Ethyl Gallate Isolated from Castanopsis cuspidata var. sieboldii Branches Inhibits Melanogenesis and Promotes Autophagy in B16F10 Cells

The Castanopsis cuspidata var. sieboldii (CCS) plant grows predominantly in temperate regions of Asian countries, such as South Korea. Research on CCS has so far concentrated on the nutritional analysis, antioxidant activity, and anti-inflammation properties of its branches. However, the isolation of compounds and structural elucidation of effective single molecules remain unexplored, necessitating further exploration of CCS branches. Therefore, this study demonstrates the antioxidant and antimelanogenic activity of a single substance of ethyl gallate (EG) isolated from CCS branch extracts. Notably, the antimelanogenic (whitening) activity of EG extracted from CCS branches remains unexplored. Tyrosinase inhibition, kinetic enzyme assays, and molecular docking studies were conducted using mushroom tyrosinase in order to examine the antioxidant mechanism and antimelanin activity of EG in B16F10 melanoma cells. Nontoxic EG concentrations were found to be below 5 µg/mL. While EG significantly reduced the levels of whitening-associated proteins, p-CREB, and p-PKA, it dose-dependently inhibited the expression of TYR, TRP-1, TRP-2, and transcription factor (MITF). In addition, EG downregulated melanogenetic gene expression and activated autophagy signals. Therefore, EG extracted from CCS branches could serve as a novel functional cosmetic material with antimelanogenic and autophagy-enhancing activity.


Introduction
As interest in well-being, health, and life expectancy grows, so does the value of healthy aging and clean skin. Various plant-derived natural compounds are currently used as functional components in cosmetics. Among the various functions of cosmetics, antioxidant activity is a significant factor in the skin's UV defense mechanism. Notably, the skin's inherent exposure to UV radiation and air induces the generation of radical and nonradical reactive oxygen species (ROS) via reactions with molecules [1]. ROS accelerates skin aging by destroying skin antioxidants and initiating lipid peroxidation, protein oxidation, DNA oxidation, chain scission, and abnormal cross-linking of collagen and hyaluronic acid, resulting in wrinkles and melanin production [2][3][4]. Because excessive UV radiation can overwhelm the skin defense system, appropriate antioxidants capable of suppressing ROS hyperproduction are needed [5][6][7][8]. Research on diverse natural products is increasing in an effort to produce effective natural antioxidants as alternatives to synthetic ones [9]. In addition to the discovery of cosmetic ingredients with antiaging and whitening activity, a novel autophagy modulator (enhancer or inhibitor) has also been developed [10]. Autophagy is a novel antiaging phenomenon essential for cells to remove intracellular waste products or unnecessary proteins and recycle them to regenerate cells in a healthy In April 2021, CCS branches were collected from Wando Arboretum (Wando, Korea) in Jeollanam-do, washed, dried with hot air (40 • C), stored, and then pulverized for use. To confirm the antioxidant activity of each solvent fraction of the pine CCS's branches, 1.5 kg of dried at 40 • C and pulverized CCS's branches was added to 15.0 L of 70% EtOH (v/v) and immersed for two weeks at room temperature for extraction. The immersed sample was filtered using a vacuum pump and Whatman No. 1 filter. After filtration, it was separated and repeated once under the same conditions. The filtrate obtained by filtration was concentrated using a rotary vacuum evaporator in a water bath at 37 • C and then lyophilized for use. In addition, 269.03 g of 70% EtOH extract was suspended in 500 mL distilled water and fractionated sequentially in order of polarity using a separation funnel to obtain n-hexane (n-Hex), chloroform (Ch), ethyl acetate (EtOAc), n-butanol (n-BuOH), and water (H 2 O) fractions of 13.03, 5.27, 51.22, 44.74, and 15.93 g, respectively ( Figure 1). Fractionation was repeated three times using 1 L of each solvent. Each fraction was used after being concentrated and lyophilized as described above, and the extraction yield was calculated using the following formula.

Separation of Active Components from EtOAc Fractions of CCS Branches
Using medium-pressure liquid chromatography (MPLC, Yamazen, Osaka, Japan), the EtOAc fraction was sequentially subdivided according to polarity among the solvent fractionation layers. After dissolving 38.22 g of the EtOAc fraction in 20 mL of MeOH and filtering the solution with a syringe filter, the separation experiment was conducted using an ODS column at a flow rate of 10 mL/min and an absorbance value of 280 nm. The solvent conditions included fractionation by sequentially increasing the MeOH ratio by 5% at a solvent ratio of H 2 O: MeOH (10-100% MeOH, 570 min) and MeOH (100%, 20 min) under isocratic conditions. Each fraction pattern was confirmed by thin-layer chromatography, and then the fractions were divided into three fractions (Fr. 3) based on their antioxidant activity and subjected to HPLC and MPLC for qualitative analysis and continuous fractionation under gradient conditions, respectively (Table S1, Figure S1). The MPLC fraction (Fr.2) with the highest antioxidant activity was subjected to MPLC under the solvent conditions of H 2 O: MeOH (10-100% MeOH, 80 min) and MeOH (100%, 20 min), and Prep-Compound 1 (47 mg) was then isolated by LC. Compound 1 was isolated by preparative high-performance liquid chromatography (Prep 150 LC, Waters, MA, USA) with an X-Bridge Prep OBD C18 column (5.0 µm, 19 mm × 150 mm). Elution was performed with a linear gradient of methanol (0 min, 50/50; 30 min, 100/0; 100 min, 100/0). AVANCE III HD 400 (FT-NMR system, 400 MHz, BRUKER) was used as the nuclear magnetic resonance (NMR) spectrometer for the structural analysis of the active component. Samples were prepared and analyzed at a concentration of 10 mg/mL using dimethyl sulfoxide-d6 (DMSO-d 6 ) (Sigma Aldrich's exclusive NMR solvent, St. Louis, MO, USA) as a solvent for NMR measurement.

Separation of Active Components from EtOAc Fractions of CCS Branches
Using medium-pressure liquid chromatography (MPLC, Yamazen, Osaka, Japan), the EtOAc fraction was sequentially subdivided according to polarity among the solvent fractionation layers. After dissolving 38.22 g of the EtOAc fraction in 20 mL of MeOH and filtering the solution with a syringe filter, the separation experiment was conducted using an ODS column at a flow rate of 10 mL/min and an absorbance value of 280 nm. The solvent conditions included fractionation by sequentially increasing the MeOH ratio by 5% at a solvent ratio of H2O: MeOH (10-100% MeOH, 570 min) and MeOH (100%, 20 min)  With a few modifications, Blois' method was used to test the DPPH free radical scavenging activity [16]. For each concentration, 200 µL of sample was placed in an Eppendorf (EP) tube, and 800 µL of 0.5 mM DPPH in MeOH (1,1-diphenyl-2-picrylhydrazyl; Sigma-Aldrich Co., St. Louis, MO, USA) reagent was mixed by vortexing for 15 min. Absorbance was then measured at 517 nm using a Biotek Synergy HT multidetection microplate reader. Each sample was repeated three times to obtain an average value, and ascorbic acid and EG were used as positive controls for comparative experiments. The radical scavenging ability of each solution was calculated using the following formula and expressed as a percentage: Radical scavenging activity (%) = (Abs control − Abs sample )/Abs control × 100 2.4.2. Measurement of ABTS Cation Radical Scavenging Activity ABTS cation radical scavenging ability was measured using Liang et al.'s method, with slight modifications [17]. The reaction of an equal volume of 7 mM ABTS (2,2 -azino-bis (3ethylbenzothiazoline-6-sulfonic acid) diammonium salt) solution with 2.45 mM potassium persulfate in the dark for 18 h produced an ABTS cationic radical. The prepared solution was diluted with distilled water until the absorbance value at 730 nm reached 0.90 ± 0.02. For each concentration, 200 µL of the sample was placed in an EP tube, mixed with 1000 µL of a 10-fold diluted ABTS solution, and vortexed in a dark room. Following a 15 min reaction, absorbance was measured at 730 nm using a Biotek Synergy HT multidetection microplate reader; each sample was repeated 3 times to obtain an average value, and ascorbic acid and EG were used as positive controls for comparative experiments. The radical scavenging activity of each solution was calculated using the following formula and expressed as a percentage, and the sample concentration (IC 50 ) was obtained when the radical scavenging activity percentage of each sample was 50%.

Total Polyphenol Content Analysis
Total polyphenol content analysis was performed using the Folin-Ciocalteu method [18]. Gallic acid was employed as a reference material in a standard calibration curve for quantitative analysis, and the R 2 value of this curve was at least 0.99. After taking 500 µL each of a sample of 1 mg/mL concentration and diluted gallic acid standard solution for each concentration, 500 µL of 0.2 M Folin-Ciocalteu's phenol reagent and 500 µL of 2% sodium carbonate aqueous solution (w/v) were also mixed in a dark room. Following a 30 min reaction, absorbance was measured at 750 nm using a Biotek Synergy HT multidetection microplate reader. The measured value was converted into the amount of gallic acid (GAE) contained per 1 g of the sample by substituting it into a standard calibration curve to obtain the total polyphenol content.

Analysis of Total Flavonoid Content
Total flavonoid content was measured using Park et al.'s method, with slight modifications [19]. Quercetin was employed as a reference material in a standard calibration curve for quantitative analysis, and the R 2 value of this curve was at least 0.99. After taking 500 µL each of a sample of 1 mg/mL concentration and diluted quercetin standard solution for each concentration, 1.5 mL of methanol, 100 µL of 10% aluminum chloride, 100 µL of 1 M potassium acetate, and 2.8 mL of distilled water were added in that order to 40 µL at room temperature and reacted for min. Absorbance was then measured at 415 nm using a Biotek Synergy HT multidetection microplate reader. The measured value was converted into the amount of quercetin (QUE) contained per 1 g of the sample by substituting it into a standard calibration curve to obtain the total flavonoid content.

Quantitative Analysis of Polyphenols Using HPLC MS/MS
The LC-MS/MS analysis instrument used in this experiment was an AB SCIEX 4000 Q Trap LC/MS/MS System (Shimadzu LC 20A System, Kyoto, Japan), and water (in 0.1% formic acid, solvent A) was used as the mobile phase in the analysis conditions, whereas acetonitrile (in 0.1% formic acid, solvent B) was used under isocratic conditions (35% B) (Table S1). Using Turbo Ion Spray, the analytical conditions of MS/MS were examined in both negative and positive modes. The ability to inhibit tyrosinase activity was measured spectroscopically by partially modifying Choi et al.'s method (2018) [20]. Briefly, 400 µL of 0.1 mM sodium phosphate buffer (pH 6.8) was used as the buffer, whereas 200 µL of 1.5 mM L-tyrosine was used as the substrate. After adding 200 µL of each sample (CCSB-Hex, CCSB-CL, CCSB-EtOAc, CCSB-BuOH), 100 µL of tyrosinase at a concentration of 1750 units was added to prepare a mixture. Ascorbic acid and EG were used as positive controls, and after reacting 900 µL of the mixture at 37 • C for 30 min, the absorbance at 475 nm was measured using a microplate reader (Infinite M200, Tecan, San Jose, CA, USA). The ability to suppress tyrosinase activity was determined using the following formula: Inhibition rate (%) = (1−absorbance of sample added group)/absorbance of non-added group × 100

Enzyme Kinetics Assay
In this study, Fan et al.'s enzyme kinetic experiment was modified and continued using L-DOPA as the substrate, with experiments conducted at concentrations of 0.5, 1.0, 1.5, and 2.0 mM [21]. Tyrosinase inhibition activity was detected using a spectrophotometer (Synergy HT, BIO-TEX, Winooski, VT, USA). The 96-well microplates were loaded with 80 µL aliquots of a solution containing 50-200 U/mL mushroom tyrosinase (Sigma Aldrich, St. Louis, MO, USA). Then, 80 µL of the substrate and 80 µL of EG (0.2-1.0 mM) were added. The absorbance of the 96 wells was measured at 510 nm (T0) using a microplate reader (Synergy HT, BIO-TEX, Winooski, VT, USA). Subsequently, the microplates were incubated at 25 ± 1 • C for 15 min, and the absorbance was measured again (T1). An additional reaction period of 15 min at 25 ± 1 • C was allowed, after which a new spectrophotometric reading was completed (T2). The inhibitory percentages at the two time points (T1 and T2) were obtained based on the following formula: where IA% is the inhibitory activity, C is the negative control absorbance, and S is the sample or positive control absorbance (the absorbance at time T0 subtracted from the absorbance at time T1 or T2) [22].

Molecular Docking Procedure
To predict the binding sites of human tyrosinase to EG, molecular docking was performed using the Glide module of the Schrodinger Package [22,23]. The X-ray crystal structure of tyrosinase (PDB ID: 2Y9X) was retrieved from the Protein Data Bank (http://www.rcsb.org, accessed on 10 October 2022). The retrieved protein structures were processed using Protein Preparation Wizard in the Schrodinger package to remove the crystallographic water molecules, add hydrogen atoms, and assign protonated states and partial charges. The missing side chains and loops were built and refined using the Prime tool of the Schrodinger suite [24]. All protein residues were parameterized using the OPLS3e force field [25,26]. Finally, restrained minimization was performed until the converged average root mean square deviation of heavy atoms was 0.3 Å.

Cell Culture
The B16F10 melanoma cells used in this experiment were purchased from the American Type Culture Collection (Rockville, MD, USA) [27]. The medium used for cell culture was maintained in Dulbecco's modified Eagle's medium (HyClone, MA, USA) supplemented with 10% fetal bovine serum (HyClone, MA, USA). After adding 50 units/mL penicillin to the medium, the experiment was conducted in a 37 • C plus 5% CO 2 environment.

MTT Cell Viability Assay
Cell viability measurement experiments were conducted according to Carmichael's method [28]. After distributing 0.18 mL of melanoma cells (B16F10) to test toxicity on a 96-well plate at a density of 1 × 10 5 cells/well, add 0.02 mL of sample solution prepared by concentration and incubate for 48 h at 37 • C in a 5% CO 2 incubator. The control group was cultured under the same conditions by adding the same amount of serum-free medium as the sample solution. A total of 300 µL of MTT solution prepared at 2.5 mg/mL was added to this and incubated for 1 h in a 37 • C, 5% CO 2 incubator; the culture medium was then removed; 100 µL of DMSO was added to each well and reacted at room temperature for 30 min; and microplate absorbance at 540 nm was measured with a reader. Cell viability was expressed as the rate of decrease in absorbance of the sample-added and non-added groups.
cell viability(%) = 1 − Absorbance of sample added group Absorbance of the non − additive group × 100

Measurement of Melanin Content
To measure the melanin content for EG, Hosoi et al.'s method was modified and implemented [29]. B16F10 cells were cultured at 1 × 10 4 cells/cm in 6-well plates. After 24 h, the cells were stimulated with α-MSH 1 µg/mL. Simultaneously, various concentrations of EG (1-5 µg/mL) were added for 48 h. After washing with phosphate-buffered saline (PBS), the cells were harvested by trypsin treatment. The collected cells were dissolved in 100 µL of 1 N NaOH and measured at 405 nm using a spectrophotometer.

Measurement of ROS Production
2 ,7 -dichlorofluorescein diacetate (DCFH-DA) fluorescent probe was used to measure the production of intracellular ROS. Cells were pretreated with EG (1 or 5 µg/mL) for 24 h, followed by staining with 10 µM DCFH-DA for 30 min at 37 • C in the dark. The cells were subsequently washed with PBS and scraped from the well. Productions of intracellular ROS were observed under a fluorescence microplate reader (Gemini, Molecular Devices, Sunnyvale, CA, USA) at excitation/emission wavelengths of 485 nm/530 nm.

Immunoblot Analysis
Protein extraction, SDS-polyacrylamide gel electrophoresis, and immunoblot analysis were performed as previously reported [26]. Briefly, cell lysates were separated by SDS-PAGE (7.5%, 12% acrylamide gels) and electrophoretically transferred to a nitrocellulose (NC) membrane (GE Healthcare, Ord, IL, USA). Subsequently, the NC membranes were blocked with 5% skim milk at 37 • C and incubated overnight at 4 • C with the primary antibody. After removing the primary antibody, the NC membranes were washed three times with PBS for 10 min, followed by incubation with a secondary antibody (Invitrogen) for 1 h at room temperature. After washing, the membranes were treated with an enhanced chemiluminescence (ECL) detection kit (Amersham Biosciences, Buckinghamshire, UK). Immunoreactive protein expression was visualized using LAS 4000 (Fujifilm, Tokyo, Japan); β-actin was used as an immunoblotting control.

Statistical Analysis
IBM SPSS online version 26.0 (SPSS, Inc., Chicago, IL, USA, an IBM company) was used for statistical analysis. A one-way analysis of variance was used to assess the statistical significance of the differences among treatment groups. For each statistically significant effect of treatment, Duncan's multiple range test was used for comparisons between multiple group means. The data were expressed as mean ± standard deviation (SD).

DPPH Radical Scavenging Activity
The antioxidant activity of natural products is commonly measured by their ability to neutralize the DPPH free radical, a rather stable free radical that causes cell aging and many diseases [34]. In this experiment, the DPPH free radical scavenging ability was measured for the 70% EtOH extract of CCSB and each solvent fraction. Without using standards, sample concentrations were tested from 25 to 1000 g/mL, and their respective

DPPH Radical Scavenging Activity
The antioxidant activity of natural products is commonly measured by their ability to neutralize the DPPH free radical, a rather stable free radical that causes cell aging and many diseases [34]. In this experiment, the DPPH free radical scavenging ability was measured for the 70% EtOH extract of CCSB and each solvent fraction. Without using standards, sample concentrations were tested from 25 to 1000 g/mL, and their respective IC 50 values were determined ( Figure 3A, Table 1). The DPPH free radical scavenging ability of CCSB extracts and fractions was found to increase concentration-dependently, and the antioxidant activity of each fraction was in the order of ethyl acetate, chloroform, n-butanol, water, and n-hexane. The IC 50 value of the EtOAc fraction was 77.77 ± 1.79 µg/mL, which demonstrated excellent DPPH radical scavenging activity, corroborating the result of an experiment in which the EtOAc fraction exhibited the highest antioxidant activity when 80% ethanol extract of CCSB was fractionated into n-hexane, dichloromethane, ethyl acetate, n-butanol, and water by Kim et al. [35]. In the study reported by Kalaivani et al., the DPPH radical scavenging activity was measured by isolating EG from leaves of Acacia Nilotica (L.) Wild. Ex. Delile Subsp. Indica (Benth.) Brenan [36]. This measurement revealed that, as the EG concentration increased, the DPPH radical scavenging activity also increased. In addition, EG had a higher DPPH radical scavenging activity than ascorbic acid, which was used as the positive control.

DPPH Radical Scavenging Activity
The antioxidant activity of natural products is commonly measured by their ability to neutralize the DPPH free radical, a rather stable free radical that causes cell aging and many diseases [34]. In this experiment, the DPPH free radical scavenging ability was measured for the 70% EtOH extract of CCSB and each solvent fraction. Without using standards, sample concentrations were tested from 25 to 1000 g/mL, and their respective IC50 values were determined ( Figure 3A, Table 1). The DPPH free radical scavenging ability of CCSB extracts and fractions was found to increase concentration-dependently, and the antioxidant activity of each fraction was in the order of ethyl acetate, chloroform, nbutanol, water, and n-hexane. The IC50 value of the EtOAc fraction was 77.77 ± 1.79 μg/mL, which demonstrated excellent DPPH radical scavenging activity, corroborating the result of an experiment in which the EtOAc fraction exhibited the highest antioxidant activity when 80% ethanol extract of CCSB was fractionated into n-hexane, dichloromethane, ethyl acetate, n-butanol, and water by Kim et al. [35]. In the study reported by Kalaivani et al., the DPPH radical scavenging activity was measured by isolating EG from leaves of Acacia Nilotica (L.) Wild. Ex. Delile Subsp. Indica (Benth.) Brenan [36]. This measurement revealed that, as the EG concentration increased, the DPPH radical scavenging activity also increased. In addition, EG had a higher DPPH radical scavenging activity than ascorbic acid, which was used as the positive control.

ABTS Radical Scavenging Activity
The chemical reaction of ABTS results in a transition from blue-green to transparent when radical cations gain electrons from antioxidants [37]. In this experiment, the ABTS Antioxidants 2023, 12, 269 9 of 21 cation radical scavenging activity was measured for the 70% EtOH extract of CCSB and each solvent fraction. Without using standards, sample concentrations were tested from 25 to 1000 g/mL, and their respective IC 50 values were determined ( Figure 3B, Table 1). Notably, the ABTS cation radical scavenging ability of CCSB extracts and fractions increased concentration-dependently, and the antioxidant activity of each fraction was in the order of ethyl acetate, chloroform, n-butanol, water, and n-hexane. The IC 50 value of the ethyl acetate fraction was 57.43 ± 0.40 µg/mL, showing excellent ABTS radical scavenging activity. The experimental results indicated that the ABTS radical had a significantly higher IC 50 value than the DPPH radical, based on the ability to measure the antioxidant capacity of hydrophilic substances and lipophilic compounds by dissolving them in water and organic solvents [38].

Total Polyphenol and Total Flavonoid Contents
Owing to their phenolic structures and double bonds, polyphenols, which are abundant in plant resources, have antioxidant, anti-inflammatory, antibacterial, and anticancer activities [39]. Plants generate polyphenols in minute quantities as secondary metabolites, and the structure of polyphenol compounds is stable even when dehydrogenation occurs due to the availability of electrons, which induces reduced characteristics and functions as antioxidants [40]. In this experiment, a standard calibration curve was prepared using gallic acid as the standard material, and the total polyphenol content of the 70% EtOH extract of CCSB and each solvent fraction was measured. The total polyphenol content of the extracts and fractions was expressed in terms of gallic acid equivalent (GAE) per mg/g of weight ( Table 1). The highest polyphenol content was found in the EtOAc fraction (368.87 ± 3.22 GAE mg/g). Therefore, CCSB contains more polyphenols than its fruits, considering Lee et al.'s study in which total phenolic content obtained from CCS fruits by extraction method using tannic acid as a standard substance reached a maximum of 27.69 mg% in water extract [41].
Furthermore, a standard calibration curve was prepared using quercetin as a standard material, and the total flavonoid content contained in the 70% EtOH extract of CCSB and each solvent fraction was measured. The total flavonoid content of the extracts and fractions was expressed in terms of quercetin equivalent (QUE) per 1 g of weight ( Table 1). The highest flavonoid content was found in the EtOAc fraction (45.14 ± 0.73 QUE mg/g).

Polyphenol Content Analysis Using HPLC MS/MS
Here, 16 types of polyphenols were identified via HPLC MS/MS, and the polyphenol content of the EtOAc fraction, which had the highest antioxidant activity among the fractions isolated from the 70% EtOH extract of CCSB, was analyzed. The polyphenols identified through HPLC MS/MS analysis were 4-hydroxybenzoic acid, caffeic acid, syringic acid, vanillic acid, coumaric acid, ferulic acid, naringenin, benzoic acid, nicotinic acid, gallic acid, protocatechuic acid, chlorogenic acid, catechin, kaempferol, EG, and epigallocatechin gallate (Figure 4). Among them, EG had the highest content at 330.00 mg/g, followed by gallic acid and chlorogenic acid. Notably, ellagic acid and its derivatives, as well as hexahydroxydiphenoyl esters and phenazine derivatives, were identified in CCS leaves [42,43]. Gallic acid, a well-known secondary metabolite of biosynthesis, was also found in high concentrations of ellagic acid and its derivatives in CCS leaves [44]. Consequently, ellagic acid and its derivatives are also present in CCSB, giving it a relatively high gallic acid content. A polyphenol analysis of CCSB leaf extract revealed that it contained large amounts of epigallocatechin gallate, EG, ρ-coumaric acid, and caffeic acid, corroborating the findings of the present study [45].

Results of EG Tyrosinase Inhibitory Activity Using a Cell-Free System
Tyrosinase, which catalyzes the rate-determining step of melanin biosynthesis, is an enzyme used to evaluate the whitening activity effect. To investigate the effect of CCSB on tyrosinase activity inhibition, the tyrosinase inhibitory activity of the extract fractions (CCSB-Hex, CCSB-Ch, CCSB-EtOAc, CCSB-BuOH, CCSB-Water) was measured. Among these fractions, CCSB-EtOAc had the highest inhibitory activity, with an IC50 value of 217.29 ± 1.76 µg/mL ( Figure 5). Ascorbic acid and EG were used as positive controls, and their IC 50 values were 30.99 ± 0.86 and 71.27 ± 0.38 µg/mL, respectively. acid, vanillic acid, coumaric acid, ferulic acid, naringenin, benzoic acid, nicotinic acid, gallic acid, protocatechuic acid, chlorogenic acid, catechin, kaempferol, EG, and epigallocatechin gallate (Figure 4). Among them, EG had the highest content at 330.00 mg/g, followed by gallic acid and chlorogenic acid. Notably, ellagic acid and its derivatives, as well as hexahydroxydiphenoyl esters and phenazine derivatives, were identified in CCS leaves [42,43]. Gallic acid, a well-known secondary metabolite of biosynthesis, was also found in high concentrations of ellagic acid and its derivatives in CCS leaves [44]. Consequently, ellagic acid and its derivatives are also present in CCSB, giving it a relatively high gallic acid content. A polyphenol analysis of CCSB leaf extract revealed that it contained large amounts of epigallocatechin gallate, EG, ρ-coumaric acid, and caffeic acid, corroborating the findings of the present study [45].

Results of EG Tyrosinase Inhibitory Activity Using a Cell-Free System
Tyrosinase, which catalyzes the rate-determining step of melanin biosynthesis, is an enzyme used to evaluate the whitening activity effect. To investigate the effect of CCSB on tyrosinase activity inhibition, the tyrosinase inhibitory activity of the extract fractions (CCSB-Hex, CCSB-Ch, CCSB-EtOAc, CCSB-BuOH, CCSB-Water) was measured. Among these fractions, CCSB-EtOAc had the highest inhibitory activity, with an IC50 value of 217.29 ± 1.76 μg/mL ( Figure 5). Ascorbic acid and EG were used as positive controls, and their IC50 values were 30.99 ± 0.86 and 71.27 ± 0.38 μg/mL, respectively.

Enzyme Kinetics Analysis of Tyrosinase
The reaction rate of the entire reaction system usually determines the Km value of an enzymatic reaction. In this study, we calculated Km and Vmax and identified the type of inhibition using the Lineweaver-Burk equation. The inhibition pattern of an enzyme depends on the binding site and type of binding mode. During competitive inhibition, the

Enzyme Kinetics Analysis of Tyrosinase
The reaction rate of the entire reaction system usually determines the Km value of an enzymatic reaction. In this study, we calculated Km and Vmax and identified the type of inhibition using the Lineweaver-Burk equation. The inhibition pattern of an enzyme depends on the binding site and type of binding mode. During competitive inhibition, the inhibitor competitively binds to the substrate noncovalently, thereby inhibiting enzyme activity. In noncompetitive inhibition, the inhibitor reversibly binds to both the free enzyme and enzyme-substrate complex to exhibit inhibitory effects. In this study, the values of Km, Vmax, and inhibition constant (Ki) of EG against tyrosinase were 1.9675 mM, 0.1175 mmol/min, and 0.4341 mM, respectively ( Figure 6). The Lineweaver-Burk plot was linear, confirming that the kinetic behavior was noncompetitive.

Molecular Docking Study
Protein-ligand docking attempts to predict the location and orientation of the ligand when it binds to a protein receptor or enzyme [24]. We used molecular docking to predict the binding between EG and human tyrosinase. Met 374, Ser 380, His 180, His 211, His 390, His 363, Phe 347, Asn 364, and Ile 368 surrounded hydrophobic pockets, as predicted by the binding model ( Figure 7A). In these hydrophobic pockets, EG formed ligand conformations that inhibited enzyme activity. When a ligand was formed between tyrosinase and EG, hydrogen bond interactions were formed at Met 374, Ser 380, and His 390. The docking results revealed that EG can bind to the active site of tyrosinase. Based on the ligand interaction diagram of EG, hydrogen bond interactions were involved with the Met 374 and Ser 380 residues of tyrosinase, and a pi-pi interaction was possible between EG and His 367 of tyrosinase ( Figure 7B) [46].

Molecular Docking Study
Protein-ligand docking attempts to predict the location and orientation of the ligand when it binds to a protein receptor or enzyme [24]. We used molecular docking to predict the binding between EG and human tyrosinase. Met 374, Ser 380, His 180, His 211, His 390, His 363, Phe 347, Asn 364, and Ile 368 surrounded hydrophobic pockets, as predicted by the binding model ( Figure 7A). In these hydrophobic pockets, EG formed ligand conformations that inhibited enzyme activity. When a ligand was formed between tyrosinase and EG, hydrogen bond interactions were formed at Met 374, Ser 380, and His 390. The docking results revealed that EG can bind to the active site of tyrosinase. Based on the ligand interaction diagram of EG, hydrogen bond interactions were involved with the Met 374 and Ser 380 residues of tyrosinase, and a pi-pi interaction was possible between EG and His 367 of tyrosinase ( Figure 7B) [46].

Cytotoxicity Evaluation and Quantitative Analysis of Intracellular ROS
Mitochondrial dehydrogenase and MTT tetrazolium react during cell metabolism to form MTT formazan, which turns purple. Using this principle, cell viability can be measured [47]. For each concentration (1-100 μg/mL), EG cytotoxicity was determined to be < 5 μg/mL ( Figure 8A). Jin et al. (2006) isolated EG from Acer okamotoanum Nakai and measured its cytotoxicity against B16F10 cells [48]. The cytotoxicity IC50 value of EG isolated from A. okamotoanum was approximately 9.29 μg/mL. In this study, cell viability was significantly reduced compared to the control at concentrations of at least 10 μg/mL. Changes in the intracellular ROS content of B16F10 after EG treatment were measured. When EG was treated at concentrations of 1, 2.5, and 5 μg/mL, the intracellular ROS significantly decreased compared to the group treated with only t-BHP ( Figure 8B).

Cytotoxicity Evaluation and Quantitative Analysis of Intracellular ROS
Mitochondrial dehydrogenase and MTT tetrazolium react during cell metabolism to form MTT formazan, which turns purple. Using this principle, cell viability can be measured [47]. For each concentration (1-100 µg/mL), EG cytotoxicity was determined to be <5 µg/mL ( Figure 8A). Jin et al. (2006) isolated EG from Acer okamotoanum Nakai and measured its cytotoxicity against B16F10 cells [48]. The cytotoxicity IC 50 value of EG isolated from A. okamotoanum was approximately 9.29 µg/mL. In this study, cell viability was significantly reduced compared to the control at concentrations of at least 10 µg/mL. Changes in the intracellular ROS content of B16F10 after EG treatment were measured. When EG was treated at concentrations of 1, 2.5, and 5 µg/mL, the intracellular ROS significantly decreased compared to the group treated with only t-BHP ( Figure 8B).

Cytotoxicity Evaluation and Quantitative Analysis of Intracellular ROS
Mitochondrial dehydrogenase and MTT tetrazolium react during cell metabolism to form MTT formazan, which turns purple. Using this principle, cell viability can be measured [47]. For each concentration (1-100 μg/mL), EG cytotoxicity was determined to be < 5 μg/mL ( Figure 8A). Jin et al. (2006) isolated EG from Acer okamotoanum Nakai and measured its cytotoxicity against B16F10 cells [48]. The cytotoxicity IC50 value of EG isolated from A. okamotoanum was approximately 9.29 μg/mL. In this study, cell viability was significantly reduced compared to the control at concentrations of at least 10 μg/mL. Changes in the intracellular ROS content of B16F10 after EG treatment were measured. When EG was treated at concentrations of 1, 2.5, and 5 μg/mL, the intracellular ROS significantly decreased compared to the group treated with only t-BHP ( Figure 8B).

Results of Melanin Content by EG in B16F10 Cells
Mushroom-derived tyrosinase is 23% identical in amino acid sequence to human tyrosinase, and mouse-derived tyrosinase is 82% similar in sequence identity to human tyrosinase, so the experiment is usually more accurate [49]. When B16F10 cells were treated with α-MSH (1 µg/mL) and EG, the melanin content reduced proportionally to the EG concentration ( Figure 9). The melanin production inhibitory activity was similar to that of 2.5 µg/mL EG and arbutin, which were positive controls. Regarding 5 µg/mL EG treatment, EG inhibitory activity surpassed that of arbutin. Mushroom-derived tyrosinase is 23% identical in amino acid sequence to human tyrosinase, and mouse-derived tyrosinase is 82% similar in sequence identity to human tyrosinase, so the experiment is usually more accurate [49]. When B16F10 cells were treated with α-MSH (1 μg/mL) and EG, the melanin content reduced proportionally to the EG concentration ( Figure 9). The melanin production inhibitory activity was similar to that of 2.5 μg/mL EG and arbutin, which were positive controls. Regarding 5 μg/mL EG treatment, EG inhibitory activity surpassed that of arbutin.

Effect of EG on Antimelanogenesis-Related Proteins/Genes and Autophagy-Related Proteins in the B16F10 Cell Line
Melanin is synthesized via various intracellular signaling pathways, including the cAMP/PKA pathway. UV boosts cAMP levels in melanin cells, activates PKA, and promotes MITF expression via CREB. MITF is an important transcriptional regulator in the melanin synthesis pathway, promoting the transcription of TYR, TRP-1, and TRP-2. EG was isolated from CCSB, and its whitening activity was confirmed by measuring the expression levels of TYR, TRP-1, TRP-2, and MITF proteins in B16F10 cells stimulated by α-MSH. When B16F10 melanoma cells were treated with EG at 1, 2.5, and 5 μg/mL, the expression levels of TYR, TRP-1, TRP-2, MITF, ρ-PKA, PKA, ρ-CREB, and CREB proteins decreased EG concentration-dependently ( Figure 10). In particular, at 5 μg/mL, an antimelanogenic effect similar to that of arbutin was confirmed. Kim et al. (2018) extracted 75% EtOH of CCS to measure tyrosinase inhibition in B16F10 cells [50]. They found that the extract exhibited 37.9% tyrosinase inhibition activity, exceeding that of the positive control arbutin (33.9%). Many studies have also explored the inhibition of melanin production using natural resources. Li et al. (2018) extracted Morus alba L. leaves with 70% EtOH; after fractionalization, the extract was used to treat B16F10 cells stimulated by α-MSH [51]. They found that the studied extract dose-dependently lowered the expression levels of CREB, MITF, TYR, and TRP-1 in B16F10 cells. Pedrosa et al. (2016) also reported the tyrosinase inhibition activity of 50% EtOH extract of Libidibia ferrea Mart in B16F10 cells [52]. In an effort to identify novel cosmetic materials with antiaging and whitening properties, research on the production of materials that control the autophagy process has

Effect of EG on Antimelanogenesis-Related Proteins/Genes and Autophagy-Related Proteins in the B16F10 Cell Line
Melanin is synthesized via various intracellular signaling pathways, including the cAMP/PKA pathway. UV boosts cAMP levels in melanin cells, activates PKA, and promotes MITF expression via CREB. MITF is an important transcriptional regulator in the melanin synthesis pathway, promoting the transcription of TYR, TRP-1, and TRP-2. EG was isolated from CCSB, and its whitening activity was confirmed by measuring the expression levels of TYR, TRP-1, TRP-2, and MITF proteins in B16F10 cells stimulated by α-MSH. When B16F10 melanoma cells were treated with EG at 1, 2.5, and 5 µg/mL, the expression levels of TYR, TRP-1, TRP-2, MITF, ρ-PKA, PKA, ρ-CREB, and CREB proteins decreased EG concentration-dependently ( Figure 10). In particular, at 5 µg/mL, an antimelanogenic effect similar to that of arbutin was confirmed. Kim et al. (2018) extracted 75% EtOH of CCS to measure tyrosinase inhibition in B16F10 cells [50]. They found that the extract exhibited 37.9% tyrosinase inhibition activity, exceeding that of the positive control arbutin (33.9%). Many studies have also explored the inhibition of melanin production using natural resources. Li et al. (2018) extracted Morus alba L. leaves with 70% EtOH; after fractionalization, the extract was used to treat B16F10 cells stimulated by α-MSH [51]. They found that the studied extract dose-dependently lowered the expression levels of CREB, MITF, TYR, and TRP-1 in B16F10 cells. Pedrosa et al. (2016) also reported the tyrosinase inhibition activity of 50% EtOH extract of Libidibia ferrea Mart in B16F10 cells [52]. In an effort to identify novel cosmetic materials with antiaging and whitening properties, research on the production of materials that control the autophagy process has been intensively conducted in recent years.
Autophagy is a revolutionary antiaging concept that is necessary for cells to eliminate intracellular wastes and old proteins, in addition to recycling and rebuilding them into healthy cells. Importantly, inducing autophagy has been shown to suppress melanin production, suggesting a connection between these two processes. ATP is required for AMP-activated protein kinase (AMPK) activation and inactivation of mTOR's target [53]. In addition, LC3B-II, an important protein marker in autophagy, induces ERK activation; ERK increases MITF expression via CREB phosphorylation; and ATG7 and Beclin-1 are positively related to MITF expression and MITF transcriptional activity, respectively [54]. To investigate EG autophagy-enhancing activity, AKT, mTOR, Beclin, and LC3B autophagy markers were induced by treating B16F10 cells with MSH, and the protein expression patterns were then measured. As a result, the protein expression of AMPK and p-AKT of the protein markers related to autophagy was increased, and the protein expression of p-m-TOR was decreased ( Figure 11). In addition, Beclin and LC3B expression levels both increased, confirming that autophagy was activated. Patrinia villosa (Thunb.) Juss extract prevented melanogenesis and induced autophagy via autophagy markers LC3B and p62 [10]. A study described a mechanism underpinning the regulation of melanin synthesis or function in antiaging, finding that autophagy responded in accordance with AKT2 concentrations [54].   Based on Western blotting data, the expression levels of melanin production-related genes, TYR, TRP-1, TRP-2, and MITF, were evaluated at the mRNA level using RT-PCR in order to confirm EG skin-whitening activity. α-MSH induced TYR, TRP-1, TRP-2, and MITF expression mediated by EG, whereas EG treatment reduced mRNA expression (1-5 µg/mL) concentration-dependently. In particular, 5 µg/mL of EG inhibited mRNA expression more effectively than the positive control arbutin ( Figure 12).  We have demonstrated that autophagy enhancers can contribute to inhibiting the melanogenic pathway ( Figure 13), but autophagy inhibition or blockage may be required for antimelanogenesis to be effective. To determine the effect of autophagy flux on melanogenesis signaling, further research is required.

Conclusions
This study demonstrated that EG isolated from Castanopsis cuspidata var. sieboldii branch (CCSB) extract promoted autophagy and inhibited melanogenesis. AMPK and p-AKT increased in the α-MSH-related pathway, with an enhanced LC3B signal in autophagy flux. EG significantly reduced the levels of whitening-associated proteins, p-CREB, and p-PKA, and it inhibited the expression of TYR, TRP-1, TRP-2, and transcription factor (MITF) in a dose-dependent manner. Therefore, CCSB extract could serve as a novel functional cosmetic material with antimelanogenic and autophagy-enhancing activity. We plan to obtain soluble expression of human tyrosinase and semisynthesis of novel derivatives of EG. By combining the result of this and future studies, EG and EG derivatives can be established as novel cosmetic ingredients with autophagy-regulating properties once the clinical study is completed.