Natural Product Sciences

The Korean Society of Pharmacognosy (한국생약학회)
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Quantitative Determination of Five Phenolic Peroxynitrite-scavengers in Nine Korean Native Compositae herbs

  • Nugroho, Agung (Department of Agro-industrial Technology, Faculty of Agricuture, Lambung Mangkurat University) ;
  • Lim, Sang-Cheol (Department of Horticulture and Landscape Architecture, Sangji University) ;
  • Karki, Subash (Department of Food Science and Nutrition, Pukyong National University) ;
  • Choi, Jae Sue (Department of Food Science and Nutrition, Pukyong National University) ;
  • Park, Hee-Juhn (Department of Pharmaceutical Engineering, Sangji University)
  • Received : 2015.04.05
  • Accepted : 2015.04.26
  • Published : 2015.09.30
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Abstract

Peroxynitrite (ONOO)-scavenging activities of nine Compositae herbs consisting of three Ixeris, two Youngia, two Cirsium and one of each Lactuca and Taraxacum species were evaluated. The contents of their ONOO scavengers in the extracts were also determined on a HPLC using seven standard compounds, chlorogenic acid (CGA), chicoric acid (CA), luteolin 7-glucoside (luteolin-7-glc), luteolin 7-glucuronide (luteolin-7-glcU), luteolin, linarin and pectolinarin. Five of those compounds exhibited potent ONOO-scavenging activities: IC50, CA (0.76 μM), CGA (1.34 μM), luteolin (0.81 μM), luteolin-7-glc (0.86 μM) and luteolin-7-glcU (3.13 μM). Both CA and luteolin-7-glc were highly contained in I. dentata (19.71 mg/g and 13.58 mg/g, respectively), I. dentata var. albiflora (17.58 mg/g and 23.83 mg/g, respectively) and I. sonchifolia (65.71 mg/g and 6.99 mg/g, respectively). Among the nine herbs, those three Ixeris species had very low IC50 values over the range of 0.48 - 1.74 μg/mL, suggesting that they could be potential therapeutic vegetables, particularly for preventing diabetic complications or obesity, which can be caused by an excess production of ONOO.

Keywords

Introduction

Peroxynitrite (ONOO−), which is formed through the reaction of nitric oxide with a superoxide anion radical, causes severe cytotoxicity, although nitric oxide itself is not cytotoxic. Excess production of ONOO− induces cytotoxicity and neurotoxicity.1 Initiation of lipid peroxidation, direct inhibition of mitochondrial respiratory chain enzymes, inactivation of glyceraldehyde-3-phosphate dehydrogenase, inhibition of membrane Na+/K+ ATPase activity, inactivation of membrane sodium channels, and other oxidative protein modifications contribute to the cytotoxic effect of ONOO−.2 Furthermore, those reactions trigger cellular responses ranging from subtle modulations of cell signaling to overwhelming oxidative injury, committing cells to necrosis or apoptosis. ONOO− generation represents a crucial pathogenic mechanism in conditions such as stroke, myocardial infarction, chronic heart failure, diabetes, circulatory shock, chronic inflammatory diseases, cancer, and neurodegenerative disorders.3

Endothelial dysfunction induced by ONOO− in obesity and diabetic diseases can result in cardiovascular diseases. Therefore, such a nitrosative stress due to a very reactive ONOO− can cause diabetic complications related to cardiovascular dysfunction.4 Pires et al.5 reported the reduction of body weight by treatment of a peroxynitrite scavenger, Mn (III) tetrakis (4-benzoic acid) porphyrin chloride, in obese mice. In addition, it was found that the reduction of nitrosative stress contributes to the amelioration of neurotoxicity, cytotoxicity, and vascular endothelial toxicity.6

In general, caffeoylquinic acids which are a group of polyphenols exhibit strong ONOO−-scavenging activities.7 We have also studied the natural products with ONOO− scavengers by analyzing caffeoylquinic acids from several plant resources.8,9 Further, it was demonstrated that the antiulcer effect of ellagic acid, a potent ONOO−-scavenger, frequently occurs in nuts and fruits, such as strawberry, raspberry, grape, and blackberry.10 Therefore, development of ONOO− scavengers from plant resources will be beneficial for cardiovascular dysfunctions, such as athero-sclerosis, cardiac failure, and hypertension, as well as for the risk of stroke accompanied by obesity or diabetic complications or for gastrointestinal diseases. ONOO−-scavengers are particularly important because humans lack the enzyme capable of scavenging it.

Koreans have used Ixeris dentata Nakai, Youngia sonchifolia Hance, Lactuca indica L. or others primarily as wild vegetables of Compositae.11 Although these plants are taxonomically or morphologically close to one another, their comparative studies have not been performed on ONOO− scavenging activities. Well-known ONOO− scavengers, chlorogenic acid (CGA)7, luteolin 7-glucoside (luteolin-7-glc), and luteolin12 together with chicoric acid (CA) and luteolin-7-glcU were used for both analysis and assay. We aimed to lead the most potent extract from those nine plant materials which were widely distributed in Korea. For the comparative study, we included both pectolinarin and linarin as the test compounds in this research. It would be meaningful to analyze ONOO− scavengers by HPLC, because plant constituents individually contribute to the genuine ONOO−-scavenging activity. In addition, the analytical data could be conveniently used for biomedical purposes, because pharmacological activities of numerous plant constituents are commonly known. In the present study, we studied the extracts of nine mountainous vegetables (Ixeris dentata Nakai, I. dentata var. albiflora Nakai, I. sonchifolia Hance, Youngia denticulata Kitamura, Y. japonica (L.) DC, Lactuca indica L., T. officinale Weber, C. setidens Nakai, and C. pendulum Fisch. ex DC) widely distributed in Korea from Compoistae in ONOO−-scavenging assay as well as in HPLC analysis.

 

Experimental

Plant materials – Leaves of Ixeris dentate (voucher number, natchem-#42), Ixeris dentata var. albiflora (natchem-#43), Ixeris sonchifolia (syn. Youngia sonchifolia, natchem-#45), Youngia japonica (natchem-#55), Lactuca indica (natchem-#61), Taraxacum officinale (natchem-#62), Cirsium pendulum (natchem-#74), and Cirsium setidens (natchem-#75) were collected in May 2012. Leaves of Youngia denticulata were collected on September 2013, considering its flowering period. All plant materials were collected from a mountain area near Wonju City. The plants were identified by Prof. Dr. Sang-Cheol Lim (Department of Horticulture and Landscape Architecture, Sangji University). Voucher specimens were deposited at the Laboratory of Natural Products Chemistry, Sangji University. The collected plants were separately dried in dark area and crushed for extraction.

Instruments and reagents – An HPLC system consisting of two Prostar 210 pumps, a Protar 325 UV-Vis detector and a Shiseido Capcell PAK C18 column (5 μm, 4.6 mm × 250 mm, Japan) was used for analysis. The HPLC solvents of H2O, MeOH, and CH3CN were purchased from J.T.Baker Co. (Phillisburg, NJ, USA). The reagents used for ONOO−-scavenging assay were diethylenetriaminepentaacetic acid (DTPA) from Sigma Chemical Co. (St. Louis, MO, USA), dihydrorhodamine 123 (DHR 123) from Molecular probes (Eugene, OR, USA) and ONOO− from Cayman Chemicals Co. (Ann Arbor, MI, USA).

Extraction and identification of the compounds – Dried, crushed, and lyophilized plant material (leaf part) (5 g) were soaked in 250 mL of 70% MeOH and extracted under reflux on a heating mantle for 5 h. After cooling, each extract solution was filtered through a filter paper. The extracted solution (2 mL) was filtered again through a disposable syringe filter (0.50 μm, Dismic-25JP Advantec, Japan) prior to the injection into the HPLC system. The extract was evaporated in vacuo using a rotary evaporator and dried on a freeze-dryer in order to obtain the extraction yield. The lyophilized extracts were also used for the ONOO−-scavenging test.

Based on literatures and our experiences on the identification of phenolic compounds in several Compositae plants, seven standard compounds were used to detect the constituents of nine extracts. Three compounds (luteolin-7-glc, luteolin-7-glcU, and pectolinarin) were obtained by isolation (purity ≥ 98% by HPLC) and CGA (Lot No. 104K0722), CA (060M1184V), and luteolin (11K4085) were purchased from Sigma-Aldrich Co. (St. Louis, MO, USA), and linarin from Extrasynthese (France, Lot No. 11011412). The detection of the standards in the extracts was performed by HPLC and TLC. Their chemical structures are presented in Fig. 1.

Fig. 1.Structures of standard compounds used for HPLC analysis.

ONOO−-scavenging assay – The measurement of peroxynitrite-scavenging activity was performed by modifying the method described by Kooy et al.13 This method is based on the measurement of highly fluorescent rhodamine 123 converted from non-fluorescent DHR-123 under the presence of ONOO−. In brief, this assay was based on the method using a rhodamine buffer (pH 7.4, 50 mM sodium phosphate diabasic, 50 mM sodium phosphate monobasic, 90 mM chlorides, 5 mM potassium chloride, 100 μM DTPA). The final concentration of DHR 123 was 5 μM. In this assay, the buffer was preserved in ice bath prior to use, and the samples were dissolved in 10% dimethylsulfoxide. The intensity of the background fluorescence was measured in 0.3N NaOH under the presence or absence of 10 μM ONOO−. Then, the fluorescent intensity was measured from the excitation and emission at 480 nm and 530 nm using a microplate fluorescencereader FL 500 (Bio-Tek Instruments Inc., Winooski, VT, USA). ONOO−-scavenging activities were calculated from the final fluorescent intensity minus the intensity of the background. The positive control was L-penicillamine.

HPLC analytical method – The mobile phase consisted of 0.05% (v/v) trifluoroacetic acid (TFA) in H2O (eluent A) and 0.05% (v/v) TFA in MeOH and CH3CN (60:40, v/v; eluent B). The gradient program was as follows: 15% B to 65% B (35 min), 65% B isocratic (5 min), 65% B to 100% B (2 min), 100% B isocratic (4 min), 100% B to 15% B (3 min), and 15% B isocratic (6 min). The total run time was 55 min at a flow rate of 1 mL/min and at 40 ℃ of column temperature. Chromatograms were recorded during a period of 0 - 40 min. The injection volume for each sample was 20 μL and simultaneous monitoring was performed at 254 nm. UV wavelength 254 nm was more sensitive for the simultaneous detection of caffeoylquinic acid, caffeoyl tartaric acid, and luteolin analogues.

To assess the linearity of the regression equations, standard stock solutions (1000 μg/mL) were prepared by dissolving each standard compound in MeOH. Stock solutions were serially diluted in order to prepare working solutions of 1.56 - 50.0 μg/mL (CGA, luteolin-7-glc, luteolin, linarin, and pectolinarin) and 3.13 - 100.0 μg/mL (CA and luteolin-7-glcU). Calibration curve equations were determined by plotting the peak area (y axis) versus the concentration (x axis), and the liniarities of equations were evaluated by R2 values. LOD (limit-of-detection) and LOQ (limit-of-quantification) were determined by signal-to-noise (S/N) ratios of 3 and 10, respectively.

 

Results and Discussion

Five compounds, CGA, CA, luteolin-7-glc, luteolin-7-glcU, and luteolin, displayed potent activities over the IC50 ranges of 0.23 - 1.45 μg/mL, although two substances, linarin and pectolinarin, had relatively higher IC50 values (Table 1). In particular, the IC50 of CA was the lowest, considering the value of the μM unit. Therefore, those five compounds can be considered as the active components of the tested plant materials.

Table 1.aValue represents mean ± S.D. (n = 2); bUnit of the value in the parenthesis is μM; cPositive control.

After testing the ONOO−-scavenging effects of nine extracts at concentrations of 0.4, 2, 10 and 50 μg/mL, the scavenging percentage and IC50 values were displayed in Table 2. The activities of Ixeris dentata, I. dentata var. albiflora, and I. sonchifolia with a range of IC50 0.48 - 1.74 μg/mL were very potent, whereas those of other plants were relatively weak. Of these, the activity of I. dentata var. albilfora (IC50 0.48 μg/mL) was the strongest. However, the activity of dandelion (T. officinale) was not so strong, although it is a very well-known crude drug in Western countries.14

Table 2.*Value represents mean ± SD (n = 2).

The following four parameters of mobile phase composition, gradient elution, UV wavelength, and column temperature were considered for the optimization of the HPLC method. The eluents, 0.05% TFA in H2O and 0.05% TFA in MeOH-CH3CN (60:40) as solvents A and B, respectively, showed better resolution, and were environment-friendly and economic compared to other solvents. The addition of TFA with a 0.05% concentration in A- and B solvents contributed to sharper peaks on the chromatograms, probably due to the deionization of phenolic substances. Gradient elution included the peaks due to a wide range of polarity within the shortest retention time. The use of a fixed column temperature and flow rate at 40 ℃ and 1.00 mL/min led to good chromatograms. The HPLC chromatograms of the mixed standard sample solution and the seven 70% MeOH extracts were shown in Fig. 2. The 70% MeOH extract was prepared since 70% MeOH solvent produces more powdery extract than 100% MeOH and that the extraction rate of flavonoids is similar between the two solvents.

Fig. 2.HPLC chromatograms of mixed standard compounds and 70% MeOH extracts of the seven Compositae herbs.

In order to determine the contents of the five ONOO− scavengers, experiments on linearity and sensitivity were performed. Regression equations of the compounds were determined as shown in Table 3. Further, linearities were proven from the R2 value of more than 0.9996. Sensitivity was also high from the LOD and LOQ values over the range of 0.07 - 0.89 μg/mL and of 0.22 - 1.44 μg/mL, respectively.

Table 3.Linearities and limits of detection and quantification (LOD - LOQ) of analytes

The contents of CGA, CA, luteolin-7-glc, luteolin-7-glcU, luteolin, linarin, and pectolinarin in nine extracts are shown in Table 4. The sum of these substances was especially high in I. sonchifolia (182.03 mg/g). In the extracts of C. setidens and C. pendulum, CGA, CA, luteolin-7-glc, luteolin-7-glcU, and luteolin were observed, but the remaining two compounds (linarin and pectolinarin) were detected. Although, the other plants did not contain linarin and pectolinarin; however, they had CGA, CA, luteolin-7-glc, luteolin-7-glcU, and luteolin. Of the CGA and CA, the former compound was quantitatively lower and the latter one was higher. The levels of CA were particularly high in I. sonchifolia (65.71 mg/g) and T. officinale (36.02 mg/g). Out of these compounds, the contents of luteolin-7-glc and luteolin-7-glcU were high, although the level of luteolin was generally very low (0.24 - 4.80 mg/g). These results suggest that luteolin was present mainly in the glycosidic form.

Table 4.Content of analytes in the extracts

Dandelion is a local name of a famous herb medicine, Taraxacum officinale, in Western countries. The herb of T. officinale has been used to mainly treat hepatic disease in Chinese medicine. This crude drug has been known to have a variety of pharmacological activities, including diuretic, choleretic, anti-inflammatory, anti-oxidative, anticarcinogenic, analgesic, anti-allergic, anti-hyperglycemic, and anti-thrombotic.14 We have also studied several mountainous vegetables mainly belonging to the Korean native Aster species, called chwinamul, on ONOO−-scavenging activities7,8 as well as the contents of phenolic substances.15

Of the nine herbs tested, the three of the plants studied, I. dentata, I. dentata var. albiflora, and I. sonchifolia, exhibited potent ONOO−-scavenging activities in the present study. The activities of these three plants were stronger than those of T. officinale (dandelion). In addition, five compounds, CGA, CA, luteolin-7-glc, luteolin-7-glcU, and luteolin, were shown to be potent ONOO−-scavengers. However, linarin and pectolinarin, exhibited considerably weaker activities.

CA and luteolon-7-glc, were quantitatively abundant in I. dentata and I. dentata var. albiflora. In particular, the content of CA was very high in I. sonchifolia (65.71 mg/g), which can also be considered to be the most significantly active substance. Although the content of phenolic substances in I. sonchifolia was reported, CA was not quantitatively determined.16 In T. officinale, the content of CA was 36.02 mg/g; but the levels of the other compounds were very low. This indicates that CA might be the main substance in T. officinale. Schütz et al.17 has also reported that CA was a main compound in the same plant. However, in C. setidens and C. pendulum, the two substances, linarin and pectolinarin, existed in high proportions, whereas the other five phenolic substances were not detected.

Certain pharmacological activities of CA have been known: apoptosis-inducing activity against preadipocyte cells,18 anti-stress activity,19 and anti-viral activity,20 although its ONOO−-scavenging activity has not been known. Park et al.21 reported potent anti-inflammatory activity due to the synergistic action between CA and luteolin. Luteolin-7-glcU has antigastritis,22 antidepressant,23 and anti-mutagenic activities.24 Further, it possesses inhibitory activities on the protein expression of inducible nitric oxide synthase and cyclooxygenase in lipopolysaccharide-induced macrophage RAW 264.7 cells.25

Pacher et al.4 suggested that cardiovascular dysfunctions, such as neuropathy, nephropathy, and hypertension, or the risk of stroke of patients with obesity or diabetic complications, are caused from the excess production of ONOO−. Therefore, I. dentata, I dentata var. albiflora, and I. sonchifolia, which were confirmed to be potent ONOO− scavengers through this study, will be beneficial for patients suffering from diabetic cardiovascular dysfunction.

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