Investigation of the Structural Properties and Antioxidant Potency of Pectic Polysaccharides Derived from Rohdea japonica (Thunb.) Roth

This study investigated the structural composition and antioxidant properties of pectic polysaccharides extracted from Rohdea japonica (Thunb.) Roth. Pectins, which belong to a complex category of acidic polysaccharides, possess a wide range of biological effects stemming from their distinctive structural domains. The polysaccharides were extracted using water, and were subsequently purified through ion exchange and gel permeation chromatography. In order to elucidate their structural features, Fourier Transform Infrared Spectroscopy and Nuclear Magnetic Resonance techniques were applied. Two specific polysaccharides, WRJP-A2a and WRJP-A3b, with molecular weights of 42.7 kDa and 64.1 kDa, respectively, were identified to contain varying proportions of homogalacturonan, rhamnogalacturonan I, and rhamnogalacturonan II domains. Regarding antioxidant capacity, WRJP-A3b exhibited superior scavenging capabilities against DPPH, ABTS, and hydroxyl radicals, potentially attributed to its higher galacturonic acid content and abundance of homogalacturonan domains. These results enhance our comprehension of the structure–activity interplay of pectic polysaccharides sourced from Rohdea japonica (Thunb.) Roth and their potential utility in the healthcare and functional food sectors.


Introduction
Pectins, a group of complex acidic polysaccharides found in plant cells, exhibit diverse biological functions [1].They primarily comprise the following three distinct domains: homogalacturonan (HG), rhamnogalacturonan I (RG-I), and rhamnogalacturonan II (RG-II).The HG domain, accounting for approximately 65% of total pectin content, consists of a linear polysaccharide made up of α-(1→4)-linked galacturonic acid (GalA) residues.Some of these GalA residues undergo methylation at the O-3 position and acetylation at either the O-2 or O-3 position [2].RG-I represents 20% to 35% of total pectin, and is composed of a backbone with repeating units of [→2)-α-Rhap-(1→4)-α-GalAp-(1→], with side chains attached to the C4 position of (1→2)-α-Rhap.The side chains comprise arabinan, galactan, arabinogalactan-I, and arabinogalactan-II (AG-II).The percentage of neutral sugar side chains in RG-I ranges from 25% to 80%, contingent on the pectin's source and extraction technique.Furthermore, the RG-II domain is a significantly conserved sequence found in plant cells, exhibiting remarkable uniformity among different plant species [3].
Pectins exhibit a remarkable ability to scavenge free radicals due to their high GalA content, positioning them as promising antioxidants.The unique physicochemical properties and low toxicity of pectins have attracted significant attention [4].The macromolecular architecture of pectin imparts it with a distinct capacity to stabilize free radicals, effectively mitigating reactive oxygen species through mechanisms such as chelating metal ions and scavenging peroxides.While phenolic compounds, owing to their lower molecular weight, may exhibit swifter reaction kinetics and elevated in vitro antioxidant activity, pectin, with its high molecular weight and multifunctional structure, offers more enduring and extensive antioxidant protection within the in vivo milieu.Furthermore, pectin's ubiquitous presence in plant cell walls, coupled with its long history of safe consumption and excellent biocompatibility, establishes a robust foundation for its safety profile [5].As complex biological macromolecules, the antioxidant effectiveness of pectins is significantly affected by factors such as solubility, molecular weight, and structural features like monosaccharide composition, glycosidic bond type, and the sequence and configuration of sugar residues [6].Moreover, plant pectins demonstrate universal structural characteristics alongside plant-source-specific traits [7].Furthermore, the biological activity of pectin is greatly influenced by the composition and structural variations within its domains.Although the main chemical structure properties of pectins are well-established, subtle structural variances like side chain composition, esterification degree, molecular weight, and branching degree differ among plant species [8].Therefore, exploring the intricate structures of different pectins is crucial for understanding the structure-activity relationship and enhancing their application in the pharmaceutical and food industries.
In recent years, there has been a surge in research focusing on pectins derived from monocotyledonous plants, which has emerged as a prominent area of scientific inquiry [9][10][11].Among these, Rohdea chinensis, a plant belonging to the Rohdea genus, has garnered particular attention.From this plant, three distinct polysaccharides have been successfully isolated and characterized [12].Rohdea japonica (Thunb.)Roth (R. japonica), another perennial herbaceous plant from the Rohdea genus, is predominantly found in various regions, including Shandong, Jiangsu, Zhejiang, Jiangxi, Hubei, Hunan, Guangxi, Guizhou, Sichuan, Anhui, Fujian, Henan, and Taiwan, along with Japan.This plant typically blooms from May to June, and bears fruit from September to November.Thriving in moist habitats, such as forest understories or grasslands at elevations between 750 and 1700 m, both its rhizome and the entire plant exhibit medicinal properties.These properties include cardiac reinforcement, diuretic effects, heat and toxin clearance, pain relief through stasis elimination, and bleeding cessation [13,14].Despite rhodexin A being the main component of R. japonica [15], research on its polysaccharides remains lacking.Certainly, there exists a notable lack of research on the intricate structure-activity relationship of R. japonica's pectins.Therefore, this study aims to extract pectins from R. japonica and ascertain their structure through a combination of chemical and instrumental analyses.Additionally, the antioxidant properties of these pectins and their related structure-activity correlations are under scrutiny.

Purity, Homogeneity, and Molecular Weight of WRJP-A2a and WRJP-A3b
WRJP-A2a exhibited no absorbance at 260 and 280 nm, indicating the absence of nu cleic acids and proteins in the fractions (Figure 2).As made evident by Figure 2, WRJP A3b contains trace amounts of nucleic acid impurities; however, this is unlikely to signif icantly impact subsequent research endeavors.Therefore, the purification process re sulted in highly pure pectin.High-performance gel permeation chromatography (HPGPC) was utilized to assess the homogeneity of WRJP-A2a and WRJP-A3b.Both pec tin fractions displayed narrow, single symmetrical peaks in the HPGPC elution curves (Figure 1C,D), suggesting homogeneity with molecular weights of 42.7 kDa (WRJP-A2a and 64.1 kDa (WRJP-A3b).

Purity, Homogeneity, and Molecular Weight of WRJP-A2a and WRJP-A3b
WRJP-A2a exhibited no absorbance at 260 and 280 nm, indicating the absence of nucleic acids and proteins in the fractions (Figure 2).As made evident by Figure 2, WRJP-A3b contains trace amounts of nucleic acid impurities; however, this is unlikely to significantly impact subsequent research endeavors.Therefore, the purification process resulted in highly pure pectin.High-performance gel permeation chromatography (HPGPC) was utilized to assess the homogeneity of WRJP-A2a and WRJP-A3b.Both pectin fractions displayed narrow, single symmetrical peaks in the HPGPC elution curves (Figure 1C,D), suggesting homogeneity with molecular weights of 42.7 kDa (WRJP-A2a) and 64.1 kDa (WRJP-A3b).

FT-IR Analysis of WRJP-A2a and WRJP-A3b
Fourier transform infrared (FT-IR) serves as a convenient and effective method for analyzing the primary structure of polysaccharides.It can be utilized to extract structural details concerning specific functional groups and sugar residue configurations within polysaccharides [16].
Both the WRJP-A2a and WRJP-A3b fractions displayed similar FT-IR spectra (Figure 1E,F).The broad and intense absorption peaks at 3319 and 3399 cm −1 were linked to the O−H stretching vibration characteristic of the hydrogen bonds in sugar residues.The faint absorption peaks around 2940 and 2936 cm −1 originated from the asymmetric C−H stretching vibrations of the −CH3, -CH2, and -CH groups.Notably, the absorption peaks near 1245, 1740, and 1610 cm −1 in the spectra indicated the presence of uronic acid [17].Specifically, the peaks near 1740 cm −1 and 1610 cm −1 represented the characteristic vibrations of C = O in carboxyl groups of methyl-esterified GalA and free carboxyl groups, respectively [18].These peaks' areas could be leveraged to calculate the degree of methylation (DM) of acidic polysaccharides.The esterification degree of pectin could be determined using the following formula: DE (%) = [A1740/(A1740 + A1610)] × 100%, where A1740 denotes the area of esterified carboxyl groups (1740 cm −1 ) and A1610 denotes the area of free carboxyl −1

FT-IR Analysis of WRJP-A2a and WRJP-A3b
Fourier transform infrared (FT-IR) serves as a convenient and effective method for analyzing the primary structure of polysaccharides.It can be utilized to extract structural details concerning specific functional groups and sugar residue configurations within polysaccharides [16].
monosaccharide compositions of WRJP-A2a-D and WRJP-A3b-D remained largely unchanged compared to the original pectin fraction (Figure 7C).In the FT-IR spectra of WRJP-A2a-D and WRJP-A3b-D (Figure 1E,F), the disappearance of the signal near 1740 cm −1 , attributed to the C = O bond in the methylated −COO− group, and the significant increase in the signal near 1610 cm −1 , indicated that the methyl groups in WRJP-A2a and WRJP-A3b had been effectively removed.

Analysis of Enzymatic Hydrolysates
Endo-PG, a specific enzyme, has the capability to degrade unesterified GalA, leading to the breakdown of the HG-type pectin domain into oligogalacturonide structural units.It also releases RG-I-and RG-II-type pectin domains from the pectin molecules.In this study, endo-PG was employed to degrade two types of pectins, resulting in two enzymatic hydrolysates known as WRJP-A2a-DE and WRJP-A3b-DE.Analysis using HPGPC (Figure 8) revealed significant alterations in the molecular weights of WRJP-A2a and WRJP-

NMR Analysis of WRJP-A3b
The 1D and 2D NMR spectra of WRJP-A3b are depicted in Figures 5 and 6, correspondingly.Based on the monosaccharide composition findings, WRJP-A3b demonstrates a high GalA content of 82.4%, indicating a predominance of HG-type structural domains in the pectin structure.In the 1 H NMR spectrum (Figure 5

Enzymatic Analysis of WRJP-A2a and WRJP-A3b
Based on the monosaccharide composition and NMR results, both WRJP-A2a and WRJP-A3b contain HG and RG-I domains.WRJP-A3b is primarily HG-type pectin, while WRJP-A2a contains an AG-II domain.For a more in-depth analysis of the pectin structure and function, WRJP-A2a and WRJP-A3b were hydrolyzed using endo-PG hydrolysis, and the different domains were separated by HPGPC.

Preparation of De-Esterified Pectin
Endo-polygalacturonase M2 (EC 3.2.1.15)specifically targets and breaks down the unesterified GalA within HG-type domains.However, the presence of methyl and acetyl groups in HG can hinder the enzymatic degradation of pectin, ultimately impacting the purity of the HG domain [19].Consequently, this study employed a lower temperature in a mildly alkaline setting to facilitate the de-esterification of pectin.To assess the effectiveness of de-esterification and the structural integrity of WRJP-A2a and WRJP-A3b, techniques such as FT-IR, HPGPC, and monosaccharide composition analysis were utilized.Analysis of HPGPC elution profiles (Figure 7A,B) revealed no significant alterations in the molecular weight distribution of WRJP-A2a and WRJP-A3b post-saponification, suggesting that the pectin's long chains remained unbroken during the process.Furthermore, the monosaccharide compositions of WRJP-A2a-D and WRJP-A3b-D remained largely unchanged compared to the original pectin fraction (Figure 7C).In the FT-IR spectra of WRJP-A2a-D and WRJP-A3b-D (Figure 1E,F), the disappearance of the signal near 1740 cm −1 , attributed to the C = O bond in the methylated −COO− group, and the significant increase in the signal near 1610 cm −1 , indicated that the methyl groups in WRJP-A2a and WRJP-A3b had been effectively removed.

Analysis of Enzymatic Hydrolysates
Endo-PG, a specific enzyme, has the capability to degrade unesterified GalA, leading to the breakdown of the HG-type pectin domain into oligogalacturonide structural units.It also releases RG-I-and RG-II-type pectin domains from the pectin molecules.In this study, endo-PG was employed to degrade two types of pectins, resulting in two enzymatic hydrolysates known as WRJP-A2a-DE and WRJP-A3b-DE.Analysis using HPGPC (Figure 8) revealed significant alterations in the molecular weights of WRJP-A2a and WRJP-A3b, with multiple chromatographic peaks observed in their respective profiles.To further purify these hydrolysates, a Sephadex G-75 column was utilized, leading to the preparation of three distinct types of hydrolysates (E1-E3) for both WRJP-A2a and WRJP-A3b.A3b, with multiple chromatographic peaks observed in their respective profiles.To further purify these hydrolysates, a Sephadex G-75 column was utilized, leading to the preparation of three distinct types of hydrolysates (E1-E3) for both WRJP-A2a and WRJP-A3b.The molecular weights of WRJP-A2a-DE1 and WRJP-A3b-DE1 were 50.3 kDa and 66.1 kDa, respectively, as indicated in Table 4.The primary constituents of the de-esterified hydrolysates were GalA, Rha, Gal, and Ara, with the Rha/GalA molar ratio approaching 1, suggesting that these hydrolysates belonged to the RG-I-type pectins.Notably, WRJP-A2a-DE1 contained a higher percentage of Gal (43.1%) and Ara (23.2%) compared to WRJP-A3b-DE1.The ratio of (Gal + Ara)/Rha serves as a metric for the average length and relative monosaccharide composition of the neutral side chains within the RG-I domain [19].In WRJP-A2a-DE1, this ratio was 4.4, which was roughly 3.4 times greater than that of WRJP-A3b-DE1, suggesting that the neutral sugar side chains in WRJP-A2a-DE1 were either longer or more extensively branched.Both WRJP-A2a-DE2 and WRJP-A3b-DE2 yielded positive results in TBA reactions, confirming their classification as RG-II-type pectins.Additionally, the molecular weights of WRJP-A2a-DE3 and WRJP-A3b-DE3 were below 2.0 kDa, and their hydrolysates were predominantly composed of GalA (ranging from 97.1% to 98.4%), indicating that they were oligogalacturonides derived from the endo-PG hydrolysis of HG-type domains.The molecular weights of WRJP-A2a-DE1 and WRJP-A3b-DE1 were 50.3 kDa and 66.1 kDa, respectively, as indicated in Table 4.The primary constituents of the de-esterified hydrolysates were GalA, Rha, Gal, and Ara, with the Rha/GalA molar ratio approaching 1, suggesting that these hydrolysates belonged to the RG-I-type pectins.Notably, WRJP-A2a-DE1 contained a higher percentage of Gal (43.1%) and Ara (23.2%) compared to WRJP-A3b-DE1.The ratio of (Gal + Ara)/Rha serves as a metric for the average length and relative monosaccharide composition of the neutral side chains within the RG-I domain [19].In WRJP-A2a-DE1, this ratio was 4.4, which was roughly 3.4 times greater than that of WRJP-A3b-DE1, suggesting that the neutral sugar side chains in WRJP-A2a-DE1 were either longer or more extensively branched.Both WRJP-A2a-DE2 and WRJP-A3b-DE2 yielded positive results in TBA reactions, confirming their classification as RG-II-type pectins.Additionally, the molecular weights of WRJP-A2a-DE3 and WRJP-A3b-DE3 were below 2.0 kDa, and their hydrolysates were predominantly composed of GalA (ranging from 97.1% to 98.4%), indicating that they were oligogalacturonides derived from the endo-PG hydrolysis of HG-type domains.

Antioxidant Activity Analysis
The antioxidant capabilities of WRJP-A2a and WRJP-A3b were assessed in vitro by evaluating their ability to scavenge DPPH, ABTS, and hydroxyl radicals.Over the tested concentration range (0.5 to 10 mg/mL), both pectins displayed a significant dose-dependent scavenging effect on these radicals, as shown in Figure 9A−F.Specifically, the Half-Maximal Inhibitory Concentration (IC 50 ) values for WRJP-A2a against the three radicals were 3.07, 1.09, and 4.75 mg/mL, respectively.In comparison, the IC 50 values for WRJP-A3b were 2.17, 1.39, and 3.27 mg/mL.These results indicate that, in the current experimental setup, WRJP-A3b exhibited a stronger radical-scavenging capacity than WRJP-A2a, although still lower than that of L-ascorbic acid.
To further explore the relationship between the antioxidant properties and structural composition of WRJP-A2a and WRJP-A3b, the radical-scavenging abilities of their de-esterified counterparts (WRJP-A2a-D and WRJP-A3b-D) and their various domains, including RG-I, RG-II, and oligogalacturonides, were evaluated.The level of methylesterification significantly influences the antioxidant activity of pectins.Specifically, the degree of methylation in pectins plays a crucial role in their antioxidant potential.Previous research has established a negative correlation between the antioxidant activity of apple pectins and their degree of methylation [20].In our study, despite WRJP-A2a showing a higher degree of methyl-esterification compared to WRJP-A3b, WRJP-A3b displayed a more potent ability to scavenge DPPH and hydroxyl radicals.After de-esterification, both WRJP-A2a-D and WRJP-A3b-D exhibited significantly enhanced antioxidant effects compared to their non-de-esterified forms.These findings highlight the intricate relationship between pectin structure and its antioxidant activity, which may result from the interaction of multiple factors.Moreover, molecular weight is another critical factor influencing the antioxidant activity of polysaccharides.It is widely accepted that high molecular weight pectins tend to form numerous intermolecular and intramolecular hydrogen bonds, thereby reducing the accessibility and reactivity of hydroxyl groups.On the other hand, pectins with lower molecular weights may have a more relaxed conformation, allowing the exposure of free hydroxyl groups and facilitating radical-scavenging reactions [21].Furthermore, the monosaccharide composition of polysaccharides significantly contributes to their antioxidant activity.A study has shown that GlcA and GalA have significant effects on the scavenging capabilities of Cissus pteroclada against DPPH, superoxide, hydroxyl, and ABTS radicals [22].Additionally, certain neutral monosaccharides, including Gal, Ara, and Glc, have been found to have substantial impacts on the DPPH radical-scavenging ability of polysaccharides [22,23].
Another study has demonstrated that 3-O-methylated-α-D-galactopyranosyl present in Pleurotus ostreatus polysaccharides possesses antioxidant properties [24].Pectins enriched with a certain amount of GalA are known to be potent antioxidants, and the antioxidant activity of these pectins can be attributed to the content of uronic acid and its degree of polymerization [25].The free radical-scavenging abilities of the three domains obtained through enzymatic hydrolysis of WRJP-A2a and WRJP-A3b are summarized in Figure 9. Significant variations in radical-scavenging capabilities were observed among the domains across a dose range of 0.5-10 mg/mL.Specifically, oligogalacturonides, characterized by the highest GalA content and lowest molecular weight, exhibited the highest radicalscavenging ability, followed by the RG-II domain (E2).The RG-I domain (E1), with lower GalA content and increased branching, demonstrated the weakest radical-scavenging capability.Notably, the radical-scavenging ability of oligogalacturonides displayed a dose-dependent pattern and surpassed that of the parent pectins (WRJP-A2a and WRJP-A3b) at the same concentration.These findings align with previous research, confirming that pectins enriched with GalA and containing HG-type domains possess an enhanced radical-scavenging capacity [26].
Molecules 2024, 29, 4135 14 of 20 ability to neutralize free radicals.The in vitro antioxidant properties of both WRJP-A2a and WRJP-A3b stem from the combined effects of various pectin domains, with the HG domain contributing the most significantly, followed by the RG-II domain.Conversely, the RG-I domain, characterized by a higher number of branches and molecular weight, had the least impact on the overall antioxidant activity of the pectins.

Materials
The rhizome material of R. japonica was collected from Qingdao, Shandong Province, China, in May 2022.This material originated from plants of the same age and location, ensuring uniformity.Professor Junlin Yu authenticated the specimens, and the voucher specimen is now safely stored in our laboratory's herbarium.Prior to further processing, the rhizome material underwent minimal preparation, involving only cleaning and washing.No peeling or removal of rhizome buds was performed.Subsequently, the rhizomes were sliced and dried in a cool, well-ventilated area for future use.DEAE-cellulose and Based on the findings, it appears that WRJP-A3b exhibits stronger antioxidant activity than WRJP-A2a, potentially attributed to its higher GalA content.Nevertheless, the presence of methyl groups and a higher molecular weight in WRJP-A3b diminished its ability to neutralize free radicals.The in vitro antioxidant properties of both WRJP-A2a and WRJP-A3b stem from the combined effects of various pectin domains, with the HG domain contributing the most significantly, followed by the RG-II domain.Conversely, the RG-I domain, characterized by a higher number of branches and molecular weight, had the least impact on the overall antioxidant activity of the pectins.

Materials
The rhizome material of R. japonica was collected from Qingdao, Shandong Province, China, in May 2022.This material originated from plants of the same age and location, ensuring uniformity.Professor Junlin Yu authenticated the specimens, and the voucher specimen is now safely stored in our laboratory's herbarium.Prior to further processing, the rhizome material underwent minimal preparation, involving only cleaning and washing.No peeling or removal of rhizome buds was performed.Subsequently, the rhizomes were sliced and dried in a cool, well-ventilated area for future use.DEAE-cellulose and Sepharose CL-6B were sourced from GE Healthcare (United States).The monosaccharide standards were purchased from Sigma.All other chemicals utilized in the study were of analytical grade.

Methods
Total carbohydrate content was determined utilizing the phenol-sulfuric acid method, with a standard composed of primary monosaccharides [27].Additionally, uronic acid content was assessed using the m-hydroxydiphenyl method, with GalA as the reference [28].Ultraviolet (UV) analysis was carried out using a UV-2700 full-wavelength UV scanner (Shimadzu, Japan) to measure absorbance from 200 to 800 nm.Homogeneity and molecular weight were evaluated using a high-performance liquid chromatography (HPLC) system (Shimadzu, Japan), featuring a RID-20A UV detector and a TSKgel G3000PWXL column (7.8 cm × 30.0 cm).Detection of 3-deoxy-D-manno-2-octulosonic acid (KDO) was conducted using the thiobarbituric acid (TBA) method as detailed in the reference [29].
3.3.Preparation of Pectin from R. japonica 3.3.1.Extraction of Pectin R. japonica material was extracted using hot water following the outlined protocol in our library reference [8].Initially, the dried material (1 kg) was crushed and soaked in deionized water (16 L).Extraction was conducted at 100 • C for 3 h, repeated three times under identical conditions.Subsequently, the supernatant was concentrated to 2 L at 80 • C and then treated with 8 L of 95% ethanol to precipitate the desired compounds, followed by an overnight incubation at 4 • C. The resulting precipitates underwent sequential washing with 95% ethanol and anhydrous ethanol before being dried under vacuum at 60 • C overnight.The final product, named water-soluble R. japonica polysaccharide (WRJP), represents the crude polysaccharide extracted from R. japonica material.

Fractionation of the Pectin
WRJP (50 g) was dissolved in 1 L of deionized water until fully dissolved.Then, the sample was centrifuged and applied to a DEAE-cellulose preparative column (12 cm × 43 cm, Cl − type).After a 30 min standing period, the crude polysaccharide was first eluted with 4.5 L of deionized water.The eluate was concentrated, freeze-dried, and yielded the neutral fraction called WRJP-N.Subsequently, the column was further eluted using 3 L of a 0.5 M NaCl solution, resulting in the crude pectin fraction, labeled as WRJP-A.The yields of both fractions were weighed and calculated.
For WRJP-A (1 g), complete dissolution in distilled water was followed by centrifugation and loading onto a DEAE-cellulose column (12 cm × 43 cm).The raw pectin was then successively eluted with deionized water, and 0.2 M, 0.3 M, and 0.5 M NaCl solutions, maintaining a flow rate of 25 mL/min.Analysis of the total carbohydrate and uronic acid content in the eluate led to the collection and labeling of corresponding fractions as WRJP-AH, WRJP-A2, WRJP-A3, and WRJP-A5.Further purification of WRJP-A2 and WRJP-A3 was accomplished using a Sepharose CL-6B column (2.5 cm × 100 cm), where they were eluted with a 0.15 M NaCl solution at a flow rate of 0.5 mL/min.This procedure resulted in two purified pectic polysaccharides, named WRJP-A2a and WRJP-A3b.Figure 10 summarizes the extraction and fractionation method for obtaining pectins from R. japonica.

Chemical Characterization Analysis
A sample of polysaccharide ranging from 2 to 4 mg underwent hydrolysis using a 2 M anhydrous HCl-methanol solution and trifluoroacetic acid, following established protocols [30].The hydrolyzed polysaccharide was then treated with 1-phenyl-3-methyl-5pyrazolone (PMP) at 70 °C for 30 min.The resulting PMP derivatives were purified via chloroform extraction and analyzed using an HPLC system, comprising an SPD-20A UVvisible diode-array detector, and a COSMOSIL 5C18-PAQ column.The mobile phase consisted of a 0.1 mol/L PBS solution (pH 6.9) with 17% acetonitrile (v/v).Set parameters included a column temperature of 35 °C, a detection wavelength of 245 nm, a flow rate of 1 mL/min, and an injection volume of 10 μL.

FT-IR Spectroscopy
Fully dried samples (2 mg) were mixed thoroughly with potassium bromide at a 1:100 (w/w) ratio and analyzed using a Spectrum Two FT-IR spectrometer (PE, USA) within the spectral range of 4000 to 400 cm −1 .

Nuclear Magnetic Resonance Analysis
For the NMR analysis, 20 mg samples were dissolved in 0.5 mL of D2O (99.9% purity).The 1 H NMR, 13 C NMR, 1 H-1 H COSY, 1 H-13 C HSQC, and HMBC spectra were recorded using a Bruker AV600 MHz NMR spectrometer (Germany) at a temperature of 25 °C.

De-Esterification and Enzymatic Hydrolysis
To produce the de-esterified pectins, 500 mg of WRJP-A2a and WRJP-A3b were separately dissolved in 15 mL of distilled water.The solutions were mixed thoroughly and then pre-cooled at 4 °C for 6 h.Subsequently, 15 mL of pre-cooled 0.2 M NaOH solution was slowly added to each sample, and the mixtures were incubated at 4 °C for 4 h with gentle stirring [8].The reaction solutions were neutralized to a pH of 7.0 using 10% glacial acetic acid, desalted on a Sephadex G-10 column, and, finally, freeze-dried to obtain the

Chemical Characterization Analysis
A sample of polysaccharide ranging from 2 to 4 mg underwent hydrolysis using a 2 M anhydrous HCl-methanol solution and trifluoroacetic acid, following established protocols [30].The hydrolyzed polysaccharide was then treated with 1-phenyl-3-methyl-5-pyrazolone (PMP) at 70 • C for 30 min.The resulting PMP derivatives were purified via chloroform extraction and analyzed using an HPLC system, comprising an SPD-20A UV-visible diode-array detector, and a COSMOSIL 5C18-PAQ column.The mobile phase consisted of a 0.1 mol/L PBS solution (pH 6.9) with 17% acetonitrile (v/v).Set parameters included a column temperature of 35 • C, a detection wavelength of 245 nm, a flow rate of 1 mL/min, and an injection volume of 10 µL.

FT-IR Spectroscopy
Fully dried samples (2 mg) were mixed thoroughly with potassium bromide at a 1:100 (w/w) ratio and analyzed using a Spectrum Two FT-IR spectrometer (PE, USA) within the spectral range of 4000 to 400 cm −1 .

Nuclear Magnetic Resonance Analysis
For the NMR analysis, 20 mg samples were dissolved in 0.5 mL of D 2 O (99.9% purity).The 1 H NMR, 13 C NMR, 1 H-1 H COSY, 1 H-13 C HSQC, and HMBC spectra were recorded using a Bruker AV600 MHz NMR spectrometer (Germany) at a temperature of 25 • C.

De-Esterification and Enzymatic Hydrolysis
To produce the de-esterified pectins, 500 mg of WRJP-A2a and WRJP-A3b were separately dissolved in 15 mL of distilled water.The solutions were mixed thoroughly and then pre-cooled at 4 • C for 6 h.Subsequently, 15 mL of pre-cooled 0.2 M NaOH solution was slowly added to each sample, and the mixtures were incubated at 4 • C for 4 h with gentle stirring [8].The reaction solutions were neutralized to a pH of 7.0 using 10% glacial acetic acid, desalted on a Sephadex G-10 column, and, finally, freeze-dried to obtain the desired de-esterified pectins (WRJP-A2a-D and WRJP-A3b-D).
WRJP-A2a-D and WRJP-A3b-D were dissolved in a 50 mM acetic acid-ammonium acetate solution adjusted to pH 5.0, achieving a concentration of 1 mg/mL.In the same solution, 50 µL of endo-polygalacturonase M2 (EC 3.2.1.15)was added, and the mixture was incubated at 40 • C for 24 h.Following this, the reaction solution underwent heating in a boiling water bath for 15 min to deactivate the pectinase.Enzymatic hydrolysates were separated using a Sephadex G-75 column (2.6 cm × 100 cm) and eluted with 0.15 M NaCl at a flow rate of 0.4 mL/min.The corresponding eluent fractions were collected, desalted through a Sephadex G-10 column, and freeze-dried.Three subfractions each were obtained from WRJP-A2a and WRJP-A3b, designated as WRJP-A2a-D-E1 to E3 and WRJP-A3b-D-E1 to E3, respectively.

DPPH Radical-Scavenging Activity
The pectin fractions' scavenging ability towards the DPPH radical was assessed using previously established methods [31].
In this procedure, 500 µL of pectin solution with varying concentrations (0.5, 1, 2, 5, and 10 mg/mL) was mixed with 2 mL of 0.5 mM DPPH solution.The mixture was then incubated in darkness for 30 min, followed by absorbance measurement at 517 nm.L-ascorbic acid was used as a positive control for comparison, while ultrapure water and an equal volume of anhydrous methanol (in place of the DPPH solution) served as blank controls.The DPPH-scavenging activity of the fractions was determined using the provided formula, as follows: A sample : This represents the absorbance value recorded for the sample solution.
A control : This represents the absorbance value recorded for the background solution, which was prepared using anhydrous methanol instead of the DPPH solution.
A blank : This represents the absorbance value recorded for the blank control.

ABTS Radical-Scavenging Activity
The scavenging capability of the pectin fractions towards ABTS radicals was evaluated using a previously established method [32].Freshly prepared daily, the ABTS working solution was used.To assess the ABTS radical-scavenging ability of the fractions, 400 µL of the sample solution at various concentrations (0.5, 1, 2, 5, and 10 mg/mL) was thoroughly mixed with 400 µL of the ABTS working solution in a reaction tube.The reaction was carried out in a dark environment at 25 • C for 30 min.The absorbance was then recorded at 732 nm.As a control, an equal volume of ultrapure water was used instead of the sample solutions.The ABTS radical-scavenging activity of the fractions was determined using the provided formula, as follows: A sample : This represents the absorbance value recorded for the sample solution.
A control : This represents the absorbance value recorded for the background solution, which was prepared using anhydrous methanol instead of the DPPH solution.
A blank : This represents the absorbance value recorded for the blank control.

Figure 3 .
Figure 3. 1D NMR spectra of WRJP-A2a (A) 1 H spectrum and (B) 13 C spectrum (A-I labeled in these spectra represent the residues corresponding to Table2).

Figure 3 .
Figure 3. 1D NMR spectra of WRJP-A2a (A) 1 H spectrum and (B) 13 C spectrum (A-I labeled in these spectra represent the residues corresponding to Table2).

Figure 5 .
Figure 5. 1D NMR spectra of WRJP-A3b (A) 1 H spectrum and (B) 13 C spectrum (A-I labeled in these spectra represent the residues corresponding to Table3).

Figure 5 .
Figure 5. 1D NMR spectra of WRJP-A3b (A) 1 H spectrum and (B) 13 C spectrum (A-I labeled in these spectra represent the residues corresponding to Table3).

Figure 8 .
Figure 8. HPGPC elution profiles of the two pectins and their de-esterified enzymatic hydrolysates.

Figure 8 .
Figure 8. HPGPC elution profiles of the two pectins and their de-esterified enzymatic hydrolysates.

Table 1 .
Yield, molecular weight, and monosaccharide composition of pectic polysaccharides extracted from Rohdea japonica.

Table 2 .
1H and 13 C NMR chemical shift assignments of the residues in WRJP-A2a.

Table 3 .
1H and 13 C NMR chemical shift assignments of the residues in WRJP-A3b.