Antibacterial Activity of Fructus forsythia Essential Oil and the Application of EO-Loaded Nanoparticles to Food-Borne Pathogens

Fructus forsythia essential oil (FEO) with excellent antibacterial activity was rarely reported. The objective of the present study was to investigate the antibacterial activity and the antibacterial mechanism of FEO against two food-borne pathogenic bacteria, Escherichia coli (E. coli) and Staphylococcus aureus (S. aureus) in vitro. When treated FEO, the zones of inhibition (ZOI) of E. coli (20.5 ± 0.25 mm) and S. aureus (24.3 ± 0.21 mm) were much larger than control (p < 0.05). The minimum inhibitory concentrations (MICs) of FEO were 3.13 mg/mL and 1.56 mg/mL for E. coli and S. aureus, respectively. The antibacterial mechanism of FEO against E. coil was due to the changes in permeability and integrity of cell membrane leading to the leakage of nucleic acids and proteins. With the superior antibacterial activity of FEO, the nano-encapsulation method has been applied in FEO. When compared to FEO and blank chitosan nanoparticles, FEO-loaded nanoparticles (chitosan to FEO of 1:1) can effectively inhibit the growth of E. coil above 90% at room temperature. It is necessary to consider that FEO and FEO-loaded nanoparticles will become promising antibacterial additives for food preservative, cosmetic, and pharmaceutical applications.


Introduction
The presence and multiplication of microorganisms in a food system may cause an important problem, which can not only reduce the quality and quantity of food products [1], but also generate the illness and disease [2,3]. Since Escherichia coli (E. coli) was recognized as a food-borne pathogen in 1982, it had been found in variety of foodstuffs [4]. Staphylococcus aureus (S. aureus) was also considered a common pathogen which produced the staphylococcal heat-stable enterotoxins [5]. Food poisoning by E. coli and S. aureus is a growing increase problems in both developing and developed countries. Under these conditions, food preservatives come to prevent food decay and maintain the freshness of the food [6]. Chemical preservatives which are synthesized in a rapid way are generally applied to food preservatives. However, it has been proven that some chemical preservatives had undesirable biological effects in animals and humans leading to immeasurable risks [7]. Currently, compared to at 4 • C and subcultured once a month. E. coli and S. aureus were activated in nutrient broth at 37 • C to a mid-log phase overnight. Before each experiment, the turbidity of the cell suspensions was measured at 600 nm and adjusted to the required concentration using the McFarland standard [22].

Measurement of ZOI
The antibacterial activity of FEO against E. coli and S. aureus was tested by the inhibition zone assay [23]. Sterile discs (6 mm diameter) impregnated with essential oil (3 mg/disc) were air dried and placed on the seeded agar plates. 3 µg Ciprofloxacin per disc was taken as a positive control and sterile 0.9% NaCl solution in 0.5% Dimethyl sulfoxide (DMSO) was taken as blank control. The plates were incubated at 37 • C for 24 h. After incubation, the diameter of the transparent inhibition zone was measured. The experiments were conducted in triplicate under the same conditions.

Measurement of MICs and MBCs
MIC and MBC values were determined using the serial two-fold dilutions method with some modifications [24]. FEO were dissolved in DMSO (0.5% (v/v)) and serially two folds diluted to the final concentration from 0.78 mg/mL to 50 mg/mL. The same volumes of activated E. coli and S. aureus suspension were co-cultured with the essential oil at 37 • C for 24 h. The MIC was defined as the lowest concentration of mixture which inhibited the growth of bacteria. The MBC was defined as the lowest concentration where no visible growth of bacteria was on the agar plate after incubation. Ciprofloxacin was used as positive control.

Time-Kill Curves
Time-kill assays of E. coli and S. aureus treated by FEO (corresponding to control, MIC and 2 MIC) was determined the number of viable cells through a colony counting method in plates [25]. Time-kill curves were constructed by plotting log 10 CFU/mL against time (h).

Scanning Electron Microscope Assay
The changes in bacterial morphology induced by FEO were observed by scanning electron microscopy (SEM) [26]. Overnight E. coli cultures were adjusted to 10 6 CFU/mL using McFarland standard and treated with FEO at different concentrations (corresponding to control, MIC, and 2 MIC) for 4 h. After incubation, the suspensions were centrifuged at 1500g/min for 10 min and washed twice with 0.1 M phosphate buffer solution (PBS, pH 7.4). Then E. coli was fixed in 5% glutaraldehyde for 4 h in dark place. After three washes with PBS, all samples were dehydrated in a sequential graded ethanol (30%, 50%, 70%, 90%, and 100%). Finally, they were sputter-coated with platinum before SEM (Quanta 200 environmental scanning electron microscope system (FEI Company, Hillsboro, OR, USA)).

Crystal Violet Assay
The alteration in membrane permeability was determined by crystal violet assay [27]. After incubation in LB medium at 37 • C for 24 h, E. coli and S. aureus were harvested and washed with PBS (pH 7.4) twice. The pellets were resuspended in sterile 0.9% NaCl solution and mixed with FEO at the concentration from 1/4MIC to 2MIC for 4 h. Cells then incubated with 10 µg/mL crystal violet in the dark for 15 min. After centrifuging, the absorbance of supernatant was determined by measuring the OD 590 nm using a UV-VIS spectrophotometer. The absorbance of crystal violet solution was considered as 100%. The crystal violet uptake was calculated using following formula: % of takeup = (OD of the sample)/(OD of the crystal violet solution) × 100

Measurement of Electrical Conductivity
The leakage of bacterial cells was investigated by measuring the leakage of electrolytes into the incubation medium with a conductivity meter (DDS-307, Precision & Scientific Instrument Co. Ltd., Shanghai, China) according to the method described by [28]. After incubation, the electric conductivities of E. coli and S. aureus suspension was adjusted to the same level of 5% glucose as isotonic bacteria. The FEO mixed with bacteria suspension with different concentrations (corresponding to control, MIC and 2 MIC) were measured the electric conductivities immediately, which was marked as L1. Then the conductivities of the mixtures were measured at 1, 2, 3, 4, 5, 6, 7, and 8 h marked as L2, respectively. The conductivities of boiled bacteria in 5% glucose were marked as L0. Untreated bacteria were served as the control. The relative electric conductivities were calculated using following formula: Relative conductivity (%) = (L2 -L1) L0 × 100

Measurement the Leakage of Cytoplasmic Materials
The cell membrane integrity of E. coli and S. aureus was examined by measuring the release of cell constituents into the supernatant [29]. The suspensions of bacteria were prepared as described above. Different concentrations of FEO (corresponding to control, MIC and 2MIC) were mixed. Untreated bacteria were served as the control. The loss of materials absorbing at 260 nm after 4 h was determined with a UV-VIS spectrophotometer. Correction was made for the absorption of the suspension with the same corresponding concentration of FEO after 2 min with two strains. The untreated cells were corrected with 0.9% NaCl solution in 0.5% DMSO, and the concentrations of proteins in supernatant were determined according to the method described by Xu [30].

SDS-PAGE of Whole-Cell Protein
The degradations of E. coli and S. aureus proteins after FEO treatment were determined by SDS-PAGE [31]. The activated bacteria were treated with FEO at different concentrations (corresponding to control, MIC and 2MIC) at 37 • C for 4 h. After treatment, the suspension were washed twice with PBS buffer and a BCA protein assay kit was used to measure the concentrations of whole-cell protein lysates. Then, the suspension was resuspended in 100 µL of the loading buffer (0.06 M Tris-HCl (pH 6.8), 5% mercaptoethanol, 10% glycerol, 2% SDS, and 0.001% bromophenol blue). The mixtures were boiled for 10 min. The SDS-PAGE was performed with a 5% stacking gel and a 12% separating gel. The gel was then dyed with silver staining.

Preparation of FEO-Loaded Nanoparticles
FEO-loaded chitosan particles were prepared according to the method modified from [32]. CS/TPP nanoparticles were prepared according to the ionotropic gelation process. Briefly, chitosan solution (0.2%, 40 mL) was prepared by dissolving in aqueous acetic acid solution (1% v/v) at room temperature overnight. Tween 80 (1% v/v) was then added to the solution and stirred at 60 • C for 2 h to obtain a homogeneous mixture. FEO (0, 40 mg and 80 mg) was dissolved in CH 2 Cl 2 (4 mL) and homogenized at a speed of 10,000 rpm for 3 min to obtain an oil-in-water emulsion. TPP solution was then dropped into the oil/water emulsion for 1 h. Thereafter, the prepared nanoparticles were isolated by centrifuging at 9000 rpm for about 30 min at 25 • C and washed severally with distilled water (20 mL). Finally, the obtained nanoparticles were stored at 4 • C. The as-prepared nanoparticles with weight ratios of chitosan to FEO (Chitosan: FEO) of 1:0, 1:0.5, and 1:1 were used for the present study.

In Situ Antibacterial Assay of Nanoparticles
The antibacterial properties of FEO and nanoparticles were evaluated with the method according to Bukvički et al. with some modifications [33]. Prepared nanoparticles with chitosan to FEO of 1:0, 1:0.5, and 1:1 were thoroughly mixed with equal amounts of activated E. coli and S. aureus cells, respectively. Experimental teams were divided in three groups: one group was kept at 50 • C, the other at 25 • C, and the last one at the 4 • C. The inhibition percentage at 50 • C, 25 • C (1), and 4 • C (2) were calculated by optical density measured by ELISA plate reader using the following equations: where OD0sample and ODsample corresponded to the absorbance of the strain growth in the presence of the nanoparticles before and after incubation at 612 nm, respectively; OD0blank and ODblank corresponded to the broth medium with dissolved compound before and after incubation, respectively; and OD0growth* and ODgrowth* to the strain growth in the absence of the nanoparticles before and after incubation at 50 • C and 25 • C, respectively. TInhibition corresponded to temperature inhibition of cells at 4 • C, measured according to the formula (3): where ODT0growth and ODTgrowth presented the growth of strain at 4 • C in medium, before and after incubation, respectively.

Statistical Analysis
All values were expressed as mean ± standard deviation (SD) of three experiments. Data were analyzed by using one-way ANOVA test. The photographs of ZOI, SEM, and SDS-PAGE showed in figures were only the representative. In all cases, a value of p < 0.05 was considered statistically significant.

Determination of Antibacterial Activity of FEO
The antibacterial activities of FEO against E. coli and S. aureus were detected by the measurement of the zone of inhibition (ZOI). The diameters of the ZOI against food-borne bacteria were shown in Table 1. The results showed that, the diameters of the ZOI for FEO treated with 3 mg/dis FEO were 20.5 ± 0.25 mm for E. coli and 24.3 ± 0.21 mm for S. aureus, respectively. Positive control (Ciprofloxacin) impregnated with 3 µg/dis were 20.1 ± 0.13 mm and 21.9 ± 0.17 mm, respectively. However, no ZOI was observed for negative control in the plate. The minimum inhibitory concentration (MIC) and minimum bacterial concentration (MBC) of FEO were depicted in Table 1. The MIC value of FEO was 3.13 mg/mL against E. coli and 1.56 mg/mL against S. aureus, respectively. The MBC values were higher than the corresponding MIC values (Table 1). These results showed that the Gram-positive S. aureus appeared more sensitive than the Gram-negative E. coli toward FEO, which was in agreement with the findings of Oussalah who reported that the antimicrobial activities of plant essential oils were more preferred to gram-positive bacterium [34]. Possibly because that Gram-negative bacteria possessed an outer membrane surrounding the cell wall, which restricted the permeation of hydrophobic compounds through lipopolysaccharide coating [35].

Effect of FEO on the Rate of Kill of E. coil and S. aureus
Further antibacterial activity of FEO was assessed by time-kill analysis, which was used to determine the speed of bactericidal activity of antibacterial agents [36]. As shown in Figure 1A,B, treatment with FEO exhibited a strong bactericidal effect on both E. coli and S. aureus, the bacterial population was inactivated within 4 h. A complete loss of viability was observed after 4 h exposure to FEO. These results suggested that the antibacterial activity of FEO was in a concentration-and time-dependent manner.

Effect of FEO on the Rate of Kill of E. coil and S. aureus
Further antibacterial activity of FEO was assessed by time-kill analysis, which was used to determine the speed of bactericidal activity of antibacterial agents [36]. As shown in Figure 1A,B, treatment with FEO exhibited a strong bactericidal effect on both E. coli and S. aureus, the bacterial population was inactivated within 4 h. A complete loss of viability was observed after 4 h exposure to FEO. These results suggested that the antibacterial activity of FEO was in a concentration-and time-dependent manner. Recently, researchers had reported that the constituents of EOs such as terpenes terpenoids, phenylpropenes, carvacrol, and thymol could inhibit the multiplication of food-borne bacteria alone or synergistically [3,31]. It had been proven that there were total of 21 components in the FEO analyzed by GC-MS and monoterpene hydrocarbons and oxygenated monoterpenes were identified the major constituents in FEO [18,37]. Studies showed that oxygenated terpenoids such as alcoholic and phenolic terpenes had more remarkable antimicrobial activity than the other constituents. Many terpenes were known to a broad spectrum of antimicrobial activity, including bacteria and fungi [38]. It might be the main reason why FEO has a broad-spectrum and excellent antimicrobial activity.

Morphological Analysis of E. coli and S. aureus
SEM was used to visually observe the morphology changes of E. coli and S. aureus cells after FEO treatment ( Figure 2). The untreated E. coli cells showed the distinctive striated cell wall (Figure 2A). Their normal morphology (rod shape) was retained. After 4 h of MIC treatment, the surface of the E. coli cell was wrinkled and irregular ( Figure 2B). At the 2MIC level, some cells were damaged, lysing to debris ( Figure 2C). As for S. aureus cells, the untreated bacteria presented the smooth cell membrane ( Figure 2D). In contrast, S. aureus cells treated with FEO at MIC level showed the destruction of the morphology ( Figure 2E). Furthermore, it was obvious to observe that the surface of the cell membrane was collapsed, broken, and lysed at 2MIC level treatment ( Figure 2F). Recently, researchers had reported that the constituents of EOs such as terpenes terpenoids, phenylpropenes, carvacrol, and thymol could inhibit the multiplication of food-borne bacteria alone or synergistically [3,31]. It had been proven that there were total of 21 components in the FEO analyzed by GC-MS and monoterpene hydrocarbons and oxygenated monoterpenes were identified the major constituents in FEO [18,37]. Studies showed that oxygenated terpenoids such as alcoholic and phenolic terpenes had more remarkable antimicrobial activity than the other constituents. Many terpenes were known to a broad spectrum of antimicrobial activity, including bacteria and fungi [38]. It might be the main reason why FEO has a broad-spectrum and excellent antimicrobial activity.

Morphological Analysis of E. coli and S. aureus
SEM was used to visually observe the morphology changes of E. coli and S. aureus cells after FEO treatment ( Figure 2). The untreated E. coli cells showed the distinctive striated cell wall (Figure 2A). Their normal morphology (rod shape) was retained. After 4 h of MIC treatment, the surface of the E. coli cell was wrinkled and irregular ( Figure 2B). At the 2MIC level, some cells were damaged, lysing to debris ( Figure 2C). As for S. aureus cells, the untreated bacteria presented the smooth cell membrane ( Figure 2D). In contrast, S. aureus cells treated with FEO at MIC level showed the destruction of the morphology ( Figure 2E). Furthermore, it was obvious to observe that the surface of the cell membrane was collapsed, broken, and lysed at 2MIC level treatment ( Figure 2F). The morphological alterations in the structure of cell wall and cell membrane were investigated by SEM analysis. The severe morphological alterations on the cells confirmed the FEO possessed excellent antibacterial activities. Meanwhile, the changes of the cell morphology demonstrated the effect of FEO on membrane permeability and integrity. It led to the damage of the bacterial cell wall and cell membrane, and the leakage of intracellular materials was outflowed to the surrounding environment. The results of SEM graphs were in agreement with some research that reported that essential oil could lyse cell walls and cell membranes with decreases of heterogeneity electron density in cytoplasm [31].

Crystal Violet Study
A number of authors had mentioned the antimicrobial activity and antimicrobial mechanism of EOs. It was generally believed that EOs changed the cell cytoplasmic membrane of microorganism. Crystal violet which was generally poorly penetrated the membrane, could easily enter the damaged cell membrane [39]. A significant enhancement in the uptake of crystal violet was observed in Figure 3, the uptake of crystal violet of E. coli and S. aureus were 21.1% and 30.2% in the absence of FEO respectively, increased their signal to 56.4% and 91.5% after FEO treatment at 2MIC. The results of SEM graphs were in agreement with some research that reported that essential oil could lyse cell walls and cell membranes with decreases of heterogeneity electron density in cytoplasm [31].

Crystal Violet Study
A number of authors had mentioned the antimicrobial activity and antimicrobial mechanism of EOs. It was generally believed that EOs changed the cell cytoplasmic membrane of microorganism. Crystal violet which was generally poorly penetrated the membrane, could easily enter the damaged cell membrane [39]. A significant enhancement in the uptake of crystal violet was observed in Figure 3, the uptake of crystal violet of E. coli and S. aureus were 21.1% and 30.2% in the absence of FEO respectively, increased their signal to 56.4% and 91.5% after FEO treatment at 2MIC.

Relative Electrical Conductivity Study
Further antibacterial mechanism of FEO against E. coli and S. aureus was confirmed with the measurement of the relative electric conductivity. As shown in Figure 4, the percentage of the relative electric conductivities of E. coli and S. aureus samples were increased to about 26.2% and 29.7% at the concentration of MIC in the first 4 h, and then reached a relative stable phage in the next 4 h. Compared to the MIC, the percentage of the relative electric conductivity of the suspensions were sharply reached to 50.2% and 41.3% in the first 4 h, and stabilized at a high level in the next 4 h at the concentration of 2MIC. The increase of the relative electric conductivity of samples treated with different concentrations of FEO suggested that the cytoplasmic membranes were disrupted, which caused the leakage of intracellular ingredient, especially losses of electrolytes including K + , Ca 2+ , Na + , and so on [40].

Leakage of Cytoplasmic Materials
The leakage of cytoplasmic material was considered as severe and irreversible damage to the cytoplasmic membrane. Measurement of specific cell leakage markers such as 260 nm absorbing materials and proteins could indicate the changes of membrane integrity compared to unexposed cells [41]. In Table 2, compared to control, after treatment with FEO at the concentration of MIC and

Relative Electrical Conductivity Study
Further antibacterial mechanism of FEO against E. coli and S. aureus was confirmed with the measurement of the relative electric conductivity. As shown in Figure 4, the percentage of the relative electric conductivities of E. coli and S. aureus samples were increased to about 26.2% and 29.7% at the concentration of MIC in the first 4 h, and then reached a relative stable phage in the next 4 h. Compared to the MIC, the percentage of the relative electric conductivity of the suspensions were sharply reached to 50.2% and 41.3% in the first 4 h, and stabilized at a high level in the next 4 h at the concentration of 2MIC. The increase of the relative electric conductivity of samples treated with different concentrations of FEO suggested that the cytoplasmic membranes were disrupted, which caused the leakage of intracellular ingredient, especially losses of electrolytes including K + , Ca 2+ , Na + , and so on [40].

Relative Electrical Conductivity Study
Further antibacterial mechanism of FEO against E. coli and S. aureus was confirmed with the measurement of the relative electric conductivity. As shown in Figure 4, the percentage of the relative electric conductivities of E. coli and S. aureus samples were increased to about 26.2% and 29.7% at the concentration of MIC in the first 4 h, and then reached a relative stable phage in the next 4 h. Compared to the MIC, the percentage of the relative electric conductivity of the suspensions were sharply reached to 50.2% and 41.3% in the first 4 h, and stabilized at a high level in the next 4 h at the concentration of 2MIC. The increase of the relative electric conductivity of samples treated with different concentrations of FEO suggested that the cytoplasmic membranes were disrupted, which caused the leakage of intracellular ingredient, especially losses of electrolytes including K + , Ca 2+ , Na + , and so on [40].

Leakage of Cytoplasmic Materials
The leakage of cytoplasmic material was considered as severe and irreversible damage to the cytoplasmic membrane. Measurement of specific cell leakage markers such as 260 nm absorbing materials and proteins could indicate the changes of membrane integrity compared to unexposed cells [41]. In Table 2, compared to control, after treatment with FEO at the concentration of MIC and

Leakage of Cytoplasmic Materials
The leakage of cytoplasmic material was considered as severe and irreversible damage to the cytoplasmic membrane. Measurement of specific cell leakage markers such as 260 nm absorbing materials and proteins could indicate the changes of membrane integrity compared to unexposed cells [41]. In Table 2, compared to control, after treatment with FEO at the concentration of MIC and 2MIC, the concentration of cell constituents (OD 260 nm) and proteins in suspensions increased 2.3, 10.2 times and 6.0, 16.0 times to E. coil, and 4.3, 12.9 times and 10.3, 19.7 times to S. aureus, respectively. These changes of the concentrations of nucleic acids and proteins suggested that essential oil damaged cytoplasmic membrane and subsequently caused leakage of intracellular constituents. Values represent means of three independent replicates ± SD.

SDS-PAGE of Protein Patterns of Bacteria Treated with FEO
To further investigate the probable antibacterial mechanisms of FEO, the whole protein patterns of bacteria were analyzed. Compared with the National Center for Biotechnology Information, SDS-PAGE of whole-cell protein lysates was to identify the possible target proteins after FEO treatment. The results demonstrated that the membrane integrity was destructed after FEO treatment ( Figure 5A,B). Lane 1, 2, 3, and 4 were corresponding to maker, control, MIC, and 2MIC when treated with FEO against E. coli (A) and S. aureus (B), respectively. The protein profiles of bacteria treated with FEO differed from those of the control. Compared with the untreated cells, the bands approximately at 60 kDa, 52 kDa, 33 kDa, and 28 kDa were degraded in E. coli samples. Whereas bands at about 30 kDa and 26 kDa were also degraded in S. aureus samples. Outer membrane protein A (OmpA: 28 kDa) was critical for the integrity of the bacterial membrane as a physical linkage with peptidoglycan layer in E. coli [42]. The membrane-associated protein TcaA (TcaA: 52 kDa) also played a critical role in the synthesis of cell wall in S. aureus [43]. The degradation and destruction of the critical functional proteins led to inactivation of the microorganism. More proteins associating with the damage of the membrane needed to be advanced investigations.  Values represent means of three independent replicates ± SD.

SDS-PAGE of Protein Patterns of Bacteria Treated with FEO
To further investigate the probable antibacterial mechanisms of FEO, the whole protein patterns of bacteria were analyzed. Compared with the National Center for Biotechnology Information, SDS-PAGE of whole-cell protein lysates was to identify the possible target proteins after FEO treatment. The results demonstrated that the membrane integrity was destructed after FEO treatment ( Figure  5A,B). Lane 1, 2, 3, and 4 were corresponding to maker, control, MIC, and 2MIC when treated with FEO against E. coli (A) and S. aureus (B), respectively. The protein profiles of bacteria treated with FEO differed from those of the control. Compared with the untreated cells, the bands approximately at 60 kDa, 52 kDa, 33 kDa, and 28 kDa were degraded in E. coli samples. Whereas bands at about 30 kDa and 26 kDa were also degraded in S. aureus samples. Outer membrane protein A (OmpA: 28 kDa) was critical for the integrity of the bacterial membrane as a physical linkage with peptidoglycan layer in E. coli [42]. The membrane-associated protein TcaA (TcaA: 52 kDa) also played a critical role in the synthesis of cell wall in S. aureus [43]. The degradation and destruction of the critical functional proteins led to inactivation of the microorganism. More proteins associating with the damage of the membrane needed to be advanced investigations.

The Application of FEO-Loaded Nanoparticles Against E. coli and S. aureus
The encapsulation of functional EOs in emulsions had been applied as a popular method to improve the utilization and stability of EOs [20]. Nano-emulsions which had the advantage of small particle size, low turbidity, and controlled ease of functional attributes had been appropriate for commercial applications, including preservatives in foods, beverages, cosmetics, and pharmaceuticals [44][45][46][47]. These EO-loaded nanoparticles were usually prepared by ionic gelation technique. In my study, the FEO-loaded nanoparticles were prepared with the positively charged primary amino groups of chitosan and the negatively charged groups TPP. This nano-encapsulation had a good effect on inhibiting the growth of two food-borne pathogens, E. coli and S. aureus. The result was presented in Table 3, the antimicrobial activity of FEO-loaded nanoparticles against E. coli and S. aureus was better in the refrigerated conditions. With the highest tested concentrations (chitosan to FEO of 1:1) 100% inhibition was achieved in 36 h at 4 • C. Inhibition percentage was quiet constant for all the concentrations used, during the storage period at a temperature of 4 • C, which was in the range from 98.43% to 95.29%. At room temperature, FEO-loaded nanoparticles (chitosan to FEO of 1:0.5 and 1:1) could also effectively inhibit the growth of the food-borne pathogens above 50%. With the temperature reached to 50 • C, the inhibition rate of pathogens with FEO-loaded nanoparticles were reduced, which was caused by the significant effect of the physical properties of oil and water system under high temperature. The increased temperature resulted in the increased release rate and diffusion coefficient of core material [48]. Compared to blank nanoparticles, encapsulation of essential oils in nano-systems represented an efficient approach to increase the physical stability of bioactive compounds and to protect them from undesirable changes. 0.00 ± 0.00 100.00 ± 0.00 100.00 ± 0.00 100.00 ± 0.00 98.21 ± 2.77 +4 0.00 ± 0.00 100.00 ± 0.00 100.00 ± 0.00 100.00 ± 0.00 100.00 ± 0.00 Values represent means of three independent replicates ± SD.

Conclusions
The results of the present study indicate that FEO is a potential antibacterial compound against two food-borne bacteria. The conversion of Fructus forsythia essential oil into nano-emulsions can greatly enhance the antibacterial activity against food-borne pathogenic bacteria. The antibacterial mechanism of FEO is the disruption of the cell membrane which changes the cell membrane permeability, and leads to the release of some cellular components such as ions, DNA, and proteins. Also, the antibacterial mechanism of FEO may degrade bacterial proteins. The present work provides strong evidence that the essential oil of Fructus forsythia is available as a green effective antibacterial additive. Further studies are needed to evaluate the efficacy and safety of EO-loaded nanoparticles in suitable food systems.