Identification of Chemical Constituents in Blumea balsamifera Using UPLC–Q–Orbitrap HRMS and Evaluation of Their Antioxidant Activities

Blumea balsamifera (L.) DC., a perennial herb in the Asteraceae family native to China and Southeast Asia, has a notable history of medicinal use due to its pharmacological properties. Using UPLC–Q–Orbitrap HRMS techniques, we systematically investigated the chemical constituents of this plant. A total of 31 constituents were identified, of which 14 were flavonoid compounds. Significantly, 18 of these compounds were identified in B. balsamifera for the first time. Furthermore, the mass spectrometry fragmentation patterns of significant chemical constituents identified in B. balsamifera were analyzed, providing important insights into their structural characteristics. The in vitro antioxidative potential of the methanol extract of B. balsamifera was assessed using DPPH and ABTS free-radical-scavenging assays, total antioxidative capacity, and reducing power. The antioxidative activity exhibited a direct correlation with the mass concentration of the extract, with IC50 values of 105.1 ± 0.503 μg/mL and 12.49 ± 0.341 μg/mL for DPPH and ABTS, respectively. For total antioxidant capacity, the absorbance was 0.454 ± 0.009 at 400 μg/mL. In addition, the reducing power was 1.099 ± 0.03 at 2000 μg/mL. This study affirms that UPLC–Q–Orbitrap HRMS can effectively discern the chemical constituents in B. balsamifera, primarily its flavonoid compounds, and substantiates its antioxidative properties. This underscores its potential utility as a natural antioxidant in the food, pharmaceutical, and cosmetics sectors. This research provides a valuable theoretical basis and reference value for the comprehensive development and utilization of B. balsamifera and expands our understanding of this medicinally valuable plant.


Introduction
Oxidative stress, a pathological condition induced by an imbalance between reactive oxygen species' (ROS) production and the biological system's ability to detoxify these reactive intermediates, contributes to several chronic diseases such as cancer, diabetes, cardiovascular diseases, neurodegenerative disorders, and aging. Antioxidants have the potential to quell this imbalance by neutralizing ROS, thereby preventing or delaying cellular damage [1]. Plant-derived antioxidants, owing to their availability, safety, and therapeutic efficacy, have been the focus of many studies. Plants, with their extensive repertoire of phytochemicals such as polyphenols, flavonoids, and terpenoids, among others, have demonstrated significant antioxidant activity [2][3][4].
Blumea balsamifera (L.) DC., a herbaceous plant from the Asteraceae family, is extensively distributed in tropical and subtropical regions, including countries such as China, Thailand, Vietnam, the Philippines, and Malaysia [5]. The first documented use of it as a medicine in China can be traced back to 652 A.D., primarily for the treatment of conditions such as colds, wind-heat headache, rheumatic arthralgia, irregular menstruation, and Flavonoids are among the primary active compounds found in B. balsamifera, with 14 flavonoid compounds being identified in both positive and negative ion modes. The fragmentation of flavonoids through mass spectrometry is generally characterized by the cleavage of flavonoid glycosides into glycosides and flavonoid aglycone fragments. Further fragmentation of flavonoid aglycones can be categorized into two primary classes: the Retro-Diels-Alder (RDA) cleavage of the ring, resulting in the division of the flavonoid aglycones into two distinct fragments, and the elimination of certain smaller molecular fragments, including CO, CHO, C 3 O 2 , CO 2 , and C 2 HO, among others [48]. The specific fragmentation pathways and resultant products are influenced by several factors, such as the reaction conditions, molecular structure, and the underlying reaction mechanism. Rutin is a type of flavonoid glycoside. In negative ion mode, its quasi-molecular ion peak is at m/z:  [49], and based on mass spectral data analysis and comparison with reference substances, it is speculated that this compound is rutin. The possible mass spectral cleavage pathways are shown in Figure 1.
343.0423. Thirdly, it loses a sugar moiety C12H20O9 to form a fragment ion m/z: 301.0359, which, through five types of cleavage pathways, yields different fragments. These pathways include: losing a molecule C7H3O2 at the C-ring's C-2 site to produce fragment m/z: 178.9989; losing a water molecule on the A-ring to yield fragment m/z: 283.0242, which continues to cleave a molecule of CO from the C-ring to yield fragment m/z: 255.0304 and, through rearrangement, further loses a molecule of CO from the C-ring to yield fragment m/z: 227.0358; undergoing a RDA cleavage on the C-ring, losing C8H6O3, to yield fragment m/z: 151.0037; losing a molecule of CH2O on the C-ring to yield fragment m/z: 271.0254, which continues to lose a molecule of CO on the C-ring to yield fragment m/z: 243.0307; and cleaving a CO molecule at the carbonyl on the C-ring to yield fragment m/z: 273.0405, which continues to cleave through three pathways, losing C7H4O4, CO2, and C8H5O4, respectively, to yield fragments m/z: 121.0300, m/z: 229.9944, and m/z: 108.0217. By comparison with the corresponding literature references [49], and based on mass spectral data analysis and comparison with reference substances, it is speculated that this compound is rutin. The possible mass spectral cleavage pathways are shown in Figure 1. Hesperidin is a flavonoid glycoside. In negative ion mode, the quasi-molecular ion peak is at m/z: 433.1154 [M−H] − . Using Xcalibar 4.0 software, the molecular formula is deduced to be C21H22O10. Upon collision-induced dissociation, it loses C3H6O3 and C4H8O4 to yield secondary fragment ions m/z: 343.0833 and m/z: 313.0727, which are characteristic C-ring from the connection between the A and B rings to yield fragment m/z: 93.0347. Thirdly, a RDA cleavage occurs on the C-ring, cleaving C 8 H 8 O from C-1 and C-3 to yield fragment m/z: 165.0196, which continues to lose a methyl group from the A-ring to yield fragment m/z: 151.0039. Fourthly, cleaving C 8 H 6 O 4 from the C-ring yields fragment m/z: 119.0506. The pseudomolecular ion peak m/z: 433.1154 loses a water molecule from the B-ring to form fragment m/z: 415.1044. By comparison with the corresponding literature references [50,51], and based on mass spectral data analysis, this compound is hypothesized to be hesperidin. The possible mass spectral cleavage pathways are illustrated in Figure 2. fragment ions of hexose flavonoid glycosides. The m/z: 313.0727 ion loses CO from the sugar moiety residue to yield fragment ion m/z: 285.0797, with four cleavage pathways. Firstly, it loses a methyl group from the C-ring to form fragment m/z: 271.0619, which continues to cleave in three pathways: losing the B-ring to yield fragment m/z: 177.0199, which further loses a carbonyl group from the A-ring to yield fragment m/z: 149.0246; cleaving C3O2 from the A-ring to yield fragment m/z: 203.0870; and losing C2H2O from the C-ring to yield fragment m/z: 229.0054, which further loses a molecule of CO from the Bring to yield fragment m/z: 201.0718. Secondly, it loses the A-ring and C-ring from the connection between the A and B rings to yield fragment m/z: 93.0347. Thirdly, a RDA cleavage occurs on the C-ring, cleaving C8H8O from C-1 and C-3 to yield fragment m/z: 165.0196, which continues to lose a methyl group from the A-ring to yield fragment m/z: 151.0039. Fourthly, cleaving C8H6O4 from the C-ring yields fragment m/z: 119.0506. The pseudomolecular ion peak m/z: 433.1154 loses a water molecule from the B-ring to form fragment m/z: 415.1044. By comparison with the corresponding literature references [50,51], and based on mass spectral data analysis, this compound is hypothesized to be hesperidin. The possible mass spectral cleavage pathways are illustrated in Figure 2.
Possible mass spectrometry fragmentation pathway of hesperidin in negative ion mode.

Identification and Fragmentation Patterns of Organic Acids
Through both positive and negative ion modes, five organic acid compounds were successfully identified in B. balsamifera. Notably, chlorogenic acid demonstrated a quasimolecular ion peak at m/z: 353.0878 [M−H] − in the negative ion mode. The molecular formula C16H18O9 was discerned utilizing the Xcalibur 4.0 software. Upon collision-induced dissociation, the molecule generated a variety of fragment ions, as described below: fragmentation through ester bond breakage resulted in a fragment at m/z: 191.0561, which,

Identification and Fragmentation Patterns of Organic Acids
Through both positive and negative ion modes, five organic acid compounds were successfully identified in B. balsamifera. Notably, chlorogenic acid demonstrated a quasimolecular ion peak at m/z: 353.0878 [M−H] − in the negative ion mode. The molecular formula C 16 H 18 O 9 was discerned utilizing the Xcalibur 4.0 software. Upon collisioninduced dissociation, the molecule generated a variety of fragment ions, as described below: fragmentation through ester bond breakage resulted in a fragment at m/z: 191.0561, which, upon further loss of a water molecule, yielded a fragment at m/z: 173.0456. Another fragmentation process involving ester bond cleavage produced a fragment at m/z: 179.0353, which, after the loss of a water molecule, formed a fragment at m/z: 161.0243. Cleavage to the left of the carbonyl group, resulting in the loss of C 7 H 12 O 6 , generated a fragment at m/z: 161.0243. The loss of C 8 H 12 O 7 led to the formation of a fragment at m/z: 133.0295. Cleavage at the alkyl group of the phenyl ring, which resulted in the loss of C 10 H 12 O 7 , generated a fragment at m/z: 109.0308. Lastly, cleavage to the left of the carbon-carbon double bond, accompanied by the loss of C 8 H 10 O 7 , produced a fragment at m/z: 135.0454. Drawing upon mass spectral data analysis, in comparison with the relevant literature references [52], and in juxtaposition with reference standards, the compound in question is Molecules 2023, 28, 4504 6 of 16 hypothesized to be chlorogenic acid. The potential mass spectral cleavage pathways are depicted in Figure 3. mentation process involving ester bond cleavage produced a fragment at m/z: 179.0353, which, after the loss of a water molecule, formed a fragment at m/z: 161.0243. Cleavage to the left of the carbonyl group, resulting in the loss of C7H12O6, generated a fragment at m/z: 161.0243. The loss of C8H12O7 led to the formation of a fragment at m/z: 133.0295. Cleavage at the alkyl group of the phenyl ring, which resulted in the loss of C10H12O7, generated a fragment at m/z: 109.0308. Lastly, cleavage to the left of the carbon-carbon double bond, accompanied by the loss of C8H10O7, produced a fragment at m/z: 135.0454. Drawing upon mass spectral data analysis, in comparison with the relevant literature references [52], and in juxtaposition with reference standards, the compound in question is hypothesized to be chlorogenic acid. The potential mass spectral cleavage pathways are depicted in Figure  3.

Identification and Fragmentation Pathways of Alkaloids
The compound under consideration, aurantiamide acetate, exhibited a quasi-molecular ion peak at m/z: 445.2121 [M+H] + in the positive ion mode. Its molecular formula, C27H28N2O4, was determined utilizing Xcalibur 4.0 software. Following collision-induced dissociation, it generated five distinct types of fragment ions as described below: the loss of C16H12NO2 yielded a fragment at m/z: 194.1179, which further underwent the loss of C2H4O2, resulting in a fragment at m/z: 134.0968. The loss of C12H14NO3 led to the formation of a fragment at m/z: 224.1074. The loss of C11H14NO2 produced a fragment at m/z: 252.1023. This fragment, upon further loss of C9H9NO, generated a fragment ion at m/z: 105.033, which was the most stable fragment ion peak under these conditions. The loss of C24H18NO2 resulted in a fragment at m/z: 88.5351. The loss of C16H14N2O2 yielded a fragment at m/z: 177.0927, which further lost C2O2 and C2H3O to yield fragments at m/z: 117.0702 and m/z: 134.0968, respectively. The loss of C16H14NO2 and C2H3O2 led to the formation of fragments at m/z: 194.1179 and m/z: 134.0968, respectively. Based on mass spectral data analysis and comparison with the related literature reference [53], this compound is conjectured to be aurantiamide acetate. The potential mass spectral cleavage pathways are illustrated in Figure 4.

Identification and Fragmentation Pathways of Alkaloids
The compound under consideration, aurantiamide acetate, exhibited a quasi-molecular ion peak at m/z: 445.2121 [M+H] + in the positive ion mode. Its molecular formula, C 27 H 28 N 2 O 4 , was determined utilizing Xcalibur 4.0 software. Following collision-induced dissociation, it generated five distinct types of fragment ions as described below: the loss of C 16 H 12 NO 2 yielded a fragment at m/z: 194.1179, which further underwent the loss of C 2 H 4 O 2 , resulting in a fragment at m/z: 134.0968. The loss of C 12 H 14 NO 3 led to the formation of a fragment at m/z: 224.1074. The loss of C 11 H 14 NO 2 produced a fragment at m/z: 252.1023. This fragment, upon further loss of C 9 H 9 NO, generated a fragment ion at m/z: 105.033, which was the most stable fragment ion peak under these conditions. The loss of C 24 H 18 NO 2 resulted in a fragment at m/z: 88.5351. The loss of C 16 H 14 N 2 O 2 yielded a fragment at m/z: 177.0927, which further lost C 2 O 2 and C 2 H 3 O to yield fragments at m/z: 117.0702 and m/z: 134.0968, respectively. The loss of C 16 H 14 NO 2 and C 2 H 3 O 2 led to the formation of fragments at m/z: 194.1179 and m/z: 134.0968, respectively. Based on mass spectral data analysis and comparison with the related literature reference [53], this compound is conjectured to be aurantiamide acetate. The potential mass spectral cleavage pathways are illustrated in Figure 4.    [54], the compound is proposed to be tanshinone IIA. The potential mass spectral cleavage pathways are illustrated in Figure 5.

DPPH Radical Scavenging Activity
The DPPH radical scavenging capacity of the methanol extract of B. balsamifera, alongside an ascorbic acid control, is depicted in Figure 6. As illustrated, an increased concentration of the various samples corresponded with a gradual increase in DPPH radical scavenging activity, eventually reaching a plateau at a specific concentration. For ascorbic acid, the DPPH scavenging rate stabilized at a concentration of 50 μg/mL, reaching a peak value at 200 μg/mL with a maximum scavenging rate of 98.72%. The methanol extract exhibited a rapid increase in scavenging rate against DPPH radicals at concentrations ranging from 3.33 to 200 μg/mL. At 200 μg/mL, the scavenging rate tended to stabilize, and the maximum scavenging rate was 75.72% at 333 μg/mL. which was lower than that of ascorbic acid.

DPPH Radical Scavenging Activity
The DPPH radical scavenging capacity of the methanol extract of B. balsamifera, alongside an ascorbic acid control, is depicted in Figure 6. As illustrated, an increased concentration of the various samples corresponded with a gradual increase in DPPH radical scavenging activity, eventually reaching a plateau at a specific concentration. For ascorbic acid, the DPPH scavenging rate stabilized at a concentration of 50 µg/mL, reaching a peak value at 200 µg/mL with a maximum scavenging rate of 98.72%. The methanol extract exhibited a rapid increase in scavenging rate against DPPH radicals at concentrations ranging from 3.33 to 200 µg/mL. At 200 µg/mL, the scavenging rate tended to stabilize, and the maximum scavenging rate was 75.72% at 333 µg/mL. which was lower than that of ascorbic acid. ascorbic acid, the DPPH scavenging rate stabilized at a concentration of 50 μg/mL, reac ing a peak value at 200 μg/mL with a maximum scavenging rate of 98.72%. The methan extract exhibited a rapid increase in scavenging rate against DPPH radicals at concentr tions ranging from 3.33 to 200 μg/mL. At 200 μg/mL, the scavenging rate tended to stab lize, and the maximum scavenging rate was 75.72% at 333 μg/mL. which was lower th that of ascorbic acid.  The value of the half-inhibitory concentration (IC 50 ) of the sample was calculated. A smaller IC 50 value indicated stronger antioxidant activity. The IC 50 values for ascorbic acid and the methanol extract in scavenging DPPH radicals were as follows: ascorbic acid (0.98 ± 0.073 µg/mL) < methanol extract (105.1 ± 0.503 µg/mL), as shown in Table 2.

ABTS Radical Scavenging Activity
As depicted in Figure 7, the methanol extract of B. balsamifera demonstrated a potent scavenging activity against ABTS radicals. This scavenging capability exhibited a positive correlation with the sample concentration within a certain range. The scavenging rate of ascorbic acid against ABTS radicals reached a plateau at a concentration of 10 µg/mL and attained a maximum value at 50 µg/mL, with the peak scavenging rate being 99.87%. The methanol extract displayed a maximum scavenging rate exceeding 99% at a concentration of 200 µg/mL, a value comparable to that of ascorbic acid.
Molecules 2023, 28, x FOR PEER REVIEW 9 o The value of the half-inhibitory concentration (IC50) of the sample was calculated smaller IC50 value indicated stronger antioxidant activity. The IC50 values for ascorbic a and the methanol extract in scavenging DPPH radicals were as follows: ascorbic acid (0 ± 0.073 μg/mL) < methanol extract (105.1 ± 0.503 μg/mL), as shown in Table 2.

ABTS Radical Scavenging Activity
As depicted in Figure 7, the methanol extract of B. balsamifera demonstrated a pot scavenging activity against ABTS radicals. This scavenging capability exhibited a posi correlation with the sample concentration within a certain range. The scavenging rat ascorbic acid against ABTS radicals reached a plateau at a concentration of 10 μg/mL attained a maximum value at 50 μg/mL, with the peak scavenging rate being 99.87%. methanol extract displayed a maximum scavenging rate exceeding 99% at a concentrat of 200 μg/mL, a value comparable to that of ascorbic acid.
The IC50 values, which signify the potency of antioxidant activity of the ascorbic a and methanol extract in scavenging ABTS radicals are as follows, listed from smalles largest: ascorbic acid (1.774 ± 0.036 μg/mL) < methanol extract (12.49 ± 0.341 μg/mL) indicated in Table 2.

Total Antioxidant Capacity Determination
The total antioxidant capacity of B. balsamifera methanol extract and ascorbic a control are shown in Figure 8. As shown in the figure, the linear total antioxidant capa of ascorbic acid and methanol extract exhibited an apparent dose-response relationsh The total antioxidant capacity of ascorbic acid reached the highest absorbance valu 3.38 ± 0.027 at a concentration of 600 μg/mL, while the methanol extract reached a m mum absorbance value of 0.454 ± 0.009 at 400 μg/mL. largest: ascorbic acid (1.774 ± 0.036 µg/mL) < methanol extract (12.49 ± 0.341 µg/mL), as indicated in Table 2.

Total Antioxidant Capacity Determination
The total antioxidant capacity of B. balsamifera methanol extract and ascorbic acid control are shown in Figure 8. As shown in the figure, the linear total antioxidant capacity of ascorbic acid and methanol extract exhibited an apparent dose-response relationship. The total antioxidant capacity of ascorbic acid reached the highest absorbance value of 3.38 ± 0.027 at a concentration of 600 µg/mL, while the methanol extract reached a maximum absorbance value of 0.454 ± 0.009 at 400 µg/mL.

Reducing Power Determination
The reducing power of B. balsamifera methanol extract and ascorbic acid contro shown in Figure 9. The reducing power of the methanol extract and ascorbic acid co showed an increasing trend, which was positively correlated with their mass conce tions. As shown in the figure, the absorbance value of ascorbic acid reached 1.935 ± at a concentration of 200 μg/mL. The methanol extract reached its maximum value of ± 0.03 at a concentration of 2000 μg/mL.

Discussion
This study analyzed the phytochemical composition and antioxidant potential balsamifera, a plant with significant ethnobotanical relevance. An advanced UPLC-Q bitrap HRMS technique was used to identify 31 compounds in the plant, includin compounds that have not been reported before. These compounds belong to variou egories such as flavonoids, organic acids, quinones, and alkaloids. The identificatio these compounds provides a chemical basis for understanding the medicinal value mechanism of action of B. balsamifera. There are still many unknown peaks in the

Reducing Power Determination
The reducing power of B. balsamifera methanol extract and ascorbic acid control are shown in Figure 9. The reducing power of the methanol extract and ascorbic acid control showed an increasing trend, which was positively correlated with their mass concentrations. As shown in the figure, the absorbance value of ascorbic acid reached 1.935 ± 0.023 at a concentration of 200 µg/mL. The methanol extract reached its maximum value of 1.099 ± 0.03 at a concentration of 2000 µg/mL.

Reducing Power Determination
The reducing power of B. balsamifera methanol extract and ascorbic acid control shown in Figure 9. The reducing power of the methanol extract and ascorbic acid con showed an increasing trend, which was positively correlated with their mass concen tions. As shown in the figure, the absorbance value of ascorbic acid reached 1.935 ± 0. at a concentration of 200 μg/mL. The methanol extract reached its maximum value of 1. ± 0.03 at a concentration of 2000 μg/mL.

Discussion
This study analyzed the phytochemical composition and antioxidant potential o balsamifera, a plant with significant ethnobotanical relevance. An advanced UPLC-Qbitrap HRMS technique was used to identify 31 compounds in the plant, including compounds that have not been reported before. These compounds belong to various egories such as flavonoids, organic acids, quinones, and alkaloids. The identification these compounds provides a chemical basis for understanding the medicinal value a mechanism of action of B. balsamifera. There are still many unknown peaks in the m spectrum that have not been identified due to the lack of reference mass spectrome data and substances for the corresponding compounds. Additional analysis is required

Discussion
This study analyzed the phytochemical composition and antioxidant potential of B. balsamifera, a plant with significant ethnobotanical relevance. An advanced UPLC-Q-Orbitrap HRMS technique was used to identify 31 compounds in the plant, including 18 compounds that have not been reported before. These compounds belong to various categories such as flavonoids, organic acids, quinones, and alkaloids. The identification of these compounds provides a chemical basis for understanding the medicinal value and mechanism of action of B. balsamifera. There are still many unknown peaks in the mass spectrum that have not been identified due to the lack of reference mass spectrometry data and substances for the corresponding compounds. Additional analysis is required to clarify these unknown compounds. Flavonoids formed the most abundant group among the identified compounds, with hemiphloin, taxifolin, rutin, and quercetin standing out in terms of their quantity. These flavonoids are well-documented for their potent antioxidant capabilities, which can be linked to the significant antioxidant activity observed in B. balsamifera. The detailed mass fragmentation patterns of these representative compounds could serve as a valuable reference for future phytochemical studies on this plant.
B. balsamifera has garnered significant interest in recent years in the quest for natural sources of antioxidants. Studies evaluating the antioxidant activity of this plant have primarily focused on its leaves. For instance, Ginting et al. investigated the antioxidant activity of n-hexane extract and its fractions from B. balsamifera leaves using a DPPH assay. However, the results showed that the antioxidant activity of the extracts was insignificant [55]. Jirakitticharoen et al. evaluated the antioxidant activity of B. balsamifera leaf extracts from different growth cycles using DPPH, ABTS, and FRAP assays. They found that the immature leaves of B. balsamifera were rich in quercetin and phenols and exhibited significant antioxidant activity [56]. Wang et al. compared and analyzed the antioxidant activity of essential oil components in the leaves of B. balsamifera picked at different times. They reported that the essential oils of B. balsamifera collected from October to December had higher antioxidant activity [57]. In this study, the antioxidant potential of methanol extract of B. balsamifera was assessed by evaluating its DPPH and ABTS free radical scavenging abilities, total antioxidative capacity, and reducing power. The results indicated that the methanol extract of the plant has considerable radical scavenging capabilities, thereby aligning with its traditional use as a natural antioxidant. There was a positive correlation observed between the antioxidant activities and the mass concentration of the methanol extract, as well as the polyphenol content, with a particular emphasis on flavonoids. Flavonoids are recognized for their strong antioxidant properties, thus contributing to the observed relationship. Although the potency was not as high as ascorbic acid, a benchmark antioxidant, it was noteworthy given the natural origin of the plant extract. This study contributes significantly to the existing body of knowledge about B. balsamifera, shedding light on its chemical diversity and antioxidant potential. These findings suggest that this plant could be a promising source of bioactive compounds for further pharmacological studies and possible drug development. Furthermore, the identification of flavonoids and other compounds could pave the way for the development of new antioxidant agents.
The study only focused on the chemical constituents and antioxidant activities of B. balsamifera methanol extract, which may not reflect the full spectrum of its bioactive components and pharmacological effects. However, the exploration of B. balsamifera's therapeutic potential should not stop here. There are avenues for further investigations, such as in vivo antioxidant tests, and evaluations of other possible bioactivities. Additionally, the interactions between the identified compounds and their collective impact on the overall antioxidant activity of B. balsamifera could be an interesting focus for future research. This will not only provide a more holistic understanding of the plant's therapeutic value but could also contribute to the optimization of extraction and formulation processes for therapeutic applications. Future research should also conduct phylogenetic and chemotaxonomic studies to clarify the relationship between B. balsamifera and other species in the genus Blumea or the family Asteraceae.

Plant Material and Extraction
B. balsamifera (L.) DC. was collected in July 2022 from the Yulin medicinal plant market in Guangxi, China. The plant material was authenticated by Associate Researcher Zheng Xilong from the School of Chinese Medicine Resources, Guangdong Pharmaceutical University. The dried aerial parts (moisture content not more than 10%) were ground using a DFY-300C swing pulverizer (Wenling LinDa Machinery Co., Ltd., Taizhou, China). The dry coarse powder of B. balsamifera was passed through a 50 mesh sieve (with a particle size ranging from 180 µm to 270 µm), and 10 g powder was accurately weighed and placed in a 50 mL flask. Methanol was added at a solid-to-liquid ratio of 1:50, and the mixture was extracted by ultrasound at a power of 300 W for 1 time, a temperature of 60 • C and time of 30 min, followed by centrifugation at 1500× g for 15 min. A volume of 200 µL of supernatant was taken and diluted to 1 mL with methanol. Then, it was filtered through a 0.22 µm membrane and stored at 4 • C before UPLC-Q-Orbitrap HRMS analysis. The remaining methanol extract was evaporated to obtain the crude methanol extract of B. balsamifera (BBME), which was stored at 4 • C for later use.

Instrumentation and Conditions
The chromatographic analysis was performed on a Vanquish Flex ultra-high-performance liquid chromatograph equipped with an Orbitrap Exploris 120 quadrupole-electrostatic orbitrap high-resolution mass spectrometer (Thermo Fisher Scientific, Waltham, MA, USA). Chromatographic separation was carried out on a Hypersil GOLD C 18 column (100 mm × 2.1 mm, 1.9 µm) with a flow rate of 0.3 mL·min -1 and a column temperature of 35 • C. The injection volume was 2.00 µL. The mobile phase consisted of acetonitrile (A) and 0.1% formic acid aqueous solution (B), using a gradient elution program (0~5 min, 95%~75% B; 15~25 min, 75%~5% B; 25~27 min, 5% B; 27.001~30 min, 95% B). The mass spectrometer was operated in positive and negative ion-switching modes with the following conditions: heated electrospray ionization (HESI) source; spray voltage, 3.5 kV; capillary temperature, 325 • C; auxiliary gas temperature, 300 • C; mass scan range (m/z), 100~1500; sheath gas, auxiliary gas, and sweep gas were all nitrogen with flow rates of 50 L·min -1 , 8 L·min -1 , and 1 L·min -1 , respectively, and; resolution, 60,000. The B. balsamifera sample was analyzed under the chromatographic and mass spectrometric conditions described above, and the total ion and MS 2 chromatograms (Supplementary Figures S1-S33) in both positive and negative ion modes were obtained.

Data Analysis and Compound Identification
The molecular formulas of the compounds corresponding to the chromatographic peaks were determined using the high-resolution exact mass values calculated by Xcalibur 4.1 software, the deviation between the measured and theoretical relative molecular masses (less than 5 × 10 -6 ), and the isotopic abundance ratios. The possible chemical constituents were identified by comparing the B. balsamifera chemical composition database information (including English names, molecular formulas, and exact relative molecular masses), reference substances, database matching (mzVault and mzCloud databases, matching scores not less than 80), and fragmentation patterns, and confirmed through literature comparison.

DPPH Free Radical Scavenging Assay
The method is rapid and simple, and has been widely used to determine the antioxidant activity of biological samples, pure compounds and extracts in vitro [58,59]. The free-radical-scavenging ability against the 2,2-diphenyl-1-picryl-hydrazyl-hydrate (DPPH) was determined. The study determined the antioxidant activity of BBME utilizing the method developed by Li with slight modifications [60]. Different concentrations of BBME solutions, namely 3.33, 33.33, 66.67, 133. 33,200,266.66, and 333 µg/mL were mixed with 2 mL of DPPH solution (2 mmol/L, dissolved in anhydrous ethanol). The resulting mixture was thoroughly blended and then reacted for 30 min at room temperature in the absence of light. The absorbance was measured at 517 nm with ascorbic acid as a positive control in the same 96-well plate. Each measurement was performed in triplicate. The percentage of DPPH-scavenging activity was calculated according to the equation: where A 1 is the absorbance of the sample, A 2 is the absorbance of the sample and ethanol without DPPH, and A 0 is the absorbance of the control (the methanol in replace of the sample). The IC 50 values of the samples were calculated by regressing the sample concentrations with the clearance rates.

ABTS Free Radical Scavenging Assay
The 2,2 -azino-bis-3-ethylbenzthiazoline-6-sulphonic acid (ABTS) is a protonated radical. The method measures the antioxidant-scavenging ability of the ABTS radical generated by potassium persulfate in the aqueous phase. It has a characteristic maximum absorbance value at 734 nm and decreases with the scavenging of protonated radicals [61]. The antioxidant activity of the BBME was evaluated using the ABTS free radical scavenging assay, with slight modifications from a previously reported method [62]. Briefly, ABTS (7 mM) was reacted with potassium persulfate (2.45 mM) and allowed to stand at room temperature for 12 h in the dark. The ABTS radical cation (ABTS •+ ) was diluted with ethanol to give an absorbance of 0.70 ± 0.02 at 734 nm. An amount of 2 mL of the BBME solutions of different concentrations (3.33, 16.67, 33.33, 50, 100, 200 and 300 µg/mL) was mixed with 2 mL of ABTS •+ solution and the mixture was left to stand in darkness for 30 min. Absorbance was measured at 734 nm. Ascorbic acid was used as a positive control. The percentage inhibition of ABTS •+ radical was calculated using the following equation: where A 1 represents the absorbance of the sample, A 2 represents the absorbance of the sample and ethanol without ABTS, and A 0 represents the absorbance of the control (the methanol in replace of the sample). The IC 50 values of the samples were calculated by regressing the sample concentrations with the clearance rates.

Total Antioxidant Capacity Assay
The total antioxidant capacity of the BBME was measured using the phosphomolybdenum method [63]. The method is based on the reduction in Mo(VI)-Mo(V) by the sample tested and the subsequent formation of green phosphate-Mo(V) complex with a maximum absorption at 695 nm. In brief, 1 mL of the BBME solutions of different concentrations (20,50,100,200, 300, and 400 µg/mL) (with methanol as the blank) were mixed with 1 mL of the reagent solution (0.6 M sulfuric acid, 28 mM sodium phospha-te, and 4 mM ammonium molybdate). The tubes were capped and incubated in a water bath at 90 • C for 90 min. After cooling, the absorbance of each solution was measured at 695 nm against a blank. The antioxidant capacity was expressed as the number of equivalents of ascorbic acid.

Reducing Power Assay
The reducing power of an active substance can be an important indicator of its potential antioxidant activity. The absorbance measured at 700 nm was used to demonstrate the reducing power. An increase in the absorbance of the measured sample indicates an increase in the reducing power of the sample tested [64]. The total reducing power of the BBME was evaluated by the method of Oyaizu [65]. In brief, 2 mL of the BBME solutions of different concentrations (20,200, 400, 600, 1000, 1600, and 2000 µg/mL, with methanol as the blank) was mixed with 2 mL of phosphate buffer (0.2 M, pH 6.6) and 2 mL of 1% potassium ferricyanide. The mixture was then incubated at 50 • C for 20 min. After the mixture was cooled, 2 mL of 10% trichloroacetic acid was added, and the mixture was centrifuged at 3000 rpm for 10 min. The upper layer of the solution (2 mL) was mixed with 2 mL of distilled water and 0.5 mL of 0.1% ferric chloride. The absorbance was measured at 700 nm against a blank solution. Ascorbic acid was used as the standard.

Statistical Analysis
All tests were conducted in triplicate. Data were presented as mean ± SD. Statistical analysis was performed using the SPSS software (Version: 20.0, Armonk, NY, USA). The data were subjected to one-way analysis of variance (ANOVA), and the significant differences were evaluated using Duncan's test (p < 0.05).