrs. Next, 10-fold serial dilutions were prepared from each treatment and 10 to 100 μL of each dilution was streaked on Muller-Hinton agar (MHA) plates. Bacterial colonies were counted after overnight incubation at 37°C. The MHA plates inoculated with untreated bacteria were used as growth control.

Determination of minimum inhibitory concentration (MIC): A broth microdilution susceptibility test was used to detect MIC as previously described20,23-25. Briefly, two-fold serially diluted AmBV was transferred into wells of 96-well plate in 90 μL volume. The serially diluted concentrations of AmBV that used to determine MIC were 4000, 2000, 1000, 500, 250, 250, 125, 62.5, 31.25, 15.625 and 7.8 μg mL1. Next, 10 μL of bacterial suspension was added to each well and the plate was incubated at 37°C for 24 hrs before reading the optical density (OD) at 630 nm using a microplate reader. The MIC value was determined as the minimum concentration of AmBV that significantly decrease the OD630 value with no visible bacterial growth.

Antifungal activities of AmBV: The antifungal activities of AmBV were evaluated through the agar-well diffusion assay as previously described26-28. The solution has been tested at different concentrations (600, 300 and 150 μg mL1).

Statistical analysis: The growth reduction was calculated relative to the growth control. Data were shown as Means±Standard Deviation (SD) of at least three independent experiments. Comparisons between various treatments were performed by t-test and one-way ANOVA. The p<0.05 was regarded as statistically significant.

RESULTS

Antibacterial activity of AmBV
Broth microdilution methods: Results from Broth microdilution methods demonstrated that AmBV significantly inhibits the growth of the tested bacterial strains in a concentration-dependent manner. AmBV was significantly inhibited the growth of E. coli ATCC8739 at concentration of 15.625 μg mL1 (p<0.05) in Fig. 1a.

Image for - Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro
Fig. 1(a-d): Antibacterial activity of different concentrations of AmBV against bacterial species, (a) E. coli ATCC 8739, (b) S. aureus ATCC 6538P, (c) S. marcescens AUH 98 and (d) S. mutans ATCC 25175
Results are shown as Means±SD of three independent experiments,* p<0.05, **p<0.01, ***p<0.001 and ****p<0.0001 vs. untreated control


Table 1: Antibacterial activity of AmBV
Concentration (μg mL1)
E. coli ATCC 8739
S. marcescens AUH 98
S. aureus ATCC 6538P
S. mutans ATCC
UT
0.2707±0.009815
0.4250±0.01803
0.3770±0.04480
0.4573±0.1249
4000
0.0580±0.002646
0.06767±0.008963
0.0630±0.006245
0.0620±0.008000
2000
0.09433±0.02977
0.1303±0.03661
0.1877±0.01102
0.07967±0.007638
1000
0.1283±0.008963
0.1583±0.01557
0.1890±0.008718
0.0774±0.006773
500
0.1287±0.007767
0.1633±0.01222
0.1940±0.01652
0.08067±0.008505
250
0.1647±0.02346
0.1670±0.001000
0.2537±0.01002
0.08633±0.01222
125
0.1710±0.01442
0.1693±0.002517
0.2700±0.004359
0.1033±0.007024
62.5
0.1787±0.02065
0.1800±0.009165
0.2830±0.005000
0.1407±0.01172
31.25
0.1967±0.01007
0.1990±0.0110
0.2910±0.02330
0.1523±0.006506
15.625
0.2140±0.03318
0.2017±0.01193
0.3387±0.01250
0.1583±0.01815
7.8
0.2377±0.01185
0.2233±0.01893
0.3770±0.04480
0.1663±0.03213

The growth of E. coli ATCC8739 was further inhibited at AmBV concentrations of 31.25, 62.50 and >125 μg mL1 (p<0.05) (Fig. 1a). The OD value of E. coli ATCC 8739 growth was decreased from 0.2707±0.009815 at untreated control to 0.2140±0.03318, 0.1967±0.01007, 0.1787±0.02065, 0.1710 ±0.01442, 0.1647±0.02346, 0.1287±0.007767, 0.1283±0.008963, 0.09433±0.02977, 0.0580±0.002646 when treated with AmBV concentrations of 15.625, 31.25, 62.5, 125, 250, 500, 1000, 2000 and 4000 μg mL1, respectively in Fig. 1a and Table 1. Similarly, the growth of S. aureus ATCC 6538P was significantly inhibited by AmBV at concentrations of 31.25, 62.50, 125 and >250 μg mL1 (p<0.05) in Fig. 1b. The OD value of bacterial growth was decreased from 0.3770±0.04480 in untreated culture to 0.2910±0.02330, 0.2830±0.005000, 0.2700±0.004359, 0.2537±0.01002, 0.1940±0.01652, 0.1890±0.008718, 0.1877±0.01102, 0.0630±0.006245 when treated with AmBV concentrations of 31.25, 62.5, 125, 250, 500, 1000, 2000 and 4000 μg mL1, respectively in Fig.1b and Table 1. Interestingly, the growth of both S. marcescens AUH 98 in Fig. 1c and S. mutans ATCC 25175 in Fig. 1d were significantly inhibited at all used AmBV concentrations (4000-7.8 μg mL1 (p<0.05)). The OD value of the growth of S. marcescens AUH 98 was decreased from 0.4250±0.01803 at untreated control to 0.2233±0.01893, 0.2017±0.01193, 0.1990±0.0110, 0.1800±0.009165, 0.1693±0.002517, 0.1670±0.001000, 0.1633±0.01222, 0.1583±0.01557, 0.1303±0.03661, 0.06767±0.008963 at AmBV concentrations of 7.8, 15.625, 31.25, 62.5, 125, 250, 500, 1000, 2000 and 4000 μg mL1, respectively (Fig.1c and Table 1). While, the OD value in case of S. mutans ATCC 25175 was decreased from 0.4573±0.1249 in untreated control to 0.1663 ±0.03213, 0.1583±0.01815, 0.1523±0.006506, 0.1407±0.01172, 0.1033±0.007024, 0.08633±0.01222, 0.08067±0.008505, 0.0774±0.006773, 0.07967±0.007638, 0.0620 ±0.008000 at AmBV concentrations of 7.8, 15.625, 31.25, 62.5, 125, 250, 500, 1000, 2000 and 4000 μg mL1, respectively in Fig.1d and Table 1. Bacterial growth inhibition by AmBV was concentration-dependent. In case of E. coli ATCC 8739, the percentages of growth inhibition were 78.56, 65.26, 52.58, 52.44, 39.26, 36.86, 34.04, 27.35, 21.13 and 16.02% at 4000, 2000, 1000, 500, 250, 125, 62.5, 31.25, 15.625 and 7.8 μg mL1 of AmBV, respectively in Fig. 2a. For S. aureus ATCC 6538P, the growth inhibition was 82.14, 46.35, 45.90, 44.58, 27.74, 22.94, 19.12, 17.2 and 3.216% at 4000, 2000, 1000, 500, 250, 125, 62.5, 31.25 and 15.625 μg mL1 of AmBV, respectively in Fig. 2b. Interestingly, all the used concentrations of AmBV inhibited the growth of S. marcescens AUH 98 in Fig. 2c. and S. mutans ATCC 25175 in Fig. 2d by more than >47.4 and >60.55%, respectively.

CFU assay: AmBV significantly reduced the CFUs of the treated bacteria. At concentrations of 250-4000 μg mL1 of AmBV, CFUs of E. coli ATCC 8739 were significantly decreased (p<0.0001) compared to untreated control in Fig. 3a. The CFUs of E. coli ATCC 8739 were 453 CFU mL1 at untreated control while at AmBV concentrations of 250, 500, 1000, 2000 and 4000 μg mL1, CFUs of E. coli ATCC 8739 were decreased to 353, 308, 219, 165 and 145 CFU mL1, respectively (Fig. 3a). Similarly, AmBV concentrations of 250-4000 μg mL1 were significantly decreased the growth of S. aureus ATCC 6538P (p<0.0001) in Fig. 3b. The CFUs of S. aureus ATCC 6538P were decreased from 505 at untreated control to 360-265, 155, 48 and 30 CFU mL1 at AmBV concentrations of 250, 500, 1000, 2000 and 4000 μg mL1, respectively (Fig. 3b). The CFUs of S. marcescens AUH 98 were significantly reduced at AmBV concentrations of 250 μg mL1 (510 CFU mL1) (p<0.0001), 500 μg mL1 (389 CFU mL1) (p<0.0001), 1000 μg mL1 (362 CFU mL1) (p<0.0001), 2000 μg mL1 (306 CFU mL1) (p<0.0001) and 4000 μg mL1 (205 CFU mL1) (p<0.0001) compared to untreated control in Fig. 3c. Similarly, the CFUs of S. mutans ATCC 25175 were significantly reduced from 750 CFU mL1 at untreated control to 535, 260, 210, 163 and 19 CFU mL1 when treated with AmBV concentrations of 250, 500, 1000, 2000 and 4000 μg mL1, respectively in Fig. 3d.

Image for - Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro
Fig. 2(a-d): Percentage of bacterial inhibition by different concentrations of AmBV against bacterial species (a) E. coli ATCC 8739, (b) S. aureus ATCC 6538P, (c) S. marcescens AUH 98 and (d) S. mutans ATCC 25175
Results are shown as Means±SD of three independent experiments


Image for - Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro
Fig. 3(a-d): Effect of different concentrations of AmBV on CFUs of bacterial species, (a) E. coli ATCC 8739, (b) S. aureus ATCC 6538P, (c) S. marcescens AUH 98 and (d) S. mutans ATCC 25175
Results are shown as Means±SD of three independent experiments,* p<0.05, **p<0.01, ***p<0.001 and ****p<0.0001 vs. untreated control


Image for - Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro
Fig. 4(a-d): Antifungal activity of different concentrations of AmBV against bacterial species, (a) Representative photographs of antifungal assays of A. niger ATCC 16404, (b) A. niger ATCC 16404 diameter of clear zone inhibition in millimeter (mm), (c) Representative photographs of antifungal assays of A. flavus and (d) A. flavus diameter of clear zone inhibition in millimeter (mm)
Results are shown as Means ±SD of three independent experiments and p-value: ****p<0.0001 vs. negative control

MIC values of AmBV: There were variations in MIC values of AmBV between treated bacterial strains. MIC values of AmBV were 15.625 μg mL1 (OD: 0.2140±0.03318), 31.25 μg mL1 (OD: 0.2910±0.02330), 7.8 μg mL1 (OD: 0.2233±0.01893) and 7.8 μg mL1 (OD: 0.1663±0.03213) against E. coli ATCC 8739, S. aureus ATCC 6538P, S. marcescens AUH 98 and S. mutans ATCC 25175, respectively in Table 2.

Antifungal activity of AmBV: AmBV exhibited a remarkable antifungal activity at concentrations of 300 and 600 μg mL1. Concentrations of 300 and 600 μg mL1 significantly (p<0.0001) inhibited the growth of A. niger ATCC 16404 in Fig. 4a. The diameter of clear zone inhibition of A. niger ATCC 16404 in the agar-well diffusion assay was 19.97±2.040 and 10.97±0.5033 mm at concentrations of 300-600 μg mL1 of AmBV, respectively in Fig. 4b.

Image for - Apis mellifera Venom Inhibits Bacterial and Fungal Pathogens in vitro
Fig. 5(a-d): Antifungal activity of different concentrations of AmBV against bacterial species, (a) Representative photographs of antifungal assays of F. oxysporum MLBM212, (b) F. oxysporum MLBM212 diameter of clear zone inhibition in millimeter (mm), (c) Representative photographs of antifungal assays of A. alternata MLBM09, (d) A. alternata MLBM09 diameter of clear zone inhibition in millimeter (mm)
Results are shown as Means±SD of three independent experiments and p-value: ****p<0.0001 vs. negative control


Table 2: MIC Values of AmBV
Bacterial isolates
MIC (μg mL1)
Escherichia coli ATCC 8739
15.625
Staphylococcus aureus ATCC 6538P
31.25
Serratia marcescens AUH 98
7.8
Streptococcus mutans ATCC
7.8

Similarly, AmBV significantly decreased the growth of A. flavus in Fig. 4c. The clear zone inhibition was 22.83±1.528 mm at a concentration of 300 μg Ml1 of AmBV and 7.333±1.041 mm

at a concentration of 300 μg mL1 of AmBV in Fig. 4d. Moreover, AmBV inhibited the growth of F. oxysporum MLBM212 in Fig. 5a and A. alternata MLBM09 in Fig. 5c. At a concentration of 300 μg mL1 of AmBV, the diameters of clear zone inhibition of F. oxysporum MLBM212 in Fig. 5b and Alternaria alternata MLBM09 in Fig. 5d were 11.67±1.258 and 9.47±0.5508 mm, respectively. Whereas at a concentration of 600 μg mL1 of AmBV, the diameters of clear zone inhibition of F. oxysporum MLBM212 (Fig. 5b) and Alternaria alternata MLBM09 (Fig. 5D) were 18.0±1.323 mm and 14.88±0.34 mm, respectively. There was no antifungal activity for AmBV against all tested fungi at a concentration of 150 μg mL1.

DISCUSSION

New untraditional antibacterial and antifungal agents are highly required to tackle the problem of microbial resistance to available commercial antimicrobial substances. BV contains a variety of bioactive molecules including amino acids (aa), peptides, proteins, enzymes, sugars, biogenic amines, volatile compounds, phospholipids and pheromones. These biomolecules could be harnessed to develop effective antibacterial and antifungal agents, yet the antimicrobial potential of BV was not fully explored. Thus, in this work, the antimicrobial effect of Apis mellifera BV (AmBV) against some medically important and common bacterial and fungal pathogens was elucidated.

Results demonstrated that AmBV is highly potent in inhibiting the growth of the tested bacterial and fungal strains. Using broth microdilution method and CFU assays, it was discovered that AmBV significantly inhibits the growth of E. coli ATCC8739, S. aureus ATCC 6538P, S. marcescens AUH 98 and S. mutans ATCC 25175 in a concentration-dependent manner. Interestingly, in this study MIC values of AmBV against all tested bacteria were markedly low compared to the majority of the reported MIC values, which indicated the efficacy of AmBV as an antibacterial agent. The MIC value of AmBV for S. aureus was 31.25 μg mL1 which is markedly lower than the MIC value reported by Samy et al.29 and Al-Ani et al.9. On the other hand, the MIC values for S. aureus were higher than what was demonstrated30,31. Similarly, the MIC values of AmBV were 15.625 μg mL1 for E. coli ATCC8739 and 7.8 μg mL1 for both S. marcescens AUH 98 and S. mutans ATCC 25175 which was much lower than the previously reported MIC values9,32-35.

Like the antibacterial activity of AmBV, antifungal activity was very prominent in the agar well diffusion assay. AmBV significantly inhibited the growth of A. niger ATCC 16404, F. oxysporum MLBM212, A. flavus and A. alternata MLBM09. Inhibition of the fungal growth required higher concentrations of AmBV compared to concentrations that were required for the inhibition of bacterial strains. Study detected a potent antifungal activity at a concentration of >300 μg mL1 from AmBV. There was a significant increase in the clear zone diameter when fungi were treated with AmBV at concentrations of 300 and 600 μg mL1. Similar to this study, the antifungal activity of AmBV has been evaluated by many other groups. Yu et al.12, demonstrated that AmBV inhibited the growth of Trichophyton mentagrophytes and Trichophyton rubrum by 92 and 32%, respectively. The antifungal inhibitory concentration reported in their study was 0.63 ppm which was higher than the current study. Similarly, BV has been reported to inhibit the growth of C. albicans and C. krusei at concentration of 60 to 125 μg mL–1 9,36.

Although, AmBV significantly decreased the growth of the tested bacteria and fungi, there were variations in antimicrobial potency and the inhibitory concentrations of AmBV between different bacterial and fungal strains. AmBV was more efficient in inhibiting the growth of E. coli ATCC8739, S. marcescens AUH 98 and S. mutans ATCC 25175 compared to S. aureus ATCC 6538P. As noted in the antibacterial activity of AmBV, there were also variations in the antifungal activities of AmBV. A. flavus and A. niger ATCC 16404 were the most sensitive to AmBV treatment followed by F. oxysporum MLBM212 and finally A. alternata MLBM09.

Variations in the antibacterial and antifungal potency of AmBV between the tested bacterial and fungal strains could be attributed to the nature of each microbial strain or the mechanism by which AmBV inhibits the growth of each microbial strain. AmBV contains a wide range of bioactive molecules that could exploit different strategies to inhibit each microbial strain37,38. Similarly, melittin which is one of the major components of AmBV is more active against gram-positive bacteria than gram-negative ones39. Similarly, PLA2 of AmBV inhibited the growth of Lactobacillus casei at a MIC value of 400 mg mL1, however, it didn’t yield any satisfactory antibacterial effect against the growth of Streptococcus salivarius, S. sobrinus, S. mutans, S. mitis, S. sanguinis and Enterococcus faecalis32. Taken together variations in the antibacterial and antifungal potency of AmBV and its bioactive molecules could be exploited to develop a microbe-specific antimicrobial agent to avoid the side effects associated with the use of broad-spectrum antimicrobial agents on the beneficial normal flora.

CONCLUSION

Microbial diseases are the most prevalent health challenge particularly in developing countries due to drug resistance, high cost and high risk of synthetic and semisynthetic antibiotics. Therefore, new antimicrobial agents are in need to control microbial diseases. Natural products like BV are considered efficient alternatives to synthetic and semisynthetic antibiotics and a promising source for the discovery of new antimicrobial agents as they contain a variety of antimicrobial bioactive compounds. In this study, the antibacterial and antifungal activities of AmBV against medically important bacterial and fungal strains were demonstrated. AmBV significantly inhibited the growth of the bacterial and fungal pathogen, in vitro. There were variations in antimicrobial potency of AmBV between microbial strains that may use in a future study to invent new antimicrobial agents that have no side effects on the beneficial normal flora. This study provides a perspective on new antibacterial and antifungal therapeutic approaches using AmBV. Results from this study may, thus, could be utilized to develop cost-effective and efficient antibacterial and antifungal therapeutic agents.

SIGNIFICANCE STATEMENT

This study discovered that AmBV has strong antibacterial and antifungal activities against many medically important pathogens. This study will help researchers to exploit the antimicrobial activity of AmBV in future preclinical and clinical studies to develop cost-effective and nontraditional antibacterial and antifungal agents.

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