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Article

New Findings in Prunus padus L. Fruits as a Source of Natural Compounds: Characterization of Metabolite Profiles and Preliminary Evaluation of Antioxidant Activity

1
Dipartimento di Scienze Agrarie, Forestali e Alimentari, Università degli Studi di Torino, Largo Braccini 2, 10095 Grugliasco, Italy
2
Département de Biologie et Écologie Végétales, Faculté des Sciences, Université d’Antananarivo, 101 Antananarivo, Madagascar
3
IMRA—Institute Malgaches des Recherches Appliqués, 101 Antananarivo, Madagascar
*
Author to whom correspondence should be addressed.
Molecules 2018, 23(4), 725; https://doi.org/10.3390/molecules23040725
Submission received: 23 February 2018 / Revised: 14 March 2018 / Accepted: 21 March 2018 / Published: 22 March 2018

Abstract

:
European bird cherry (Prunus padus L.) has been known since the Middle Ages for its medical/food use and high health-promoting value. This study aimed to assess the potential of these fruits as a source of bioactive compounds through the characterization of its physicochemical traits, nutraceutical properties, phytochemical composition via HPLC fingerprint, and antioxidant capacity. Fully ripened fruits of Prunus padus L. (Colorata cv) were collected in mid-July 2017 in Chieri, north-western Italy. The TPC (194.22 ± 32.83 mgGAE/100 gFW) and TAC (147.42 ± 0.58 mgC3G/100 gFW) values were obtained from the analyzed extracts. The most important phytochemical class was organic acids (48.62 ± 2.31%), followed by polyphenols (35.34 ± 1.80%), monoterpenes (9.36 ± 0.64%), and vitamin C (6.68 ± 0.22%). In this research the most important flavonols selected as marker were quercitrin (16.37 ± 3.51 mg/100 gFW) and quercetin (11.86 ± 2.36 mg/100 gFW). Data were reported based on fresh weight. Moreover, fresh fruits showed a mean antioxidant activity value of 17.78 ± 0.84 mmol Fe2+·kg−1. Even though the seeds and leaves contain cyanogenic glycosides, this study showed that these fruits could be a natural source of bioactive compounds with high antioxidant properties, due to the contents of organic and phenolic acids, catechins, and a synergetic effect of vitamin C and flavonoids.

1. Introduction

In recent years, a global interest in the traditional use of plants in folk medicinal and food applications was observed, also in many European countries. Unfortunately, information on traditional use of these neglected fruits is scarce, but it is very important for the evaluation of the chemical composition and biological activity (antioxidant capacity) of fruits used in traditional medical and food systems. The correlation between the use of traditional food resources and culinary practices with people’s health is also of great importance. Much of the knowledge has been developed before conventional medications were introduced; however, some studies reported the remaining recipes of traditional remedies based on neglected fruits [1].
European bird cherry (Prunus padus L.) is a boreal-temperate Eurasian species, known since the Middle Ages for its medical/food use and high health-promoting value. The species, which belongs to the Prunus-genus of Rosaceae family, is widely distributed in Europe, in woods or river banks. Wild Prunus-species belong to three subgenera: Prunus (plum-species), Cerasus (cherry-species), and Padus (bird cherry-species). It grows quickly and has strong adaptability [1]. Bird cherry growth power is related to the latitude of growing-site, habitats and age: growth is fastest and most variable at young age and on rich loamy soils overlying limestone [2]. There are three bird cherry subspecies (padus, borealis, petraea) depending on the differences in morphology and distribution area.
Prunus padus belongs to the same genus of several cultivated species as almond, peach and nectarine, plum, sloe and sweet cherry, and it has also been used as graftstock for sour cherry: it can be potentially used as a gene donor for crop improvement. It is an excellent garden ornamental plant: in the past this species was often moved from natural growing-sites into home gardens especially in the areas where the climate is harsh (northern Europe). Bird cherries are easy to cultivate for many reasons: they grow fast and are easily reproduced by seeds or by bending twigs which root easily. Bird cherries can also produce ground shoots and root suckers [3].
European bird cherries are host plants for many herbivores and pathogens and for this reason they were sometimes removed from urban or rural sites. The subspecies borealis is rare and locally threatened in some countries as identified by International Union for Conservation of Nature (IUCN) in the “Red List of Threatened Species” European assessment: therefore, a national level monitoring is required. Germplasm collection, incorporation of targeted monitoring, management of this species in protected areas where it is present, and duplicated ex situ storage are priorities for this species.
This deciduous tree or shrub presents ornamental flowers and edible fruits [4]. P. padus is a honey plant and germplasm resource because the flower has a good nectar [1]. It flourishes in May and June and its stone fruits with dark purple-red skin and light pulp have high ornamental value. The sticky and flavorless fruits ripen from July to September and fall early [5]. Bird cherry is a subglobose or globose-ovoidal drupe, 10–12 mm long and about 10 mm wide with a weight of 2–3 g. Bird cherries seem to produce very active metabolites, as cyanogenic glycosides and specific phenols, for qualitative defenses of valuable immature vegetative parts and seeds against herbivores [4]. Fruits contain up to 5% of sugars, oxalic and citric acids, a lot of tannins, terpenes, and volatile oils. Most of the phytochemical compounds (flavonoids, anthocyanins, phenolic acids, as well as vitamins) present in P. padus fruits, exhibit a proved and high antioxidant capacity [6]: these molecules inhibit the free radical generation and prevent protein, lipids, and also nucleic acids oxidative damage [7].
Bird cherry shows a high chemical variability: flowers, fruits, and leaves are used for relieving cough and invigorating the spleen. People have utilized the bark as pesticide before the industrial products were available [4]. For example, the bark was spread on potato fields and apple orchards for its smell and bitter taste. For several years its cyanogenic glycosides and phenols protected cultivations from rodent and insect attacks. Fruits, bark, powdered leaves, and flowers are still used as anesthetics and disinfectants in Russia and in Scandinavian countries. Moreover, fruits can solve dysentery and digestion problems and stomach-ache (similar to blueberries). People in Eastern and Northern Europe usually dry, crush, and grain the fruits, use them in tart fillings or mix them up with flour for baking. Russians make bird cherry liqueur or thickened juices. The fruits are added to alcoholic beverages or juices and dye the liquids dark red [4].
Recently, traditional food plants have become very attractive to the food industry, prompting their use as replacements for synthetic chemicals and nutraceuticals, but neglected and underutilized natural food resources, as P. padus, are suffering from few attention and research, and their phytochemical potential is not fully exploited. Therefore, investigation of such properties has been of interest mainly for finding new sources for natural antioxidants for food supplements or other food applications: in this sense, European bird cherry is a very important resource for its phytochemical composition, nutritional value, and antioxidant properties. This work aimed at describing bird cherry fruit physicochemical traits and evaluate its potential as a source of natural bioactive compounds through the characterization of its nutraceutical properties and antioxidant capacity. Furthermore, the assessment and quantification of several phytochemicals, selected as health-promoting markers with demonstrated efficacy on the human organism, were performed using high-performance liquid chromatography-diode array detection (HPLC-DAD) to define plant material as potential health-promoting foods.

2. Results and Discussion

2.1. Morphological and Quality Parameters

Table 1 presents the fruit weight and size, total soluble solids (TSS), pH, and titratable acidity (TA) of the analyzed bird cherry genotype. Results showed that the bird cherry fruit is quite spheroidal in shape (11.11 ± 0.08 mm in length and 11.94 ± 0.09 mm in width), with a mean weight value of 2.08 ± 0.02 g and a dark red color.
Quality analysis produced a mean TSS value of 16.17 ± 0.45 Brix, while TA showed a mean value of 245.33 ± 13.32 meq·L−1 with a pH mean value of 2.93 ± 0.03 in accordance with previous studies [4]. In the present research, ripe bird cherry fruits contained significantly high levels of TSS. However, sugar contents might be significantly affected by the process of maturation: indeed, individual and total sugars content increase with maturity due to starch mobilization and translocation from other plant organs as reported by Mikulic-Petkovsek et al. [8] for different fruit species. Moreover, TA and relative pH value determine consumer perceptions of fruit sweetness and sourness. Titratable acidity significantly decreases at full maturity and the lowest levels are generally measured at the last harvest stage: in this study, only one maturation stage (ripe fruits for fresh consumption) were considered in order to better characterize the P. padus fruit quality as health-promoting fresh product. Sugar to acid ratio represents the ratio between total sugars (TSS) and total organic acids (TA) content in fruits: the sugar/acid ratio, important for the taste and flavor of fruits, is often used as an index of sweetness for specific fruits. In this research, bird cherry fruits showed a high sugar to acid ratio value (9.80), due both to high TSS value and to low TA value.

2.2. Nutraceutical Properties

Polyphenols are molecules with demonstrated positive effects against oxidative stress and inhibition of macromolecular oxidation. Moreover, a considerable interest in the potential health-promoting and protective effects of anthocyanin-rich fruits or their derived-products in humans and animals has been recently reported [9]. These molecules are mainly found in the external layers of the skin while flesh tissue contains little or no anthocyanins [10] as in Prunus padus fruits. The evolution of anthocyanins is parallel to sugar accumulation, but no direct relationship has been established yet.
In this research the methods used allowed an accurate and rapid measurement of total anthocyanin content (TAC) and total polyphenolic content (TPC). The TPC, 194.22 ± 32.83 mg of gallic acid equivalents (GAE) on 100 g of fresh weight (FW), and TAC, 147.42 ± 0.58 mg of cyanidin 3-O-glucoside (C3G) on 100 gFW, values obtained from the analyzed extracts (Table 1) were similar to values reported by Kucharska and Oszmianski [5] and Pasko et al. [1]: in these and other similar studies, TAC in P. padus ranged from 190 to 281 mgC3G/100 gFW, while TPC ranged from 60 to 370 mgGAE/100 gFW. Several internal and external factors such as genetic variability as well as many climatic and environmental conditions (light intensity, humidity, temperature, the use of specific agrotechniques, infections or other stress factors) could determine the differences in phenolic and anthocyanin [11].
Antioxidant bioactive compounds may act as reducing agents, hydrogen donators, and singlet oxygen quenchers thanks to their redox properties. In this research, the ferric reducing antioxidant power (FRAP) assay, based on the ability of antioxidants to reduce ferric(III) ions to ferrous(II) ions, was used to evaluate antioxidant capacity of bird cherry fruits. Although the FRAP protocol is an in vitro chemical-based assay without large application in biological systems (antioxidant action is not limited to scavenging free radicals but includes up-regulation of antioxidant and detoxifying enzymes, modulation of redox cell signaling and gene expression), many studies showed that it may highlight the potential of a sample as inhibitor of a target molecule oxidation: this chemical-based method is useful for screening, it is low cost, high throughput and yields an index value (expressed as ferrous iron equivalents) that allows comparing and ordering different samples in order to sense the antioxidant power of natural products [12,13]. In any case, there are many oxidative stress biomarkers to investigate, and therefore, to define the antioxidant and nutraceutical properties of a food as shown by Frijhoff et al. [14]. Fresh fruits showed a mean FRAP value of 17.78 ± 0.84 mmol Fe2+·kg−1 (Table 1), according to other studies [1]. Moreover, FRAP assay showed a FRAP value similar to raspberry, orange, and black mulberry [6,7], but lower than other common berry fruits as blueberry, blackcurrant, and blackberry [15]. Different bioactive compounds contribute to the antioxidant activity of fruit extracts. For example, the antioxidant capacity of some polyphenols, as anthocyanins, is higher than vitamin C activity: antioxidant activity of cyanidin is 4–4.5 times higher than ascorbic acid [10]. In this study, the correlation between TPC/TAC and antioxidant activity was strongly positive, with significant Pearson correlation coefficients (R = 0.938 for TPC and R = 0.998 for TAC).

2.3. Phytochemical Composition

Antioxidant compounds (polyphenols and vitamin C), terpenes, and organic acids may be nutritionally important and play an health-promoting critical role in humans for disease prevention due to their synergistic or additive biological effects (phytocomplex) [15]. The current practice for chemical characterization is carried out measuring the quantity of the main bioactive compounds, called ‘‘markers’’: in this study 28 biologically active compounds were selected as markers for fingerprint analysis because they have been described as important health-effective substances in humans [15].
This study contributed to the knowledge of the phytochemical composition and antioxidant properties of the bird cherry fruits, supporting a larger exploitation of this fruit tree-species. In particular, these fruits could be useful for the food industry, as a potential natural source of bioactive compounds with high antioxidant properties, due to their contents of organic and phenolic acids, catechins, flavonoids, and vitamin C.
The chemical fingerprint of P. padus fruits is reported in Table 2 and Table 3 (polyphenolic compounds and other health-promoting agents, respectively). The total bioactive compound content (TBCC) was calculated as the sum of the main molecules selected for their healthy properties and detected in the extracts: results showed a mean TBCC value of 1139.23 ± 19.15 mg/100 gFW.
Synergistic and additive antioxidant effects of bioactive compounds were evaluated via FRAP assay as preliminary test: Pearson’s correlation coefficient (R) between antioxidant activity and the other phytochemical parameters was used to assess the correlation between each bioactive class and total antioxidant activity as reported in Table 4.
A preliminary phytochemical fingerprint of bird cherry fruits was described. 23 bioactive compounds were separated and identified via HPLC-DAD: adding other markers with demonstrated biological activity would be a necessary step for a better identification of the chromatographic pattern in further fingerprint studies together with a mass spectrometry detection of unknown peaks. In particular, polyphenolic compounds detected in these fruits have not yet been fully identified in literature: liquid chromatography coupled to mass/mass spectrometry (LC–MS/MS) is a very effective technique for complex plant extract analysis providing a rapid and accurate identification of phytochemicals, as phenolics [16,17]. Mass/mass spectrometry data of selected and identified polyphenols in P. padus fruits were reported in supplementary materials (Table A1). P. padus fruits showed the following bioactive compound composition: four cinnamic acids (caffeic, chlorogenic, coumaric, and ferulic acids), four flavonols (hyperoside, quercetin, quercitrin, rutin), two benzoic acids (ellagic and gallic acids), two catechins ((+)catechin, (−)epicatechin), two tannins (castalagin, vescalagin), four monoterpenes (limonene, phellandrene, sabinene, γ-terpinene), three organic acids (citric, oxalic, and quinic acids), and vitamin C (expressed as the sum of ascorbic and dehydroascorbic acids). Isoquercitrin, terpinolene, malic acid, succinic acid, and tartaric acid were not detected, in agreement with P. padus fruit phytochemical fingerprints reported in similar studies [1,5].
The single contribution of each class to total fruit phytocomplex was evaluated grouping the identified health-promoting molecules into bioactive classes. The most important class was organic acids (48.62 ± 2.31%), followed by polyphenols (35.34 ± 1.80%) as the sum of anthocyanins, phenolic acids, flavonols, catechins and tannins, monoterpenes (9.36 ± 0.64 5%), and vitamin C (6. 68 ± 0.22%) (mean values were considered).
Therefore, organic acids represented the first component of the P. padus fruit fingerprint (553.88 ± 51.27 mg/100 gFW) as already reported by Pasko et al. [1]. These compounds, in particular citric acid (217.24 ± 14.95 mg/100 gFW) and quinic acid (324.48 ± 57.21 mg/100 gFW), are mainly used to determine fruit maturity stage because they affect some fruit quality properties (e.g., stability, color, and flavor) indicating the spoilage of fruit products [8], but they are also antioxidants with multi-purpose uses in pharmacology as reported by Eyduran et al. [18]. These molecules are also used as chemical markers to identify adulteration in fruit juices and considered as food acidifiers by food industry.
Moreover, results showed that bird cherry fruits could be a good source of phenolic constituents and deserved special attention focused on studying their phytochemical profile as reported in other studies on different genotypes [1]: the most important polyphenolic classes (Figure 1) were anthocyanins (147.42 ± 0.58 mg/100 gFW) > catechins (82.09 ± 19.58 mg/100 gFW) > tannins (80.61 ± 14.61 mg/100 gFW) > cinnamic acids (39.29 ± 3.59 mg/100 gFW) > flavonols (38.29 ± 6.43 mg/100 gFW) > benzoic acids (14.94 ± 2.05 mg/100 gFW). In this study, the correlation between polyphenolic class and antioxidant activity was positive, with a significant Pearson correlation coefficient (R = 0.682). HPLC fingerprint of identified polyphenols in P. padus fruits was reported in Figure 2. For many years biological protective effects of polyphenols have been often ascribed mainly to their antioxidant activity [19]: however, more complex actions are now being considered [20]. Plants containing flavonoids are often used to treat diabetes in several natural medicines; these compounds show glucose-lowering effects repressing hepatic glucose production in animals [21]. Flavonoids are polyphenolic compounds comprising 15 carbons with two aromatic rings connected by a three-carbon bridge and they occur widely throughout the plant kingdom with the exception of fungi and algae. In particular, flavonols show the potential to quench active oxygen species and inhibit in vitro oxidation of low-density lipoproteins reducing thrombotic tendency. Flavonols may inhibit cyclooxygenase modulating arachidonic acid metabolism and attenuating inflammation. Many natural flavonoids have also shown anti-carcinogenic activity in several animal models. In addition, they may interact with carcinogens in the gastrointestinal tract reducing their adsorption [22]. In the flavonoid group, flavonols may exert critical beneficial features related to human health. In this research the most important flavonols selected as marker were quercitrin (16.37 ± 3.51 mg/100 gFW) and quercetin (11.86 ± 2.36 mg/100 gFW), followed by hyperoside (7.38 ± 0.41 mg/100 gFW) and rutin (2.67 ± 1.02 mg/100 gFW), according to previous studies [1]. Moreover, the presence of cinnamic acids, in particular chlorogenic acid (10.48 ± 0.28 mg/100 gFW), may be important when fruits are processed, as these compounds are considered a preferential substrate for the catecholase activity of polyphenol oxidase [23]. Cinnamic acids, as caffeic, ferulic and coumaric acids, could also influence the oxidation and color development processes occurring during technological processing [24]. As previously discussed, anthocyanins (147.42 ± 0.58 mg/100 gFW) are of prominent importance in P. padus fruits for two reasons: they constitute an important part of the quality traits, because their levels directly pertain to the fruit coloration, and, on the other hand, they have been claimed to possess several biological properties and an high potential nutraceutical value [25]. Ellagic (11.41 ± 1.25 mg/100 gFW) and gallic acids (3.54 ± 0.81 mg/100 gFW) were also detected in P. padus extracts: these molecules are very important in human nutrition and are related to many biological properties, including, anticancer, anti-atherosclerotic, anti-inflammatory, antihepatotoxic, and anti-HIV replication activities [26]. The presence of tannins in adequate amounts (80.61 ± 14.61 mg/100 gFW) in bird cherry extracts are advantageous as they are able to very effectively quench free radicals [27]. The identification of (+)catechin (56.66 ± 16.88 mg/100 gFW) and (−)epicatechin (25.43 ± 3.16 mg/100 gFW) is an important result as they are involved in the inhibition of lipid peroxidation, and inhibition of human cancer cell line proliferation and cyclooxygenase enzymes as similar compounds belonging to the bioactive class of catechins [28]. In Figure A1 spectroscopic information of 4 polyphenolic compounds (chlorogenic acid, quercitrin, ellagic acid, and (+)catechin) with high demonstrated health-promoting properties were reported.
Monoterpenes represent an important fraction of the TBCC of bird cherry fruits (106.65 ± 7.51 mg/100 gFW): the plant terpenoids are potential health-promoting groups because they are a large class of naturally bioactive molecules used extensively for their aromatic qualities together with their antioxidant capacity and anti-inflammatory properties [29]. Monoterpenes are non-nutritive dietary components found in the essential oils of several plants. An high number of these molecules have antibacterial and antitumor activity [30]. In this study, γ-terpinene (65.52 ± 6.25 mg/100 gFW) and limonene (31.40 ± 5.65 mg/100 gFW) were the most abundant monoterpenes: several studies reported their chemopreventive activity against rodent mammary, skin, liver, lung and forestomach cancers [31].
Vitamin C was evaluated as the sum of ascorbic and dehydroascorbic acids (25.20 ± 3.48 mg/100 gFW and 50.87 ± 16.23 mg/100 gFW, respectively) due to their biological activity in human organisms [32]. Bird cherry fruits showed a total vitamin C content (76.07 ± 13.34 mg/100 gFW) similar to the most common fruits, as kiwifruit (74.56 ± 9.84 mg/100 gFW) and orange (71.12 ± 1.96 mg/100 gFW), as previously reported by several pieces of research [15]. For this reason, a portion of 100 g of bird cherry fruits may contribute to the recommended daily intake of vitamin C (60–90 mg) [33]. However, the use of bird cherry fresh fruits as functional food is limited by their slightly more bitter taste if compared to other common fruit species [2].

3. Materials and Methods

3.1. Plant Material, Harvesting Site and Pedoclimatic Information

Fully ripened fruits (0.5 kg for each biological replication) of a cultivated genotype of Prunus padus L. (Colorata cv) were collected in the in mid-July 2017, in Chieri (45°1′0′′ N, 7°49′0′′ E, at 305 m A.S.L.), Piedmont (north-western Italy), in a germplasm repository of the Department of Agricultural, Forest and Food Sciences, University of Turin (voucher specimens were deposited). Fruits were manually harvested from the plants based on selected qualitative parameters (firmness and total soluble solids), considering also literature and experience of the University researchers. The climate of the area is temperate, with rains in spring and autumn, and average precipitation of approximately 810 mm/year; the soil is loam–clay.
The fruits were selected, having removed those with cuts or those damaged by insects, and then divided into two equal portions. One portion was used to determine their morphological and physico-chemical parameters, on the same day of harvest. The second portion was stored at 4 °C and 95% relative humidity (RH) for one day and then used for phytochemical extraction.

3.2. Solvents and Chemicals

Sodium carbonate, Folin-Ciocalteu phenol reagent, sodium acetate, citric acid, potassium chloride, hydrochloric acid, iron(III) chloride hexahydrate, 2,4,6-tripyridyl-S-triazine (TPTZ), 1,2-phenylenediamine dihydrochloride (OPDA), all polyphenolic (caffeic acid, chlorogenic acid, coumaric acid, ferulic acid, hyperoside, isoquercitrin, quercetin, quercitrin, rutin, ellagic acid, gallic acid, (+)catechin, (−)epicatechin, castalagin, and vescalagin) and terpenic standards (limonene, phellandrene, sabinene, γ-terpinene, and terpinolene), potassium dihydrogen phosphate, phosphoric acid and HPLC-grade methanol and acetonitrile were purchased from Sigma-Aldrich (St. Louis, MO, USA). Ethylenediaminetetraacetic acid disodium salt was purchased from AMRESCO (Solon, OH, USA). Sodium fluoride was purchased from Riedel-de Haen (Seelze, Germany). Milli-Q ultrapure water was produced by Sartorius Stedim Biotech mod. Arium (Sartorius, Göttingen, Germany). Cetyltrimethylammonium bromide (cetrimide), ascorbic acid (AA) and dehydroascorbic acid (DHAA) were purchased from Extrasynthése (Genay, France). Acetic acid, ethanol, organic acids (citric acid, malic acid, oxalic acid, quinic acid, succinic acid, and tartaric acid) and HPLC-grade formic acid were purchased from Fluka BioChemika, Buchs, Switzerland.

3.3. Determination of Quality Properties

The fruit width and length were measured using a 0.01 mm sensitive digital caliper (Traceable Digital Caliper-6′′, VWR International, Milano, Italy) and their weight determined to the nearest 0.01 g (Mettler, Greifensee, Switzerland). The fruit without kernel was then homogenized in a blender and centrifuged (4000 rpm, 10 min) to separate solid parts from juice, and pH, total soluble solids (TSS), and titratable acidity (TA) were evaluated.
The TSS was measured with a digital refractometer (Tsingtao Unicom-Optics Instruments, Laixi, China) and results were expressed as °Brix. The TA (meq·L−1) was determined by titration of a mixture of bird cherry juice (10 mL) diluted in Milli-Q water (90 mL) with a 0.2 M NaOH solution using an automatic titrator (Crison, Alella, Spain) to an end-point of pH 8.2. The pH of the fruit juice was directly measured with the aid of a potentiometric pH-meter (Crison, Alella, Spain).

3.4. Bioactive Compound Extraction

3.4.1. Polyphenolic Compounds

For the extraction of bioactive compounds, 10 g of fruit without kernel (three replications) were put into a 50-mL test tube and 25 mL of extraction solution (methanol:bi-distilled water, 95:5 v/v, pH adjusted with 1.5 mL of 37% HCl) and were then added to the weighed samples. After 60 min in the dark, the extracts were homogenized with an Ultra-Turrax (IKA-Werkemodel T25, Staufen, Germany) for about 1 min and then centrifuged for 15 min at 3000 rpm in a Centrifuge (ALC Centrifuge model PK 120, Cologno Monzese, Italy). This operation was carried out 3 times. All the supernatants were recovered and transferred to small glass tubes and kept frozen at −20 °C for further analysis.

3.4.2. Organic Acids and Monoterpenes

For the extraction of organic acids and monoterpenes, three replications were considered. Five grams of fruit without kernel were put into a test tube and 25 mL of 95% ethanol solution were then added. After 30 min in the dark, the extracts were homogenized with an Ultra-Turrax (T25, IKA WERKE) for about 1 min and then centrifuged for 10 min at 4000 rpm in an ALC Centrifuge PK 120 (ALC International, Cologno Monzese, Italy). This operation was carried out 2 times. All the supernatants were recovered and transferred to small glass tubes and kept frozen at −20 °C for further analysis.

3.4.3. Vitamin C

A total of 10 g of fruit without kernel (three replications) was put into a 50-mL test tube and 10 mL of extraction solution (0.1 M citric acid, 2 mM EDTA disodium salt and 4 mM sodium fluoride in methanol–water, 5:95 v/v) were then added. The extracts were homogenized with an Ultra-Turrax (IKA-Werke T25) for about 1 min and then centrifuged for 10 min at 4000 rpm at room temperature in an ALC Centrifuge PK 120. The supernatants were recovered and transferred to a 15-mL test tube through filter cloth and then acidified with 4 N HCl to decrease pH solution to a value of 2.2–2.4 pH units. Acidified samples were centrifuged for 5 min at 12,000 rpm at 4 °C with an ALC Multispeed refrigerated centrifuge PK 121R (ALC International, Cologno Monzese, Italy) [34].

3.5. Spectrophotometric Analysis

The total polyphenol content (TPC) was determined using the Folin-Ciocalteu assay [35], reporting results as mg of gallic acid equivalents (GAE) per 100 g of fresh weight (FW). A total of 0.5 g of fruit extract and 30 mL of bi-distilled water was added to 2.5 mL of Folin–Ciocalteu reagent and 10 mL of Na2CO3 15%; after 2 h in the dark, absorbance was 765 nm. The standard calibration curve was plotted using gallic acid at concentrations of 0.02–0.1 mg/mL.
The total anthocyanin content (TAC) was obtained using the pH-differential method [36], and expressed as milligrams of cyanidin 3-O-glucoside (C3G) per 100 gm of fresh weight (mgC3G/100 gFW). A molar absorptivity of 26,900 was used for cyanidin 3-O-glucoside (molecular weight 449.2). Extracts in 0.025 M potassium chloride buffer (pH 1.0) and 0.4 M sodium acetate buffer (pH 4.5) were measured at 510 and 700 nm after 20 min of incubation at 23 °C. Anthocyanins demonstrate maximum absorbance at 515 nm at pH 1.0 and at 700 nm at pH 4.5. The colored oxonium form of anthocyanin predominates at pH 1.0, and the colorless hemiketal form at pH4.5. The pH-differential method is based on the reaction producing oxonium forms.
For the evaluation of antioxidant activity the ferric reducing antioxidant power (FRAP) assay [37] was used and results were expressed as millimoles of ferrous iron (Fe2+) equivalents per kilogram (solid food) of FW. The method is based on the reduction of the ferric (Fe3+) 2,4,6-tris(2-pyridyl)-s-triazine (TPTZ) complex to its ferrous form (Fe2+). The FRAP reagent was prepared daily by mixing a TPTZ solution and a FeCl3·6H2O solution with acetate buffer (0.3 M), and then warmed at 37 °C before using; 30 µL of sample (15 µL of extracted sample and 15 µL of extraction buffer, dilution 1:2) was added to 90 µL of bi-distilled water and 900 µL of FRAP reagent in a 2-mL microtube and then incubated at 37 °C for 30 min in a Shaking Water Bath (G.F.L. Shaking Water Bath mod.1083, Burgwedel, Germany). Absorbance was read at 595 nm. Standard curve was obtained using FeSO4·7H2O (concentration range: 100–1000 mmol/L).

3.6. Chromatographic Analysis

3.6.1. Sample Preparation Protocols for HPLC Analysis

Samples were filtered with circular pre-injection filters (0.45 µm, polytetrafluoroethylene membrane) prior to HPLC-DAD analysis. In the case of vitamin C analysis, a C18 cartridge for solid phase extraction (Sep-Pak® C-18, Waters, Milford, MA, USA) was used to separate the polyphenolic fraction from vitamin C (ascorbic acid–AA plus dehydroascorbic acid–DHAA). Then, o-phenylenediamine (OPDA) solution (18.8 mmol·L−1) was added to each sample for DHAA derivatization into the fluorophore 3-(1,2-dihydroxyethyl)furo(3,4-b)quinoxaline-1-one. After 37 min in the dark, these samples were analyzed using HPLC-DAD [34].

3.6.2. Apparatus and Chromatographic Conditions

An Agilent 1200 High-Performance Liquid Chromatograph coupled to an Agilent UV-Vis diode array detector (Agilent Technologies, Santa Clara, CA, USA) was used for the chromatographic analysis.
Bioactive substances were separated on a Kinetex C18 column (4.6 × 150 mm, 5 μm, Phenomenex, Torrance, CA, USA). Five different chromatographic methods were used to analyze the samples, two for polyphenols and one for terpenic compounds, organic acids, and vitamins, respectively [9]. Several mobile phases were used for compound separation and identification and UV spectra were recorded at different wavelengths, as listed in Table 5.
The chromatographic conditions were set to obtain a phytochemical fingerprint containing compositional information with a good resolution and a reasonable analysis time. Different linear gradients in different slopes were used for optimizing the molecule separation because some compounds were similar in structure with each other in the same chemical class. Formic and phosphoric acid was added for enhancing the resolution and eliminating peak tailing because most of the compounds were also weakly acidic. Selected wavelengths were suitable to achieve more specific peaks as well as a smooth baseline after a full-scan on the chromatogram from 190 to 400 nm.

3.6.3. Identification and Quantification of Bioactive Compounds in the Extracts

External standard calibration method was used for quantitative determinations by plotting the peak area (y) of the compound versus the sample concentration (x): for each analytical standard: three manual injections (20 µL) at each concentration were performed. The approach for accounting for matrix effects was to build a calibration curve using standard samples with known analyte concentration approximating the matrix of the sample as much as possible. The limit of detection (LOD) and the limit of quantification (LOQ) of the used chromatographic methods, defined as the lowest amount of analyte that gives a reproducible peak with a signal to-noise ratio (S/N) of 3 and 10 respectively, were reported in Table 6. All the samples were analyzed in triplicate, and the results were reported as means ± standard deviation (SD) to assess the repeatability of the used methods. Accuracy was checked by spiking samples with a solution containing each bioactive compound in a concentration of 10 mg·mL−1.
In this preliminary study, compounds were identified by the comparison of the retention times (tR) and maximum absorbance values of detected peaks in samples with those obtained by injection of pure standards in the same matrix conditions. Total bioactive compound content (TBCC) was determined as the sum of selected markers having a positive role in human health as reported in the “multi-marker approach” by Mok and Chau [38]. Five polyphenolic classes were considered: benzoic acids, catechins, cinnamic acids, flavonols, and tannins. Monoterpenes, organic acids, and vitamin C (as the sum of ascorbic and dehydroascorbic acids) were also considered to obtain an analytical fingerprint. All the results were expressed as mg/100 g of FW (fresh weight).

3.7. Statistical Analysis

Analysis of variance was performed by one-way ANOVA analysis (SPSS 22.0) followed by Tukey’s HSD post hoc comparison test at p < 0.05 (N = 3). Correlation between antioxidant activity and the other phytochemical parameters was evaluated with Pearson’s coefficient (R) at p < 0.05 (N = 3).

4. Conclusions

The results revealed that European bird cherry fruit is rich in anthocyanins and other health-promoting agents, similarly to berry and other common fruits reported as antioxidant rich sources, and particularly useful as fresh functional foods or fruit-derived products (e.g., juices, fruit drinks, and wines). It is worth emphasizing that bioactive compounds from bird cherry are not only important components for cheap natural food suitable for consumption, but they could also be valuable substances for pharmaceutical products due to their antioxidative potential. For these reasons, the determination of the natural antioxidant compounds from P. padus fruits may help develop at least a potential template for functional food candidates for antioxidant therapy.
Additional research should be carried out to improve knowledge regarding the health benefits, antioxidant activity, and phytochemical profile of P. padus. Specific cultivars should be harvested and included in food products and daily nutrition for their high healthy properties as potential functional foods.

Acknowledgments

This research was supported by the University of Turin (Fondo per la Ricerca Locale 2017). The authors thank Mauro Caviglione and Marco D’Oria for the field activities (plant management and fruit collection) in the germplasm repository of the Department of Agricultural, Forest and Food Sciences, University of Turin.

Author Contributions

Dario Donno and Gabriele L. Beccaro conceived and designed the experiments; Dario Donno performed the chemical experiments and instrumental HPLC analysis; Maria Gabriella Mellano and Marta De Biaggi contributed to statistical data analysis; Isidoro Riondato proceeded to collect plant material and performed quality analysis; Dario Donno and Ernest N. Rakotoniaina statistically analyzed the data; Dario Donno wrote the paper. All authors have read and approved the final manuscript.

Conflicts of Interest

The authors declare no conflict of interest.

Appendix A

Table A1. Mass/mass spectrometry data of the polyphenolic compounds detected in bird cherry fruits.
Table A1. Mass/mass spectrometry data of the polyphenolic compounds detected in bird cherry fruits.
ClassCompoundIonization Mode aIonization Type bParent Ion c MS2 Ions d,eCollision Energy f
(eV)
(m/z)
Cinnamic acidscaffeic acidpositiveESI181.1689, 11730
chlorogenic acidpositiveESI355.31163, 164, 33710
coumaric acidpositiveESI165.16147, 119, 915–60 (ramp)
ferulic acidpositiveESI195.18195, 177, 14530
FlavonolshyperosidepositiveESI465.38303, 30430
isoquercitrinpositiveESI465.38303, 304, 12730
quercetinpositiveESI303.26303, 304, 25735
quercitrinpositiveESI435.35303, 8530
rutinpositiveESI611.52303, 304, 46530
Benzoic acidsellagic acidnegativeESI301.19229, 257, 18430
gallic acidnegativeESI169.1279, 51, 6750
Catechins(+)catechinpositiveESI291.27139, 123, 1475–60 (ramp)
(−)epicatechinpositiveESI291.27139, 123, 16535
TanninscastalaginnegativeESI933.63301, 631, 91550
vescalaginnegativeESI933.63301, 613, 91550
a Mass spectra were acquired operating in both positive [M − H]+ and negative [M − H] ionization modes (Quadrupole time-of-flight mass spectrometer—QTOF); b ESI source was chosen instead of APCI (Atmospheric Pressure Chemical Ionization) and APPI (Atmospheric Pressure Photoionization) sources as the phenolic compounds were small and relatively polar molecules; c Parent ion (m/z): molecular ions of the standard compounds (mass to charge ratio); d MS2: fragments for the related molecular ions. Tandem mass spectrometry was used due to its fragmented ion stability; e Most intense signal/s in MS/MS spectra is/are highlighted in bold; f Collision energy (CE) refers to related collision energies of the fragment ions.
Figure A1. Chemical structure and spectroscopic information of 4 polyphenolic compounds selected for their high health-promoting properties.
Figure A1. Chemical structure and spectroscopic information of 4 polyphenolic compounds selected for their high health-promoting properties.
Molecules 23 00725 g0a1

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Sample Availability: Samples of the compounds are not available from the authors.
Figure 1. Polyphenolic composition in bird cherry fruits. Mean value and standard deviation (SD) of each polyphenolic class is given (N = 3). Different letters for each class indicate the significant differences at p < 0.05. Results are expressed as mg/100 gFW (FW = fresh weight).
Figure 1. Polyphenolic composition in bird cherry fruits. Mean value and standard deviation (SD) of each polyphenolic class is given (N = 3). Different letters for each class indicate the significant differences at p < 0.05. Results are expressed as mg/100 gFW (FW = fresh weight).
Molecules 23 00725 g001
Figure 2. HPLC fingerprint of selected polyphenolic compounds with high health-promoting properties. For peak identification: caffeic acid—1, chlorogenic acid—2, coumaric acid—3, ferulic acid—4, hyperoside—5, isoquercitrin—6, quercetin—7, quercitrin—8, rutin—9, ellagic acid—10, gallic acid—11, (+)catechin—12, (−)epicatechin—13, castalagin—14, and vescalagin—15. Isoquercitrin (6) was searched but not detected in the extracts.
Figure 2. HPLC fingerprint of selected polyphenolic compounds with high health-promoting properties. For peak identification: caffeic acid—1, chlorogenic acid—2, coumaric acid—3, ferulic acid—4, hyperoside—5, isoquercitrin—6, quercetin—7, quercitrin—8, rutin—9, ellagic acid—10, gallic acid—11, (+)catechin—12, (−)epicatechin—13, castalagin—14, and vescalagin—15. Isoquercitrin (6) was searched but not detected in the extracts.
Molecules 23 00725 g002
Table 1. Quality and nutraceutical traits of bird cherry fruits.
Table 1. Quality and nutraceutical traits of bird cherry fruits.
TraitsParametersMean Value ± SD
QualityWeight a2.08 ± 0.02
Width b11.94 ± 0.09
Length c11.11 ± 0.08
Total soluble solids d16.17 ± 0.45
Titratable acidity e245.33 ± 13.32
pH f2.93 ± 0.03
NutraceuticalTotal polyphenolic content g194.22 ± 32.83
Antioxidant activity h17.78 ± 0.84
Total anthocyanin content i147.42 ± 0.58
Mean value and standard deviation (SD) of each sample is given (N = 3). Results were expressed as: a g; b mm; c mm; d Brix; e meq·L−1; f pH-units; g mgGAE/100 gFW; h mmol Fe2+/kg; i mgC3G/100 gFW.
Table 2. Phytochemical fingerprint of the polyphenolic compounds found in bird cherry fruits.
Table 2. Phytochemical fingerprint of the polyphenolic compounds found in bird cherry fruits.
Polyphenolic ClassCompoundMean ValueSD
Cinnamic acidscaffeic acid6.161.35
chlorogenic acid10.480.28
coumaric acid12.203.07
ferulic acid10.453.65
Flavonolshyperoside7.380.41
isoquercitrinn.d./
quercetin11.862.36
quercitrin16.373.51
rutin2.671.02
Benzoic acidsellagic acid11.411.25
gallic acid3.540.81
Catechins(+)catechin56.6616.88
(−)epicatechin25.433.16
Tanninscastalagin53.958.90
vescalagin26.665.97
Mean value and standard deviation (SD) of each sample is given (N = 3). Results are expressed as mg/100 gFW (FW = fresh weight).
Table 3. Phytochemical fingerprint (vitamin C and other health-promoting molecules) of bird cherry fruits.
Table 3. Phytochemical fingerprint (vitamin C and other health-promoting molecules) of bird cherry fruits.
Bioactive ClassCompoundMean ValueSD
Monoterpeneslimonene31.405.65
phellandrene8.512.69
sabinene1.210.18
γ-terpinene65.526.25
terpinolenen.d./
Organic acidscitric acid217.2414.95
malic acidn.d./
oxalic acid12.162.19
quinic acid324.4857.21
succinic acidn.d./
tartaric acidn.d./
Vitamin Cascorbic acid25.203.48
dehydroascorbic acid50.8716.23
Mean value and standard deviation (SD) of each sample is given (N = 3). Results are expressed as mg/100 gFW (FW = fresh weight).
Table 4. Correlation between antioxidant activity and the other phytochemical parameters in analyzed fruits by Pearson’s correlation coefficient (R).
Table 4. Correlation between antioxidant activity and the other phytochemical parameters in analyzed fruits by Pearson’s correlation coefficient (R).
RPearson’s Correlation Coefficient
TPCTACPolyphenolsMonoterpenesOrganic AcidsVitamin C
Antioxidant activity0.9370.9980.6820.8080.4370.361
Correlation was evaluated at p < 0.05 (N = 3).
Table 5. Chromatographic conditions of the used methods.
Table 5. Chromatographic conditions of the used methods.
MethodCompounds of InterestMobile PhaseFlow
(mL min−1)
Wavelength
(nm)
Acinnamic acids, flavonolsA: 10 mM KH2PO4/H3PO41.5330
B: CH3CN
Bbenzoic acids, catechins, tanninsA: H2O/CH3OH/HCOOH (5:95:0.1 v/v/v)0.6280
B: CH3OH/HCOOH (100:0.1 v/v)
CmonoterpenesA: H2O1.0210, 220,
B: CH3CN 235, 250
Dorganic acidsA: 10 mM KH2PO4/H3PO40.6210, 214
B: CH3CN
Evitamin CA: 5 mM C16H33N(CH3)3Br/50 mM KH2PO40.9261, 348
B: CH3OH
Elution conditions: Method A: gradient analysis: 5%B to 21%B in 17 min + 21%B in 3 min (2 min conditioning time); Method B: gradient analysis: 3%B to 85%B in 22 min + 85%B in 1 min (2 min conditioning time); Method C: gradient analysis: 30%B to 56%B in 15 min + 56%B in 2 min (3 min conditioning); Method D: gradient analysis: 5%B to 14%B in 10 min + 14%B in 3 min (2 min conditioning time); Method E: isocratic analysis: ratio of phase A and B: 95:5 in 10 min (5 min conditioning time).
Table 6. Calibration parameters for all the used analytical standards.
Table 6. Calibration parameters for all the used analytical standards.
ClassStandardtR a (min)Calibration Curve EquationR2Calibration Curve Range (mg L−1)Wavelength (nm)LOD b (mg L−1)LOQ c (mg L−1)
Cinnamic acidscaffeic acid4.54y = 59.046x + 200.60.996111–5003300.3051.016
chlorogenic acid3.89y = 13.583x + 760.050.984 0.9403.134
coumaric acid5.74y = 8.9342x + 217.40.997 2.9079.690
ferulic acid7.99y = 3.3963x − 4.95241.000 1.2454.150
Flavonolshyperoside10.89y = 7.1322x − 4.5830.999111–5003303.37211.241
isoquercitrin11.24y = 8.3078x + 26.6210.999 0.2520.840
quercetin17.67y = 3.4095x − 98.3070.998 4.05513.518
quercitrin13.28y = 2.7413x + 5.63670.998 5.45618.187
rutin12.95y = 6.5808x + 30.8310.999 2.9379.790
Benzoic acidsellagic acid18.65y = 29.954x + 184.520.99862.5–2502800.6112.035
gallic acid6.26y = 44.996x + 261.860.999 0.4351.451
Catechins(+)catechin10.31y = 8.9197x + 66.9521.00062.5–2502802.3437.809
(−)epicatechin14.30y = 12.88x − 43.8160.999 0.7632.543
Tanninscastalagin16.35y = 4.236x − 8.5351.00062.5–2502801.0093.363
vescalagin17.25y = 4.939x − 1.2321.000 0.6032.010
Monoterpeneslimonene3.35y = 0.1894x − 5.4200.999125–10002508.65428.847
phellandrene4.85y = 8.783x − 145.30.998 2100.5621.874
sabinene3.65y = 18.14x − 10040.998 2200.0940.314
γ-terpinene5.28y = 0.4886x − 23.020.999 23517.57758.590
terpinolene4.83y = 26.52x + 876.80.999 2200.2410.804
Organic acidscitric acid5.30y = 1.0603x − 22.0921.000167–1000210, 21418.80562.682
malic acid4.03y = 1.415x − 80.2540.996 15.72152.404
oxalic acid7.85y = 6.4502x + 6.15030.998 0.5501.835
quinic acid3.21y = 0.8087x − 38.0210.998 26.10687.021
succinic acid3.46y = 0.9236x − 8.08230.995 7.13523.783
tartaric acid5.69y = 1.8427x + 15.7961.000 8.52028.401
Vitamin Cascorbic acid5.03y = 42.71x + 27.9690.999100–10002610.8362.786
dehydroascorbic acid3.30y = 4.1628x + 140.010.99930–3003481.0953.649
a tR = retention time; b LOD = limit of detection; c LOQ = limit of quantification.

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Donno, D.; Mellano, M.G.; De Biaggi, M.; Riondato, I.; Rakotoniaina, E.N.; Beccaro, G.L. New Findings in Prunus padus L. Fruits as a Source of Natural Compounds: Characterization of Metabolite Profiles and Preliminary Evaluation of Antioxidant Activity. Molecules 2018, 23, 725. https://doi.org/10.3390/molecules23040725

AMA Style

Donno D, Mellano MG, De Biaggi M, Riondato I, Rakotoniaina EN, Beccaro GL. New Findings in Prunus padus L. Fruits as a Source of Natural Compounds: Characterization of Metabolite Profiles and Preliminary Evaluation of Antioxidant Activity. Molecules. 2018; 23(4):725. https://doi.org/10.3390/molecules23040725

Chicago/Turabian Style

Donno, Dario, Maria Gabriella Mellano, Marta De Biaggi, Isidoro Riondato, Ernest Naivonirina Rakotoniaina, and Gabriele Loris Beccaro. 2018. "New Findings in Prunus padus L. Fruits as a Source of Natural Compounds: Characterization of Metabolite Profiles and Preliminary Evaluation of Antioxidant Activity" Molecules 23, no. 4: 725. https://doi.org/10.3390/molecules23040725

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