Abstract
Inhibition of digestive lipases refers to the suppression of dietary fat absorption and, to some extent, to a strategy against overweight and obesity. In this study, the effect of five commercial black chokeberry juices on pancreatic lipase as a key enzyme relevant to obesity was investigated using as substrates triolein, sunflower oil, and rapeseed oil emulsions as well as 4-methylumbelliferyl oleate. The juices were also analyzed for antioxidant capacity (ABTS·+, DPPH·, FRAP methods), qualitative and quantitative composition of phenolic compounds and nutrients. Significant differences were observed among their chemical compositions and biological activities. Chokeberry juices were rich in proanthocyanidins, followed by the hydroxycinnamic acids, anthocyanins, and flavonols. Their inhibitory activity against pancreatic lipase was related to polyphenol content, that of proanthocyanidins. The results reported herein have shown the influence of proanthocyanidin degree of polymerization on the inhibitory activity, especially in lipid emulsions. In conclusion, this work suggests that chokeberry juice may be a potential source of dietary fat absorption inhibitors, especially if it contains high molecular phenolic compounds.
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Introduction
Black chokeberry (Aronia melanocarpa) fruit is known as a potent source of phenolic compounds, especially anthocyanins and proanthocyanidins [1–4]. Nevertheless, chokeberry berries are rarely consumed directly because of their specific organoleptic properties, such as unpleasant astringent taste and their smell of bitter almonds [5]. So, it is preferable to use them for syrup, juice, jam, liqueur, and wine production. Moreover, processed berries have better flavor and are less bitter than the fresh fruits. One of the valuable products is chokeberry juice because one liter of the juice can contain up to 9 g of polyphenols, and chokeberry juice is one of the richest sources of these natural antioxidants among fruit juices [6].
An interest in chokeberry juices production has increased considerably in recent years, with a growing number of reports on their potential health benefits. Results of in vitro and in vivo studies indicate that chokeberry juice has cardioprotective [7, 8], hepatoprotective [9], and anti-diabetic effects [1] as well as anticancer activity [10]. Recent human studies also showed that Aronia melanocarpa juice may be useful in the treatment of obesity disorders [11]. Black chokeberry constituents may help in reducing dietary fat absorption by inhibiting digestive lipases activity. Pancreatic lipase inhibitory activity of black chokeberry extracts has been shown in in vitro studies using simple, different p-nitrophenyl esters or 4-methylumbelliferyl oleate as substrates [12, 13]. The cited studies have shown anti-lipase activity dependence on the method of lipase activity determination [12] and on type of extraction agent [13].
Despite the data on anti-lipase activity of black chokeberry fruit extracts, there are no studies concerning chokeberry juices. The need for such data still exists due to insufficient intake of unprocessed berries, changes of bioactive compounds during chokeberry juice production, and increasing interest in healthy food consumption. Therefore, the objective of this study was to evaluate the inhibitory activities of five commercial 100 % black chokeberry juices against porcine pancreatic lipase using different in vitro assays. The pancreatic lipase is one of the most widely studied targets for phytochemicals acting as anti-obesity agents because it is responsible for the hydrolysis of 50–70 % of total dietary fats in the intestinal lumen [14]. Because in gastrointestinal tract the substrates for the water-soluble pancreatic lipase are usually lipid droplets embedded in an aqueous medium [15], we decided to use systems with triolein (glycerol trioleate), rapeseed oil, and sunflower oil emulsions in order to better simulate physiological conditions. Porcine pancreatic lipase activity was also determined by the method using 4-methylumbelliferyl oleate (4-MUO) as substrate because of its wide application. Basic chemical composition and qualitative and quantitative phenolic compounds composition as well as antioxidant capacity of juices were also evaluated.
Materials and methods
Materials and reagents
Chokeberry juices (100 % of fruit) of five different brands in glass bottles, rapeseed oil (Kruszwica S.A., Poland), and sunflower oil (PPHU Olmaj, Poland) were purchased from local markets (Łódź, Poland). Juice samples for analysis were obtained after mixing the contents of three bottles. Lipase (EC 3.1.1.3) from porcine pancreas type II, Tris-base, triolein (glycerol trioleate), bile acids from bovine and ovine, 4-methylumbelliferyl oleate (4-MUO), organic acids and sugars standards, sorbitol, quercetin, (+)-catechin, (−)-epicatechin, gallic acid, naringenin, ascorbic acid, 2,2′-azino-bis(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS), 2,2-diphenyl-1-picrylhydrazyl (DPPH), 2,4,6-tris-2-pyridyl-s-triazine (TPTZ), 6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid (Trolox), phloroglucinol, potassium persulfate, dimethyl sulfoxide (DMSO), formic acid, methanol, and acetonitrile were obtained from Sigma-Aldrich (Steinheim, Germany). Cyanidin 3-glucoside, cyanidin 3-galactoside, 5-O-caffeoylquinic acid, p-coumaric acid, protocatechuic acid, quercetin 3-O-glucoside, quercetin 3-O-galactoside, quercetin 3-O-rutinoside, quercetin, isorhamnetin 3-O-galactoside were obtained from Extrasynthese (Lyon, France). Procyanidins B2 and B3, 3-caffeoylquinic acid, and 4-caffeoylquinic acid were purchased from TransMIT (Gießen, Germany), and procyanidin B1 from PhytoLab (Vestenbergsgreuth, Germany). Acetic acid was obtained from J.T. Baker (Łódź, Poland). Sodium hydroxide and sodium carbonate were purchased from Chempur (Piekary Śląskie, Poland). Other reagents were obtained from POCH (Gliwice, Poland). Ultrapure water (Simplicity™ Water Purification System, Millipore, Marlborough, MA, USA) was used to prepare all solutions.
Quality parameters
Total soluble solids, pH, organic acids, and sugars contents were evaluated as quality indexes. The pH values were measured using a pH-meter (CyberScan pH 510, Eutech Instruments, Singapore). The total soluble solids were recorded in a refractometer Abbe 2 WAY (Vanco Industries, Ningbo, China) at 20 °C, with values being expressed as °Brix. Individual sugars (glucose, fructose, sucrose) and sorbitol were determined by HPLC method described by Sójka and Król [16] using Aminex HPX87C column (300 × 7.8 mm) from BioRad (Hercules, California, USA) at 85 °C and the refractive index (RI) detector (Knauer K-2301) with a Knauer integrating system (Berlin, Germany). The mobile phase was water, and the flow rate was 0.5 ml/min. The injection volume was 20 µl. The juice before injection was cleaned on SPE column containing cation exchanger resin Amberlite IR120 and anion exchanger resin Amberlite IRA420 at a volumetric ratio of 1:2. The results were expressed as gram of individual sugar per 1 l of juice. Individual organic acids (citric, malic, oxalic, and tartaric) were analyzed by HPLC method using the HPLC Knauer system (Berlin, Germany) consisted of a UV–Vis detector set at 210 nm and a LiChrospher-100 RP-18 column (250 × 4.6 mm; 5 μm) operated at 25 °C. The isocratic mobile phase consisted of mixture of 0.5 % water solution of diammonium hydrogen phosphate adjusted to pH 2.24 with phosphoric acid and acetonitrile (99.98:0.02, v/v). Samples were eluted at a flow rate of 1 ml/min. The injection volume was 20 µl. The juices were centrifuged at 13,000 rpm for 5 min, and each supernatant was filtered through a 0.20-μm Minisart RC4 filter (Sartorius, Stedim Biotech GmbH, Germany) before injection into the HPLC system. The results were expressed as gram of individual organic acid per 1 l of juice.
Spectrophotometric determination of phenolic compounds
Total phenolics content was determined using Folin–Ciocalteu reagent as we described in our previous work [12]. The absorbance of reaction mixture (juice, Folin–Ciocalteu reagent, sodium carbonate, and water) was read at 760 nm after 20 min incubation at ambient temperature. Total phenolics content was expressed as g of gallic acid equivalents (GAE) per 1 l of juice. Total anthocyanins content was quantified by a pH-differential [6]. Juices were diluted (50–200 times) with two buffer solutions at pH 1 and 4.5, and absorbance was measured at 515 and 700 nm after 1 h incubation at ambient temperature in the dark. The results were expressed as g of cyanidin 3-glucoside equivalents (CGE) per 1 l of juice using a molar extinction of cyanidin 3-glucoside of 26,900 l/mol cm and molar weight of 449.2 g/mol. The content of total proanthocyanidins in juices was determined after acid depolymerization to the corresponding anthocyanidins as described by Rösch et al. [17]. In fact, 0.1 ml of diluted (2–20 times) juice was mixed with 9.9 ml of a solution of concentrated hydrochloric acid in n-butanol (1:9, v/v) and heated for 90 min in a boiling water bath. After cooling in ice, the absorbance of sample was measured at 550 nm. The content of proanthocyanidins was calculated by the molar extinction coefficient of cyanidin (ε = 17,360 l/mol cm and molar mass 287 g/mol) and was expressed as gram of cyanidin equivalents (CYE) per l l of juice.
Identification of individual phenolic compounds by UPLC–MS
Phenolic compounds were identified using the Acquity UPLC system coupled with a quadrupole–time-of-flight (Q-TOF) MS instrument (Waters Corp., Milford, MA, USA) with an electrospray ionization (ESI) source. Separation was achieved on an AcquityTM BEH C18 column (100 × 2.1 mm, 1.7 µm; Waters). The mobile phase was a mixture of 0.1 % formic acid (A) and acetonitrile (B). The gradient program was as follows: initial conditions—1 % B in A, 12 min—25 % B in A, 12.5 min—100 % B, 13.5 min—1 % B in A. The flow rate was 0.42 ml/min, and the injection volume was 5 µl. The column was operated at 30 °C. The major operating parameters for the Q-TOF–MS were described in the previous work [18]. The juices were centrifuged at 13,000 rpm for 5 min, and each supernatant was filtered through a 0.20-μm Minisart RC4 filter (Sartorius, Stedim Biotech GmbH, Germany) before injection into the UPLC system. The data were collected by Mass-LynxTM V 4.1 software. Polyphenolic compounds were putatively identified using their UV–Vis characteristic, MS, and MS2 properties using data gathered in-house and from the literature.
Quantitative determination of phenolics by HPLC
Phenolic compounds were quantified using Dionex HPLC system (Germering, Germany) equipped with the Ultimate 3000 model diode array detector. The detector cooperated with the LPG-3400A pump, EWPS-3000SI autosampler, column thermostat TCC-3000SD, and Chromeleonv 6.8 software. Cadenza Imtakt column C5-C18 (75 × 4.6 mm) with a guard column was used. The mobile phase was composed of solvent A (4.5 % formic acid, v/v) and solvent B (acetonitrile). The elution system was as follows: 0–1 min 5 % B; 20 min 25 % B; 21 min 100 % B; 26 min 100 % B; 27 min 5 % B. The flow rate of the mobile phase was 1.0 ml/min, and the injection volume was 20 μl. The column was operated at 30 °C. The runs were monitored at 245 nm (protocatechuic acid and depside), 280 nm (flavanone), 320 nm (phenolic acids), 360 nm (flavonols), and 520 nm (anthocyanins) wavelengths. Caffeoylquinic acid isomers were quantified as 5-O-caffeoylquinic acid, p-coumaric acid derivatives as p-coumaric acid, anthocyanins as cyanidin 3-O-glucoside, quercetin derivatives as quercetin 3-O-glucoside, izorhamnetin derivative as isorhamnetin 3-O-galactoside, and protocatechuic acid and depside 1 as protocatechuic acid, eriodictyol 7-glucuronide as naringenin. The results were calculated as mg of compound in 1 l of juice.
Determination of mean degree of polymerization of proanthocyanidins
Acid-catalyzed degradation of polymeric proanthocyanidins in the excess of phloroglucinol was used to determine proanthocyanidins mean degree of polymerization (mDP). Direct phloroglucinolysis of freeze-dried chokeberry juices (40–60 mg) was performed as described Wojdyło et al. [19]. The products of acid degradation of proanthocyanidins were separated by the use of the HPLC system (Waters, Milford, MA) that consisted of a gradient pump (1525), fluorescence detector (2475), auto-injector (2707), and Breeze 2 system controller equipped with a 250 × 4.6 mm id, 5 µm Symmetry C18 column (Waters). The mobile phase was a binary gradient with A, water/acetic acid (97.5:2.5, v/v), and B, water/acetonitrile (20:80, v/v), with a flow rate of 1 ml/min, and the gradient program used was according to Sójka et al. [20]. The injection volume was 20 μl. The fluorescence detection was recorded at an excitation wavelength of 278 nm and an emission wavelength of 360 nm. The calibration curves, which were based on peak area, were established using (+)-catechin, (−)-epicatechin, procyanidins B1, B2, and B3 after hydrolysis reaction as (+)-catechin-phloroglucinol and (−)-epicatechin-phloroglucinol adducts standards. The mDP was calculated as the molar ratio of all the flavan-3-ol units (phloroglucinol adducts + terminal units) to (−)-epicatechin and (+)-catechin, which correspond to terminal units.
Assays for pancreatic lipase activity
The release of free fatty acids from three emulsified lipids (i.e., triolein, sunflower oil, and rapeseed oil) catalyzed by porcine pancreatic lipase was calculated on the basis of the volume of NaOH added as described in our previous work [21]. Titration was carried out using an automatic pH–stat titrator (SCHOTT Instruments GmbH). All assays were carried out at 37 °C and pH 7.4. The oil-in-water emulsions were prepared by mechanical stirring of lipid substrates with 20 mM Tris-base buffer (pH 7.4) containing 150 mM NaCl and 1.3 mM CaCl2, and bile acids (triolein emulsion) or both bile acids and gum arabic (oil emulsions) in high-speed blender (PRO200, Bioeko) in an ice bath for 5 min at 20,000 rpm. Triolein emulsion contained 2.34 g of triolein, 1.56 g of bile acids, and 100 ml of buffer, while oil emulsion included 4 g of oil, 1 g of bile acids and 1 g of gum arabic, and 100 ml of buffer. Pancreatic lipase was dissolved in the same Tris-base buffer at 10 mg/ml and then centrifuged at 13,000 rpm for 5 min. Directly before analysis, the juices were adjusted to pH 7.2–7.4 with 6 M NaOH (the initial pH values were 3.42–3.72). Briefly, 4 ml of the emulsified substrate solution and 2 ml of juice or buffer (control sample) were transferred into a clean 25-ml glass bottle. The reaction mixtures were pre-incubated at 37 °C for 5 min before adding lipase supernatant—0.5 ml into triolein emulsion or 1 ml into oil emulsion. For each sample, a separate blank without lipase was used for background subtraction. Finally, the reaction mixtures were incubated in a shaking bath (200 rpm) at 37 °C for 30 min. The reaction was terminated by adding 14 ml of ethanol, and the resultant mixture was automatically titrated to pH 8 using a pH–stat with 10 mM NaOH solution. All samples were assayed in triplicate. The inhibition of lipase activity (percentage) was calculated using the following formula:
where V is the volume (ml) of 10 mM NaOH required to neutralize the free fatty acids produced.
Lipase activity was also measured using 4-MUO as substrate according to our previous work [12]. The amount of 4-methylumbelliferone released by lipase was measured with a microplate reader (Synergy™2, BioTek Instruments Inc.) at an excitation wavelength of 360 nm and at an emission wavelength of 460 nm. The inhibition (%) was calculated by using the following formula:
where F control and F control blank are fluorescence values of the solvent control with and without 4-MUO, respectively; F sample and F sample blank are fluorescence values of the juice with and without 4-MUO, respectively.
The concentration which inhibits pancreatic lipase activity by 50 % (IC50) was determined on the basis of the graph of inhibition rate against the juice concentration. The lower IC50 indicates the higher anti-lipase activity.
Analysis of antioxidant capacity
Free radical scavenging activity of chokeberry juices using the free radical cation ABTS·+ was performed as described by Re et al. [22]. The DPPH scavenging radical assay was conducted according to Kim et al. [23]. FRAP was performed according to Benzie and Strain [24]. For all methods, juices were diluted with water 30–400 times. The antioxidant capacity was evaluated by measuring the absorbance at 734 nm after 6 min of reaction with the radical (ABTS·+), at 517 nm after 30 min (DPPH·), and at 593 after 10 min for FRAP. For all methods, standard curves were prepared using different concentrations of Trolox (water-soluble derivative of vitamin E). The results obtained were expressed as mmol Trolox equivalents (TE) per 1 l of juice.
Statistical analysis
Data were expressed as mean ± SD. Data were analyzed by means of a one-way analysis of variance (ANOVA). A Duncan post hoc test was used to determine differences between the means with significance level p < 0.05. Pearson’s correlation coefficients (r) were determined using Microsoft Excel XP in order to define the relationships between selected parameters.
Results
Effect of chokeberry juices on pancreatic lipase activity
The effect of five commercial black chokeberry juices on the porcine pancreatic lipase activity was assessed in vitro using a pH–stat method with three different lipid substrates: triolein (glycerol trioleate), sunflower oil, and rapeseed oil. Independently, lipase activity was determined by fluorimetric method with 4-MUO as substrate. The results, expressed as IC50 values, are given in Table 1. The IC50 values varied from 0.59 to 5.84 μl of juice/ml of reaction mixture in the fluorimetric method and from 27.79 to 221.66 μl of juice/ml in the pH–stat method. Two juices (brands 4 and 5) at the highest doses (307.7 μl of juice/ml of reaction mixture) in the conditions of the assay did not inhibit pancreatic lipase in triolein emulsion. In the case of both oil emulsion systems, three juices at the highest concentration (285.7 μl of juice/ml of reaction mixture) did not affect enzyme activity.
Antioxidant capacity of chokeberry juices
In the present work, three methods (ABTS, DPPH, and FRAP) were selected for the evaluation of the antioxidant capacity of the chokeberry juices tested because the determination of antioxidant capacity of complex food matrix is still an unresolved problem. The Trolox equivalents (TE) values were calculated in order to compare the chokeberry juices, as shown in Fig. 1. Significant differences (p < 0.05) in the antioxidant capacity were found for the analyzed juices. The TE values varied in the ranges 20.39–91.21 mmol/l of juice, 19.02–106.13 mmol/l, and 12.19–61.09 mmol/l as determined by ABTS, DPPH, and FRAP method, respectively. The ranking order of the antioxidant capacities was the same for ABTS and FRAP methods, while juice of brand 3 was more active than juice brand 1 in DPPH method.
Phenolic compounds of chokeberry juices
The black chokeberry juices were analyzed for the content of total phenolics, total anthocyanins, and total proanthocyanidins using a Folin–Ciocalteu, a pH-differential, and acid depolymerization methods, respectively. As it is shown in Table 2, significant differences have been observed for the commercial juices tested (p < 0.05), which were about fourfold for total phenolics (2.73–10.35 g GAE/l) and about sevenfold in the case of total anthocyanins (0.10–0.67 g CGE/l) and total proanthocyanidins (0.64–4.17 g CYE/l). Proanthocyanidins accounted for 29.8–40.3 %, while anthocyanins contributed only for 3.6–6.7 % of total phenolic content. The mean size of proanthocyanidin molecules described by their mDP was very diverse for the juices tested and ranged from 12 to 52.
Additionally, the juices with the highest anti-lipase and antioxidant activities (three brands) were analyzed for the phenolic profiles by UPLC–MS and for the content of individual phenolic compounds using HPLC system. Representative HPLC chromatograms of chokeberry juice are presented in Fig. 2. The results of qualitative and quantitative phenolic composition in black chokeberry juices are summarized in Table 3. The results showed that chlorogenic acids dominated in the group of low molecular phenolic compounds and they represented 67.7–82.4 % of phenolics. Flavonols in chokeberry juices were mainly a mixture of quercetin glycosides and constituted only 4.5–18.8 % of phenolics. The contribution of anthocyanins in total phenolics varied from 4.4 % in juice brand 3 to 9.6 % in juice brand 1. Cyanidin 3-O-galactoside and cyanidin 3-O-arabinoside were the main anthocyanins in the tested chokeberry juices.
Basic parameters of the juices studied
The basic chemical composition of five commercial chokeberry juices is given in Table 4. Statistically significant differences (p < 0.05) in all quality parameters tested were found in chokeberry juices produced by different companies. The minimum and maximum pH values were measured as 3.42 and 3.72, and the total soluble solids (°Brix) values ranged from 12.5 to 20.1. Total content of fructose, glucose, sucrose, and sorbitol varied significantly from 89.5 to 162.4 g/l of juice. Sorbitol dominated in all juices and amounted to 39.5–47.6 % of total sugars. Sucrose was noted only in two juices at 1.7 and 3.0 g/l. The total organic acids content in the juices tested varied from 12.3 g/l to 21.9 g/l with significant differences dependently on the brands (p < 0.05). The amounts of organic acids analyzed were ordered as malic acid > tartaric acid > citric acid > oxalic acid. Malic acid amounted to 52.6–60.9 % of total organic acids content.
Discussion
Obesity is one of the most rapidly expanding metabolic disorders, and therefore, its prophylaxis is a big challenge for the world. Reduced absorption of dietary fat from the intestine by the inhibition of digestive lipases, especially pancreatic lipase, is an approach to decreasing the risk of obesity [15]. The presence of pancreatic lipase inhibitors has recently been reported in some edible fruits, including black chokeberry [12, 13, 21, 25–29]. Inhibition of this enzyme by fruits is attributed to the phenolic compounds, such as proanthocyanidins [12, 21, 27], ellagitannins [25, 26], anthocyanins [13, 28], and flavones [29]. The present study reports that proanthocyanidins accounted for 29.8–40.3 %, while anthocyanins contributed only for 3.6–6.7 % of total phenolic content (2.73–10.35 g/l) in the black chokeberry juices commercially available in Poland (Table 2). The total phenolic content estimated by HPLC method ranged from 1.00 to 1.45 g/l and was six- or sevenfold lower than total phenolic content determined by Folin–Ciocalteu method (Tables 2, 3). It may confirm the significant contribution of polymeric proanthocyanidins in the phenolic compounds present in chokeberry juices. On the other hand, the Folin–Ciocalteu reagent is nonspecific to phenolic compounds and can react with a wide range of thiol derivatives, some vitamins and aromatic amino acids [30]. According to the literature data, proanthocyanidins are the dominant phenolic components of black chokeberry fruit and chokeberry juices [2, 3]. Additionally, Wu et al. [4] found that chokeberry fruits contained only procyanidins and polymers with DP > 10 accounted for nearly 82 % of total procyanidins content. Furthermore, the levels of total phenolics (2.73–10.35 g/l) and total anthocyanins (0.10–0.67 g/l) estimated in this study agree with the literature data. Total phenolic content determined by the Folin–Ciocalteu method varied from 5.46 [31] to 18.54 g/l [32], while total anthocyanin content estimated by pH-differential method ranged from 0.15 [11] to 3.04 g/l [6]. The large differentiation noticed in both the present and previous studies may be due to differences in chokeberry cultivars, maturation stages as well as technology of juice production, and time of the juice storage. Among chokeberry phenolic constituents, in particular, anthocyanins were extensively degraded (losses 93 %) during juice processing, while levels of hydroxycinnamic acids decreased by 37 %, proanthocyanins by 45 %, and flavonols by 48 % [33]. On the other hand, Mayer-Miebach et al. [34] demonstrated high stability of phenolic compounds during chokeberries processing without enzyme treatment of mash.
The results of the present study revealed that all the chokeberry juices tested decreased pancreatic lipase activity in 4-MUO assay, while the inhibitory effect in lipid emulsions showed practically only two of them (Table 1). From a nutritional point of view, the use of different lipid emulsions as substrates for pancreatic lipase better resembles physiological conditions because dietary long-chain triglycerides are broken down into oil-in-water emulsions in mouth, stomach, and small intestine during digestion process [35]. The chokeberry juice brand 1 exhibited the lowest IC50 values and, therefore, the greatest inhibitory effect on pancreatic lipase (Table 1). This juice had the highest concentration of total phenolics and total proanthocyanidins (Table 2) as well as phenolic acids and anthocyanins determined by HPLC method (Table 3). The anti-lipase activity measured by fluorimetric method was correlated with the total phenolics (r = −0.855), total anthocyanins (r = −0.788), total proanthocyanidins (r = −0.857), and the mDP of proanthocyanidins (r = −0.830). For comparison, a Pearson’s correlation coefficient between the IC50 value in triolein emulsion and total phenolics was 0.149, total anthocyanins 0.460, and total proanthocyanidins 0.063. Gironés-Vilaplana et al. [28] observed strong correlation between the lipase inhibition and anthocyanin content for Latin-American fruits. On the other hand, Boath et al. [25] suggested that anthocyanins are not necessary for lipase inhibition by berry polyphenols.
The lipase inhibition determined in triolein emulsion was correlated only with the mDP of proanthocyanidins (r = −0.999). The mean size of proanthocyanidin molecules described by their mDP in the chokeberry juices tested was very diverse and ranged from 12 to 52, while for two more efficient juices was >40 (Table 2). For comparison, the mDP value for chokeberry juice obtained from heated fruits followed by decantation of raw juice was 24 [34]. The very high mDP values obtained in this study for juice brands 1 and 2 may indicate lack of enzyme treatment of chokeberry mash during fruit processing as well as decantation or filtration process of raw juice. The mDP of proanthocyanidins occurring in chokeberry fruit was determined as 59 [36] or in the acetone fruit extract as 19 [34]. The published studies have shown that anti-lipase activity of proanthocyanidins depends upon the degree of polymerization and more potent effect was observed for higher DP [27, 37]. For example, the IC50 values determined with the use of 4-MUO as the substrate were as follows: for dimer >125 μg/ml, but 32.9 and only 0.9 μg/ml for trimer and procyanidins over nonamer, respectively [27]. Proanthocyanidins have been also postulated as the major factor responsible for the anti-lipase effect of apple, cocoa, and Salacia reticulata [27, 38, 39]. The role of proanthocyanidins in reducing obesity was recently reviewed by Salvadó et al. [40]. In vivo studies with different animal models confirm anti-obesity action of proanthocyanidins from various plant sources. Additionally, they also reduce the mass of adipose tissues and decrease body weight gain.
Nevertheless, chokeberry juice contains several classes of phenolic compounds which in combination might differently affect the lipase activity due to the different interaction between them as well as with other juice components. The results of qualitative and quantitative analyses of low molecular phenolic compounds by UPLC-MS and HPLC methods allowed to conclude that all most active juices had the same phenolic profile (Table 3), which was in accordance with the data published [9, 34]. The major low molecular phenolic compounds of chokeberry juice were chlorogenic acids such as 3- and 5-O-caffeoylquinic acid. The results published by Worsztynowicz et al. [13] used p-nitrophenol palmitate as substrate demonstrated that chlorogenic acids and anthocyanins, except for cyanidin 3-glucoside, isolated from chokeberry fruit did not inhibit the pancreatic lipase. Unfortunately, authors of the above paper have not determined proanthocyanidins content in the extracts tested. In the assay using 4-MUO as substrate, the IC50 value for chlorogenic acid (the second low molecular phenolic in juices tested) was higher than that one for dimer but lower than the IC50 values for higher oligomers [27]. The differences in anti-lipase activity of chokeberry juices tested may be also due to nonphenolic components that may affect a surface property of the substrate emulsion and absorption of lipase at an oil–water interface. The juices tested in our studies differed also in terms of the basic chemical composition (Table 4). Total soluble solid, organic acid, sugars, and sorbitol contents were consistent with other report [1]. The low levels of sucrose in the juices studied are evidence that they were made purely from fruits without addition of sucrose. Additionally, the juice brand 1 with the highest anti-lipase activity had the highest soluble solids, glucose, sorbitol, and organic acids content.
Our results have also shown that commercially available black chokeberry juices may improve antioxidant status. It is a desired effect in the case of obesity which is considered as a state of chronic oxidative stress and inflammation related to reduced antioxidant defense and high reactive oxygen species production [41]. Antioxidant capacity was affected by the type of assay system and phenolic compounds contents. Additionally, the antioxidant capacity ranking order of the juices tested was slightly different than that one regarding the anti-lipase activity of the juices. The juice brand 3 with no anti-lipase activity in oils emulsions was the second in the order in terms of scavenging free radicals and ferric reducing power (Fig. 1). The antioxidant capacity as TE values was strongly correlated with total phenolics, anthocyanins, and proanthocyanidins (r > 0.934). We also observed a high correlation between antioxidant capacity and inhibition of pancreatic lipase measured by 4-MUO assay with a Pearson’s correlation coefficient of r > −0.740. On the other hand, we have noticed lack of correlation between lipase inhibitory activity in triolein emulsion and antioxidant capacity. According to Zheng and Wang [42], among polyphenols present in chokeberry juice anthocyanins contribute the most to the total antioxidant activity (42 %). Besides the anthocyanins, proanthocyanidins present in very high amounts in chokeberry juice are also very potent scavengers of free radicals as well as the inhibitors of lipid peroxidation [43, 44]. Moreover, black chokeberry juice phenolics were efficient in regenerating or protecting α-tocopherol against oxidation [32].
Conclusions
In summary, the present study provides the first evidence that black chokeberry juices exhibited pancreatic lipase inhibition in vitro, which depends on the test method used. Additionally, our results suggested that the proanthocyanidins degree of polymerization was a very important factor responsible for the high inhibitory activity against pancreatic lipase. Therefore, proanthocyanidins-rich chokeberry juices as potent inhibitors of pancreatic lipase should be a component of a diet addressed to obese people as a natural alternative for obesity prophylaxis and treatment. This was the first study on inhibitory activity of chokeberry juice against pancreatic lipase. Moreover, consumption of black chokeberry juice may be a convenient and efficient way to supplement our diet with natural antioxidants capable of scavenging free radicals. Further studies are needed to examine the exact mechanism of the pancreatic lipase inhibition as well as influence of the chokeberry juice components on other digestive enzymes involved in degradation of carbohydrates and proteins.
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Sosnowska, D., Podsędek, A., Kucharska, A.Z. et al. Comparison of in vitro anti-lipase and antioxidant activities, and composition of commercial chokeberry juices. Eur Food Res Technol 242, 505–515 (2016). https://doi.org/10.1007/s00217-015-2561-4
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DOI: https://doi.org/10.1007/s00217-015-2561-4