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Preventive Nutrition and Food Science logoLink to Preventive Nutrition and Food Science
. 2018 Mar 31;23(1):35–45. doi: 10.3746/pnf.2018.23.1.35

Antioxidant Activities of Selected Berries and Their Free, Esterified, and Insoluble-Bound Phenolic Acid Contents

Ji-Sang Kim 1,
PMCID: PMC5894784  PMID: 29662846

Abstract

To explore the potential of berries as natural sources of bioactive compounds, the quantities of free, esterified, and insoluble-bound phenolic acids in a number of berries were determined. In addition, the antioxidant activities of the berries were determined using 2,2-diphenyl-1-picrylhydrazyl radical scavenging activity, ferric reducing antioxidant power, and Trolox equivalent antioxidant capacity assays, in addition to determination of their metal ion chelating activities. Furthermore, several phenolic compounds were detected using high-performance liquid chromatography. Of the 6 tested berries, black chokeberry and blackberry exhibited the strongest antioxidant activities, and the various berry samples were found to contain catechin, caffeic acid, p-coumaric acid, epicatechin, vanillic acid, quercitrin, resveratrol, morin, naringenin, and apigenin. Moreover, the antioxidant activities and total phenolic contents of the fractions containing insoluble-bound phenolic acids were higher than those containing the free and esterified phenolic acids. The results imply that the insoluble-bound fractions of these berries are important natural sources of antioxidants for the preparation of functional food ingredients and preventing diseases associated with oxidative stress.

Keywords: antioxidant activity, alkaline hydrolysis, phenolic profile, berries

INTRODUCTION

Berries, which are particularly important in the Finnish diet, contain many essential functional components, including flavonoids and phenolic acids, which constitute two large and heterogeneous groups of biologically active non-nutrients. Although the contents of flavonoids and phenolic acids vary widely within berries, the contents of phenolic compounds within a single species also vary due to differences in the berry varieties (1) and growth conditions (2).

In a structural context, phenolic compounds are composed of aromatic rings that bear one or more hydroxyl groups, and are generally categorized as phenolic acids, flavonoids, anthocyanins, or tannins (3). Indeed, such phenolic compounds constitute one of the most numerous and ubiquitously distributed groups of plant secondary metabolites, and have been demonstrated to exhibit various beneficial effects in the treatment of a multitude of diseases (4). In the case of the phenolic acids, these compounds exist in three main forms, namely soluble free acids, esterified acids, which are esterified with sugars and low-molecular mass components, and insoluble-bound acids, which are covalently bound to the structural components of cell walls (5,6). In terms of their biological activities, phenolic compounds are considered to contribute to the antioxidant, anti-carcinogenic, anti-inflammatory, and anti-angiogenic properties of berries (79), while also improving the nutritional value of processed foods by preventing the oxidation of lipids and proteins in such products (10). Although a number of studies have examined the nutritional and chemical components of berries in addition to their bioactivities (11,12), few reports on the free, esterified, and insoluble-bound phenolic acid contents of berries and their resulting antioxidant capacities are available. Thus, we herein aim to investigate the contents and antioxidant capacities of these three classes of phenolics following their isolation from selected berries. In addition, the polyphenols present in the free, esterified, and insoluble-bound components were identified and quantified by high-performance liquid chromatography (HPLC).

MATERIALS AND METHODS

Chemicals and reagents

2,2-Diphenyl-1-picrylhydrazyl (DPPH), 6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid (Trolox), gallic acid, p-hydroxybenzoic acid, chlorogenic acid, catechin, caffeic acid, epicatechin, epigallocatechin gallate, p-coumaric acid, ferulic acid, m-coumaric acid, o-coumaric acid, quercitrin, myricetin, resveratrol, morin, quercetin, naringenin, apigenin, vanillic acid, kaempferol, and formic acid were purchased from Sigma Chemical Co. (St. Louis, MO, USA). Aluminum chloride, anhydrous sodium sulfate, Folin-Ciocalteu reagent, methanol, n-hexane, sodium carbonate, and sodium nitrite were obtained from Merck (Darmstadt, Germany). All other chemicals used in the experiments were of analytical grade, and deionized water was used throughout.

Sample preparation

Six berries were studied, namely, raspberry (Rubus idaeus L.), blackcurrant (Ribes nigrum), blackberry (Rubus croceacanthus), cranberry (Vaccinium macrocarpon), black chokeberry (Aronia melanocarpa), and blueberry (Vaccinium spp). The berries were collected from local markets in Gimhae, Korea. After washing with deionized water and immediately freeze-drying, the lyophilized berries were ground into powders using a grinder and stored at −80°C prior to analysis.

Extraction and separation of the phenolic fractions

Free phenolic acid fractions

Extraction of the free phenolic acid fraction was carried out following the method described by Neo et al. (13) with slight modifications. More specifically, a sample of the desired berry powder (1 g) was homogenized using a mixture of aqueous methanol (MeOH) and acetone (both 70%, 1:1, v/v) at room temperature. Each homogenized mixture was then subjected to centrifugation and the supernatants were combined prior to reducing their volumes by evaporation under reduced pressure. The pH of the resulting aqueous suspension was adjusted to pH 2, then extracted with n-hexane to remove lipid contaminants. Subsequently, the free phenolics present in the aqueous phase were extracted using a mixture of diethyl ether/ethyl acetate (EtOAc) (1:1, v/v), and the combined organic extracts were dried over anhydrous Na2SO4, filtered (Whatman No.1 filter paper), and evaporated to dryness under reduced pressure at 45°C, prior to re-dissolving the residue in MeOH (5 mL). The recovered aqueous extract was then combined with the precipitate obtained following the initial centrifugation step for extraction of the esterified phenolic acid components.

Esterified phenolic acid fractions

The esterified phenolic acid fraction was extracted according to the method described by Neo et al. (13) using the aqueous phase obtained following extraction of the free phenolic acid-containing fraction. Initially, this aqueous phase was directly hydrolyzed using 4 N NaOH at room temperature, after which the pH of the hydrolyzed solution was adjusted to pH 2, and n-hexane was added to remove any residual oils. The pH-adjusted extract was then washed using the above described diethyl ether/EtOAc mixture, and the resulting extracts were combined and evaporated to dryness under vacuum at 45°C to give the esterified phenolic compounds, which were re-dissolved in MeOH (5 mL).

Insoluble-bound phenolic acid fractions

The insoluble-bound phenolic acids were extracted from the above residue according to the method described by Neo et al. (13). In this case, the berry samples obtained following extraction with methanol/acetone were hydrolyzed using 4 N NaOH at room temperature. The pH of the solution was then adjusted to pH 2, and the resulting solution subjected to centrifugation. The obtained supernatant was extracted using n-hexane, followed by diethyl ether/EtOAc, prior to evaporation to dryness and re-dissolving in MeOH (5 mL).

Qualitative and quantitative analysis of the phenolic acid fractions

Determination of the total phenolic content (TPC)

The TPC of each extract was colorimetrically estimated using the Folin-Ciocalteu method (14). More specifically, a portion of the Folin-Ciocalteu reagent (0.5 mL) was added to each extract (0.1 mL), after which distilled water was added (7 mL). The resulting mixtures were allowed to stand at room temperature for 5 min prior to the addition of an aqueous 7.5% Na2CO3 solution (1.5 mL). The obtained solutions were then allowed to stand at room temperature for a further 2 h, after which time their absorbances at 765 nm were measured using gallic acid and methanol as the reference standard and blank solutions, respectively. All values were expressed as milligrams of gallic acid equivalents (GAE) per 100 g of sample dry matter.

HPLC analysis of the phenolic fractions

HPLC was used to separate and identify the individual polyphenolic compounds present in the berry samples according to a previously reported method (15) with slight modifications. Each extract was filtered through a 0.45 μm filter prior to injection into the HPLC system (Agilent 1260 Infinity Quaternary liquid chromatograph, Hewlett Packard, Wilmington, NC, USA), which was equipped with a multiple wavelength detector operating at 280 nm. Chromatographic separations were achieved using an Agilent Zorbax RRHD SB-C18 column (2.1 mm i.d.×100 mm, 1.8 μm particle size; Agilent Technologies, Santa Clara, CA, USA). The column temperature and flow rate were set at 30°C and 0.3 mL/min, respectively. Two solvents (solutions A and B) were used to achieve a gradient elution. Solution A was composed of water containing 0.1% formic acid, while solution B was composed of acetonitrile containing 0.1% formic acid, and the following gradient was employed: 0% B (0 min), 5% B (0~3.5 min), 15% B (3.5~7.1 min), 40% B (7.1~25 min), 40% B (25~26 min), 100% B (26~27 min), 100% B (27~29 min), and 0% B (29~35 min). The standards employed for analysis were caffeic acid, chlorogenic acid, ferulic acid, gallic acid, m-coumaric acid, o-coumaric acid, p-coumaric acid, p-hydroxybenzoic acid, vanillic acid, catechin, epicatechin, epigallocatechin gallate, quercitrin, myricetin, resveratrol, morin, quercetin, naringenin, apigenin, and kaempferol.

Evaluation of the antioxidant activities of the phenolic acid fractions

DPPH radical scavenging activity

The radical scavenging activities of the extracts were estimated according to the procedure described by Delgado-Andrade et al. (16). An aliquot of the desired extract (200 μL) was added to a solution of the DPPH radical in MeOH (1 mL, 74 mg/L). It should be noted that a freshly prepared solution of the DPPH radical gave a final absorption of 1.8 AU at 520 nm. The above mixture (i.e., containing the DPPH radical and the sample extract) was then shaken for 30 min, after which time its absorption at 520 nm was measured. Trolox solutions of various concentrations were used for calibration (0.15~1.15 mM), and the results were expressed as mM equivalents of Trolox (TE)/g of sample.

Ferric reducing antioxidant power (FRAP) assay

The ferric reducing antioxidant power of each extract was evaluated according to the Benzie and Strain method (17). A portion of the freshly prepared FRAP reagent warmed to 37°C (900 μL) was mixed with distilled water (90 μL), and either the desired extract or water (as a blank) was added (30 μL). The final dilution of each test sample was 1:34. The FRAP reagent employed herein contains a 10 mM 2,4,6-tripyridyl-S-triazine solution (2.5 mL) prepared in 40 mM aqueous HCl, in addition to 20 mM FeCl3·6H2O (2.5 mL), and 0.3 M acetate buffer (25 mL) at pH 3.6. The absorption of each solution was recorded at 595 nm every 15 s using a Synergy HTX spectrophotometer (Biotech Instruments, Winooski, VT, USA), and the reaction was monitored for 30 min at 37°C. Trolox solutions of various concentrations were used for calibration, and the results were expressed as mM TE/g of sample.

Determination of the total antioxidant capacity using the Trolox equivalent antioxidant capacity (TEAC) assay

The antioxidant capacity of each extract was estimated according to the procedure reported by Re et al. (18). Thus, the 2,2′-azino-bis(3-ethylbenzothiazoline-6-sulphonic acid) radical cation (ABTS) was prepared by reacting a 7 mM ABTS stock solution with a 2.45 mM aqueous solution of K2S2O8. The resulting ABTS solution was diluted using 5 mM phosphate-buffered saline buffer (pH 7.4) to obtain an absorbance of 0.70±0.02 at 730 nm. Following addition of the desired extract (10 μL), the Trolox standard was added to a portion of the diluted ABTS solution (4 mL), and the absorbance was recorded over 20 min (Synergy HTX spectrophotometer, Biotech Instruments). Trolox solutions of various concentrations were used for calibration, and the results were expressed as mM TE/g of sample.

Metal ion chelating activity

The metal ion chelating abilities of the extracts were investigated according to the procedures reported by Wang and Xiong (19) and Dinis et al. (20). To determine the Cu2+ chelating ability, a 2 mM solution of CuSO4 (1 mL) was mixed with pyridine (1 mL) at pH 7.0, and a 0.1% solution of pyrocatechol violet (20 μL) was added. Following the addition of the desired extract (1 mL), the blue color of the CuSO4 solution disappeared, due to dissociation of the Cu2+ ions. After allowing the reaction to proceed for 5 min, the absorbance was recorded at 632 nm (Synergy HTX spectrophotometer). To determine the Fe2+ chelating ability, a portion of each extract (100 μL) was added to a mixture of distilled water (600 μL) and 0.2 mM FeCl2·4H2O (100 μL), and the resulting mixture allowed to stand at room temperature for 30 s. After this time the reaction mixture was added to a 1 mM solution of ferrozine (200 μL), and the absorbance was recorded at 562 nm (Synergy HTX spectrophotometer, Biotech Instruments) after allowing to stand for 10 min at room temperature. The Cu2+ and Fe2+ chelating activities were calculated using the following equation:

Chelating activity (%)=A0-AsA0×100

where A0 and As are the absorbance values of the control and the extract samples, respectively.

Statistical analysis

The experimental data were analyzed by analysis of variance (ANOVA), and the significant differences between the mean values determined from measurements carried out in quintuples (i.e., P<0.05) were obtained by Duncan’s multiple range test using statistical analysis software (SPSS 17.0, IBM Inc., Armonk, NY, USA).

RESULTS AND DISCUSSION

Total phenolic contents of the berry samples

The TPCs of the berry samples and their isolated fractions are presented in Table 1. As indicated, the TPCs of the free, esterified, and insoluble-bound phenolic acids from the various berry samples were within the range of 86.67~372.33, 130.00~735.00, and 272.67~801.67 mg GAE/100 g of dry weight (DW) samples, respectively. More specifically, the free phenolic acid fraction of black chokeberry had the highest TPC, followed by cranberry, blackberry, blueberry, and blackcurrant, while raspberry had the lowest TPC. For the esterified phenolic acid fraction, the highest TPC was observed for black chokeberry, followed by blackberry, cranberry, blueberry, blackcurrant, and raspberry. In the insoluble-bound phenolic acid fraction, black chokeberry again exhibited the highest TPC, followed by blackberry, cranberry, blueberry, blackcurrant, and raspberry. Upon combination of the obtained values for the three fractions of the different berry samples, the total TPCs ranged from 489.67 to 1,909.33 mg GAE/100 g DW, with black chokeberry, blackberry, and cranberry giving the highest values. In addition, we found that for all samples, the TPCs in the insoluble-bound phenolic acid fractions were significantly (P<0.05) higher than those of the free and esterified phenolic acid fractions, with a contribution of 39.78~55.68%.

Table 1.

The total phenolic contents of the berry samples and their isolated fractions (mg gallic acid equivalents/100 g of sample)

Free Esterified Insoluble-bound Total
Raspberry 86.67±1.53fC 130.00±1.00fB 272.67±0.58fA 489.67±2.52f
Blackcurrant 189.67±0.58eC 227.67±1.53eB 292.33±1.53eA 710.33±2.52e
Blackberry 272.00±1.73cC 476.67±2.08bB 559.00±5.20bA 1,307.33±9.24b
Cranberry 285.00±1.73bC 355.67±2.08cB 492.33±2.31cA 1,133.00±3.00c
Black chokeberry 372.33±2.08aC 735.00±2.65aB 801.67±1.53aA 1,909.33±5.51a
Blueberry 214.67±3.06dC 349.33±2.52dB 372.67±2.52dA 936.67±2.08d
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Data represent the mean value for each sample±standard deviation (n=5).

Different letters within the same row (A–C) and column (a–f) indicate significant differences at P<0.05.

More specifically, the TPCs of the insoluble-bound fractions obtained from the raspberry, blackcurrant, blackberry, cranberry, black chokeberry, and blueberry samples were 55.68, 41.15, 42.76, 43.45, 41.99, and 39.79%, respectively. Interestingly, Acosta-Estrada et al. (5) reported that insoluble-bound phenolic acid constituents were covalently bound to structural components of the cell walls, and that they play important roles in providing chemical and physical barriers, in determining the antioxidant properties of the berries, and in protecting against pathogen invasion by animals, insects, and microorganisms (21). In addition, release of the phenolic compounds was previously reported to be more efficient by alkaline hydrolysis than by acid hydrolysis (22), as alkaline hydrolysis resulted in cleavage of the ester bonds linking the phenolic acids to the polysaccharides present in the cell walls (5).

Identification and quantification of the phenolic acid compounds

The phenolic acid compounds present in the various berry samples were then identified and quantified as outlined in Table 2, with catechin, caffeic acid, p-coumaric acid, epicatechin, vanillic acid, quercitrin, resveratrol, morin, naringenin, and apigenin being present in all berry samples. In the free phenolic acid fraction, the TPC ranged from 2,960.71 to 18,936.78 μg/100 g DW, with the blackberry sample containing the highest content, followed by the blueberry, black chokeberry, cranberry, blackcurrant, and raspberry fractions. In addition, the esterified fraction contained a TPC ranging from 6,910.83 to 32,644.08 μg/100 g DW. In this case, black chokeberry contained the highest TPC, followed by blueberry, raspberry, blackberry, cranberry, and blackcurrant. Furthermore, the TPC of the insoluble-bound phenolic acid fraction ranged from 16,152.67 to 35,497.91 μg/100 g DW, with the raspberry extract containing the highest TPC, followed by the black chokeberry, blueberry, blackberry, blackcurrant, and cranberry extracts. Although the TPC of the esterified fraction obtained from the blueberries was significantly (P<0.05) higher than those of the free and insoluble-bound fractions, a different trend was observed for the other berries, with higher TPCs being detected in their insoluble-bound fractions. More specifically, high catechin contents were found in the free phenolic acid fractions of blueberry (12,072.87 μg/100 g DW), black chokeberry (10,985.48 μg/100 g DW), blackberry (4,150.90 μg/100 g DW), cranberry (1,982.41 μg/100 g DW), and blackcurrant (626.05 μg/100 g DW), while high contents of p-coumaric acid were detected in the free phenolic acid fractions of blackberry (10,491.54 μg/100 g DW), blueberry (2,170.81 μg/100 g DW), and black chokeberry (1,576.64 μg/100 g DW). In addition, high contents of morin were found in the cranberry (1,047.81 μg/100 g DW) and raspberry (407.38 μg/100 g DW) extracts, while in the case of the blackcurrant and cranberry samples, high contents of vanillic acid were detected in the free phenolic fractions (i.e., 1,102.24 and 584.78 μg/100 g DW, respectively). In the case of the esterified fraction, high catechin contents were found in the blueberry (10,615.92 μg/100 g DW), black chokeberry (5,288.70 μg/100 g DW), and blackcurrant (1,565.89 μg/100 g DW) samples, while high caffeic acid contents were detected for the blackberry, blueberry, blackcurrant, and raspberry extracts (i.e., 2,526.80, 1,804.70, 1,546.96, and 766.47 μg/100 g DW). For the insoluble-bound fractions, high catechin contents were found in the blueberry (6,970.62 μg/100 g DW), black chokeberry (4,391.78 μg/100 g DW), blackberry (1,708.61 μg/100 g DW), and blackcurrant (1,216.04 μg/100 g DW) samples, whereas high p-coumaric acid contents were detected in the insoluble-bound fractions of raspberry, blueberry, and blackberry (i.e., 10,597.95, 3,311.30, and 3,254.54 μg/100 g DW, respectively). To date, a number of studies have reported that the polyphenol components present in plants correlated with their respective antioxidant activities (23, 24). Indeed, Intra and Kuo (25) reported that the antioxidant activity of catechin was related to its free radical scavenging and metal chelating activities, which rendered catechin a more potent lipid antioxidant than vitamins C and E. In addition, it should be noted that catechin does not exhibit pro-oxidant activity in physiological achievable concentrations. In terms of its structure, catechin contains two aromatic rings and a dihydropyran heterocyclic moiety bearing a hydroxyl group at the C-3 position (26), which can chelate to metal ions (27). As such, catechin could be considered a powerful antioxidant for the neutralization of free radicals (28). In addition, vanillic acid is a phenolic derivative present in numerous edible plants and fruits, and is also an intermediate in the production of vanillin from ferulic acid (29). Furthermore, morin is a type of flavonoid belonging to the flavonol group, while p-coumaric acid is a hydroxyl derivative of cinnamic acid. Interestingly, this compound exhibits a range of medicinal properties, including antifilarial, anticancer, and antimicrobial activities (30), which can be attributed to its free-radical scavenging ability (31).

Table 2.

The main phenolic compounds and their contents of selected berries (unit: μg/100 g dry weight)

Phenolics Free Esterified Insoluble-bound
Raspberry
 p-Hydroxybenzoic acid ND ND ND
 Gallic acid ND 10.64±0.58B 51.95±3.43A
 Chlorogenic acid ND 18.90±0.25B 701.07±37.55A
 Catechin 107.86±4.32C 657.72±4.68A 189.66±7.09B
 Caffeic acid 139.95±1.05C 766.47±10.05A 636.23±24.01B
 p-Coumaric acid 66.11±1.51C 5,518.41±168.49B 10,597.95±101.55A
 Epicatechin 168.97±2.63C 10,838.60±145.40A 9,561.10±123.49B
 Epigallocatechin gallate ND 250.09±3.64A 186.61±9.27B
 Ferulic acid 467.26±7.87A 5.18±0.43C 66.15±4.29B
 m-Coumaric acid 339.71±3.90C 6,281.16±31.04B 9,369.64±180.92A
 o-Coumaric acid ND ND 48.02±6.01
 Vanillic acid 18.66±0.83C 703.40±31.31A 376.55±26.26B
 Quercitrin 939.21±8.28A 30.93±0.22C 146.99±5.03B
 Myricetin 11.89±0.33B ND 39.15±1.32A
 Resveratrol 237.19±1.63A 53.89±0.06C 72.25±1.34B
 Morin 407.38±2.26B 1,006.23±3.74A 173.46±2.28C
 Quercetin 1.86±0.08C 7.79±0.26B 17.43±1.08A
 Naringenin 14.06±0.30B 9.34±0.28C 38.24±2.46A
 Apigenin 40.59±0.39B 12.65±0.17C 103.88±1.95A
 Kaempferol ND ND 3,121.59±31.77
 Total 2,960.71±21.97C 26,171.39±80.97B 35,497.91±227.42A
Blackcurrant
 p-Hydroxybenzoic acid 575.37±2.17A 495.47±6.69B ND
 Gallic acid 51.13±1.83B 27.74±4.36C 66.98±2.39A
 Chlorogenic acid 382.59±40.76A 37.13±4.04C 173.18±1.04B
 Catechin 626.05±15.14C 1,565.89±10.51A 1,216.04±4.90B
 Caffeic acid 167.01±14.08C 1,546.96±48.97A 774.27±12.39B
 p-Coumaric acid 474.76±21.44A 299.85±14.93B 168.97±15.28C
 Epicatechin 194.24±2.66B 152.97±2.43C 236.56±6.52A
 Epigallocatechin gallate 16.17±1.03C 2,216.32±43.98A 1,269.71±29.88B
 Ferulic acid ND 222.47±2.54B 283.20±13.66A
 m-Coumaric acid ND ND ND
 o-Coumaric acid 29.88±1.48 ND ND
 Vanillic acid 1,102.24±21.19A 14.95±1.50C 696.85±9.63B
 Quercitrin 155.97±2.00A 164.02±8.93A 91.07±7.34B
 Myricetin 20.44±0.95A 3.68±0.48B ND
 Resveratrol 55.59±2.15C 88.22±3.78B 151.87±6.04A
 Morin 11.50±0.95C 45.00±2.76A 24.74±1.47B
 Quercetin ND 2.28±0.21B 3.91±0.16A
 Naringenin 27.66±0.84A 9.31±0.36C 22.98±0.66B
 Apigenin 28.88±1.75B 18.59±1.04C 80.89±2.57A
 Kaempferol ND ND 11,466.97±149.81
 Total 3,919.47±38.51C 6,910.83±31.69B 16,728.16±140.56A
Blackberry
 p-Hydroxybenzoic acid 685.01±2.16 ND ND
 Gallic acid 163.39±3.27A 21.11±2.80B ND
 Chlorogenic acid ND ND 63.24±17.81
 Catechin 4,150.90±183.57A 2,364.52±28.53B 1,708.61±43.24C
 Caffeic acid 1,296.79±54.11C 2,526.80±10.2A 1,587.30±15.06B
 p-Coumaric acid 10,491.54±152.65A 1,560.84±101.78C 3,254.54±102.45B
 Epicatechin 176.51±6.80C 2,418.42±33.17B 5,023.41±55.78A
 Epigallocatechin gallate 226.39±13.44C 2,114.32±12.47A 1,155.83±18.02B
 Ferulic acid 179.18±5.16A 92.94±7.98C 127.75±4.09B
 m-Coumaric acid 363.10±32.54C 7,046.05±334.46A 5,686.20±213.23B
 o-Coumaric acid 191.08±2.22 ND ND
 Vanillic acid 432.90±19.20C 519.66±47.92B 693.35±21.43A
 Quercitrin 129.25±13.30C 868.90±15.50A 307.57±41.50B
 Myricetin 6.62±0.59B 4.33±0.44B 25.07±5.84A
 Resveratrol 228.89±8.16A 104.14±0.41C 181.59±2.68B
 Morin 98.40±0.33B 257.49±2.61A 86.27±7.29C
 Quercetin 8.12±0.94B 3.81±0.26C 24.42±0.50A
 Naringenin 20.63±0.68A 13.05±0.38B 13.59±0.60B
 Apigenin 88.09±1.54A 9.72±0.88C 49.94±5.21B
 Kaempferol ND ND 249.48±14.83
 Total 18,936.78±101.81C 19,926.11±273.06B 20,238.14±272.13A
Cranberry
 p-Hydroxybenzoic acid 435.41±0.06A 415.26±0.21B 413.64±5.47B
 Gallic acid ND 27.03±1.10 ND
 Chlorogenic acid ND 41.95±1.12B 1,134.36±25.22A
 Catechin 1,982.41±5.05A 294.40±14.87C 676.34±20.34B
 Caffeic acid 651.92±9.54B 37.71±20.65B 1,523.64±56.92A
 p-Coumaric acid 94.01±2.99C 228.38±6.42B 1,051.06±54.95A
 Epicatechin 1,343.81±9.28A 26.32±1.90C 1,140.79±9.24B
 Epigallocatechin gallate 373.38±11.62C 4,001.21±54.26B 4,870.57±82.50A
 Ferulic acid 129.23±5.43C 350.46±9.39B 444.71±30.91A
 m-Coumaric acid 110.14±8.30A 24.70±0.96B ND
 o-Coumaric acid 39.66±1.01C 57.96±1.04B 368.49±14.95A
 Vanillic acid 584.78±13.69B 119.20±1.93C 1,626.01±55.84A
 Quercitrin 97.87±0.91B 75.58±1.41C 366.36±11.65A
 Myricetin 113.93±5.39A 7.27±0.84B ND
 Resveratrol 233.78±1.58A 79.29±1.96C 87.10±3.22B
 Morin 1,047.81±15.70A 912.02±9.24B 434.03±10.79C
 Quercetin 5.06±0.17C 24.57±0.15A 22.88±0.50B
 Naringenin 17.25±0.28B 23.01±3.39A 10.11±0.38C
 Apigenin 29.60±0.38A 7.18±0.08C 19.73±1.22B
 Kaempferol ND ND 1,962.86±93.33
 Total 7,290.03±25.27B 7,353.50±112.99B 16,152.67±133.48A
Black chokeberry
 p-Hydroxybenzoic acid 424.40±7.33 ND ND
 Gallic acid 289.27±17.13A 211.19±16.94B ND
 Chlorogenic acid 1,707.39±21.75C 4,896.15±131.98B 13,253.03±579.46A
 Catechin 10,985.48±80.44A 5,288.70±497.19B 4,391.78±339.28C
 Caffeic acid 235.20±4.32C 2,603.96±401.22B 11,818.82±177.50A
 p-Coumaric acid 1,576.64±85.08B 1,718.38±19.09A 796.57±94.40C
 Epicatechin 30.28±6.07C 1,760.75±77.11A 518.93±10.51B
 Epigallocatechin gallate ND 2,348.95±23.43A 1,426.52±23.86B
 Ferulic acid ND 1,212.88±23.81A 539.83±12.67B
 m-Coumaric acid 73.17±4.83 ND ND
 o-Coumaric acid 12.99±0.72B 29.56±4.65A ND
 Vanillic acid 325.76±33.36B 1,152.81±91.05A 21.62±3.09C
 Quercitrin 603.76±15.18B 9,754.80±176.79A 215.68±12.90C
 Myricetin 38.79±0.15B 151.35±3.72A 28.36±1.33C
 Resveratrol 246.32±1.88A 92.23±1.22B 95.13±5.38B
 Morin 177.90±9.91C 1,386.48±5.57A 530.75±27.82B
 Quercetin 5.80±0.55B 1.77±0.10C 14.94±1.69A
 Naringenin 18.28±1.23A 18.82±0.88A 19.51±1.67A
 Apigenin 13.82±0.35B 15.30±0.59B 912.63±17.98A
 Kaempferol ND ND 501.35±29.62
 Total 16,765.25±197.45C 32,644.08±716.22B 34,952.25±477.52A
Blueberry
 p-Hydroxybenzoic acid 454.35±5.38A ND 421.76±0.79B
 Gallic acid ND ND ND
 Chlorogenic acid ND 29.56±1.97B 156.06±1.92A
 Catechin 12,072.87±189.74A 10,615.92±436.88B 6,970.62±109.02C
 Caffeic acid 286.52±19.74C 1,804.70±90.11B 6,680.09±115.81A
 p-Coumaric acid 2,170.81±320.36C 10,598.66±145.29A 3,311.30±78.62B
 Epicatechin 334.77±28.30B 71.19±5.62C 366.69±19.32A
 Epigallocatechin gallate ND 709.56±21.56B 759.16±22.42A
 Ferulic acid 4.42±0.52C 302.70±3.74A 248.16±11.52B
 m-Coumaric acid ND 102.42±12.89 ND
 o-Coumaric acid 458.18±18.26A 122.62±8.67B ND
 Vanillic acid 571.09±31.64C 3,261.67±9.81A 975.37±9.15B
 Quercitrin 344.30±11.18A 111.68±4.28B 112.45±2.28B
 Myricetin 69.87±2.43A 34.62±0.80A 54.48±52.93A
 Resveratrol 147.73±4.35A 98.74±2.99B 148.60±17.82A
 Morin 45.26±1.13C 403.05±40.44B 841.43±2.61A
 Quercetin 50.03±0.31A 28.29±1.95C 31.71±0.83B
 Naringenin 24.62±0.70A 17.02±1.52B 15.93±0.75B
 Apigenin 8.45±0.15C 10.02±0.25B 14.64±1.42A
 Kaempferol ND ND 2,995.57±263.63
 Total 17,043.27±565.13C 28,322.43±489.79A 24,104.01±372.49B
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Data represent the mean value for each sample±standard deviation (n=5).

Different letters (A–C) within a row indicate significant differences at P<0.05 level.

ND, not detected.

DPPH radical scavenging activity

The scavenging activities of the phenolic acids extracted from the various berry samples were then investigated using the DPPH radical scavenging assay. This assay was selected due to the greater stability of the DPPH radical compared to the superoxide and hydroxyl radicals (32). Thus, Table 3 shows the DPPH radical scavenging capacities of the free, esterified, and insoluble-bound phenolic acid fractions obtained from the berry samples, which were in the range of 86.67~156.95, 78.11~183.11, and 97.90~272.75 μmol TE/g DW, respectively. Upon combination of the results obtained for these three fractions, the total radical scavenging activities were calculated to range from 265.58 to 568.80 μmol TE/g DW. Interestingly, for all samples the DPPH radical scavenging activities of the insoluble-bound fractions were significantly (P<0.05) higher than those of the free and the esterified fractions. In addition, black chokeberry exhibited the highest DPPH scavenging activity (i.e., 568.80 μmol TE/g DW), followed by the raspberry, blackberry, cranberry, blueberry, and blackcurrant extracts. Interestingly, Madhujith and Shahidi (33) reported that the DPPH radical scavenging activities of insoluble-bound phenolic acids were higher than of free and esterified phenolic acids. Other studies have also indicated that insoluble-bound phenolics acids exhibit higher antioxidant activities than free phenolics (34,35). It therefore appears that the antioxidant activities of plant extracts are related to the presence of certain individual phenolic compounds and their corresponding structures (36), where the positions and quantities of the hydroxyl groups are likely of particular importance (37). The results obtained herein therefore indicate that the insoluble-bound phenolic acids present in the various berry samples could effectively react with DPPH radicals to convert them into stable products and terminate the radical chain reaction.

Table 3.

The DPPH radical scavenging capacities of the free, esterified, and insoluble-bound phenolic acid fractions obtained from the berry samples (unit: μmol Trolox equivalent/g dry weight)

Free Esterified Insoluble-bound Total
Raspberry 86.67±6.92cC 130.37±1.60bB 272.75±5.22aA 489.79±13.75b
Blackcurrant 67.63±7.28dB 100.04±6.02cA 97.90±4.04dA 265.58±17.34e
Blackberry 156.95±6.68aB 98.33±4.01cC 199.58±4.47bA 454.87±15.16c
Cranberry 93.30±6.13cB 99.67±4.42cB 123.58±5.22cA 316.55±15.77d
Black chokeberry 114.59±6.92bC 183.11±2.02aB 271.10±3.62aA 568.80±12.56a
Blueberry 109.99±6.57bA 78.11±4.84dB 116.14±5.26cA 304.25±16.67d
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Data represent the mean value for each sample±standard deviation (n=5).

Different letters within the same row (A–C) and column (a–e) indicate significant differences at P<0.05.

FRAP assay

Two main mechanisms exist for the scavenging of free radicals by antioxidants, namely hydrogen atom transfer and single electron transfer (38,39). The FRAP assay is a typical electron transfer-based method that measures the reduction of ferric ions (Fe3+) to intensely blue colored ferrous ions (Fe2+) by antioxidants in acidic media. Thus, we determined the FRAP values of the free, esterified, and insoluble-bound phenolic acid fractions from the various berry samples, and the results are outlined in Table 4. In general, the samples exhibiting higher ferric-reducing antioxidant powers also contained the highest TPCs. As shown in Table 4, for the fraction containing the free phenolic acids, the FRAP values varied from 17.27 to 111.63 μmol TE/g DW, with blackberry giving the highest value, followed by the black chokeberry, raspberry, cranberry, blackcurrant, and blueberry samples. In the fraction containing the esterified phenolic compounds, the FRAP values ranged 18.27 to 177.90 μmol TE/g DW. In this case, black chokeberry gave the highest FRAP value, followed by raspberry, blackberry, blackcurrant, cranberry, and blueberry. Furthermore, for the insoluble-bound phenolic acid fraction, the FRAP values ranged from 23.55 to 238.80 μmol TE/g DW, with black chokeberry again exhibiting the highest FRAP value, in this case followed by raspberry, blackberry, blueberry, cranberry, and blackcurrant. With the exception of the blackcurrant sample, the FRAP values of the insoluble-bound phenolic acid fractions were significantly (P<0.05) higher than those of the free and esterified phenolics. Upon combination of the results obtained for the three fractions, the total FRAP values ranged from 65.84 to 449.86 μmol TE/g DW. Similarly, Liyana-Pathirana and Shahidi (40) reported that the contribution of insoluble-bound phenolic acids to the TPC in wheat was significantly higher than those of the free and esterified fractions, with the insoluble-bound phenolics demonstrating a significantly higher antioxidant capacity. The berry samples examined herein that contain significant quantities of insoluble-bound phenolic acids should therefore be considered a good source of phenolics that exhibit numerous potential health benefits.

Table 4.

The ferric reducing antioxidant power of free, esterified, and insoluble-bound phenolic fractions obtained from the berry samples (unit: μmol Trolox equivalent/g dry weight)

Free Esterified Insoluble-bound Total
Raspberry 28.11±5.91bcC 133.97±2.47bB 218.36±2.90bA 380.44±11.29b
Blackcurrant 17.81±1.46dC 27.46±1.50dA 23.55±1.33dB 68.83±4.29d
Blackberry 111.63±7.26aB 63.51±8.13cC 135.35±6.70cA 310.49±22.09c
Cranberry 22.41±3.26cdB 22.87±0.77deB 29.38±1.15dA 74.65±5.17d
Black chokeberry 33.16±4.75bC 177.90±4.67aB 238.80±6.90aA 449.86±16.31a
Blueberry 17.27±2.33dB 18.27±0.97eB 30.30±2.18dA 65.84±5.48d
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Data represent the mean value for each sample±standard deviation (n=5).

Different letters within the same row (A–C) and column (a–e) indicate significant differences at P<0.05.

Determination of the total antioxidant capacity using the TEAC assay

The total antioxidant activities of the free, esterified, and insoluble-bound phenolic acid components isolated from the various berry samples were determined using the TEAC assay, and the results are given in Table 5, where values ranging from 47.10~178.35, 58.15~231.69, and 80.44~243.35 μmol TE/g DW are indicated, respectively. In this case, the black chokeberry samples in the insoluble-bound fraction exhibited the highest TEAC value (243.35 μmol TE/g DW), followed by blackberry, cranberry, raspberry, blueberry, and blackcurrant. In addition, the TEAC values of the raspberry, blackberry, cranberry, and black chokeberry extracts containing the insoluble-bound phenolic acids were significantly (P<0.05) higher than those containing the free and esterified phenolics. However, a different trend was observed for the blackcurrant and blueberry samples, with the fractions containing the esterified and free phenolic acids giving higher TEAC values than that containing the insoluble-bound phenolics. Combination of the results for the three fractions gave total TEAC values ranging from 230.27 to 552.15 μmol TE/g DW, where the black chokeberry sample exhibited the highest total TEAC value, followed by the blackberry, cranberry, raspberry, blueberry, and blackcurrant samples.

Table 5.

The ABTS radical cation scavenging activity of the free, esterified, and insoluble-bound phenolic acid components isolated from the various berry samples (unit: μmol Trolox equivalent/g dry weight)

Free Esterified Insoluble-bound Total
Raspberry 51.48±1.57eC 111.06±1.88cB 158.56±3.13cA 321.10±6.58d
Blackcurrant 47.10±0.96fC 102.73±2.53dA 80.44±1.88eB 230.27±5.36f
Blackberry 178.35±2.20aB 99.19±1.86dC 186.90±2.53bA 464.44±6.60b
Cranberry 88.77±1.91cC 125.23±2.82bB 162.31±1.66cA 376.31±6.38c
Black chokeberry 77.10±1.58dC 231.69±3.75aB 243.35±1.58aA 552.15±6.90a
Blueberry 102.31±2.26bA 58.15±2.20eB 100.44±1.88dA 260.90±6.33e
Open in a new tab

Data represent the mean value for each sample±standard deviation (n=5).

Different letters within the same row (A–C) and column (a–f) indicate significant differences at P<0.05.

However, the total TEAC values of the tested samples did not appear to show any clear relationship with the TPCs. In this case, the TEAC value of a compound represents the concentration of Trolox that exhibits the same antioxidant capacity as the compound or compounds of interest (41). Thus, the TEAC value can be considered to be a stoichiometric number related to a Trolox value of 1. Indeed, Alshikh et al. (39) suggested that the TEAC value was dependent not only on the phenolic concentration but also on the identity of the phenolic compounds and the reaction mechanisms taking place. This suggests that the TPCs may not sufficiently explain the observed antioxidant activities of fruit and plant phenolic extracts, which are mixtures of different compounds exhibiting variable activities.

Metal ion chelating activity

In their higher valence states, metals such as iron, copper, manganese, nickel, and cobalt are known to participate in the direct initiation of lipid oxidation via electron transfer and lipid alkyl radical formation, while lower valence metals can directly initiate lipid oxidation via the formation of reactive oxygen species (ROS) (42). In addition, the chelation of iron can prevent the formation of free radicals in addition to preventing the impairment of vital organ functions in vivo. More specifically, the formation of a complex between the antioxidant and the metal renders the metal ions inactive and so they cannot act as initiators of lipid oxidation (43). Thus, the metal ion chelating activities of the free, esterified, and insoluble-bound phenolic acid fractions from the various berry samples are given in Table 6. In the case of the cupric ion (Cu2+) chelating ability, values of 33.58~54.34, 41.60~54.95, and 42.61~59.23% were obtained for the berry extracts containing the free, esterified, and insoluble-bound phenolics, respectively. Combination of the results for the three different fractions gave total Cu2+ chelating abilities ranging from 135.35 to 160.18%, where the black chokeberry sample exhibited the highest Cu2+ chelating ability. In addition, in the case of ferrous ion (Fe2+) chelating ability, the values obtained for the berry extracts containing free phenolic acids and those released from their esterified and insoluble-bound forms were in the range of 33.25~47.60, 44.21~53.56, and 44.21~55.53%, respectively, with combination of these results giving total Fe2+ chelating abilities of 132.19~145.51%. However, the Cu2+ and Fe2+ chelating abilities of the tested samples showed no clear trend between the free, esterified, and insoluble-bound phenolic acid fractions. Although the phenolic compounds present in these berry samples are the main components responsible for chelation to metal ions, it is also possible that nonphenolic constituents present in the extracts may also participate in this process (44).

Table 6.

The metal ion chelating activity of the free, esterified, and insoluble-bound phenolic acid fractions from the various berry samples (unit: %)

Cu2+ chelating ability Fe2+ chelating ability
Free Esterified Insoluble-bound Total Free Esterified Insoluble-bound Total
Raspberry 54.34±2.19aA 43.40±0.11eB 42.61±0.19fB 140.36±2.48b 37.27±0.41dC 53.56±0.30aA 47.60±0.39bB 138.43±1.10b
Blackcurrant 44.32±1.67cB 46.32±0.10dA 46.64±0.09dA 137.28±1.86c 45.57±0.39bA 44.21±0.40dB 44.89±0.40dAB 134.66±1.18c
Blackberry 49.51±1.21bA 47.68±0.82cB 44.64±0.10eC 141.83±2.13b 45.57±0.39bB 47.35±0.08cA 44.21±0.40dC 137.12±0.86b
Cranberry 33.58±0.50dC 53.36±0.87bA 48.50±0.09bB 135.44±1.45c 47.60±0.39aA 45.11±0.40dB 45.79±0.40cB 138.50±1.18b
Black chokeberry 45.99±0.25cC 54.95±0.14aB 59.23±0.10aA 160.18±0.48a 42.84±0.40cC 47.15±1.06cB 55.53±0.38aA 145.51±1.80a
Blueberry 46.37±0.25cB 41.60±0.11fC 47.38±0.16cA 135.35±0.52c 33.25±0.42eC 52.47±0.75bA 46.47±0.39cB 132.19±1.56d
Open in a new tab

Data represent the mean value for each sample±standard deviation (n=5).

Different letters within the same row (A–C) and column (a–f) indicate significant differences at P<0.05.

Thus, in conclusion, we herein investigated the antioxidant capacities and total phenolic acid contents (free, esterified, and insoluble-bound fractions) of 6 selected berries, in addition to identifying and quantifying a number of phenolic compounds present in the berry samples using HPLC. Interestingly, we found that the contents and antioxidant capacities of the free, esterified, and insoluble-bound phenolic acid components varied considerably. More specifically, the black chokeberry and blackberry samples exhibited superior antioxidant activities to the other berry samples, as determined by a combination of the results obtained from DPPH, FRAP, and TEAC assays, in addition to determination of their metal ion chelating activities.

Furthermore, catechin, caffeic acid, p-coumaric acid, epicatechin, vanillic acid, quercitrin, resveratrol, morin, naringenin, and apigenin were found to be widely abundant in the selected berry samples. Moreover, the antioxidant activities and TPCs of the fractions containing the insoluble-bound phenolics were higher than those of the fractions containing the free and esterified phenolic acids. Our results therefore suggest that the insoluble-bound fractions of the various berries examined herein could be regarded as good sources of natural antioxidants, and so may be suitable for application in the preparation of functional food ingredients and preventing diseases associated with oxidative stress.

ACKNOWLEDGEMENTS

This work was supported by Kyungnam University Foundation Grant, 2013.

Footnotes

AUTHOR DISCLOSURE STATEMENT

The author declares no conflict of interest.

REFERENCES

  • 1.Prior RL, Cao G, Martin A, Sofic E, McEwen J, O’Brien C, Lischner N, Ehlenfeldt M, Kalt W, Krewer G, Mainland CM. Antioxidant capacity as influenced by total phenolic and anthocyanin content, maturity, and variety of Vaccinium species. J Agric Food Chem. 1998;46:2686–2693. doi: 10.1021/jf980145d. [DOI] [Google Scholar]
  • 2.Dixon RA, Paiva NL. Stress-induced phenylpropanoid metabolism. Plant Cell. 1995;7:1085–1097. doi: 10.1105/tpc.7.7.1085. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 3.Masisi K, Beta T, Moghadasian MH. Antioxidant properties of diverse cereal grains: a review on in vitro and in vivo studies. Food Chem. 2016;196:90–97. doi: 10.1016/j.foodchem.2015.09.021. [DOI] [PubMed] [Google Scholar]
  • 4.Soobrattee MA, Neergheen VS, Luximon-Ramma A, Aruoma OI, Bahorun T. Phenolics as potential antioxidant therapeutic agents: mechanism and actions. Mutat Res. 2005;579:200–213. doi: 10.1016/j.mrfmmm.2005.03.023. [DOI] [PubMed] [Google Scholar]
  • 5.Acosta-Estrada BA, Gutiérrez-Uribe JA, Serna-Saldívar SO. Bound phenolics in foods, a review. Food Chem. 2014;152:46–55. doi: 10.1016/j.foodchem.2013.11.093. [DOI] [PubMed] [Google Scholar]
  • 6.Ayoub M, de Camargo AC, Shahidi F. Antioxidants and bioactivities of free, esterified and insoluble-bound phenolics from berry seed meals. Food Chem. 2016;197:221–232. doi: 10.1016/j.foodchem.2015.10.107. [DOI] [PubMed] [Google Scholar]
  • 7.Clifford MN. Anthocyanins-nature, occurrence and dietary burden. J Sci Food Agric. 2000;80:1063–1072. doi: 10.1002/(SICI)1097-0010(20000515)80:7&#x0003c;1063::AID-JSFA605&#x0003e;3.0.CO;2-Q. [DOI] [Google Scholar]
  • 8.Kong JM, Chia LS, Goh NK, Chia TF, Brouillard R. Analysis and biological activities of anthocyanins. Phytochemistry. 2003;64:923–933. doi: 10.1016/S0031-9422(03)00438-2. [DOI] [PubMed] [Google Scholar]
  • 9.Rossi A, Serraino I, Dugo P, Di Paola R, Mondello L, Genovese T, Morabito D, Dugo G, Sautebin L, Caputi AP, Cuzzocrea S. Protective effects of anthocyanins from blackberry in a rat model of acute lung inflammation. Free Radic Res. 2003;37:891–900. doi: 10.1080/1071576031000112690. [DOI] [PubMed] [Google Scholar]
  • 10.Viljanen K, Kivikari R, Heinonen M. Protein-lipid interactions during liposome oxidation with added anthocyanin and other phenolic compounds. J Agric Food Chem. 2004;52:1104–1111. doi: 10.1021/jf034785e. [DOI] [PubMed] [Google Scholar]
  • 11.de Souza VR, Pereira PA, da Silva TL, de Oliveira Lima LC, Pio R, Queiroz F. Determination of the bioactive compounds, antioxidant activity and chemical composition of Brazilian blackberry, red raspberry, strawberry, blueberry and sweet cherry fruits. Food Chem. 2014;156:362–368. doi: 10.1016/j.foodchem.2014.01.125. [DOI] [PubMed] [Google Scholar]
  • 12.Namiesnik J, Vearasilp K, Nemirovski A, Leontowicz H, Leontowicz M, Pasko P, Martinez-Ayala AL, González-Aguilar GA, Suhaj M, Gorinstein S. In vitro studies on the relationship between the antioxidant activities of some berry extracts and their binding properties to serum albumin. Appl Biochem Biotechnol. 2014;172:2849–2865. doi: 10.1007/s12010-013-0712-2. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 13.Neo YP, Ariffin A, Tan CP, Tan YA. Determination of oil palm fruit phenolic compounds and their antioxidant activities using spectrophotometric methods. Int J Food Sci Technol. 2008;43:1832–1837. doi: 10.1111/j.1365-2621.2008.01717.x. [DOI] [Google Scholar]
  • 14.Singleton VL, Rossi JA. Colorimetry of total phenolics with phosphomolybdic-phosphotungstic acid reagents. Am J Enol Vitic. 1965;16:144–158. [Google Scholar]
  • 15.Mattila P, Kumpulainen J. Determination of free and total phenolic acids in plant-derived foods by HPLC with diode-array detection. J Agric Food Chem. 2002;50:3660–3667. doi: 10.1021/jf020028p. [DOI] [PubMed] [Google Scholar]
  • 16.Delgado-Andrade C, Seiquer I, Navarro MP. Bioavailability of iron from a heat treated glucose-lysine model food system: assays in rats and in Caco-2 cells. J Sci Food Agric. 2004;84:1507–1513. doi: 10.1002/jsfa.1839. [DOI] [Google Scholar]
  • 17.Benzie IF, Strain JJ. The ferric reducing ability of plasma (FRAP) as a measure of “antioxidant power”: the FRAP assay. Anal Biochem. 1996;239:70–76. doi: 10.1006/abio.1996.0292. [DOI] [PubMed] [Google Scholar]
  • 18.Re R, Pellegrini N, Proteggente A, Pannala A, Yang M, Rice-Evans C. Antioxidant activity applying an improved ABTS radical cation decolorization assay. Free Radic Biol Med. 1999;26:1231–1237. doi: 10.1016/S0891-5849(98)00315-3. [DOI] [PubMed] [Google Scholar]
  • 19.Wang LL, Xiong YL. Inhibition of lipid oxidation in cooked beef patties by hydrolyzed potato protein is related to its reducing and radical scavenging ability. J Agric Food Chem. 2005;53:9186–9192. doi: 10.1021/jf051213g. [DOI] [PubMed] [Google Scholar]
  • 20.Dinis TC, Maderia VM, Almeida LM. Action of phenolic derivatives (acetaminophen, salicylate, and 5-aminosalicylate) as inhibitors of membrane lipid peroxidation and as peroxyl radical scavengers. Arch Biochem Biophys. 1994;315:161–169. doi: 10.1006/abbi.1994.1485. [DOI] [PubMed] [Google Scholar]
  • 21.Sancho AI, Bartolomé B, Gómez-Cordovés C, Williamson G, Faulds CB. Release of ferulic acid from cereal residues by barley enzymatic extracts. J Cereal Sci. 2001;34:173–179. doi: 10.1006/jcrs.2001.0386. [DOI] [Google Scholar]
  • 22.Kim KH, Tsao R, Yang R, Cui SW. Phenolic acid profiles and antioxidant activities of wheat bran extracts and the effect of hydrolysis conditions. Food Chem. 2006;95:466–473. doi: 10.1016/j.foodchem.2005.01.032. [DOI] [Google Scholar]
  • 23.Lizcano LJ, Bakkali F, Ruiz-Larrea MB, Ruiz-Sanz JI. Antioxidant activity and polyphenol content of aqueous extracts from Colombian Amazonian plants with medicinal use. Food Chem. 2010;119:1566–1570. doi: 10.1016/j.foodchem.2009.09.043. [DOI] [Google Scholar]
  • 24.Wu CR, Lin WH, Hseu YC, Lien JC, Lin YT, Kuo TP, Ching H. Evaluation of the antioxidant activity of five endemic Ligustrum species leaves from Taiwan flora in vitro. Food Chem. 2011;127:564–571. doi: 10.1016/j.foodchem.2011.01.041. [DOI] [PubMed] [Google Scholar]
  • 25.Intra J, Kuo SM. Physiological levels of tea catechins increase cellular lipid antioxidant activity of vitamin C and vitamin E in human intestinal Caco-2 cells. Chem Biol Interact. 2007;169:91–99. doi: 10.1016/j.cbi.2007.05.007. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 26.Braicu C, Ladomery MR, Chedea VS, Irimie A, Berindan-Neagoe I. The relationship between the structure and biological actions of green tea catechins. Food Chem. 2013;141:3282–3289. doi: 10.1016/j.foodchem.2013.05.122. [DOI] [PubMed] [Google Scholar]
  • 27.Zhang HY, Ge N, Zhang ZY. Theoretical elucidation of activity differences of five phenolic antioxidants. Zhongguo Yao Li Xue Bao. 1999;20:363–366. [PubMed] [Google Scholar]
  • 28.Zheng LT, Ryu GM, Kwon BM, Lee WH, Suk K. Anti-inflammatory effects of catechols in lipopolysaccharide-stimulated microglia cells: inhibition of microglial neurotoxicity. Eur J Pharmacol. 2008;588:106–113. doi: 10.1016/j.ejphar.2008.04.035. [DOI] [PubMed] [Google Scholar]
  • 29.Civolani C, Barghini P, Roncetti AR, Ruzzi M, Schiesser A. Bioconversion of ferulic acid into vanillic acid by means of a vanillate-negative mutant of Pseudomonas fluorescens strain BF13. Appl Environ Microbiol. 2000;66:2311–2317. doi: 10.1128/AEM.66.6.2311-2317.2000. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 30.Delaquis P, Stanich K, Toivonen P. Effect of pH on the inhibition of Listeria spp. by vanillin and vanillic acid. J Food Prot. 2005;68:1472–1476. doi: 10.4315/0362-028X-68.7.1472. [DOI] [PubMed] [Google Scholar]
  • 31.Prince PSM, Dhanasekar K, Rajakumar S. Preventive effects of vanillic acid on lipids, bax, bcl-2 and myocardial infarct size on isoproterenol-induced myocardial infarcted rats: a biochemical and in vitro study. Cardiovasc Toxicol. 2011;11:58–66. doi: 10.1007/s12012-010-9098-3. [DOI] [PubMed] [Google Scholar]
  • 32.Siriwardhana SSKW, Shahidi F. Antiradical activity of extracts of almond and its by-products. J Am Oil Chem Soc. 2002;79:903–908. doi: 10.1007/s11746-002-0577-4. [DOI] [Google Scholar]
  • 33.Madhujith T, Shahidi F. Antioxidant potential of barley as affected by alkaline hydrolysis and release of insoluble-bound phenolics. Food Chem. 2009;117:615–620. doi: 10.1016/j.foodchem.2009.04.055. [DOI] [Google Scholar]
  • 34.Chandrasekara A, Shahidi F. Determination of antioxidant activity in free and hydrolyzed fractions of millet grains and characterization of their phenolic profiles by HPLCDAD-ESI-MSn. J Funct Foods. 2011;3:144–158. doi: 10.1016/j.jff.2011.03.007. [DOI] [Google Scholar]
  • 35.Govardhan Singh RS, Negi PS, Radha C. Phenolic composition, antioxidant and antimicrobial activities of free and bound phenolic extracts of Moringa oleifera seed flour. J Funct Foods. 2013;5:1883–1891. doi: 10.1016/j.jff.2013.09.009. [DOI] [Google Scholar]
  • 36.Djeridane A, Yousfi M, Nadjemi B, Boutassouna D, Stocker P, Vidal N. Antioxidant activity of some algerian medicinal plants extracts containing phenolic compounds. Food Chem. 2006;97:654–660. doi: 10.1016/j.foodchem.2005.04.028. [DOI] [Google Scholar]
  • 37.Silva FA, Borges F, Guimarães C, Lima JL, Matos C, Reis S. Phenolic acids and derivatives: studies on the relationship among structure, radical scavenging activity, and physicochemical parameters. J Agric Food Chem. 2000;48:2122–2126. doi: 10.1021/jf9913110. [DOI] [PubMed] [Google Scholar]
  • 38.Albishi T, John JA, Al-Khalifa AS, Shahidi F. Phenolic content and antioxidant activities of selected potato varieties and their processing by-products. J Funct Foods. 2013;5:590–600. doi: 10.1016/j.jff.2012.11.019. [DOI] [Google Scholar]
  • 39.Alshikh N, Costa de Camargo A, Shahidi F. Phenolics of selected lentil cultivars: antioxidant activities and inhibition of low-density lipoprotein and DNA damage. J Funct Foods. 2015;18:1022–1038. doi: 10.1016/j.jff.2015.05.018. [DOI] [Google Scholar]
  • 40.Liyana-Pathirana CM, Shahidi F. Importance of insoluble-bound phenolics to antioxidant properties of wheat. J Agric Food Chem. 2006;54:1256–1264. doi: 10.1021/jf052556h. [DOI] [PubMed] [Google Scholar]
  • 41.van den Berg R, Haenen GRMM, van den Berg H, Bast A. Applicability of an improved Trolox equivalent antioxidant capacity (TEAC) assay for evaluation of antioxidant capacity measurements of mixtures. Food Chem. 1999;66:511–517. doi: 10.1016/S0308-8146(99)00089-8. [DOI] [Google Scholar]
  • 42.Kanner J, Harel S, Hazan B. Muscle membranal lipid peroxidation by an “iron redox cycle” system: initiation by oxy radicals and site-specific mechanism. J Agric Food Chem. 1986;34:506–510. doi: 10.1021/jf00069a034. [DOI] [Google Scholar]
  • 43.Shahidi F, Zhong Y. Measurement of antioxidant activity in food and biological systems. In: Shahidi F, Ho CT, editors. Antioxidant Measurement and Applications. American Chemical Society; Washington, DC, USA: 2007. pp. 36–66. [DOI] [Google Scholar]
  • 44.Wettasinghe M, Shahidi F. Iron (II) chelation activity of extracts of borage and evening primrose meals. Food Res Int. 2002;35:65–71. doi: 10.1016/S0963-9969(01)00120-X. [DOI] [Google Scholar]

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