Essential Oils from the Fruits and Leaves of Spondias mombin Linn.: Chemical Composition, Biological Activity, and Molecular Docking Study

This work focused on characterizing the chemical constituents and evaluating the antioxidant and antimicrobial activities of the essential oils obtained from the fruit and leaves of Spondias mombin—a flowering plant of the Anacardiaceae family. Essential oils were extracted through steam distillation and characterized by gas chromatography-mass spectrometry. For the fruit essential oil, 35 compounds were obtained, and 25 compounds were identified in the leaf essential oil. The dominant compounds present in the fruit essential oil were (E)-ethyl cinnamate (14.06%) and benzyl benzoate (12.27%). Methyl salicylate (13.05%) and heptacosane (12.69%) were the abundant compounds in the leaf essential oil. The antioxidant activity of the essential oils was evaluated via phosphomolybdenum, hydrogen peroxide scavenging, 2, 2-diphenyl-1-picrylhydrazyl (DPPH) free radical scavenging, and thiobarbituric acid reactive substances (TBARS) assays. The total antioxidant capacity of fruit and leaf essential oils was 48.5 ± 0.7 μg/gAAE and 48.5 ± 0.7 μg/g AAE, respectively. The half maximal scavenging concentrations of the essential oils in the hydrogen peroxide; DPPH and TBARS assays ranged from 252.2 μg/mL to 2288 μg/mL. The antimicrobial activity of the essential oils was tested using broth dilution and disc diffusion assays against eight microorganisms. The essential oils exhibited broad-spectrum antimicrobial activity against the microorganisms with minimum inhibitory concentrations of 9.75–50 mg/mL. Also, the zones of inhibition of the oils ranged from 12 mm to 25 mm. The biofilm inhibitory activities of the oils were dose-dependent with BIC50 values of 42.49 ± 0.1 mg/mL and 97.34 ± 0.6 mg/mL for fruit and leaf essential oils, respectively. Molecular docking studies revealed that the antibiofilm action of the fruit and leaf essential oils could be due to inhibition of the quorum sensing protein, LasR. The results suggest a possible application of the oils as antioxidant and antimicrobial agents.


Introduction
Essential oils are aromatic oily liquids made up of mixtures of volatile compounds and usually represent a small fraction of a plant's composition. ese oils are strongly scented and have a lower density in comparison to water [1]. e aroma of each oil results from the combination of the aromas of all components, with minor oil constituents, even playing critical roles [2]. Essential oils can be isolated from all plant organs-fruits, leaves, stem bark, twigs, and roots-and are mainly composed of terpenes, fatty acids, phenols, alcohols, ketones, and aldehydes [3]. Essential oils have a wide range of biological activities such as antimicrobial, antioxidant, antifungal, and anti-inflammatory activities, and these activities have been attributed to the individual components in the essential oils. Due to the importance of essential oils, they have wide applicability in the food, cosmetic, and fragrance industries.
Essential oils are able to mop up free radicals and hence suppress the action of reactive oxygen and nitrogen species in various matrices. Free radicals, including hydroxyl, superoxide, and nitric oxide radicals, react with molecules in biological systems, leading to oxidative stress. Oxidative stress can cause damage to biologically relevant molecules such as DNA, proteins, carbohydrates, and lipids and has also been implicated in diabetes and neurological malfunctions [4]. e actions of free radicals also cause lipid peroxidation, and this can lead to a significant reduction in food quality [5]. In general, antioxidants function as radical scavengers and inhibit lipid peroxidation and other free radical-mediated processes. As such, they can protect the human body as well as processed foods from oxidative damage. Butyl hydroxytoluene (BHT) and butylated hydroxyanisole (BHA) are synthetic antioxidants that are widely used in the food industry to overcome the action of some free radicals, yet they have not been wholly received by consumers due to negative perceptions about synthetic chemicals and toxicity [6]. ere is therefore a high demand for new agents from natural sources to replace some of these synthetic antioxidants. e use of plant-derived antioxidants, such as those containing phenolic substances like flavonoids and phenolic acids in foods, as well as therapeutic medicine, is gaining much recognition. Essential oil components such as phytol and menthol have also been reported to possess antioxidant properties, making their use a potential route for curbing free radical-mediated challenges.
Essential oils and their components have also shown significant activity against microorganisms. Microorganisms are the major drivers of the emergence and reemergence of various infectious diseases. Microbial resistance to existing antimicrobial agents and the absence of new compound scaffolds in the antimicrobial drug pipelines has prompted an urgent need for innovative solutions to this menace. Resistance to the effects of antimicrobial agents occurs due to microorganisms developing strict mechanisms such as making their cell membrane impermeable to drugs, changing drug target sites, or producing enzymes that may degrade antibiotics. Biofilm formation and spore-forming capacity are additional strategies that help the microorganisms to survive in harsh conditions [7]. In the formation of biofilm, microorganisms rely on quorum sensing (QS).
is event enables bacteria to express virulence factors such as pyocyanin and pyoverdine. In Pseudomonas aeruginosa, QS is regulated by various proteins that are part of a complex structure. e transcriptional activator protein, LasR, sits at the top of the QS hierarchy as it is a primary protein responsible for the activation of the other QS systems, as well as a key player in biofilm formation and virulence genes activation. Inhibition of LasR could interfere with QS and hence biofilm formation [8]. Downregulation of QS, and thus, inhibition of biofilm formation, has therefore been suggested as an innovative approach to tackle the antimicrobial resistance menace. Antimicrobial drugs that interfere with QS and impede biofilm formation are therefore desired. Essential oils, such as those obtained from Chrysophyllum albidum and Synsepalum dulcificum, have been shown to possess antimicrobial and antibiofilm activities [9,10]. Essential oil constituents such as p-cymene, thymol, eugenol, and carvacrol have also been shown to possess antibiofilm and anti-QS activities [11]. Essential oils could therefore be integral in developing new strategies for antimicrobial resistance.
Spondias mombin Linn. (S. mombin) is a flowering plant that belongs to the Anacardiaceae family. e fruits of the plant have leathery skin and a thin layer of pulp, and this has been used in making jelly, juice, jams, and ice cream. e fruit pulp of S. mombin is rich in potassium, magnesium, phosphorus, and copper, and these confer high nutritional and functional value [12]. S. mombin fruits are used in local medicinal practices for managing ailments such as stomachache, toothache, diarrhea, cough, sore throat, nausea, leprosy, and fungal infections [13]. It has been reported that extracts from the leaves of S. mombin exhibit antimicrobial, leishmanicidal, antiviral, hypoglycemic, and antioxidant properties [14]. A concoction from S. mombin leaves is widely used for the treatment of diarrhea, dysentery, stomachache, and inflammation [15]. e leaves are also used in folk medicine for the treatment of several topical and systemic diseases like inflammation of the mouth and throat [16]. e essential oils from S. mombin from different countries have been reported in other studies, with marked differences in chemical composition. In Nigeria, both Olufunke and Oladimeji analyzed essential oils from S. mombin leaves, and in both cases, terpenes such as β-caryophyllene and c-cadinene were the dominant constituents [17,18]. In Brazil, different studies have reported alkanes and terpenes as the major constituents in S. mombin leaf and fruit essential oils [19][20][21]. Since essential oil composition is influenced by environmental conditions such as temperature and light, and cultivation conditions like soil type and soil properties [22], essential oils from the fruits and leaves of S. mombin from Ghana were analyzed in this study. e antioxidant, antimicrobial, and biofilm inhibitory activities of the essential oils were also evaluated in different assays. Molecular docking was used to investigate the interactions between the constituents of the oils and the LasR protein, as a means of shedding light on molecular events that may be implicated in biofilm inhibition. Even though many Gram-positive and Gram-negative bacteria form biofilms, biofilm formation in P. aeruginosa is well-characterized and the organism is widely used in many studies as a model biofilm-forming organism [23,24]. P aeruginosa was therefore used in this work to study biofilm and QS inhibition capabilities of the essential oils.

Sample Collection.
Fruits and leaves of S. mombin were collected in August 2020 from a farm at Ahinsan (6°40′04.8″N 1°35′28.6″W) in the Ashanti Region of Ghana. e samples were authenticated at the Herbarium Section of the Department of Herbal Medicine, Kwame Nkrumah University of Science and Technology (KNUST). Voucher specimen identification codes were generated for the fruit (KNUST/HMI/2021/FR002) and the leaves (KNUST/HMI/ 2021/L013) of the plant, after which specimens were deposited in the herbarium.

Sample Preparation.
e fruits of S. mombin were washed under running water to remove any debris. e pulp of the fruits was separated from the seeds, placed in plastic bags, sealed, and stored at 4°C till extraction. e leaves were washed and air dried under ambient temperature for about 5 days before extraction. Fruits and leaves of S. mombin were subjected to steam distillation using the Clevenger apparatus for 3 hours. e oils were concentrated under a vacuum and dried with anhydrous Na 2 SO 4 . e oils were then weighed, and their respective percentage yields were calculated using % Yield of oil � Mass of oil Mass of sample used × 100. (1)

Gas Chromatography-Mass Spectrometry.
e composition of the essential oils was analyzed on a gas chromatography-mass spectrometry system (Perkin Elmer GC Clarus 580 Gas chromatograph with a Perkin Elmer (Clarus SQ 8 S) mass spectrometer). e mass analyzer of the system was quadrupole. GC-MS conditions were the same as that reported in earlier works from our group [25,26]. e total GC-MS run time was 34.5 min.

Compound Identification.
To identify the compounds present in the essential oils, the mass spectra obtained from the GC-MS analyses were compared to the mass spectra of compounds housed in the National Institute of Standard and Technology (NIST) and Wiley mass spectra databases. Assignment of compound names was made based on the similarity indices with compounds in the NIST and Wiley repositories used in the GC-MS system, as well as spectral data from some published literature [27]. e relative percentages of the various constituents were expressed as percentages calculated by normalization of the peak area.

Antioxidant Activities.
e antioxidant activities of the fruit and leaf essential oils of S. mombin were assessed using the phosphomolybdenum, 2,2-diphenyl-1-picrylhydrazyl (DPPH) radical scavenging, hydrogen peroxide scavenging, and inhibition of lipid peroxidation assays.

Total Antioxidant Capacity (TAC).
e phosphomolybdenum assay was used to evaluate the total antioxidant capacity of the essential oils. e method used was the same as that used by Afu et al. [28]. Absorbances were measured on an Analytik Jena Specord 200 Plus (Germany) against a blank solution.
e standard drug used in the assay was ascorbic acid. Equation (2) was used to compute the TAC (in ascorbic acid equivalent).
where M represents essential oil mass (g) in the reaction mixture, V is the total volume (mL) of the reaction mixture, and C is the concentration of ascorbic acid used (μg/mL).

DPPH Free Radical Scavenging
Activity. e method used by Gyei and coworkers was used in assessing the DPPH free radical scavenging activity of the essential oils [25]. Different concentrations of the oils were prepared in 5% DMSO. e total reaction volume was 200 μL (DPPH solution, 0.1 mM, 150 μL, and essential oil, 50 μL). Incubation of the mixture was done in the dark for a period of 30 minutes, followed by absorbance measurements of 517 nm on an Analytik Jena Specord 200 Plus spectrophotometer (Germany). e reaction blank was made by using methanol to replace essential oils in the reaction. Positive control for the assay was ascorbic acid. e DPPH scavenging capacity of the essential oils was calculated using where Asample is the absorbance of the test sample and Acontrol is the absorbance of the blank. e IC 50 values (extract concentration required to scavenge 50% of DPPH radicals) were obtained from a graph of % inhibition against concentration.

Hydrogen Peroxide Scavenging Assay.
In this assay, 130 μL of a 5 mM solution of hydrogen peroxide was added to 500 μL of a 1 mM solution of (NH 4 ) 2 Fe(SO 4 ) 2 ·6H 2 O. After this, 3 mL of various concentrations of essential oil or gallic acid (which was used as standard) was added to the mixture and incubated for 30 mins in the dark at ambient conditions. To this mixture was added 1,10-phenanthroline (3 mL, 1 mM). is mixture was uniformly mixed by vigorous shaking, incubated for another 10 mins, and the absorbance of the reaction was measured at 510 nm (Specord 200 Plus, Germany). Water was used in place of essential oils for the blank. Equation (4) was used in computing the percent hydrogen peroxide scavenged. % Hydrogen peroxide scavenged � Atest Acontrol × 100, where Atest is the absorbance of the test sample and Acontrol is the absorbance of the blank. e IC 50 values (extract concentration required to scavenge 50% of hydrogen peroxide radical) were obtained from a graph of % inhibition against concentration [29].

Inhibition of Lipid Peroxidation (TBARS Assay).
For the inhibition of lipid peroxidation assay, Nartey and coworkers' method was employed for this work. e oxidable substrate used for this work was egg yolk. Absorbance measurements were taken at 532 nm (Specord 200 Plus, Germany). Positive controls were butylated hydroxytoluene (BHT) and ascorbic acid. e percentage inhibition of lipid peroxidation was calculated from the absorbance obtained using equation (3). e IC 50 values (extract concentration required to achieve 50% inhibition of lipid peroxidation) were obtained from a graph of % inhibition against concentration [24].

Data Analysis.
Triplicates of all the experiments were made, and the mean and standard deviations were computed. All statistical analyses were made using the GraphPad Prism software 6.0 for Windows (GraphPad Software, San Diego, CA, USA). When p < 0.05, it was considered as being statistically significant. . Candida albicans which is a fungus was also used. All microorganisms were obtained from the Department of Pharmaceutics, KNUST. e bacterial strains were cultured at 37°C in nutrient broth overnight, whereas sabouraud dextrose agar was used in culturing C. albicans. Microbial cultures were streaked on nutrient agar (Oxoid, UK) plates and incubated at 37°C for 18-24 h. A colony suspension was made in sterile saline, adjusted to 0.5 McFarland standard before further diluting it in sterile double-strength nutrient broth to obtain a concentration of about 2 × 10 5 CFU/mL.

Minimum Inhibitory Concentrations (MIC).
e broth dilution method was employed in determining the minimum inhibitory concentrations (MICs) of the essential oils. Twofold serial dilution (100 μL) of the essential oil or standard antibiotic (ciprofloxacin) was prepared in sterile 96-well microtiter plates. To each well, 100 μL of appropriate microorganisms in double-strength nutrient broth was added. Following a 24-hour incubation of plates at 37°C, 20 μL of 1.25 mg/mL 3-(4, 5-dimethylthiazol-2-yl)-2,5diphenyltetrazolium bromide solution (MTT) was added to each well. is was then incubated for 30 min at 37°C. e lowest concentration of test essential oil or standard antibiotic that completely inhibited the growth of the organism as detected by the absence of the purple coloration after MTT addition during a 24-hour incubation period at 37°C was defined as the MIC. Triplicate of each test was performed [30].

Zones of Inhibition.
e zones of inhibition of the essential oils were measured in the agar disc diffusion assay. A suspension containing ∼2.0 × 10 5 CFU/mL of the microorganism was spread on agar media in agar plates. Filter discs were prepared by individually soaking each disc in 30 μL of 30 mg/mL essential oil or 10 μg/mL standard drug. e discs were then impregnated onto the agar plates that had previously been inoculated with the test microorganisms. Discs with solvents, instead of essential oils, were used as the negative control. Ciprofloxacin was used as the standard drug. Plates were incubated at 37°C for 24 hours. Zones of inhibition were measured to assess the antimicrobial activity against each test organism [30].

Biofilm Inhibition.
Biofilm inhibitory activities of test essential oils were determined in the crystal violet staining assay. Sterile microtiter plates were filled with 100 μL of MIC and sub-MIC concentrations of test essential oils or gentamicin (used as standard). e bacterial suspension (at 0.5 McFarland standard) was then added to each well to make a total volume of 200 μL. A control experiment, in which solvent was used in place of essential oils, was also set up using the same procedure. e plates were incubated for 24 hours at 37°C, and thereafter, the content of the wells was discarded.
is was followed by washing 3 times with deionized water to remove loosely attached cells. Crystal violet (0.1%) was used to stain each well, followed by elution with 30% acetic acid into a new microtiter plate. e absorbances were read at 595 nm (Specord 200 Plus, Germany). Biofilm inhibition was estimated using equation (3). e BIC5 0 values (drug concentration required to inhibit biofilm formation by 50%) were obtained from a graph of % inhibition against concentration [31].

Molecular Docking Studies.
e 3D structure of LasR was obtained from the Protein Data Bank with the PDB code 6V7X [32]. e protein was cocrystallized with the native substrate N-3-oxo-dodecanoyl-l-homoserine lactone and a quorum sensing antiactivator protein AQS1. Prior to docking, the protein was prepared using AutoDockTools-1.5.7rc1. Cocrystallized ligands and water molecules were removed, Gasteiger charges were calculated for atoms, and polar hydrogens were added [33]. e output file was saved in the pdbqt format. Most abundant compounds identified in the fruit and leaf essential oils and compounds that have been reported in the literature to possess antimicrobial activities were used in the molecular docking study. e compounds used from the fruit were (E)-ethyl cinnamate, benzyl benzoate, n-hexadecanoic acid, cis vaccenic acid, geraniol, methyl eugenol, terpineol, linalool, a-amyrin, and caryophyllenyl alcohol. For the leaves, hexan-1-ol, 2methoxy-4-vinylphenol, heptacosane, methyl salicylate, humulene, caryophyllene, longifolene, n-hexadecanoic, and aromadendrene oxide were considered. e 3D structures of the compounds were modeled and optimized in Spartan '14 using quantum mechanical methods [34]. To validate the docking protocol in precision docking, the autoinducer AHL was redocked in the ligand-binding domain of LasR. Validation was confirmed based on low RMSD (<2Å) of the redocked ligand from the orientation of the cocrystallized ligand and the reproduction of observed interactions from the pdb structure [35]. For the compounds, an initial blind docking was performed using PyRx, with an AutoDock Vina extension.
is was done to identify the regions on the protein that the ligands preferred to bind. e grid box was defined to cover the whole protein in this blind docking. Compounds that bound in the ligand-binding domain of LasR after blind docking were later subjected to precision docking to probe further into the protein-ligand interactions using the following grid dimensions: center-X � 20.
Results from the phosphomolybdenum assay estimated the total antioxidant capacity of the fruit and leaf essential oils as 48.5 and 83.5 μg/g AAE, respectively. e half maximal concentration of the fruit essential oil required for scavenging hydrogen peroxide (IC 50 ) was 352.2 ± 0.5 μg/mL and that of the leaf essential oil was 947.2 ± 0.6 μg/mL. e fruit essential oil was therefore a better hydrogen peroxide scavenger compared to the leaf oil. Gallic acid, with an IC 50 of 9.1 ± 1.3 μg/mL, was used as the standard in this assay. In the DPPH assay, the IC 50 values for the fruit and leaf essential oils of S. mombin were 2112 ± 0.8 μg/mL and 2063 ± 0.7 μg/mL, respectively. Ascorbic acid was used as the standard drug in this assay and its IC 50 was 14.30 ± 4.3 μg/ mL. In the TBARS assay, the fruit essential oil showed better activity in the inhibition of lipid peroxidation compared to the leaf essential oil with IC 50 values of 1294.0 ± 1.0 μg/mL and 2288.0 ± 0.6 μg/mL for fruit and leaf, respectively. e IC 50 value of butylated hydroxytoluene (BHT) used in this assay as the standard was 9.2 ± 1.7 μg/mL. Table 4 summarizes the antioxidant activities of the fruit and leaf essential oils of S. mombin. e antimicrobial activities of the fruit and leaf essential oils of S. mombin were evaluated against a panel of microorganisms using both broth dilution and agar disc diffusion methods. e fruit essential oil exhibited zones of inhibition against the tested microorganisms at diameters ranging from 12 mm to 25 mm. e Gram-positive bacteria, S. aureus and S. pneumoniae, were the most susceptible microorganisms against the fruit essential oil with zones of inhibition of 25 mm and 21 mm, respectively. e fungus, C. albicans, recorded a lower zone of inhibition of 12 mm. For P. aeruginosa, a Gram-negative bacterium, no zone of inhibition at the concentration of essential oil tested was recorded. e zones of inhibition of the leaf essential oil against S. pneumoniae and K. pneumoniae were 17 mm and 12 mm, respectively. However, the leaf essential oil showed no zones of inhibition against S. aureus, P. aeruginosa, or C. albicans (Table 5). e MICs for the essential oils ranged from 9.75 mg/mL to 50 mg/mL ( Table 6). S. pneumoniae, K. pneumoniae, and E. coli were the most susceptible organisms to the fruit essential oil with an MIC of 9.75 mg/mL in all cases. A concentration of 19.5 mg/mL of the fruit essential oil was required to inhibit the growth of S. aureus, B. subtilis, E. faecalis, and C. albicans. Other than S. aureus and P. aeruginosa, the leaf essential oil was able to inhibit the growth of all tested microorganisms at 23 mg/mL. S. aureus was the least susceptible microorganism against the leaf essential oil with its MIC above the concentration tested. e biofilm inhibitory activity of the essential oils was assessed using the crystal violet staining assay with P. aeruginosa as the test organism. ere was over 40% inhibition of biofilm formation at all concentrations of leaf and fruit essential oils tested. e maximum biofilm inhibition was observed at the MIC for both fruit and leaf essential oils at 62% and 59%, respectively (Table 7). e concentration of the fruit essential oil required for 50% inhibition of biofilm formation (BIC 50 ) was 42.49 ± 0.1 mg/mL, which was better than that of the leaf essential oil (BIC 50 of 97.34 ± 0.6 mg/mL).
Selected compounds present in the leaf and fruit essential oils of S. mombin were docked against the LasR protein. is was done to investigate the potential of the docked compounds in modulating the activity of LasR in order to explain the observed anti-biofilm activity. LasR has two domains: an N-terminal ligand-binding domain (LBD) and a C-terminal DNA-binding domain (DBD) (Figure 3(a)). LasR is stabilized and dimerized when its autoinducer 3-oxo-C12-homoserine lactone binds to it. e resultant LasR-AI homodimer complex then attaches to the target DNA promoter and leads to the stimulation of gene transcription. From the crystal structure, the autoinducer interacted with LasR via hydrogen bonding to Trp60, Asp73, Tyr39, Ser129, and hydrophobic interactions with Val76, Cys79, Leu125, and Ala127. Redocking of the cocrystallized acyl-homoserine lactone (AHL) gave a binding affinity of 8.6 kcal/mol. Observed interactions in the redocked structure were hydrogen bond contacts with Trp60, Asp73, r75, and Ser129 and hydrophobic contacts with Val76, Cys79, and Leu125. Together, these made up 86% of the reproduced interactions. e root mean squared deviation (RMSD) of the redocked conformation compared to that obtained from pdb was 1.158 Ả (<2 Ả), confirming the docking protocol to be valid for further studies (Figure 3(b)). e selected ligands were docked to LasR in a blind docking experiment. From the blind docking results, it was      Evidence-Based Complementary and Alternative Medicine linalool (Figure 4(a)). ese compounds were subjected to precision docking to probe further into the protein-ligand interactions. Benzyl benzoate formed hydrogen bond contacts with Asp73, r75, and r115 and hydrophobic interactions with Leu36, Tyr64, Asp73, Val76, Ala105, Leu110, Ser129, and Ile52 with a binding affinity of −10.1 kcal/mol. (E)-ethyl cinnamate also had a binding affinity of −7.8 kcal/mol while establishing hydrophobic interactions with Trp88, Phe101, Ala101, and Leu110. Geraniol established hydrogen bonds with r75 and hydrophobic interactions with Leu36, Tyr56, Tyr64, Trp88, Phe101, Ala105, Trp88, and Leu110 with a binding affinity of −6.7 kcal/mol. Methyl eugenol had a binding affinity of −6.8 kcal/mol and formed hydrophobic interactions with Tyr56, Tyr64, Asp73, Trp88, Ala105, and Leu110. With a binding affinity of −7.4 kcal/mol, terpineol established hydrogen bond interaction with Asp73 and hydrophobic interactions with Tyr64, Trp88, Leu110, Ala105, and Phe101. Linalool also had hydrogen bond contact with Ser129 and hydrophobic contacts with Trp88, Phe101, Ala105, and Leu110 with a binding affinity of −6.6 kcal/mol. A summary of the interactions between the compounds and LasR has been provided in Table 8 and Figure 4.

Evidence-Based Complementary and Alternative Medicine
Methyl salicylate established hydrogen bond interactions with Tyr56, r75, r115, Ser129 and hydrophobic contacts with Leu36, Tyr64, Asp73, and Trp88 with a binding affinity of −6.9 kcal/mol, as shown in Table 8 and

Discussions
Essential oils have been isolated from different plant organs like fruits, leaves, stem bark, twigs, and roots. In this study, steam distillation was utilized in the extraction of essential oils from fruits and leaves of S. mombin. e yields of essential oils from the fruits and leaves were 0.07% and 0.06%, respectively. e yields obtained were higher in comparison with the yields reported by de Assis (0.03% and 0.002% for leaves and fruits, respectively) where hydrodistillation was used in the extraction. e yield obtained for the leaf essential oil was also higher than that obtained by Olufunke et al. (0.002%) who subjected fresh leaves to hydrodistillation [17]. e variation in yield may be due to the different methods of extractions used. It has been reported that steam distillation gives a higher yield of essential oils in comparison to hydrodistillation [36]. It could also be due to differences in harvesting seasons and variations in the genetic make-up of the different cultivars [37].
Essential oils are essential in the sense that they contain the essence of the different fragrances and the properties of the plants from which they are obtained [38]. Essential oils are mainly composed of terpenes, fatty acids, phenols, alcohols, ketones, and aldehydes. Gas chromatography coupled with a mass spectrometer (GC-MS) was used to identify the compounds present in the essential oils. e most abundant compound in the leaf essential oil was methyl salicylate.
is compound was reported to be present in studies carried out by both Santos and Olufunke [17,21]. Olufunke and Oladimeji identified caryophyllene as the major component in the leaf essential oil (Table 9) [17,18]. Even though present in the leaf essential oil in this study, caryophyllene (6.77%) was not the most abundant compound. Other compounds like humulene, naphthalene, and aromadendrene present in this study were also found in the leaf essential oil of S. mombin from the other works [20,21]. For the fruit essential oil, the most dominant compounds were (E)-ethyl cinnamate and benzyl benzoate. Terpineol, which was identified as one of the major components in Santos' work, was present in this study as well. e class of compounds dominant in the fruit essential oil was esters while alkanes dominated in the leaf essential oil. e difference in chemical composition in the fruits and leaves may be due to the nutritional status of the plant as well as genetic and environmental factors [39].
Essential oils exhibit biological properties including antimicrobial, anti-inflammatory, antioxidant, and   Data presented as mean ± standard deviation, n � 3; concentrations of essential oils or gentamicin used were based on their minimum inhibitory concentration (MIC) against P. aeruginosa; * gentamicin was used for comparison purposes.
Evidence-Based Complementary and Alternative Medicine 9 antimalarial. In nature, essential oils play an important role in the attraction of insects to promote the dispersal of pollens and deter herbivores from feeding on plants by reducing their appetite for plants [40]. e antioxidant activity of essential oils is a biological property of great interest because they may preserve foods from the toxic effects of oxidants [41]. Also, if essential oils can scavenge free radicals, they may play an important role in the prevention of some diseases. e antioxidant activities of the oils were therefore analyzed using various assays (Table 4). e leaf essential oil showed a better total antioxidant capacity compared to the fruit essential oil. In the hydrogen peroxide scavenging assay, the fruit essential oil had a higher scavenging ability than the leaf essential oil. However, the leaf essential oil was observed to be a better DPPH radical scavenger compared to the fruit essential oil. Lipid peroxidation is a complex reaction that can be generated through different pathways [3]. In assessing lipid peroxidation, several lipids' substrates like oils, fats, and fatty acid methyl esters have been used. In this work, the ability of essential oils to inhibit 50% of lipid peroxidation was assessed using the TBARS assay with egg yolk as the substrate. From the results, the fruit essential oil showed a better inhibitory activity compared to the leaf essential oil. Esters and acids have been reported to possess antioxidant activity. Hence, the high antioxidant activity of the fruit essential oil compared to the leaf essential oil may be due to the high composition (63%) of esters and acids in the fruit essential oil. Compounds such as linalool, geraniol, and palmitic acid have been reported to possess antioxidant activity and may be great contributors to the antioxidant activity of the fruit essential oil [42]. e multicomponent chemical composition and complex mechanism of action of essential oils on different bacterial sites make it difficult for bacteria to develop resistance to them [43]. Terpenes such as p-cymene have been shown to cause membrane permeability of bacteria by taking part in membrane swelling. Once the membrane becomes permeable, other essential oil components which target internal organelles (like carvacrol) can then act. is synergy permits the inhibition of the growth of microorganisms [44]. e fruit and leaf essential oils of S. mombin showed different activities against tested microorganisms in the antimicrobial assays. S. mombin fruit essential oil showed the greatest activity against S. pneumoniae and K. pneumoniae with an MIC of 9.75 mg/mL. In addition, high zones of inhibition were observed for these microorganisms in the agar disc diffusion assay. e leaf essential oil did not show any zone of inhibition or MIC against S. aureus within the concentrations tested. In general, it was observed that the fruit essential oil exhibited a better antimicrobial activity compared to the leaf essential oil. is may be due to the presence of linalool [45], geraniol [46], and methyl eugenol [47] in the fruit essential oil which have been reported to possess antimicrobial activities. Bacteria can escape the lethal effects of antimicrobials through the formation of  biofilm.
erefore, inhibiting biofilm formation is a potential route for eliminating bacteria. e biofilm inhibitory activities of the fruit and leaf essential oils were therefore investigated. From the results, the essential oils showed moderate activities with BIC 50 values of 42.49 ± 0.1 mg/mL and 97.34 ± 0.6 mg/mL for fruit and leaf essential oils, respectively. It was observed that the biofilm inhibition of both oils was dose-dependent, and inhibition increased with increased concentration. is trend was also observed in a study conducted by Nartey et al. in 2021 [9][10][11][12][13][14][15][16][17][18][19][20][21][22][23][24][25][26]. Essential oils from Chrysophyllum albidum, Averrhoa carambola, and several plants have been shown to inhibit biofilm formation. Previous studies have also reported the antibiofilm activities of compounds such as linalool, geraniol, methyl eugenol, and methyl salicylate. ese compounds were also identified in the fruit and leaf essential oil and can contribute greatly to its biofilm inhibitory activity. To understand how the compounds in the fruit and leaf essential oils potentially contributed to biofilm inhibition, molecular docking was employed.
Molecular docking was used to predict the binding of the compounds against LasR, a protein that plays a key role in biofilm formation in P. aeruginosa. LasR is made up of two protein domains: an amino-terminal ligand-binding domain and a carboxy-terminal DNA-binding domain. In solution, the LasR ligand-binding domain occurs as a homodimer. A long loop, L3, comprising residues Leu40 through Phe51 in the ligand-binding domain, covers the pocket and sequesters the ligand inside the receptor's core, away from the solvent. Residues, such as Tyr56, Trp60, Ser 129, and Asp73, form hydrogen bond contacts with the head group of the autoinducer. A number of hydrophobic residues, including Leu36, Leu40, Ile52, Val76, and Leu125, engage the hydrophobic tail of the N-3-oxododecanoyl homoserine lactone through van der Waals interactions at the other end of LasR's ligand-binding pocket. In the absence of the autoinducer, the loss of these beneficial interactions would presumably result in loop flexibility and subsequent exposure of the buried hydrophobic residues in this pocket to bulk solvent, causing protein aggregation. Similarly, the lack of the autoinducer's interaction with the hydrophobic residues would jeopardize the integrity of the beneficial hydrophobic contacts, resulting in an unstable complex [48].
Of the 10 compounds selected from the fruits for docking, 6 of them had a binding preference for the ligandbinding domain of LasR. Stronger interactions by the six compounds with pocket residues, coupled with their high binding affinities, could probably be responsible for the antibiofilm property of the fruit essential oil. Notably, benzyl benzoate and (E)-ethyl cinnamate, the most abundant compounds in the fruit essential oil, had the highest binding affinities with values of −10.1 kcal/mol and −7.8 kcal/mol, respectively, making them the major probable contributors to antibiofilm action. e other four compounds (geraniol, methyl eugenol, terpineol, and linalool) could collectively contribute to the antibiofilm activity of the fruit essential oil as seen in their binding affinities. From the leaf essential oil, three compounds (2-hexan-1-ol, 2-methoxy-4-vinylphenol, and methyl salicylate) were well accommodated in the ligand-binding domain of LasR while making strong interactions with pocket residues. Observations of the binding affinities of the compounds and their interactions with some key residues in the active site of LasR suggest that the compounds could elicit their biological activity by inhibiting LasR. e abundance of methyl salicylate in the leaf essential oil and its strong affinity for LasR could play a major role in the antibiofilm action, with 2-hexan-1-ol and 2-methoxy-4vinylphenol fairly contributing to inhibition. e compounds from the fruit essential oil had higher binding affinities for LasR compared to the compounds from the leaf essential oil. is may be the reason the antibiofilm activities of the fruit essential oil observed in vitro were better in comparison to the leaf essential oil.

Data Availability
All data generated or analyzed during this study are included within the article.

Conflicts of Interest
All authors declare no competing financial, professional, or personal interest that might have influenced the performance or presentation of the work described in this manuscript.