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Article

Antioxidant Activity and Volatile Oil Analysis of Ethanol Extract of Phoebe zhennan S. Lee et F. N. Wei Leaves

by
Liping Yu
1,†,
Wang Cheng
1,†,
Meifen Tian
2,
Zhigang Wu
1,3,*,
Xiaoli Wei
1,*,
Xing Cheng
4,
Mingwei Yang
5 and
Xuan Ma
5
1
College of Forestry, Guizhou University, Guiyang 550025, China
2
Xifeng County Bureau of Natural Resources, Guiyang 551100, China
3
International Joint Research Center for Biomass Materials, Southwest Forestry University, Kunming 650224, China
4
Dozheng County Bureau of Forestry, Zunyi 563500, China
5
Zhejiang Academy of Forestry, Hangzhou 310000, China
*
Authors to whom correspondence should be addressed.
These authors contributed equally to this work.
Forests 2024, 15(2), 236; https://doi.org/10.3390/f15020236
Submission received: 30 November 2023 / Revised: 2 January 2024 / Accepted: 23 January 2024 / Published: 26 January 2024
(This article belongs to the Special Issue Advances in the Cultivation, Protection and High-Value Utilization of Forest Resources)
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Abstract

:
The medicinal value of P. zhennan has been documented in traditional Chinese medicine books. The aim of this paper was to study the antioxidant activity of alcoholic extracts of P. zhennan leavesusing 1,1-diphenyl-2-picrylhydrazyl (DPPH) and 2-phenyl-4,4,5,5-tetramethylimidazolineoxyl-1-oxyl-3-oxide (PTIO) radical scavenging and ferric ion reducing antioxidant power (FRAP) assays. The active components of the leaves were identified via headspace solid-phase microextraction and gas chromatography–mass spectrometry (HS-SPME-GC-MS). The results showed that the scavenging rate of DPPH was 94.67%with an EC50 value of 0.674 mg/mL at a concentration of 2 mg/mL. The maximum scavenging rate was 47.40% at a Trolox equivalent of 0.33 mg TE/mL for PTIO radicals. The FRAP reached 84.80% at 0.20 mg/mL concentration. The results confirmed the strong antioxidant activity of the extracts. Furthermore, 44 compounds, mostly terpenoids, obtained from the alcoholic extracts of P. zhennan leaves were analyzed using HS-SPME-GC-MS and 15 of these compounds had a relative content exceeding 1%. The strong antioxidant activity of the alcoholic extracts of P. zhennan leaves could be attributed to the presence of copaene (33.97%), β-caryophyllene (4.42%), δ-cadinene (11.04%), γ-muurolene (4.78%), cis-calamenene (2.02%), linalool (1.04%), α-pinene (1.46%), borneol acetate (1.5%), and γ-terpinene (0.66%). This study demonstrates the potential medicinal value of alcoholic extracts of P. zhennan leaves.

1. Introduction

Phoebe zhennan is a member of the Lauraceae family; its use in infectious, internal, and dermatological diseases is clearly documented in traditional Chinese pharmacological books, such as Zheng lei ben cao, Taiping Shenghui Fang, and Puji Fang. Numerous studies have shown that antioxidant can effectively prevent aging and many diseases. Antioxidation is the abbreviation of antioxidant free radicals. When the human body is in continuous contact with the external environment, free radicals are continuously produced in the body through factors such as respiration (oxidation reaction), external pollution, and radiation exposure. Free radicals break down cells and tissues, affecting metabolic function and causing varying degrees of health problems. For example, common cancers [1], aging [2], diabetes [3], respiratory diseases [4], nervous system diseases [5], and so on are all related to oxidative free radicals. If excessive oxidative free radicals are eliminated, many aging and related diseases caused by free radicals can be prevented. Many natural plant extracts have been shown to have antioxidant activity, so the search for plant-derived antioxidants is increasing [6,7,8]. However, there are few reports on the antioxidant activity of P. zhennan. The antioxidant activity can be reflected by an in vitro antioxidant activity test, that is, the scavenging ability of the tested samples to synthetic free radicals is evaluated [9,10,11,12]. Common artificial free radicals include 1,1-diphenyl-2-picrylhydrazyl radical (DPPH), ABTS radical, 3-oxo-2-phenyl-4,4,5,5-tetramethylimidazoline-1-oxygen radical (PTIO) [13,14,15], etc. The determination of iron ion reducing power (FARP) is also a common method to evaluate antioxidant activity [16]. The evaluation indexes of free radical scavenging activity include free radical scavenging rate, half inhibitory concentration (IC50) [17], half effective concentration (EC50), and Trolox equivalent [18,19,20,21,22].
The antioxidant activity of a plant is related to the chemical composition of the extract. Traditional extraction methodsall suffer from low extraction efficiency and a serious waste of resources. However, as an emerging plant extraction method, ultrasonic-assisted extraction technology accelerates extraction efficiency, saves energy, and protects the environment. It is regarded as a “green technology” and has been widely used to extract and separate active ingredients in plants. In this study, absolute ethanol was used to extract the active ingredients of P. zhennan leaves via ultrasonic technology. Headspace solid-phase microextraction and gas chromatography–mass spectrometry (HS-SPME-GC-MS) technology was used to analyze the active ingredients in P. zhennan leaves to clarify their mechanism of action further. Based on the record of its medical effects in traditional Chinese pharmaceutical works, this study explores the novelty and significance of its antioxidant activity.

2. Materials and Methods

2.1. Materials

The leaves of Phoebe zhennan S. Lee et F. N. Wei were harvested on 18 October 2021, from QingLang Village, Zhouxi Town, Kaili City, Guizhou Province, China (107.8679997 E, 26.4462369 N). The main reagents used were DPPH, water-soluble vitamin E (Trolox), PTIO, dihydrogen phosphate, sodium chloride, 1% potassium ferricyanide, 10% trichloroacetic acid solution, 0.1% ferric chloride solution, and anhydrous ethanol. All reagents were analytically pure and bought from Shanghai Aladdin Biochemical Technology Co. (Shanghai, China).
The main instruments and equipment used were an SY-2000 rotary evaporator (Shanghai Yarong Biochemical Instrument Factory; Shanghai, China), a 7890A-5975C gas chromatograph (Agilent Technologies; Santa Clara, CA, USA), and 50/30 μm PDMS/CAR/DVB (2 cm) extraction fiber (Supelco; Bellefonte, PA, USA).

2.2. Ultrasonic-Assisted Ethanol Extraction

After picking the samples, the leaves of P. zhennan were placed in a clean, cool, and dry place to dry in the shade. Dried leaves of the appropriate quantity were crushed and passed through a 60-mesh sieve. Thereafter, a 15 g sample was transferred into a 250 mL wide-mouth bottle, and anhydrous ethanol was added as the extraction solution. The extraction was repeated three times; the extract was centrifuged at 3000 r/min for 10 min and then vacuum filtered and concentrated with a rotary evaporator.

2.3. DPPH Radical Scavenging Assay

We used the reference [13] method with slight modifications. Exactly 6.9 mg of the DPPH standard sample was weighed and dissolved in anhydrous ethanol to make a final volume of 250 mL under light-proof conditions. Anhydrous ethanol was used as the blank control. The absorbance (OD) was measured at 517 nm for 30 min after the reaction under light-proof conditions, with three replicates. The concentration of the DPPH solution on the X-axis and the OD value on the Y-axis gave the DPPH standard curves.
Different concentrations of the alcoholic extracts of P. zhennan and Trolox standard (water-soluble vitamin E) solutions were also prepared. Measure the absorbance of the DPPH solution as A1. Measure the absorbance of the experimental group (P. zhennan and Trolox) as A. Measure the blank absorbance of the sample as A0. The above measurements were zeroed with anhydrous ethanol, and the free radical scavenging rate was calculated using the formula shown in the following equation. The EC50 was calculated using GraphPad Prism 9 software (Graphstats Technologies, Bengaluru, India).
Scavenging   Rate   of   DPPH   Radical   ( % ) = A 1   ( A     A 0 ) A 1 × 100 %

2.4. PTIO Radical Scavenging Assay

We used the method described in the literature [15] with slight modifications. The PTIO solution was prepared by weighing 45 mg of the PTIO standard sample and fixing the volume to 200 mL with anhydrous ethanol; it was stored at 4 °C until use. Trolox standard solutions were prepared at concentrations of 4, 2, 1, 0.5, 0.25, and 0.125 mg/mL, and the scavenging rate of PTIO radicals by Trolox at different concentrations was determined. The Trolox standard curves were plotted with the Trolox concentration as the X-axis and the scavenging rate as the Y-axis. The different concentrations of the alcohol extract solution of P. zhennan leaves were configured sequentially. The absorbance was measured at 557 nm after a 30 min reaction at 37 °C in a water bath. Measure the absorbance of the PTIO solution as A1. Measure the absorbance of the experimental group (P. zhennan and Trolox) as A. Measure the blank absorbance of the sample as A0. The above measurements were zeroed with anhydrous ethanol, and each measurement was repeated 3 times to calculate the free radical scavenging rate using the formula shown in the following equation.
Scavenging   Rate   of   PTIO   Radical   ( % ) = A 1   ( A A 0 ) A 1 × 100 %

2.5. PRAP Assay

The reference method [16] was used with slight modifications. We made a 0.2 mol/L phosphate-buffered solution (pH = 6.6). Then, 1.74 g of sodium dihydrogen phosphate, 2.7 g of disodium hydrogen phosphate, and 1.7 g of sodium chloride with an analytical balance were dissolved in distilled water, and the volume was made up to 400 mL. A 1 mL aliquot each of 0.2 mol/L phosphate buffer and 1% potassium ferricyanide solution was added to 1.2 mL each of 0.05, 0.1, 0.15, 0.2, 0.25, and 3 mg/mL concentrations of selenium alcohol extract. The resulting mixture was placed in a constant-temperature water bath at 50 °C for 20 min and then cooled rapidly. Then, we added 1 mL of a 10% trichloroacetic acid solution and centrifuged at 3000 r/min for 10 min.
Further, we added 0.5 mL of 0.1% ferric chloride solution to 2.5 mL of the supernatant, mixed well, and added distilled water to obtain a final volume of 5 mL. Absorbance A was measured at 700 nm after 10 min. The solvent was replaced with distilled water to determine the absorbance of the sample blank A0; the absorbance of the test control was recorded as A1, and Trolox was used as the positive control. Three replicates of each measurement were used to calculate the ferric ion-reducing capacity using the formula in the following equation.
FRAP   ( % ) = A   A 1 A 0 A × 100 %

2.6. HS-SPME-GC-MS Analysis

Sample treatment: To perform HS-SPME-GC-MS, the leaves were crushed separately and sieved through a 60-mesh sieve; 1 g of leaf powder was weighed into a 15 mL extraction vial and sealed quickly. The fiber head was aged at 250 °C in the GC-MS inlet until there were no spurious peaks. The sample vial was placed in the SPME device, and the temperature was set at 35 °C. The sample vial was placed in the extraction device to preheat for 15 min, and the SPME head was inserted into the headspace portion of the sample through the vial cap. The fiber head was pushed out. The extraction head was approximately 1.0 cm above the upper surface of the sample, and the headspace extraction was performed for 40 min. The fiber head was withdrawn, and the extraction head was pulled out of the sample vial. Then, the extraction head was inserted into the GC-MS inlet, the fiber head was pushed out, and the sample was analyzed at 250 °C for 3 min.
Chromatographic conditions: The chromatographic column used was DB-WAX (30.0 m × 250 μm, 0.25 μm). The column was started at 40 °C and held for 5 min, ramped up to 180 °C at 10 °C/min, held for 5 min, and then ramped up at 20 °C/min to 250 °C. The gas chamber temperature was 250 °C, and the transfer line temperature was 250 °C. The carrier gas was He, and the carrier gas flow rate was 1.0 mL/min; there was no shunt.
Mass spectrometer conditions: EI source; electron energy 70 eV; ion source temperature 230 °C; quadrupole 150 °C; scan mode Scan; scan mass range 35–550 µ.
Qualitative and quantitative analyses: Using the MS database NIST11, we detected the retention time and retention index. Database screening of the results was performed to deduct parameters such as column loss peak. The area normalization method was used to quantify the quantitative results, i.e., the percentage of the peak area of the identified component to the sum of the areas of all identified components. The following formula was used:
C i = A i A 1 + A 2 + A i + A n × 100 %
where:
  • Ci = content of an identified component, %;
  • Ai = the peak area corresponding to an identified component;
  • n = the total number of identified components.

3. Results and Discussion

3.1. DPPH Radical-Scavenging Activities

The DPPH standard curve is shown in Figure 1A, and the fitted equation is Y = 0.008058X + 0.003886, R2 = 0.9966. The absorbance of DPPH was significantly linearly correlated with the concentration. According to Beer’s law, the spectrophotometer transmission ratio has the highest accuracy in the range of 20% to 60% absorbance [23], i.e., absorbance in the range of 0.222–0.699 is appropriate. The analytical equation showed that the absorbance was 0.555 Abs when the concentration was 70 μmol/L, which met the accuracy requirement. Thus, the concentration was selected for the subsequent test.
The scavenging ability of DPPH radicals and the correlation between the two at different concentrations of the alcoholic extracts of P. zhennan leaves are shown in Figure 1 and Figure 2. As shown in Figure 1B and Figure 2C, with Trolox as the positive control, trolox at 0.125–4 mg/mL had a scavenging rate of approximately 96.41%, and it showed strong antioxidant activity. The concentration-dependent scavenging rate of DPPH by the alcoholic extracts of P. zhennan leaves was extremely significant (p < 0.0001) before reaching 2 mg/mL, and the scavenging rate reached 49.04% when the concentration was 0.125 mg/mL. The scavenging rate increased rapidly with increasing concentration. As the concentration increased to 2 mg/mL, the scavenging rate of DPPH by the alcoholic extracts of P. zhennan leaves reached 94.67% and then became stable. This was only 1.74% lower than Trolox’s scavenging rate of 96.41%, indicating that the scavenging effect of Siberian hemlock alcoholic extracts on DPPH was significant. Considering the utilization rate and scavenging effect, the optimal concentration of DPPH radicals scavenged by the alcoholic extracts of P. zhennan leaves was 2 mg/mL.
EC50 is the antioxidant concentration that reduces the concentration of DPPH free radicals by 50%; the lower the EC50 value, the stronger the scavenging ability. The EC50 value for DPPH free radicals from the alcoholic extract of P. zhennan leaves was 0.674 mg/mL, as calculated using the regression model in the program GraphPad Prism 9 (Figure 1D). According to the results, Wild Z. spina-christi of Ethiopia and Z. jujube fruit species of India are rich in antioxidant elements, such as magnesium, zinc, and selenium. They have been reported to have an EC50 of 2.94–7.75 mg/mL of DPPH free radicals [24,25]. In contrast, the EC50 of the alcoholic extract of P. zhennan leaves is only 8.69%–22.92% of theirs, which somehow corresponds to a decrease of 77.08%–91.31%. The analysis of its bioactive components also suggests that it could be a potential antioxidant.

3.2. PTIO Radical-Scavenging Activities

The color of the PTIO solution is bluish purple, which fades when it reacts with antioxidants. PTIO solution has a strong absorption peak at 557 nm. The absorbance of PTIO at a concentration of 0.225 mg/mL was tested to be 0.347, which conforms to Beer’s law; thus, this concentration was chosen for the test. The results of PTIO radical-scavenging activities were shown in Figure 2. As shown in Figure 2A, the scavenging effect of PTIO radical scavenging increases slowly with increasing concentration when the concentration is below 4 mg/mL, with a linear fit slope of 0.02445 and R2 = 0.8203. In the range of 4–8 mg/mL, the linear fit slope is 0.07837 and R2 = 0.9572, with strong linearity of the quantitative-efficacy relationship. The scavenging rate increased rapidly, approximately 3.2 times that at concentrations below 4 mg/mL. At 8 mg/mL concentration, the scavenging rate reached 47.40 %, followed by a flattening of the quantitative-efficacy curve, indicating a maximum scavenging rate of 47.79 % for free radicals.The scavenging rate of PTIO by the extract of P. zhennan leaves at maximum concentration is similar to that of the water extracts of six traditional Chinese medicine plants selected in theexperiment by Li [15], including Angelicae sinensis radix, at similar concentrations.
As shown in Figure 2B, the EC50 value of the ethanol extract of P. zhennan leaves to PTIO free radical was 5.405 mg/mL by regression model calculation. As shown in Figure 2C, PTIO is more stable than DPPH, and Trolox reaches an 86.63% scavenging rate only at a concentration of 4 mg/mL. The fitted equation for the scavenging rate of PTIO radicals by Trolox is Y = −0.4225e (−x/0.1320) − 0.5008e (−x/1.029) + 0.8750, R2 = 0.9941. The antioxidant capacity can be reflected by the TEAC, which compares the antioxidant capacity of a given substance with that of the standard antioxidant substance Trolox. The higher the TEAC value, the higher the antioxidant capacity. The TEAC for PTIO radical scavenging ability of the alcoholic extracts of P. zhennan leaves was found to be 0.33 mg TE/mL.

3.3. PRAP Test Analysis

The ferric ion reduction method refers to the ability of the sample to reduce the trivalent iron of potassium ferricyanide to divalent iron, yielding potassium ferrocyanide. Under acidic conditions, potassium ferricyanide reacts with ferric chloride to form ferricyanide, which has an absorption peak at 700 nm. The stronger the reducing ability of the sample is, the higher the absorbance at 700 nm, and the stronger the antioxidant performance is. The reducing ability of ferric ions is shown in Figure 3A. The figure shows that the reducing ability of Trolox increases with concentration and reaches a strong reducing ability of 94.98% at aconcentration of 0.25 mg/mL. In contrast, the ferrous ion reduction capacity of the alcoholic extract of the leaves of P. zhennan increased with increasing concentration and then slightly decreased and stabilized at concentrations above 0.20 mg/mL. The highest reducing capacity of the alcoholic extract of P. zhennan leaves was 84.80%, which was lower than that of the positive control Trolox; however, the extract had a strong reducing capacity, proving its strong antioxidant capacity. As shown in Figure 3B, the fitting equation of Trolox PRAP is Y = −246.1 + (0.9462 + 246.1)/(1 + 10 ^ (−0.3684 − x) × 8.026), R2 = 0.9816. Through analysis, the Trolox equivalent was 0.03 mg TE/mL when the iron ion reduction ability of P. zhennan ethanol extract reached itsmaximum. It is worth noting that the research results proposed by Wojtunik [26] indicate that in the case of spectrophotometric determination, isoterpenol and linalool exhibit high reducing activity. In addition, α-terpenes, γ-terpenes, and other compounds have reducing activity. This is consistent with the composition analysis in the following text, which mainly focuses on terpenoids. Therefore, the abundance of terpenoids can be considered as the reason for the reducing ability of P. zhennan leaves. However, further investigation is needed.

3.4. Active Constituents

The HS-SPME-GC-MS total ion flow diagram is shown in Figure 4. There are many peaks in the volatile component spectrum of P. zhennan leaves. These peaks were searched with the NIST database. As described in Section 2.6, impurity peaks such as polyoxysilane (the column loss component) are subtracted and normalized using the area method. A total of 99 compounds were obtained from the leaves using HS-SPME-GC-MS, and 44 compounds were analyzed for each compound after excluding the data with a match lower than 80%. Among them, there are 21 kinds of sesquiterpenes, 6 kinds of alkenes, 7 kinds of monoterpenes, 2 kinds of monoterpene alcohols, 3 kinds of aromatic hydrocarbons, 1 kind of acid, 1 kind of aromatic ester, and 3 other kinds.
A total of 15 compounds had a relative content of more than 1%, and the highest relative content was copaene (33.97%). Other compounds included δ-cadinene (11.04%), γ-muurolene (4.78%), α-muurolene (4.68%), β-caryophyllene (4.42%), and eucalyptol (3.31%), 1,4,7,-cycloundecatriene, 1,5,9,9-tetramethyl-, Z,Z,Z- (2.99%), cis-calamenene (2.02%), β-elemene (1.7%), benzocyclobutene (1.63%), borneol acetate (1.5%), α-pinene (1.46%), ylangene (1.34%), β-patchoulene (1.07%), and linalool (1.04%), as detailed in Table 1. The active ingredients in P. zhennan leaves are mostly terpenoids. These terpenoids possess similar structures and activities, such as bacteriostatic, anticancer, and antioxidant qualities.
Copaene, γ-muurolene, and δ-cadinene were also reported in the bark of Cinnamomum loureirii from the Lauraceae family. Copaene, γ-muurolene, and δ-cadinene are sesquiterpenes, and their contents are significantly and positively correlated with the antioxidant activity of FRAP and ABTS [27]. Studies have shown that many sesquiterpenes have good antioxidant activity and antibacterial effects. As the most abundant sesquiterpene in this study, copaene is widely found in many plants [28,29] and has antibacterial and antioxidant properties [30]. Its chemical properties are active, andit has a variety of reaction capabilities and great potential for modification. It can prepare a variety of derivatives, and its derivatives also have anti-tumor cell proliferation activity [31,32]. It can also synthesize flame retardants, sweeteners, plasticizers, attractants, functional materials, etc. [33]. Therefore, the product development of copaene and its derivatives has become the focus. cis-Calamenene is a sesquiterpene; along with α-pinene, it is also a major component of plants such as Juniperus oxycadrus that have good antioxidant activity [34,35]. β-Caryophyllene is a natural terpene. Caryophyllene is a natural bicyclic sesquiterpene with strong antioxidant activity. Dahham reported that caryophyllene’s IC50 values for DPPH and FRAP were 1.25 and 3.23 µM, respectively [36]. Linalool is an oxygenated monoterpene with an EC50 of only 6.78 µg/mL for ABTS [37]; this reveals the pharmacological potential of linalool.
γ-Terpinene (0.66%) is also a terpene, and although its relative content in P. zhennan leaves is low, it has strong antioxidant activity and xanthine oxidase inhibitory capacity with borneol acetate [38]. γ-Terpinene has antioxidant potential, with an IC50 against DPPH of only 122 ± 2.5 μg/mL [39]. Both α-curcumene (0.29%) and β-bourene (0.09%) belong to sesquiterpenes. Although they account for only 0.35% and 0.32% ofanhydrous ethanol extract, α-curcumene has a certain inhibitory effect on Escherichia coli and Staphylococcus aureus [40]. β-Bourenes hows a wide range of antibacterial activity against Gram-positive and Gram-negative bacteria and three pathogenic fungi [41].
The antioxidant activity of P. zhennan leaves may result from the combined effects of its compounds. Considering the year-round harvest ability and short-term reproducibility of P. zhennan leaves, they have potential medicinal value. However, this study didnot fractionally extract the active components of P. zhennan leaves, and its antioxidant mechanism has not been fully revealed. In the future, we can consider further research in this direction.

4. Conclusions

It was determined that the P. zhennan leaves have strong antioxidant activity through in vitro antioxidant activity methods. Furthermore, based on HS-SPME-GC-MS analysis, 44 compounds, mainly terpenoids, were identified from P. zhennan leaves in this paper. P. zhennan leaves have potential medicinal value. Other properties, such as toxicology, should be evaluated before they can be used in humans. In addition, this study had some limitations. Fractional extraction of the active components of P. zhennan leaves was not performed. Thus, the antioxidant mechanism has not been fully revealed, and an in-depth study in this direction can be considered in the future.

Author Contributions

Conceptualization, methodology, L.Y. and W.C.; validation, L.Y., W.C., M.T. and X.C.; formal analysis, L.Y., W.C., M.Y. and X.M.; resources, M.T., X.C., M.Y. and X.M.; writing—original draft preparation, L.Y. and W.C.; writing—review and editing, W.C., M.T. and X.C.; investigation, visualization, supervision, Z.W. and X.W. All authors have read and agreed to the published version of the manuscript.

Funding

This work was supported by the National Natural Science Foundation of China (31870613 and 32160413), the High-level Innovative Talents Training Plan Project of Guizhou Province of China ([2016]5661), and the Outstanding Youth Science and Technology Talent Project of Guizhou Province of China (YQK[2023]003), International Joint Research Center for Biomass Materials Open Fund (2023-GH05) and Supported by the 111 Project (D21027).

Data Availability Statement

The data presented in this study are available upon reasonable request from the corresponding author.

Conflicts of Interest

The authors declare no conflicts of interest.

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Forests 15 00236 g001
Figure 1. (A) The DPPH standard curve. (B) The dose–effect curve of Trolox and P. zhennan to DPPH. (C) Correlation analysis of the DPPH scavenging rate between Trolox and P. zhennan at different concentrations. ****, significant difference (p < 0.0001); ns, no significant difference (p > 0.05). (D) The EC50 of P. zhennan on DPPH.
Figure 1. (A) The DPPH standard curve. (B) The dose–effect curve of Trolox and P. zhennan to DPPH. (C) Correlation analysis of the DPPH scavenging rate between Trolox and P. zhennan at different concentrations. ****, significant difference (p < 0.0001); ns, no significant difference (p > 0.05). (D) The EC50 of P. zhennan on DPPH.
Forests 15 00236 g001
Forests 15 00236 g002
Figure 2. (A) The dose–effect curve of P. zhennan to PTIO. (B) The EC50 of P. zhennan on DPPH. (C) The clearance rate of PTIO by Trolox.
Figure 2. (A) The dose–effect curve of P. zhennan to PTIO. (B) The EC50 of P. zhennan on DPPH. (C) The clearance rate of PTIO by Trolox.
Forests 15 00236 g002
Forests 15 00236 g003
Figure 3. (A) The reduction ability of P. zhennan and Trolox; (B) The EC50 of P. zhennan on PRAP.
Figure 3. (A) The reduction ability of P. zhennan and Trolox; (B) The EC50 of P. zhennan on PRAP.
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Forests 15 00236 g004
Figure 4. TIC of volatile components in P. zhennan leaves.
Figure 4. TIC of volatile components in P. zhennan leaves.
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Table 1. Main active components and relative contents of P. zhennan leaves.
Table 1. Main active components and relative contents of P. zhennan leaves.
NO.TR/minCompoundMWCASContent/%Structure
11.24α-Pinene136.1280-56-81.46Forests 15 00236 i001
22.35Camphene136.1279-92-50.48Forests 15 00236 i002
37.08α-Terpinene136.1299-86-50.47Forests 15 00236 i003
47.66D-Limonene136.125989-27-50.88Forests 15 00236 i004
57.89(±)-Sabinene136.123387-41-50.48Forests 15 00236 i005
67.96Eucalyptol154.14470-82-63.31Forests 15 00236 i006
78.83trans-β-Ocimene136.123779-61-10.82Forests 15 00236 i007
88.95γ-Terpinene136.1299-85-40.66Forests 15 00236 i008
99.15Benzocyclobutene104.06694-87-11.63Forests 15 00236 i009
109.48m-Cymene134.11535-77-30.74Forests 15 00236 i010
119.78Terpinolene136.12586-62-90.23Forests 15 00236 i011
1213.3Ylangene204.1914912-44-81.34Forests 15 00236 i012
1313.46Copaene204.193856-25-533.97Forests 15 00236 i013
1413.79β-Bourene204.195208-59-30.09Forests 15 00236 i014
1513.9Alloaromadendrene204.1917334-55-30.26Forests 15 00236 i015
1613.95(−)-α-Gurjunene204.19489-40-70.51Forests 15 00236 i016
1713.99(+)-Sativene204.193650-28-00.38Forests 15 00236 i017
1814.16Linalool154.1478-70-61.04Forests 15 00236 i018
1914.46α-Bergamotene204.1917699-05-70.41Forests 15 00236 i019
2014.59Borneol acetate196.155655-61-81.5Forests 15 00236 i020
2114.64Fenchol154.141632-73-10.52Forests 15 00236 i021
2214.68Zingiberene204.19495-60-30.27Forests 15 00236 i022
2314.73β-Elemene204.19110823-68-21.7Forests 15 00236 i023
2414.83β-Caryophyllene204.1987-44-54.42Forests 15 00236 i024
2514.96β-Patchoulene204.19514-51-21.07Forests 15 00236 i025
2615.16α-Elemene204.195951-67-70.3Forests 15 00236 i026
2715.38(+)-γ-Cadinene204.1939029-41-90.39Forests 15 00236 i027
2815.45Aromandendrene204.19489-39-40.27Forests 15 00236 i028
2915.731,4,7,-Cycloundecatriene, 1,5,9,9-tetramethyl-, Z,Z,Z-204.191000062-61-92.99Forests 15 00236 i029
3015.82-Isopropenyl-4a,8-dimethyl-1,2,3,4,4a,5,6,7-octahydronaphthalene204.191000192-43-50.92Forests 15 00236 i030
3115.96γ-Muurolene204.1930021-74-04.78Forests 15 00236 i031
3216.09(+)-Borneol154.141000150-76-30.47Forests 15 00236 i032
3316.22Isoledene204.191000156-10-80.76Forests 15 00236 i033
3416.38α-Muurolene204.1931983-22-94.68Forests 15 00236 i034
3516.53Cedr-8-ene204.19469-61-40.02Forests 15 00236 i035
3616.75δ-Cadinene204.19483-76-111.04Forests 15 00236 i036
3716.89α-Curcumene202.17644-30-40.29Forests 15 00236 i037
3817.15α-Cadinene204.1924406-05-10.39Forests 15 00236 i038
3917.58cis-Calamenene202.17483-77-22.02Forests 15 00236 i039
4021.046-Isopropyl-1,4-dimethylnaphthalene198.14489-77-00.03Forests 15 00236 i040
4121.49Dimethyl phthalate194.06131-11-30.32Forests 15 00236 i041
4222.14Cadalene198.14483-78-30.01Forests 15 00236 i042
4325n-Hexadecanoic acid256.2457-10-30.13Forests 15 00236 i043
4425.74Erucamide337.33112-84-50.23Forests 15 00236 i044
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Yu, L.; Cheng, W.; Tian, M.; Wu, Z.; Wei, X.; Cheng, X.; Yang, M.; Ma, X. Antioxidant Activity and Volatile Oil Analysis of Ethanol Extract of Phoebe zhennan S. Lee et F. N. Wei Leaves. Forests 2024, 15, 236. https://doi.org/10.3390/f15020236

AMA Style

Yu L, Cheng W, Tian M, Wu Z, Wei X, Cheng X, Yang M, Ma X. Antioxidant Activity and Volatile Oil Analysis of Ethanol Extract of Phoebe zhennan S. Lee et F. N. Wei Leaves. Forests. 2024; 15(2):236. https://doi.org/10.3390/f15020236

Chicago/Turabian Style

Yu, Liping, Wang Cheng, Meifen Tian, Zhigang Wu, Xiaoli Wei, Xing Cheng, Mingwei Yang, and Xuan Ma. 2024. "Antioxidant Activity and Volatile Oil Analysis of Ethanol Extract of Phoebe zhennan S. Lee et F. N. Wei Leaves" Forests 15, no. 2: 236. https://doi.org/10.3390/f15020236

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