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Article

Comparative Analysis of Chemical Composition and Antibacterial Activity of Essential Oils from Five Varieties of Lavender Extracted via Supercritical Fluid Extraction

by
Lijing Lin
1,†,
Zhencheng Lv
2,†,
Meiyu Wang
1,3,
Ankang Kan
3,
Songling Zou
2,
Bin Wu
4,
Limin Guo
4,
Salamet Edirs
4,
Jiameng Liu
1,* and
Lin Zhu
1,*
1
Hainan Key Laboratory of Storage and Processing of Fruits and Vegetables, Agricultural Products Processing Research Institute, Chinese Academy of Tropical Agricultural Sciences, Zhanjiang 524001, China
2
School of life Sciences, Huizhou University, Huizhou 516007, China
3
Merchant Marine College, Shanghai Maritime University, Shanghai 201306, China
4
Institute of Agro-Production Storage and Processing, Xinjiang Academy of Agricultural Sciences, Urumqi 830091, China
*
Authors to whom correspondence should be addressed.
These authors contributed equally to this work.
Molecules 2025, 30(2), 217; https://doi.org/10.3390/molecules30020217
Submission received: 22 October 2024 / Revised: 3 January 2025 / Accepted: 4 January 2025 / Published: 7 January 2025
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Abstract

:
This study aimed to determine the chemical composition of five Lavender essential oils (LEOs) using the gas chromatography–mass spectroscopy technique and to assess their antibacterial activity against four marine Vibrio species, including Shewanella algae, Shewanella maridflavi, Vibrio harveyi, and Vibrio alginolyticus. Sensitivity tests were performed using the disk diffusion and serial dilution methods. The results showed that all five LEOs exhibited antibacterial activity against the four tested marine Vibrio species. The antibacterial activities of all five LEOs were above moderate sensitivity. The five LEOs from French blue, space blue, eye-catching, and true Lavender showed high sensitivity, particularly against Shewanella maridflavi. The compounds of LEOs from different varieties of Lavender were similar and mainly comprised linalool, linalyl acetate, eucalyptol, and isoborneol. Different varieties of LEOs possessed unique components besides common components, and the percentage of each one was different, which led to different fragrance loads. The major fragrances were lily of the valley, an aromatic compound fragrance, and an herbal fragrance. The antibacterial activity of LEO from eye-catching Lavender was better than that of others, which could provide a reference for its application in the prevention and control of marine Vibrio spp. and the development of antibacterial products.

1. Introduction

Essential oils, compounds extracted from plants, are volatile and aromatic liquids. The unique aromatic compounds give each essential oil its distinctive essence. Essential oils can retard or inhibit the growth of many bacteria and fungi [1]. For example, tea tree essential oil and thyme essential oil showed significant antibacterial activity against Staphylococcus aureus. Cinnamon essential oil and clove essential oil have inhibitory effects on Escherichia coli. Rosemary essential oil and Lavender essential oil show antibacterial effect on Pseudomonas aeruginosa [2]. Lindera subumbelliflora Kosterm essential oil has antifungal activity against Candida albicans [3]. Oregano essential oil and thyme essential oil have inhibitory effects on Aspergillus, while lemon grass essential oil and cinnamon essential oil have antifungal effects on Penicillium [4]. These oils are composed of various aldehydes, phenols, alcohols, and other compounds, mainly terpenes and phenylpropanoids, with the former being the principal constituent [5]. Essential oils were initially used as fragrances. As research progressed, these oils were identified to possess multiple biological activities. Currently, they are used in traditional Chinese medicine compound preparations, aromatherapy agents, and insect repellents and have widespread applications in medicine, aquaculture, food, cosmetics, etc. [6]. Essential oils can be used as anesthetics, sedatives, and substitutes for synthetic drugs. Nalan Ozgur Yigit [7] found that Lavender and laurel essential oil had remarkable anesthetic effects on rainbow trout. The induction time of Lavender essential oil at 200 mg/L and laurel essential oil at 400 mg/L was 258.0 s and 189.5 s, respectively, and the recovery time was 41 s and 129.5 s. Histopathological evaluation showed no abnormalities in the gill, liver, and kidney. Soon-Il Kim [8] found that plant essential oil has the potential to become a new pesticide. Bakiaydn [9] also found that Lavender essential oil as a natural anesthetic may be a more environmentally friendly, cost-effective, and safer product than synthetic drugs. Essential oil can be used as a new antibacterial substance. Temitayo Margaret Omoyeni [10] uses freeze-dried polyvinyl alcohol (PVA)/Arabic gum (GA) to synthesize hydrogel, in which 0.2 mL of black Vitex negundo oil has an obvious inhibitory effect on Staphylococcus aureus and Bacillus subtilis and can be used for wound healing and other biomedical applications. With people’s quality of life continuously improving and the government’s increasing emphasis on sustainable development [11], plant essential oils can meet the requirements of being healthy, green, environmentally friendly, and pollution-free in their applications.
Lavender (Lavandula angustifolia Mill.) is a perennial subshrub plant belonging to the Lamiaceae family and the Lavandula genus and is native to the Mediterranean coast. Lavender essential oil (LEO) is known for its calming effect on the nerves [12], pain relief, and the treatment of neurological diseases. LEO is light yellow, extracted from Lavender, and has an aromatic fragrance. Studies have reported that LEO has a broad-spectrum antibacterial ability [13]. At present, GC-MS can be used to analyze the components of essential oil and study its antibacterial activity. Othman El Faqer [14] studied the antibacterial potential of Allium sativum essential oil. By GC/MS analysis, it was found that diallyl disulfide was the main component, and Allium sativum essential oil showed strong activity against methicillin-resistant Staphylococcus aureus. Gunja Sah [15] studied and analyzed the chemical constituents and biological activities of Mentha longifolia. By GC-MS analysis, it is confirmed that the main components are piperitone oxide and cis-piperitone oxide. The essential oil showed remarkable nematicidal activity, antioxidant activity (through DPPH and H2O2 scavenging experiments), and antibacterial activity against a variety of bacteria and fungi. Salvia dumetorum essential oil was extracted by Yana K. Levaya [16] by steam distillation, and its chemical constituents were analyzed by GC-MS, among which sesquiterpenes accounted for 54.15%. Salvia dumetorum essential oil showed strong antibacterial activity against Staphylococcus aureus and Bacillus subtilis and inhibited the biofilm formation of Streptococcus mutans on 1% sucrose medium.
The genus Vibrio (Vibrio spp.) comprises Gram-negative bacteria that are widely distributed in bays, coastal waters, open oceans, sediments, and marine environments [17]. Those organisms are opportunistic pathogens. Marine fisheries often suffer from vibriosis caused by Vibrio infections, resulting in substantial economic losses. Furthermore, this organism exerts a negative effect on the sustainable development of the marine ecological environment [18]. In addition, Vibrio can infect humans through the food chain via contaminated seafood, posing a severe threat to human health [19]. Currently, there are few reports on the antibacterial activity of essential oils against marine Vibrio.
Five varieties of Lavender were selected in this study, as follows: French blue Lavender (Lavandula stoechas), Xinjiang Ili 701 Lavender, space blue Lavender (Lavandula stoechas), eye-catching Lavender (Lavandula hybrida), and true Lavender (Lavandula angustifolia). Four bacterial strains were tested in this study, namely Shewanella maridflavi, Shewanella algae, Vibrio alginolyticus, and Vibrio harveyi, to investigate the antibacterial activity of the five LEOs. The main components of the essential oils were qualitatively and quantitatively analyzed using gas chromatography–mass spectroscopy (GC–MS). Moreover, their aroma characteristics were studied to provide a scientific basis for the development and utilization of essential oils in the aquaculture industry.

2. Results and Discussion

2.1. Supercritical Fluid Extraction of LEO

The results of the supercritical fluid extraction of LEOs are shown in Table 1. The essential oils obtained by supercritical fluid extraction were yellow liquids, with extraction yields ranging from 3.72% to 4.17%. Eye-catching Lavender had the highest extraction yield of 4.17 ± 0.11%. In terms of color, the essential oils were basically yellow, with true Lavender having a lighter color.

2.2. Analysis of Antibacterial Activity

2.2.1. Antibacterial Activity of Essential Oils (Disk Diffusion Method)

The bacteriostatic effect of LEO against S. maridflavi is shown in Figure 1a. The sensitivity levels and diameters of the inhibition zones were as follows: eye-catching LEO, highly sensitive (17.17 mm) > French blue LEO, highly sensitive (16.00 mm) > true LEO, highly sensitive (15.50 mm) > space blue LEO, highly sensitive (15.33 mm) > 701 LEO, moderately sensitive (12.5 mm).
The bacteriostatic effect of LEOs against S. algae is shown in Figure 1b. The sensitivity levels and diameters of the inhibition zones were as follows: French blue LEO, moderately sensitive (12.75 mm) > eye-catching LEO, moderately sensitive (12.58 mm) > 701 LEO, moderately sensitive (12 mm) > space blue LEO, moderately sensitive (11.83 mm) > true LEO, moderately sensitive (10.83 mm).
The bacteriostatic effect of LEOs against V. alginolyticus is shown in Figure 1c. The sensitivity levels and diameters of the inhibition zones were as follows: eye-catching LEO, moderately sensitive (14.83 mm) > French blue LEO, moderately sensitive (13.67 mm) > space blue LEO, moderately sensitive (12.33 mm) > 701 LEO, moderately sensitive (12.33 mm) > true Lavender LEO, moderately sensitive (12 mm).
The bacteriostatic effect of LEOs against V. harveyi is shown in Figure 1d. The sensitivity levels and diameters of the inhibition zones were as follows: space blue LEO, moderately sensitive (13.83 mm) > eye-catching LEO, moderately sensitive (13.75 mm) > true LEO, moderately sensitive (13.17 mm) > 701 LEO, moderately sensitive (11 mm) > French blue LEO, moderately sensitive (10.83 mm).

2.2.2. Results of Gradient Dilution Filter Paper Disk Method for LEO

According to the data in Table 2, the bacteriostatic effects of the five LEOs all reached moderate sensitivity or above. Notably, when Shewanella maridflavi was used as the test strain, the essential oils of French blue Lavender (16 mm), space blue lave Lavender (15.33 mm), eye-catching Lavender (17.17 mm), and true Lavender (15.5 mm) all reached the highly sensitive standard. Overall, the essential oil of eye-catching Lavender demonstrated good activity against Shewanella maridflavi, Shewanella algae, Vibrio alginolyticus, and Vibrio harveyi.

2.3. Volatile Components of Essential Oils

The volatile components of French blue LEO were analyzed under the aforementioned GC–MS conditions. The total ion chromatogram of the volatile components is shown in Figure 2a. Through NIST/WILEY mass spectral library searching and the area normalization method, 29 compounds were identified from the volatile substances of French blue LEO, accounting for 96.33% of the total volatile components, as can be seen from Table 3, including 15 terpenes (15.9%), 7 alcohols (40.5%), 2 ketones (0.69%), and 5 esters (38.93%). The compounds with higher contents were linalool (32.72%), linalyl acetate (31.18%), eucalyptol (1.27%), trans-β-ocimene (4.72%), β-ocimene (2.02%), 1-octen-3-yl-acetate (1.14%), isoborneol (2.26%), terpinene-4-ol (2.56%), α-terpineol (1.17%), lavandulyl acetate (6.17%), β-caryophyllene (3.81%), and (E)-β-famesene (1.41%). These were the main components of French blue LEO, with compounds having a relative content > 1% accounting for 90.43%.
The volatile components of 701 LEO were analyzed under the aforementioned GC–MS conditions. The total ion chromatogram of the volatile components is depicted in Figure 2b. Through NIST/WILEY mass spectral library searching and the area normalization method, 29 volatile substances were identified from 701 LEO (99.14%), as can be seen from Table 4, including 16 terpenes (14.64%), 7 alcohols (44.30%), 2 ketones (0.6%), and 5 esters (38.07%). The compounds with higher contents were linalool (35.38%) and linalyl acetate (33.91%), followed by eucalyptol (1.51%), trans-β-ocimene (3.67%), β-ocimene (1.49%), isoborneol (1.94%), 4-carvomenthenol (3.71%), α-terpineol (1.05%), lavandulyl acetate (3.15%), β-caryophyllene (5.88%), and (E)-β-famesene (1.34%). These were the main components of 701 LEO, with compounds having a relative content > 1%, accounting for 93.03%.
The volatile components of space blue LEO were analyzed under the aforementioned GC–MS conditions. The total ion chromatogram of the volatile components is shown in Figure 2c. Through NIST/WILEY mass spectral library searching and the area normalization method, 33 compounds were identified from the volatile substances of space blue LEO, accounting for 99.29% of the total volatile components, as can be seen from Table 5, including 16 terpenes (20.49%), 8 alcohols (39.21%), 2 ketones (0.75%), and 7 esters (38.84%). The compounds with higher contents were linalool (31%) and linalyl acetate (30.27%), followed by 3-carene (1.17%), D-limonene (1.84%), eucalyptol (1.34%), trans-β-ocimene (4.75%), β-ocimene (1.96%), 1-octenyl-3-acetate (1.04%), isoborneol (2.87%), terpinene-4-ol (1.68%), α-terpineol (1.46%), lavandulyl acetate (6.51%), β-caryophyllene (5.04%), and (E)-β-Famesene (1.31%). These were the main components of space blue LEO, with compounds having a relative content > 1% accounting for 92.24%.
The volatile components of eye-catching LEO were analyzed under the aforementioned GC–MS conditions. The total ion chromatogram of the volatile components is shown in Figure 2d. Through NIST/WILEY mass spectral library searching and the area normalization method, 32 compounds were identified from the volatile substances of LEO, accounting for 99.78% of the total volatile components, as can be seen from Table 6, including 18 terpenes (17.92%), 7 alcohols (52.03%), 2 ketones (12.07%), and 5 esters (17.76%). The compounds with higher contents were linalool (27.51%), linalyl acetate (15.58%), eucalyptol (18.16%), and camphor (11.87%), followed by α-pinene (1.18%), β-pinene (1.35%), D-limonene (1.57%), trans-β-ocimene (1.85%), β-ocimene (2.88%), isoborneol (3.29%), α-terpineol (1.66%), lavandulyl acetate (1.46%), and β-caryophyllene (3.92%). These were the main components of eye-catching LEO, with compounds having a relative content > 1% accounting for 92.28%.
The volatile components of true LEO were analyzed under the aforementioned GC-MS conditions. The total ion chromatogram of the volatile components is shown in Figure 2e. Through NIST/WILEY mass spectral library searching and the area normalization method, 27 compounds were identified from the volatile substances of true LEO, accounting for 100% of the total volatile components, as can be seen from Table 7, including 10 terpenes (18.12%), 9 alcohols (33.74%), 4 ketones (2.34%), and 4 esters (46.05%). The compounds with higher contents were linalyl acetate (40.81%) and linalol (24.6%), followed by 3-octanone (1.17%), trans-β-ocimene (3.18%), β-ocimene (1.57%), isoborneol (1.63%), terpinene-4-ol (3.7%), lavandulyl acetate (4.14%), β-caryophyllene (5.83%), trans-2-hydroxycinnamic acid (1.62%), and (E)-β-Famesene (4.09%), which were the main components of true LEO. Compounds with a relative content > 1% accounted for 92.34%.

2.4. Aroma Analysis of Essential Oils

Volatile aromatic components are the material basis for the aroma of essential oils. By combining the ABC quantitative values of the odor of each essential oil substance with its relative content, a radar chart of the aroma distribution (Figure 3) can be drawn to visually express the overall aroma of different essential oils.
The aroma distribution radar chart of French blue LEO (Figure 3a) showed that this essential oil covered 17 aroma types. Of these, the aroma with the highest load was the lily of the valley, followed by aromatic compounds and orchids. Additionally, citrus, frankincense, fruity, iris, rose, jasmine, green, cool, camphor, pine, woody, spicy, herbaceous, and toasted aromas displayed high loads and constituted the chief aroma of French blue LEO.
701 LEO (Figure 3b) covered 20 aroma types. Of these, the aromas with the highest loads were the lily of the valley and aromatic compounds, followed by herbaceous. Moreover, fatty, cool, citrus, frankincense, food, fruity, green, iris, jasmine, pine, orchid, rose, spicy, toasted, woody, earthy, and camphor aromas exhibited high loads and constituted the primary aroma of 701 LEO.
Space blue LEO (Figure 3c) encompassed 18 aroma types, of which the one with the highest load was aromatic compounds, followed by herbaceous. Furthermore, fatty, cool, citrus, frankincense, food, fruity, green, iris, pine, lily of the valley, orchid, rose, spicy, woody, earthy, and camphor aromas had high loads and comprised the main aroma of space blue LEO.
Eye-catching LEO (Figure 3d) covered 19 aroma types, of which the one with the highest load was herbaceous, followed by cool and lily of the valley. Moreover, citrus, frankincense, food, fruity, green, herbaceous, iris, jasmine, pine, aromatic compounds, orchid, rose, spicy, woody, earthy, and camphor aromas exhibited high loads and constituted the primary aroma of eye-catching LEO.
True LEO (Figure 3e) covered 20 aroma types. Of these, the aroma with the highest load was aromatic compounds, followed by lily of the valley and herbaceous. In addition, fatty, cool, citrus, frankincense, food, fruity, green, iris, jasmine, pine, orchid, rose, spicy, toasted, woody, earthy, and camphor aromas had high loads and comprised the main aroma of true LEO.

2.5. Discussion

The essential oils of the five Lavender varieties, including French blue, caused moderate-to-high sensitivity in the four marine Vibrio strains, including Shewanella maridflavi. GC–MS findings indicated that the major components of the essential oils from all Lavender varieties were linalool and linalyl acetate. These observations agree with those from a previous report [35]. Linalool has been reported to exhibit bacteriostatic activity against Pseudomonas putida [36]. Several studies have shown that the antibacterial activity increases when the contents of linalool and linalyl acetate in LEOs are increased, which suggests that these two compounds are the main substances responsible for the antibacterial activity of LEOs. Linalool and linalyl acetate can play an antibacterial role by destroying the cell membrane of microorganisms, increasing the permeability of the membrane, leading to the leakage of important components of cells, thus causing cell death and inhibiting the synthesis of essential biological macromolecules (such as RNA, DNA, protein, and polysaccharides), further enhancing their antibacterial properties. At the same time, the stability of linalyl acetate in the process of thermal- and photo-oxidation affects its antibacterial efficacy, and proper treatment can enhance its activity [37,38]. In addition, linalool shows significant antifungal activity, which may interfere with the metabolic processes of fungi by inhibiting the activities of some key enzymes, destroy the biofilm structure of fungi, and inhibiting the formation and maturity of their biofilm [39]. The antibacterial effect of linalyl acetate may be partly due to the disturbance of the lipid part of the microbial plasma membrane, which leads to a change in membrane permeability and the leakage of intracellular substances. In addition, these compounds may penetrate the cell membrane and interact with key targets in the cell, thus exerting antibacterial activity [40]. LEOs exhibited good antimicrobial activities against E. coli and S. aureus at concentrations > 2000 ppm [41]. GC–MS data indicated that the essential oils of the five Lavender varieties used in this study contained approximately 30% linalool and linalyl acetate, which agrees with the moderate-to-high sensitivity demonstrated in the antibacterial activity assays. For the antibacterial mechanism of Lavender essential oil, we can deeply study its effects on the microbial cell membrane, protein synthesis, and nucleic acid structure, so as to better understand its mechanism.
The essential oil extracted from different lavender varieties produces distinct compounds. The unique compound found in 701 LEO is 4-Carvomenthenol. For space blue LEO, the distinctive compounds include Nerol, Hexyl 2-methylbutyrate, Bornyl acetate, and Neryl acetate. Eye-catching LEO is characterized by α-Sabine, γ-Terpinene, (E)-Hexyl 2-methylbut-2-enoate, and Neryl propionate. Lastly, the unique compounds identified in true LEO are 3-Octanol, trans-2-Hydroxycinnamic acid, caryophyllene oxide, and Herniarin.
The essential oil samples were characterized based on sensory attributes, such as sweet, floral, woody, camphor, fruity, and herb notes [41]. According to the aroma radar charts, different Lavender varieties exhibited different aroma types. Five substances, namely caryophyllene, geraniol acetate, geraniol, linalool, and linalyl acetate, have been shown to be the key compounds that differentiate the aromatic profiles of LEOs [42]. Linalool contributed the most to the lily of the valley aroma [43], linalyl acetate contributes the most to the aromatic compounds aroma [44], and isoborneol contributes the most to the herbaceous aroma. The essential oil of French blue Lavender had the highest aroma load of lily of the valley, followed by aromatic compounds and orchid; 701 LEO had the highest aroma load of lily of the valley and aromatic compounds, followed by herbaceous; space blue LEO had the highest aroma load of aromatic compounds, followed by herbaceous; eye-catching LEO had the highest aroma load of lily of the valley and aromatic compounds, followed by herbaceous; true LEO has the highest aroma load of aromatic compounds, followed by lily of the valley and herbaceous. All Lavender varieties displayed either the lily of the valley aroma from linalool or the aromatic compounds aroma from linalyl acetate. These findings imply that diversified Lavender varieties, including French blue, 701, space blue, eye-catching, and true Lavender, share common aroma components of Lavender. Nonetheless, each variety also possesses its unique aroma.

3. Materials and Methods

3.1. Materials

Lavender flowers: eye-catching Lavender, space blue Lavender, French blue Lavender, 701 Lavender, and true Lavender were all collected from Yining County, Ili Kazakh Autonomous Prefecture, Xinjiang (Latitude: 43.9779° N; Longitude: 81.5296° E).
Bacterial strains: Shewanella algae and Shewanella maridflavi were isolated from Bahaba taipingensis; Vibrio harveyi and Vibrio alginolyticus were isolated from Ostrea gigas. All strains were marine Vibrio provided by the Marine Products Research Laboratory of Huizhou University.
Dimethyl sulfoxide (DMSO) (Beijing Solarbio Science & Technology Co., Ltd., Beijing, China), marine culture medium, Luria Bertani Broth (LB broth), LB agar, agar, and peptone (Shanghai Acmec Biochemical Technology Co., Ltd., Shanghai, China) were used.

3.2. Instruments and Equipment

An HA121-50-2 Supercritical extraction device (Jiangsu Nantong Hua’an Supercritical Extraction Co., Ltd., Nantong, China); 7890B-5977A GC-MS (Agilent, Santa Clara, CA, USA), Shimadzu UV-2550 UV-visible spectrophotometer (Shimadzu (China) Co., Ltd., Shanghai, China), HP-5MS chromatographic column (30 m × 250 μm × 0.25 μm) (Agilent, USA), and Synergy H1 multi-function microplate detector (BioTek Instruments, Inc., Charlotte, VT, USA) were used.

3.3. Methods

3.3.1. Extraction of LEO

Lavender flowers were accurately weighed (500 g) and placed into an extraction vessel (18 MPa, 40 °C, 2 h). The obtained oil was released from the separation vessel to obtain the essential oil. The extraction yield was finally calculated using the following formula:
Extraction   yield   % = Mass   of   essential   oil   /   Mass   of   raw   material ×   100

3.3.2. Antibacterial Activity of LEOs

Preparation of Bacterial Suspensions

Experimental strains were stored in a −80 °C refrigerator. Each time, 2 μL of bacterial strains were inoculated into a liquid marine culture medium. The inoculation was performed in a laminar flow cabinet. After inoculation, the cultures were shaken and incubated at 35 °C for 10 h in an incubator shaker. Subsequently, the optical density (OD) values were measured at 600 nm using a spectrophotometer [45]. The optimal OD value range for the bacterial suspensions was 0.8–1.2 [46]. Finally, the suspensions were diluted to an OD of 0.05 and stored for later use.

Determination of Inhibition Zones

For this procedure, 1 mL of each of the four bacterial suspensions was added to preprepared sterile LB agar plates. The suspensions were thoroughly spread on the LB agar plates. After the suspensions had settled, the excess liquid was removed using a pipette, and the plates were air-dried [47]. A sterile tweezer was used to pick up a 6 mm diameter sterile filter paper disk, and a pipette was used to add 5 μL of the test essential oil onto the corresponding filter paper disk. The disks were then placed onto the corresponding LB agar medium. The culture plates were inverted and incubated overnight in a 37 °C incubator. After 24 h, the diameters of the inhibition zones were measured. The diameters of the inhibition zones formed by the corresponding essential oil filter paper disks were measured using the cross method. Three parallel experiments were conducted, and the average values were taken to evaluate the bacteriostatic effect of the plant essential oils [48]. DMSO [49] was used as a negative control.

Sensitivity Level Test of Essential Oil

For the inhibition zone test, 6 mm-diameter filter paper disks were used. Bacterial sensitivity to the essential oils was determined based on the size of the inhibition zones. The judgment criteria followed the “Standards for the Implementation of Antimicrobial Susceptibility Testing” issued by the CLSI and were as follows: diameter > 20 mm, extremely sensitive; 15–20 mm, highly sensitive; 10–15 mm, moderately sensitive; <10 mm, low sensitivity.

3.3.3. Analysis of LEOs

GC–MS was used for the analysis, and the system was a 7890B-5977A with an HP-5MS chromatographic column (30 m × 250 μm × 0.25 μm).
GC conditions: initial temperature of 40 °C, held for 3 min; increased to 160 °C at a rate of 5 °C/min, then increased to 200 °C at a rate of 10 °C/min, and held for 10 min; injection port temperature of 250 °C; flow rate of 1.0 mL/min; carrier gas was high-purity He; and splitless injection.
MS conditions: electron impact ion source; electron impact energy of 70 eV; ion source temperature of 230 °C; transfer line temperature of 250 °C; scan range of 50–500 m/z; and MS quadrupole temperature of 150 °C.
The five LEOs were diluted 20-fold, and 0.2 μL of each oil was manually injected. The experiments were repeated thrice, and the final results were expressed as the mean ± standard deviation.

3.3.4. Qualitative Analysis of Volatile Components in LEOs

The volatile components of the plant essential oils were detected and analyzed by using GC–MS to obtain their total ion chromatograms. The NIST/WILEY mass spectral library was used for searching, and the MS, retention index (RI), and literature-reported RI values were combined to identify each compound and determine the volatile substances [14].
RI: the RIs of each component were calculated using the retention times of n-alkanes. The following formula was used to calculate the RI:
RI = 100   × tR i     tR N   /   tR N + 1     tR N +   100 N
where [tR(i)] is the retention time of the analyte; [tR(N)] and [tR(N + 1)] are the retention times of n-alkanes with carbon numbers N and N + 1, respectively.
The volatile components of the plant essential oils were detected and analyzed using GC–MS to obtain their total ion chromatograms. The NIST/WILEY mass spectral library was used for searching, and the area normalization method was applied for the semiquantitative analysis of the relative content of each component to identify the volatile substances [15].
Relative   content   % = Peak   area   of   a   component   /   Total   peak   area   ×   100 %

3.3.5. Aroma Analysis of LEOs

Aroma does not have an exact unit of measurement and is primarily derived from human olfactory perception. It describes the olfactory impression of a particular fragrance tone in perfumes and fragrances and is mostly expressed using descriptive language. Essential oils are extracted from plant materials and exhibit complex and diverse aromas.
Volatile aromatic components are the material basis for the aroma of essential oils [50]. The “ABC” method proposed by Lin Xiangyun in “The Art of Perfumery” was used to quantitatively describe the odors of the volatile components. This system classifies the odors of different volatile components in nature into 26 types, using the initial letter of their representative aroma as an abbreviation. This classification method is the only system to quantitatively describe and distinguish orders quantitatively. By combining the ABC quantitative values of the odor of each fragrance substance with its relative content, a radar chart of the aroma distribution can be drawn.

3.3.6. Data Analysis

SPSS 18.0 (IBM, Armonk, NY, USA) software was used to process the data statistically, and the one-way analysis of variance (ANOVA) was applied to analyze the significance of the difference between groups. The difference was considered significant in the case of p < 0.05, and the results were expressed as ±SD.

4. Conclusions

In this study, the extraction rate of essential oil by supercritical fluid extraction is 3.72–4.17%. The extraction rate of Lavender is the highest, which is 4.17%. Essential oil is basically yellow, and real Lavender is lighter in color. The volatile components of five LEOs were identified using GC–MS, and the antibacterial activities of the LEOs against four marine Vibrio species were evaluated using disk diffusion and serial dilution methods. The findings suggested that all five LEOs exhibited antibacterial activity against the four tested marine Vibrio species. The antibacterial effects of the LEOs exceeded moderate sensitivity. The antibacterial effects of French blue (16 mm), space blue (15.33 mm), wakeful (17.17 mm), and real (15.5 mm) reached highly sensitive standards, particularly against S. maridflavi. The essential oil of eye-catching Lavender demonstrated good activity against S. maridflavi, S. algae, V. alginolyticus, and V. harveyi. For French blue LEO, a total of 29 compounds were identified (96.33%). The main components are linalool (32.72%) and linalyl acetate (31.18%), of which the compounds with content greater than 1% account for 90.43%. For 701 LEO, 29 kinds of volatile substances (99.14%) were identified, among which linalool (35.38%) and linalyl acetate (33.91%) were the main components, and the compounds with content greater than 1% accounted for 93.03%. For space blue LEO, 33 compounds (99.29%) were identified, and the main components were linalool (31%) and linalyl acetate (30.27%), and the compounds with content greater than 1% accounted for 92.24%. For eye-catching LEO, 32 compounds (99.78%) were identified, and the main components were linalool (27.51%) and linalyl acetate (15.58%), and the compounds with content greater than 1% accounted for 92.28%. For true LEO, 27 kinds of compounds (100%) were identified, and the main components were linalyl acetate (40.81%) and linalool (24.6%), and the compounds with content greater than 1% accounted for 92.34%. Different varieties of LEOs possessed similar types of compounds, with the major ones being linalool and linalyl acetate. The main fragrances were the lily of the valley fragrance, aromatic compound fragrance, and herbal fragrance. This study’s findings can provide a reference basis for the prevention and control of Vibrio and the development and application of antibacterial drugs, as well as offer insights into the aroma analysis of the five LEOs.

Author Contributions

Conceptualization, L.L.; methodology, M.W.; software, L.Z.; validation, A.K. and J.L.; formal analysis, L.Z. and Z.L.; resources, S.Z.; data curation, Z.L.; writing—original draft preparation, L.L.; writing—review and editing, B.W.; supervision, L.L.; project administration, L.G. and S.E.; funding acquisition, B.W., L.Z. and L.L. All authors have read and agreed to the published version of the manuscript.

Funding

This study was funded by “The Regional Collaborative Innovation Project of Xinjiang Province–Supercritical carbon dioxide extraction of aromatic plant resources in Central Asia and its instrument application (Grant No. 2022E01023)”, “Central Public-interest Scientific Institution Basal Research Fund (No. 1630122024011, No. 1630122024006, No. 1630062022006, No. 1630122024018)”, and “the Key Laboratory of Storage & Processing of Fruits and Vegetables of Hainan Province (No. HNGS202406)”.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

Data are contained within the article.

Conflicts of Interest

The authors declare no conflicts of interest.

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Molecules 30 00217 g001
Figure 1. (a) Bacteriostatic effect of five Lavender essential oils against Shewanella maridflavi. (b) Inhibition zone effect of five LEOs against Shewanella algae. (c) Inhibition zone effect of five LEOs against Vibrio alginolyticus. (d) Inhibition zone effect of five LEOs against Vibrio harveyi.
Figure 1. (a) Bacteriostatic effect of five Lavender essential oils against Shewanella maridflavi. (b) Inhibition zone effect of five LEOs against Shewanella algae. (c) Inhibition zone effect of five LEOs against Vibrio alginolyticus. (d) Inhibition zone effect of five LEOs against Vibrio harveyi.
Molecules 30 00217 g001
Molecules 30 00217 g002
Figure 2. Total ion chromatogram of volatile components in LEOs ((a) French blue LEO; (b) 701 LEO; (c) space blue LEO; (d) eye-catching LEO; (e) true LEO).
Figure 2. Total ion chromatogram of volatile components in LEOs ((a) French blue LEO; (b) 701 LEO; (c) space blue LEO; (d) eye-catching LEO; (e) true LEO).
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Molecules 30 00217 g003
Figure 3. Radar chart of aroma distribution for each essential oil. Note: (a) French blue Lavender; (b) 701 Lavender; (c) space blue Lavender; (d) eye-catching Lavender; (e) true Lavender; each letter represents a different aroma: A—fatty; B—cool; C—citrus; D—frankincense; E—food; F—fruity; G—green; H—herbaceous; I—iris; J—jasmine; K—pine; L—aromatic compounds; M—lily of the valley; N—narcotic; O—orchid; P—phenolic; R—rose; S—spicy; T—toasted; Ve—vegetable; W—woody; Y—earthy; Z—organic solvent; Ca—camphor.
Figure 3. Radar chart of aroma distribution for each essential oil. Note: (a) French blue Lavender; (b) 701 Lavender; (c) space blue Lavender; (d) eye-catching Lavender; (e) true Lavender; each letter represents a different aroma: A—fatty; B—cool; C—citrus; D—frankincense; E—food; F—fruity; G—green; H—herbaceous; I—iris; J—jasmine; K—pine; L—aromatic compounds; M—lily of the valley; N—narcotic; O—orchid; P—phenolic; R—rose; S—spicy; T—toasted; Ve—vegetable; W—woody; Y—earthy; Z—organic solvent; Ca—camphor.
Molecules 30 00217 g003
Table 1. Extraction of essential oil from Lavender.
Table 1. Extraction of essential oil from Lavender.
VarietyExtraction Yield/%Color
Eye-catching Lavender4.17 ± 0.11 aYellow
Space blue Lavender3.72 ± 0.20 bYellow
French blue Lavender3.95 ± 0.16 cYellow
701 Lavender3.74 ± 0.18 bYellow
True Lavender3.78 ± 0.22 bLight Yellow
Note: different letters in a column indicate significant differences (p < 0.05).
Table 2. Sensitivity levels of different Vibrio strains to various essential oils (unit/mm).
Table 2. Sensitivity levels of different Vibrio strains to various essential oils (unit/mm).
Essential Oil TypeShewanella maridflaviShewanella algaeVibrio alginolyticusVibrio harveyi
French blue Lavender16.00 ± 0.5012.75 ± 2.3813.67 ± 2.3610.83 ± 1.04
701 Lavender12.50 ± 2.2712.00 ± 1.4712.33 ± 1.4311.00 ± 0.71
Space Lavender15.33 ± 5.5111.83 ± 2.7512.33 ± 2.5213.83 ± 2.75
Eye-catching Lavender17.17 ± 1.7012.58 ± 0.9614.83 ± 1.2513.75 ± 0.54
True Lavender15.50 ± 5.2710.83 ± 1.4412.00 ± 3.4613.17 ± 2.93
Table 3. Compound composition of French blue LEO.
Table 3. Compound composition of French blue LEO.
NO.ComponentsMolecular FormulaRT/minRI (cal)RI (ref)Relative Content/%CASMS
1α-pineneC10H169.50930.819390.27 ± 0.0280-56-8RI, MS
2CampheneC10H169.97945.759360.27 ± 0.0279-92-5RI, MS
31-Octen-3-olC8H16O11.07986.779790.30 ± 0.023391-86-4RI, MS
4MyrceneC10H1611.42991.319910.52 ± 0.03123-35-3RI, MS
53-CareneC10H1612.001009.6710110.45 ± 0.0313466-78-9RI, MS
6Hexyl acetateC8H16O212.171023.2610110.27 ± 0.02142-92-7RI, MS [20]
7p-CymeneC10H1412.471024.5810260.29 ± 0.0299-87-6RI, MS
8D-LimoneneC10H1612.601028.6910360.72 ± 0.055989-27-5RI, MS
9EucalyptolC10H18O12.691031.6310371.27 ± 0.07470-82-6RI, MS
10trans-β-OcimeneC10H1612.931039.1810454.72 ± 0.283779-61-1RI, MS
11β-OcimeneC10H1613.251049.3510442.02 ± 0.1213877-91-3RI, MS [21]
12α-terpineneC10H1614.501088.6910850.17 ± 0.01586-63-0RI, MS
13LinaloolC10H18O14.941102.62110232.72 ± 1.9678-70-6RI, MS
141-Octen-3-yl-acetateC10H18O215.271112.9511081.14 ± 0.062442-10-6RI, MS [22]
15CamphoreC10H16O16.241143.7611510.48 ± 0.03464-48-2RI, MS [23]
16IsoborneolC10H18O16.921165.2411552.26 ± 0.13124-76-5RI, MS
17terpinene-4-olC10H18O17.241175.2611772.56 ± 0.14562-74-3RI, MS
18CryptoneC9H14O17.511178.9711870.21 ± 0.01500-02-7RI, MS
19α-TerpineolC10H18O17.641187.8711931.17 ± 0.0798-55-5RI, MS
20Isobornyl formateC11H18O218.711228.5912390.17 ± 0.011200-67-5RI, MS
21Linalyl acetateC12H20O219.501247.94125331.18 ± 1.84115-95-7RI, MS
22Lavandulyl acetateC12H22O320.441291.7612936.17 ± 0.3820777-39-3RI, MS [24]
23α-FencheneC10H1622.411338.70 0.22 ± 0.02471-84-1MS
24α-CopaeneC15H2422.911379.9113790.4 ± 0.023856-25-5RI, MS
25β-CaryophylleneC15H2423.931437.3614193.81 ± 0.2487-44-5RI, MS
26(E)-β-FameseneC15H2424.781465.5814591.41 ± 0.0918794-84-8RI, MS
27D-GermacreneC15H2425.481488.9315030.72 ± 0.0518252-44-3RI, MS [25]
28γ-CadineneC15H2426.271515.4115130.22 ± 0.0139029-41-9RI, MS [26]
29τ-CadinolC15H26O28.981605.77 0.22 ± 0.015937-11-1MS
SUM ---96.33
Table 4. Compound composition of 701 LEO.
Table 4. Compound composition of 701 LEO.
NO.ComponentsMolecular FormulaRT/minRI (cal)RI (ref)Relative Content/%CASMS
1α-PineneC10H169.50 930.819390.25 ± 0.0080-56-8RI, MS
2CampheneC10H169.97 945.729360.29 ± 0.0079-92-5RI, MS [27]
31-Octen-3-olC8H16O11.07 986.949790.21 ± 0.003391-86-4RI, MS
4MyrceneC10H1611.42 991.319910.50 ± 0.01123-35-3RI, MS
53-CareneC10H1611.99 1009.5110110.40 ± 0.0013466-78-9RI, MS
6Hexyl acetateC8H16O212.17 1023.2310110.21 ± 0.00142-92-7RI, MS [28]
7p-CymeneC10H1412.47 1024.5810260.41 ± 0.0099-87-6RI, MS
8D-LimoneneC10H1612.60 1028.6910360.53 ± 0.005989-27-5RI, MS
9EucalyptolC10H18O12.69 1031.4710371.51 ± 0.01470-82-6RI, MS
10trans-β-OcimeneC10H1612.93 1039.1810453.67 ± 0.023779-61-1RI, MS [20]
11β-OcimeneC10H1613.25 1049.3510441.49 ± 0.0113877-91-3RI, MS [21]
12terpinoleneC10H1614.53 1089.8310880.19 ± 0.00586-63-0RI, MS
13LinaloolC10H18O14.94 1102.78110235.38 ± 0.1878-70-6RI, MS
141-Octen-3-yl-acetateC10H18O215.27 1112.9511080.62 ± 0.002442-10-6RI, MS [22]
15CamphoreC10H16O16.24 1143.7611510.40 ± 0.00464-48-2RI, MS [23]
16IsoborneolC10H18O16.89 1164.2711551.94 ± 0.01124-76-5RI, MS
174-CarvomenthenolC10H18O17.23 1175.0711773.71 ± 0.02562-74-3RI, MS
18CryptoneC9H14O17.51 1178.7911870.20 ± 0.00500-02-7RI, MS
19α-TerpineolC10H18O17.63 1187.7111931.05 ± 0.0198-55-5RI, MS
20Isobornyl formateC11H18O218.70 1228.4212390.18 ± 0.001200-67-5RI, MS
21Linalyl acetateC14H24O219.50 1247.94125333.91 ± 0.30115-95-7RI, MS
22Lavandulyl acetateC13H22O320.44 1291.5712933.15 ± 0.0120777-39-3RI, MS [24]
23α-FencheneC10H1622.40 1338.52 0.21 ± 0.00105-91-9MS
24α-CopaeneC12H20O222.91 1379.9113790.36 ± 0.00141-12-8RI, MS
25β-CaryophylleneC15H2423.93 1437.1914195.88 ± 0.0487-44-5RI, MS
26(E)-β-FameseneC15H2424.78 1465.5814591.34 ± 0.0218794-84-8RI, MS
27D-GermacreneC15H2425.47 1488.7615030.68 ± 0.0018252-44-3RI, MS [25]
28γ-CadineneC15H2426.27 1515.2415130.24 ± 0.0039029-41-9RI, MS [26]
29τ-CadinolC15H26O28.97 1605.57 0.23 ± 0.005937-11-1MS
SUM ---99.14
Table 5. Compound composition of space blue LEO.
Table 5. Compound composition of space blue LEO.
NO.ComponentsMolecular FormulaRT/minRI (cal)RI (ref)Relative Content/%CASMSNO.
1CampheneC10H169.97 945.569369360.46 ± 0.0179-92-5RI, MS [27]
2β-PineneC10H1610.89 974.769809800.18 ± 0.00127-91-3RI, MS
31-Octen-3-olC8H16O11.07 986.779799790.28 ± 0.013391-86-4RI, MS
4MyrceneC10H1611.42 991.319919910.75 ± 0.03123-35-3RI, MS
53-CareneC10H1611.99 1009.51101110111.17 ± 0.0213466-78-9RI, MS
6Hexyl acetateC8H16O212.17 1023.23101610160.25 ± 0.01142-92-7RI, MS [29]
7o-CymeneC10H1412.39 1021.96102310230.22 ± 0.00527-84-4RI, MS
8p-CymeneC10H1412.47 1024.58102610260.49 ± 0.0199-87-6RI, MS
9D-LimoneneC10H1612.60 1028.85103610361.84 ± 0.045989-27-5RI, MS
10EucalyptolC10H18O12.69 1031.63103710371.34 ± 0.03470-82-6RI, MS [20]
11trans-β-OcimeneC10H1612.93 1039.18104510454.75 ± 2.153779-61-1RI, MS [21]
12β-OcimeneC10H1613.25 1049.35104410441.96 ± 0.0513877-91-3RI, MS
13α-terpineneC10H1614.50 1088.69108510850.21 ± 0.0099-86-5RI, MS
14LinaloolC10H18O14.94 1102.621102110231.00 ± 0.8178-70-6RI, MS [22]
151-Octenyl-3-acetateC10H18O215.27 1112.95110811081.04 ± 0.012442-10-6RI, MS [23]
16CamphoreC10H16O16.24 1143.76115111510.38 ± 0.01464-48-2RI, MS
17IsoborneolC10H18O16.91 1164.93115511552.87 ± 0.09124-76-5RI, MS
18terpinene-4-olC10H18O17.23 1175.07117711771.68 ± 0.07562-74-3RI, MS
19CryptoneC9H14O17.51 1178.79118711870.37 ± 0.03500-02-7RI, MS [30]
20α-TerpineolC10H18O17.63 1187.71119311931.46 ± 0.0498-55-5RI, MS
21NerolC10H1618.70 1221.48122812280.24 ± 0.00106-25-2RI, MS [31]
22Hexyl 2-methylbutyrateC11H22O219.04 1239.85123812380.17 ± 0.0110032-15-2RI, MS
23Linalyl acetate C12H20O219.50 1258.851253125330.27 ± 0.63115-95-7RI, MS
24Bornyl acetateC12H20O220.34 1288.55129212920.25 ± 0.0176-49-3RI, MS [31]
25Lavandulyl acetateC12H22O320.44 1292.25129312936.51 ± 0.1820777-39-3RI, MS [24]
26Neryl acetateC12H20O222.41 1362.20136613660.35 ± 0.01141-12-8RI, MS
27α-CopaeneC15H2422.91 1403.27137913790.59 ± 0.043856-25-5RI, MS
28β-CaryophylleneC15H2423.93 1437.36143114315.04 ± 0.1587-44-5RI, MS
29trans-α-bergamoteneC15H2424.29 1449.30143614360.24 ± 0.0113474-59-4RI, MS
30(E)-β-FameseneC15H2424.78 1465.74145914591.31 ± 0.0318794-84-8RI, MS
31D-GermacreneC15H2425.48 1488.93150315030.86 ± 0.0223986-74-5RI, MS [25]
32γ-CadineneC15H2426.27 1515.41151315130.42 ± 0.0139029-41-9RI, MS
33τ-CadinolC15H26O28.98 1605.74 0.34 ± 0.015937-11-1MS
SUM -- -99.29
Table 6. Compound composition of eye-catching LEO.
Table 6. Compound composition of eye-catching LEO.
NO.ComponentsMolecular
Formula		RT/minRI (cal)RI (ref)Relative
Content/%		CASMS
1α-pineneC10H169.50930.819391.18 ± 0.0080-56-8RI, MS
2CampheneC10H169.97945.759360.72 ± 0.0079-92-5RI, MS [27]
3α-SabineneC10H1610.81972.299700.43 ± 0.003387-41-5RI, MS
4β-PineneC10H1610.90974.919801.35 ± 0.01127-91-3RI, MS
51-Octen-3-olC8H16O11.07986.979790.23 ± 0.013391-86-4RI, MS
63-OctanoneC8H16O11.30994.339860.20 ± 0.00106-68-3RI, MS [32]
7MyrceneC10H1611.42991.319910.79 ± 0.02123-35-3RI, MS
83-CareneC10H1612.201016.2410180.19 ± 0.0013466-78-9RI, MS [33]
9p-Cymene C10H1412.471024.7410260.21 ± 0.0099-87-6RI, MS
10D-LimoneneC10H1612.601028.8510361.57 ± 0.015989-27-5RI, MS
11EucalyptolC10H18O12.701031.97103718.16 ± 0.06470-82-6RI, MS
12trans-β-OcimeneC10H1612.931039.1810451.85 ± 0.013779-61-1RI, MS [20]
13β-OcimeneC10H1613.261049.5110442.88 ± 0.0113877-91-3RI, MS [21]
14γ-Terpinene C10H1613.571059.4910630.19 ± 0.0099-85-4RI, MS
15α-terpineneC10H1614.501088.6910850.54 ± 0.0199-86-5RI, MS
16LinaloolC10H18O14.941102.78110227.51 ± 0.0878-70-6RI, MS
171-Octen-3-yl-acetateC10H18O215.271113.1111080.19 ± 0.052442-10-6RI, MS [22]
18CamphoreC10H16O16.251144.11115111.87 ± 0.0521368-68-3RI, MS [23]
19IsoborneolC10H18O16.891164.4211553.29 ± 0.03124-76-5RI, MS
20terpinene-4-ol C10H18O17.241175.2611770.85 ± 0.02562-74-3RI, MS
21α-TerpineolC10H18O17.641187.8711931.66 ± 0.0298-55-5RI, MS
22Linalyl acetate C12H20O219.491258.50125315.58 ± 0.04115-95-7RI, MS
23Lavandulyl acetateC12H20O220.441292.0712931.46 ± 0.0120777-39-3RI, MS [24]
24(E)-Hexyl 2-methylbut-2-enoateC11H20O221.521322.5113310.15 ± 0.0016930-96-4RI, MS
25α-FencheneC10H1622.411338.70 0.25 ± 0.17471-84-1MS
26β-CaryophylleneC15H2423.931437.3614193.92 ± 0.0387-44-5RI, MS
27trans-α-bergamoteneC15H2424.291449.4714360.28 ± 0.0113474-59-4RI, MS [34]
28(E)-β-FameseneC15H2424.781465.7414590.55 ± 0.0118794-84-8RI, MS
29D-GermacreneC15H2425.481489.0915030.70 ± 0.0123986-74-5RI, MS [25]
30Neryl propionateC13H22O226.081504.9115150.38 ± 0.01105-91-9RI, MS
31γ-CadineneC15H2426.281515.5815130.32 ± 0.0039029-41-9RI, MS [26]
32τ-CadinolC15H26O28.981605.94 0.33 ± 0.015937-11-1MS
SUM ---99.78
Table 7. Compound composition of true LEO.
Table 7. Compound composition of true LEO.
NO.ComponentsMolecular FormulaRT/minRI (cal)RI (ref)Relative Content/%CASMS
1α-PineneC10H169.50930.659390.23 ± 0.0080-56-8RI, MS
21-Octen-3-olC8H16O11.07986.779790.21 ± 0.003391-86-4RI, MS
33-OctanoneC8H16O11.28993.809861.17 ± 0.01106-68-3RI, MS [32]
4β-MyrceneC10H1611.41991.159910.28 ± 0.01123-35-3RI, MS
53-OctanolC8H18O11.591004.069970.27 ± 0.00589-98-0RI, MS
6Hexyl acetateC8H16O212.171023.0610110.27 ± 0.00142-92-7RI, MS [28]
7p-CymeneC10H1412.471024.5810260.26 ± 0.0099-87-6RI, MS
8D-LimoneneC10H1612.601028.6910360.95 ± 0.015989-27-5RI, MS
9EucalyptolC10H18O12.691031.4710370.90 ± 0.01470-82-6RI, MS
10trans-β-OcimeneC10H1612.931039.0210453.18 ± 0.033779-61-1RI, MS [20]
11β-OcimeneC10H1613.251049.1910441.57 ± 0.0113877-91-3RI, MS
12LinalolC10H18O14.931102.46110224.60 ± 0.1978-70-6RI, MS
131-Octenyl-3-acetateC10H18O215.261112.8011080.83 ± 0.012442-10-6RI, MS
14CamphoreC10H16O16.241143.7611510.24 ± 0.0021368-68-3RI, MS
15IsoborneolC10H18O16.921165.0911551.63 ± 0.00124-76-5RI, MS
16terpinene-4-olC10H18O17.231175.0711773.70 ± 0.03562-74-3RI, MS
17CryptoneC9H14O17.501178.6411870.25 ± 0.02500-02-7RI, MS
18α-TerpineolC10H18O17.631187.7111930.42 ± 0.0110482-56-1RI, MS
19Linalyl acetateC12H20O219.521248.58125340.81 ± 0.21115-95-7RI, MS
20Lavandulyl acetateC12H20O220.441291.7612934.14 ± 0.0120777-39-3RI, MS [24]
21β-Caryophyllene C15H2423.931437.3614195.83 ± 0.0187-44-5RI, MS
22trans-2-Hydroxycinnamic acidC9H8O324.341388.87 1.62 ± 0.01614-60-8MS
23(E)-β-FameseneC15H2424.781465.7414594.09 ± 0.0218794-84-8RI, MS
24D-GermacreneC15H2425.471488.7615030.91 ± 0.0123986-74-5RI, MS [25]
25Caryophyllene oxideC15H24O27.891569.58 0.81 ± 0.011139-30-6MS
26τ-CadinolC15H26O28.981605.77 0.22 ± 0.005937-11-1MS
27HerniarinC10H8O330.351589.70 0.67 ± 0.03531-59-9MS
SUM ---100
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Lin, L.; Lv, Z.; Wang, M.; Kan, A.; Zou, S.; Wu, B.; Guo, L.; Edirs, S.; Liu, J.; Zhu, L. Comparative Analysis of Chemical Composition and Antibacterial Activity of Essential Oils from Five Varieties of Lavender Extracted via Supercritical Fluid Extraction. Molecules 2025, 30, 217. https://doi.org/10.3390/molecules30020217

AMA Style

Lin L, Lv Z, Wang M, Kan A, Zou S, Wu B, Guo L, Edirs S, Liu J, Zhu L. Comparative Analysis of Chemical Composition and Antibacterial Activity of Essential Oils from Five Varieties of Lavender Extracted via Supercritical Fluid Extraction. Molecules. 2025; 30(2):217. https://doi.org/10.3390/molecules30020217

Chicago/Turabian Style

Lin, Lijing, Zhencheng Lv, Meiyu Wang, Ankang Kan, Songling Zou, Bin Wu, Limin Guo, Salamet Edirs, Jiameng Liu, and Lin Zhu. 2025. "Comparative Analysis of Chemical Composition and Antibacterial Activity of Essential Oils from Five Varieties of Lavender Extracted via Supercritical Fluid Extraction" Molecules 30, no. 2: 217. https://doi.org/10.3390/molecules30020217

APA Style

Lin, L., Lv, Z., Wang, M., Kan, A., Zou, S., Wu, B., Guo, L., Edirs, S., Liu, J., & Zhu, L. (2025). Comparative Analysis of Chemical Composition and Antibacterial Activity of Essential Oils from Five Varieties of Lavender Extracted via Supercritical Fluid Extraction. Molecules, 30(2), 217. https://doi.org/10.3390/molecules30020217

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