G. lemaneiformis was purchased from Nan’ao Island (Shantou, Guangdong, China). Alkaline protease was provided by Hefei Bomei Biotechnology Co., Ltd. (Hefei, China). 1,1-diphenyl-2-picrylhy-drazyl (DPPH), 2, 2′-azino-bis (3-ethylbenzothiazoline-6-sulfonic acid) (ABTS) and tripyridyltriazine (TPTZ) were provided by Sigma-Aldrich Co., Ltd. (St. Louis, MO, United States). HepG2 was provided by Chinese Academy of Sciences. DMEM medium and fetal bovine serum (FBS) were supported by Gibco Co., Ltd. (Guangzhou, China). Superoxide dismutase (SOD) activity detection kit and malondialdehyde (MDA) assay kit were provided by Beijing Solarbio Science and Technology Co., Ltd. (Beijing, China).

In this study, the dried G. lemaneiformis powder was immersed in 0.2 M NaOH at the proportion of 1:24 (w/v). Next, in this study, the mixtures were employed in G. lemaneiformis protein extraction using ultrasonic assisted alkali extraction and acid precipitation. Ultrasonic treatment was implemented at 30°C in 70 min at a power of 482 W, and the frequency parameter is set to 20 kHz. We centrifuged later solution at 11,000 g in 15 min at 4°C. In addition, the pH in supernatant was set to 4.5, and centrifugated at 11,000 g for 15 min at 4°C. Then, the collected precipitate was dialyzed and lyophilized. Finally, the obtained G. lemaneiformis protein was preserved at −20°C for future application.

G. lemaneiformis protein were dissolved into ultrapure water for preparation of solutions with different protein concentration. The protein solution was hydrolyzed with alkaline protease at their optimal condition. Followed by centrifugation of protein hydrolysates at 11,000 g in 15 min at 4°C, the reaction ceased after heating at 100°C for 20 min. Next, in order to perform the analysis, the obtained supernatant received freeze drying treatment and was preserved at −20°C. The degree of hydrolysis was calculated from the ratio of α-amino nitrogen to total nitrogen (the amino nitrogen content was measure by the formaldehyde titration method, and the total nitrogen content as well as protein concentration were measured by the Kjeldahl method).

Firstly, the GLPH solution (filtered by 0.22 μm microporous membrane) was fractionated on a Sephadex G-25 gel filtration column (1.6 × 50 cm) with the flow rate of 0.5 mL/min. In the meanwhile, the column was eluted in ultrapure water. Every eluate was gathered for monitoring at 214 nm, and four fractions (A–D) were gathered and lyophilized. The highest antioxidant activity fraction C was further separated using RP-HPLC. The peptide fraction was filtered through a microporous membrane (0.22 μm) before being loaded into Athena C18 (5 μm, 4.6 × 250 mm). Besides, the mobile phases of gradient elution included eluent A including 0.1% concentration of TFA in ultrapure water (v/v) and eluent B including 0.1% concentration of TFA in acetonitrile. In addition, the gradient elution program was 0–5 min, 0% A; 5–25 min, 0–50% A; 25–30 min, 50–100% A. The eluate was monitored at 220 nm, and three peptides (C1–C3) were isolated and then lyophilized.

The fraction C1 having the highest antioxidant activity was further analyzed the amino acid sequence by nano-HPLC-MS/MS on a Q Exactive Plus mass spectrometry (Thermo Fisher Scientific, Waltham, MA, United States). We loaded 9 μL sample into a chromatographic analytical column (Acclaim PepMap C18, 75 μm × 15 cm) at a flow rate of 300 nL/min. Elution conditions included mobile phase A (0.1% formic acid in water); mobile phase B (0.1% formic acid in ACN); column temperature (40°C); linear elution program (0–30 min, 8–30% B). Besides, mass spectra were documented within an m/z scope of 100–1,500. In addition, we had the electrospray voltage of 2 kV. Tandem mass spectra were processed by PEAKS Studio version X+ (Bioinformatics Solutions Inc., Waterloo, ON, Canada).

Synthesis of identified antioxidant peptides followed the solid-phase technique of GL Biochemistry Co., Ltd. (Shanghai, China). Besides, the resulting peptides had a purity over 95% (w/w) measured using high-performance liquid chromatography at mobile phase A, 0.1% TFA in 100% acetonitrile; mobile phase B, 0.1% TFA in 100% water; flow rate, 1 mL/min; column, Kromasil-C18, 5 μm particle size, 4.6 × 250 mm. Using the MS spectrum, molecular masses of synthesized peptides were measured. The ABTS radical scavenging activity of synthesized peptides with varying concentrations (0–1 mg/mL) was measured as mentioned previously. Using non-linear regression analysis, the half inhibitory concentration (IC₅₀) of the peptide was measured.

In this study, the molecular docking in the identified peptides with Keap1 was performed using the procedure by Han et al. (21). The semi flexible docking of Keap1 with antioxidant peptide was calculated by molecular docking software AutoDock 4.2. Before docking, we downloaded the crystal structure of Keap1 (PDB ID: 2FUL) from the PDB database. Simultaneously, water molecules and Nrf2 16-mer were removed by PyMOL software to obtain the receptor molecules to be docking. Adding polar hydrogen to the receptor molecule, calculate the charge and add the protein type. The 3D structure of small molecule ligands was obtained in Chem3D software and the energy was minimized. In autodock, small molecule ligands can be detected. The central coordinates of the docking range were set as the active site of Keap1 (x: 5; y: 9; z: 1) (22). At the same time, and a reaction constraint box with a spacing of 0.375 Å was established. Lamarck genetic algorithm is used to optimize the docking energy. In the cluster analysis of conformational energy, the tolerance of root mean square deviation is 2.0 Å. The interaction between antioxidant peptides from G. lemaneiformis and Keap1 protein was analyzed by discovery studio 2020 client.

H₂O₂-induced oxidative damage model was established, and the influence of the antioxidant peptide on oxidative damage was evaluated by measuring cell viability, SOD activity and MDA content. HepG2 cells suspension was absorbed and seeded on 96-well plates with the density of 1 × 104 cells/well, followed by cultivation under a humidified atmosphere (37°C, 5% CO₂) via DEME medium (with 10% FBS and 1% penicil-lin-streptomycin). After 24-h cultivation of HepG2, the cells were categorized into control and treatment groups. In addition, the control group was added with 100 μL culture medium and cultured for 4h. Besides, the treatment group (peptide-treated group) was pre-pared through supplementing 100 μL of 100 μg/mL of GSH or PGPTY (DMEM dissolved) and cultured for 4 h. Next, 10 μL H₂O₂ (800 μM) was introduced to every well, followed by incubation for 2 h. Besides, the treatment group (H₂O₂-treated group) was added with 100 μL culture medium and cultured for 4 h. Then, 10 μL H₂O₂ (800 μM) was introduced, which was also cultured for 2 h. Light density value at 595 nm was calculated, and cell viability (%) was computed as below:

Where A_{treatment group} indicates the absorbance in treatment group, A_{control group} denotes the absorbance in control group.

SOD activity and MDA content were determined using SOD kit and MDA kit (Beijing Solarbio Science and Technology Co., Ltd.).

Through one-way analysis of variance (ANOVA) on the IBM SPSS statistics 25.0 software, Duncan’s t-tests were conducted. It was shown that differences showed statistical significance at p < 0.05.

The G. lemaneiformis protein was hydrolyzed by alkaline protease. The effects of enzyme dosage, enzyme hydrolysis time, substrate concentration, pH on the degree of hydrolysis and the ABTS free radical scavenging rate of protein hydrolysates (2 mg/mL) were investigated by single factor experiment. Optimization of enzymatic hydrolysis conditions (such as substrate concentration, enzyme dosage, enzymatic hydrolysis time, and pH) is crucial for the production of hydrolyzed proteins with desired functional properties (23). Enzymatic hydrolysis program was carried on with different enzyme dosage from 1 to 6%, and other hydrolysis conditions were fixed with temperature of 50°C, enzyme hydrolysis time of 4h, substrate concentration of 1 g/100 mL and pH 8.0. As shown in Figure 1A, the degree of hydrolysis and the ABTS free radical scavenging rate rapidly enhanced from 1 to 3%. After enzyme dosage more than 3%, the degree of hydrolysis and the ABTS free radical scavenging rate increased slightly. Nevertheless, the ABTS free radical scavenging rate appeared a downward trend with enzyme dosage more than 5%. Moreover, no significant difference was found in hydrolysis degree and ABTS free radical scavenging rate between 4 and 5%. The principle of reagent saving and antioxidant activity were used as the main criteria, and the 2–4% of enzyme dosage was chosen as the subsequent optimized experimental conditions.

As an important factor affecting the activity and degree of hydrolysis of enzymatic hydrolysis products, the optimal conditions of substrate concentration were also explored varying from 0.5 to 3 g/100 mL. Figure 1B exhibits the impact of substrate concentration on hydrolysis degree and ABTS free radical scavenging rate. As substrate concentration grew to 1 g/100 mL, hydrolysis degree and ABTS radical scavenging rate both shown an upward trend, and the maximum antioxidant activity was reached at 1 g/100 mL. As substrate concentration continually increases, hydrolysis degree and ABTS radical scavenging rate gradually decrease. The reason for this may be that too high substrate concentration will cause the solution to be too viscous, slow molecular diffusion, and cause substrate inhibition and enzyme inactivation. Thus, substrate concentrations ranged from 0.5 to 1.5 g/100 mL were chosen as the subsequent optimized experimental conditions.

The impact of enzyme hydrolysis time on hydrolysis degree and ABTS free radical scavenging rate was within a range of 1–10h. According to Figure 1C, as nzymatic hydrolysis time increased from 1 to 2 h, hydrolysis degree and ABTS free radical scavenging rate showed a fast increase. As enzymatic hydrolysis time enhanced, hydrolysis degree presented a slow increase, but ABTS continually decreased. It was possibly because the prolonged hydrolysis time made hydrolysis more complete. But excessive hydrolysis could produce more amino acids, resulting the decreased antioxidant activity. In addition, the highest value of the ABTS free radical scavenging rate (66.71%) was found at enzymatic hydrolysis time of 2 h. In order to make the peptides obtained in the subsequent experiments have better biological activity, the enzymatic hydrolysis time from 1 to 3 h was selected as the subsequent optimized experimental conditions.

The effect of pH on both hydrolysis degree and ABTS free radical scavenging rate was within a range of 7.0–9.5. Figure 1D shows the results. As pH increased, hydrolysis degree and ABTS free radical scavenging rate showed a fast increase. As pH approached 8, hydrolysis degree and ABTS free radical scavenging rate reached the maximum. Hydrolysis degree and ABTS radical scavenging rate progressively reduced as pH continually increased. Therefore, pH ranged from 7.5 to 8.5 was selected.

By performing the single-factor experiment, the orthogonal experiment was performed using the 2.3.2 method, in which ABTS free radical scavenging rate served as an evaluation index. The experiment results and analysis are shown in Table 2. The extreme value R shows that the primary and secondary order of the influence of different factors on the scavenging rate of ABTS free radicals within the experimental range is A (substrate concentration) > B (enzyme dosage) > C (hydrolysis time) > D (pH). The theoretical optimal combination of each factor is A2B1C2D2. The analysis of variance of orthogonal experiment was shown in Table 3. The impacts of A, B, C, and D on the clearance rate of ABTS radical scavenging rate were significant (p < 0.05). Finally, the optimal process parameters were determined (enzyme dosage of 2%, hydrolysis time of 2 h, substrate concentration of 1 g/100 mL and pH at 8.0).

Peptide size is among the influencing factors of its antioxidant activity. Gel filtration chromatography and RP-HPLC are commonly used to isolate and enrich peptides (24, 25). The antioxidant peptides from GLPH were isolated using the Sephadex G-25 gel filtration column according to the differences of molecular dimensions. Figure 2A displayed that GLPH was separated into four fractions (A, B, C, and D). Every fraction was gathered for freeze drying, to investigate its antioxidant activity. As shown in Figure 2B, the fraction C exhibited the strongest antioxidant activity. Its ABTS free radical scavenging rate and FRAP value of the fraction C (2 mg/mL) was 74.95% and 163.08 μg/mL, respectively. Therefore, the fraction C was chosen in further separation and purification.

Fraction C was isolated using RP-HPLC on an Agilent ZORBAX XDB-C18 (21.2 × 150 mm, 5 μm) column. According to Figure 3A, the elution consisted of three major peaks (C1, C2, and C3). Their antioxidant activities are displayed in Figure 3B. It was found that the fraction C2 (2 mg/mL) had the highest DPPH and ABTS free radical scavenging rate and FRAP value, which were 90.96, 80.95, and 190.17 μg/mL, respectively. Using nano-HPLC-MS/MS, the amino acid sequences of antioxidant peptides in fraction C2 were further measured.

According to Figure 4, the three antioxidant peptides were identified as Leu-Ser-Pro-Gly-Glu-Leu (LSPGEL), Val-Tyr-Phe-Asp-Arg (VYFDR) and Pro-Gly-Pro-Thr-Tyr (PGPTY) with molecular weight of 614.68, 698.76, and 533.57 Da, respectively. The molecular weight of most antioxidant peptides is lower than 1,000 Da. This could be attributed to the peptides with lower molecular weight are more likely to have interactions with target free radicals to end the chain reaction, and they usually have stronger antioxidant activity than that of the peptides with higher molecular weight (26). As shown in Table 4, the corresponding proteins of the antioxidant peptides were verified, and the peptides of LSPGEL, VYFDR and PGPTY were found derived from allophycocyanin α chain (18th–23th), phycocyanin beta subunit (162th–166th), and phycocyanin α subunit (70th–74th), respectively. Synthesis of the identified peptides was performed to verify antioxidant activity. PGPTY had clearly higher antioxidant activity compared with LSPGEL and VYFDR.

Keap1-Nrf2 pathway is the most important regulator of oxidative stress induced by various exogenous and endogenous factors (27). Keap1 (Kelch-like ECH-associated protein 1) could bind to Nrf2 (nuclear factor erythroid 2-related factor 2) via its Kelch domains, leading to a degradation of Nrf2 (28). However, the accumulation of Nrf2 is very important for the expression of a series of phase II detoxication enzymes such as superoxide dismutase (SOD) in the cells (29). Therefore, the external molecules (like peptides) able to bind to Keap1 could prohibit Keap1-Nrf2 interaction and increase cell resistance to oxidative stress. The docking of antioxidant peptide with Keap1 by Autodock 4.2 will help to further analyze the anti-oxidation mechanism. As shown in Figures 5A,B, LSPGEL forms seven hydrogen bonds with ASN382, ARG380, ASN414, SER363, TYR334, SER602, and ARG336 of Keap1, forms hydrocarbon bond with ARG415, and forms PI alkyl with TYR572, with docking energy of −3.88 kcal/mol and inhibition constant of 1.43 mM. As shown in Figures 5C,D, four hydrogen bonds were formed between VYFDR and Keap1’s ARG380, ASN382, SER602, and GLN530, with docking energy of −3.49 kcal/mol and inhibition constant of 2.79 mM. According to Figures 5E,F, six hydrogen bonds were formed between PGPTY and keyap1’s GLY574, HIS575, ARG553, ASP529, TYR572, ARG483, with docking energy of −4.49 kcal/mol and inhibition constant of 0.51 mM. The results suggested that the PGPTY docked with Keap1 was easier than the other two peptides, which might be the cause of the PGPTY had the higher antioxidant activity.

Active peptides are mainly combined with macromolecules through hydrogen bond interaction, van der Waals force and electrostatic interaction. Besides, hydrogen bond interaction is particularly important, and can play a role in stabilizing docking complex. Keap1 is a key component of Nrf2 regulation that plays a part in cytoplasm. The peptide LSPGEL and VYFDR occupied the amino acid residues ARG380 and ASN382, while the peptide PGPTY occupied the amino acid residues ARG483. These amino acid residues are very important for the Keap1 in the Keap1-Nrf2 pathway. Thus, the antioxidant peptide from G. lemaneiformis has a favorable effect on the cell oxidative stress and exogenous damage.

By adopting the H₂O₂-induced oxidative stress cell model, the antioxidant activity of PGPTY was assessed. Figure 6A demonstrates that different concentrations (100, 200, 400 μg/mL) of PGPTY had no significant (p > 0.05) toxicity impact on HepG2 cells in contrast to the control group. With the purpose of exploring the protective impact of PGPTY on H₂O₂-induced cell damage, PGPTY (100 μg/mL) and positive control glutathione (100 μg/mL) were pretreated and then exposed to 800 μM of H₂O₂, respectively. As illustrated in Figure 6B, the cell viability of HepG2 cells cultured with H₂O₂ (800 μM) was significantly decreased (p < 0.05) to 56.71%, indicating that the oxidative damage model for HepG2 cells was successfully constructed. When HepG2 cells were pretreated with PGPTY or GSH and then treated with H₂O₂, the cell viability was significantly enhanced (p < 0.05). Research showed PGPTY and GSH could both alleviate the damage of HepG2 cells induced by H₂O₂, and the cytoprotective effect of the PGPTY was as well as that of the GSH.

For illustrating the protective mechanism of PGPTY against H₂O₂-induced oxidative stress injury in HepG2 cells, SOD activity and MDA content in HepG2 cells were studied. Besides, the antioxidant enzymes (such as SOD) in cell are very important for the cell against oxidative stress damage, and the cell with high antioxidant enzyme activity could have good antioxidation ability (30, 31). Malondialdehyde (MDA) could be produced from the degradation of cell membrane induced by lipid peroxidation, and the reduced content of MDA in the cell could reflect the alleviated oxidative damage (32, 33). As shown in Figure 6C, when HepG2 cells were processed using 800 μM H₂O₂ in 2h, SOD activity in HepG2 cells was drastically decreased and MDA content obviously ascended. However, the PGPTY protective group had obviously higher SOD activity (p < 0.05) in relative to the H₂O₂-injured group, indicating that the capacity of PGPTY to prevent H₂O₂-induced oxidative damage on HepG2 cells was in part associated with its ability to enhance antioxidant enzyme (such as SOD) activity in HepG2 cells. Besides, the MDA content in PGPTY-pretreated HepG2 cells was notably lower (p < 0.05) when compared with that of H₂O₂-injured group, implying cell membrane could be protected by the peptide from H₂O₂-induced degradation or damage. Similar regulation effect of SOD and MDA in the H₂O₂-injured HepG2 cells was also observed in the GSH-pretreated group, and no significant (p > 0.05) difference was reported between groups.