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Exploring the Phytochemical Composition and the Bioactive Properties of Malbec and Torrontés Wine Pomace from the Calchaquíes Valleys (Argentina) for their Sustainable Exploitation

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28 May 2024

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29 May 2024

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Abstract
Hydroalcoholic extracts from Malbec and Torrontés wine pomace (Vitis vinifera L.) originating from the high-altitude vineyards of Argentina's Calchaquí Valleys were characterized. Total phenolics, hydroxycinnamic acids, orthodiphenols, anthocyanins, non-flavonoid phenolics, total flavonoids, flavones/flavonols, flavanones/dihydroflavonols, and tannins were quanti-fied through spectrophotometric methods, with Malbec extract exhibiting higher concentra-tions in most of phytochemical groups when compared to Torrontés. HPLC-DAD identified more than 30 phenolic compounds in both extracts. Malbec displayed superior antiradical ac-tivity (ABTS cation, nitric oxide, and superoxide anion radicals), reduction power (iron, copper and phosphomolybdenum), hypochlorite scavenging, and iron chelating ability, compara-tively to Torrontés. The cytotoxicity assessments revealed that Torrontés affected the viability of HT29-MTX and Caco-2 colon cancer cells by 70% and 50%, respectively, at the highest tested concentration (1 mg/mL). At the same time, both extracts did not demonstrate acute toxicity in Artemia salina or in red blood cell assays at 500 µg/mL. Both extracts inhibited the lipoxygen-ase enzyme, with Malbec also reducing the tyrosinase activity and neither inhibited the xan-thine oxidase. The substantial phenolic content and diverse biological activities in Calchaquí Valleys' pomaces underline their potentialities to be valorized for pharmaceutical, cosmetic, and food industries.
Keywords: 
Subject: Biology and Life Sciences  -   Food Science and Technology

1. Introduction

Agroindustries are currently valued not only due to their productive and economic performance in each country, but also for their relationship and actions with the environment. Although most of the agro-industrial companies generate wastes whose management or final disposal has been highly questioned in recent decades, they seek to obtain benefits by taking advantage of them, achieving a pollution reduction, and generating economic profits derived from the added value that may generate [1,2,3]. In recent years, food industry has embraced green technologies, clean labeling, and the incorporation of natural ingredients to benefit consumers and the industry itself. In wine industry, grapes are one of the most produced crops worldwide, with an estimated production of more than 78 million tons in 2020 [2]. It is estimated that for every 100 L of wine, about 30 kg of pomace are generated, mainly consisting of skins, pulp, and stems [4,5]. Although grape pomace can be used for animal feed and compost, among other uses, only a small amount is reused, and its disposal poses environmental problems [6]. Leveraging wine pomace for sustainable purposes represents an effective strategy to mitigate environmental pollution and serves as a substitute to minimize carbon emissions across the winery`s manufacturing process. The biological properties of wine pomace residues are of interest to several industries such as food, cosmetic, and pharmaceutical ones [5].
In previous studies, it was observed that the secondary metabolites present in wine pomace could be used as natural additives due to their antioxidant capacity and ability to improve microbial stability and inhibit the growth of pathogenic microorganisms [5]. Grape pomace extracts offer numerous health benefits due to their antioxidant, anti-inflammatory, anticancer, and hypoglycemic properties [2,5]. These benefits are attributed to the rich content of nutrients and polyphenols, which underscore their potential as novel pharmacological agents for the treatment and prevention of various diseases [7]. These diseases include cancer, metabolic syndrome, neurological disorders, liver and cardiovascular diseases, and other conditions related to oxidative stress [2,5,7]. Grape pomace is a raw material for the production of dietary supplements (powders, tablets, capsules), providing an auxiliary source of polyphenols that avoids wine consumption [8]. Among polyphenolic, flavonoids (anthocyanins, flavan-3-ols, flavonols, among other), tannins and non-flavonoids such as phenolic acids, and stilbenes, are mainly responsible for the well-established antioxidant and anti-inflammatory effects. Due to these properties, phenolic compounds can be used in the cosmetic industry [7,9], inhibiting the enzyme tyrosinase, which is over expressed in diseases such as melasma, freckles, and senile lentigines [10].
According to Wani et al. [7], about 70% of phenolic compounds remain in grape pomace after fermentation-maceration. Therefore, its use and valorization through extraction of phenolic compounds is an attractive strategy that aims to recover compounds while reducing the environmental impact of their by-products [11]. However, the biological activity of grape pomace extracts depends on grape variety, geographical origin, climate, vineyard soil conditions, and winemaking process [2].
Considering the wide range of possible uses of pomace extracts and the recognition that the polyphenolic composition depends on the plant material’s origin and winemaking techniques, it is of special interest to explore the chemical and functional properties of the pomace of each region and cultivar with the aim of finding industrial applications.
In previous studies, white and red wine pomace extracts from the Calchaquí Valleys were found to inhibit the virulence of pathogenic bacteria (Pseudomonas aeruginosa and Staphylococcus aureus) [12,13]. These extracts demonstrated inhibition of P. aeruginosa’s swarming motility, biofilm production, and metabolic activity in a biofilm environment. The antibiofilm activities showed a positive correlation with the polyphenol content of the extracts [12]. Calchaquíes Valleys wine pomaces also exhibited efficacy against Leishmania amazonensis, the responsible agent of American tegumentary leishmaniasis. The extracts also displayed significant anticholinesterase activity, suggesting potentialities for the palliative treatment of Alzheimer [14].
Given the limited information on the phenolic composition and biological properties of Torrontés and Malbec wine pomace from this geographical area, the present study aims to investigate the polyphenolic composition, antioxidant capacity, cytotoxicity, and enzyme inhibition potential (tyrosinase, lipoxygenase, and xanthine oxidase) of Torrontés and Malbec pomace from the Calchaquí Valleys.

2. Materials and Methods

2.1. Chemicals

For HPLC analysis, methanol and formic acid were HPLC grade from Merck (Darmstadt, Germany). The different standards of phenolic compounds, namely the phenolic acids: gallic acid (≥99%), protocatechuic acid (99.63%), neochlorogenic acid (≥98%), caftaric acid (≥97%), chlorogenic acid (> 95%), 4-caffeyolquinic acid (≥98%), va-nillic acid (≥97%), caffeic acid (≥98%), syringic acid (≥98%), p-coumaric acid (≥98%), trans-ferulic acid (≥99%), sinapic acid (≥99%), 3,5-di-O-caffeyolquinic acid (≥95%), ellag-ic acid (≥95%), 4,5-di-O-caffeyolquinic acid (≥90%), cinnamic acid (≥99%); flavonoids: (+)-catechin (≥98%), (-)-epicatechin (≥90%), naringin (≥95%), quecetin-3-O-galactoside (≥97%), quercetin-3-O-glucopyranoside (≥99%), rutin hydrate (≥94%), myricetin (≥96%), quercitrin (≥97%), kaempferol-3-O-glucoside (≥95%), kaempferol-3-O-rutinoside (≥98%), isorhamnetin-3-O-glucoside (≥98%), isorhamnetin-3-O-rutinoside (≥99%), naringenin (98%), quercetin (95%), kaempferol (≥98%), apigenin (≥99%), chrysin (≥99%), tiliroside (≥98%); chalcones: phloridzin dehydrate (99%) and phloretin (≥98.5%); stilbenoids: trans-polydatin (≥98%), trans-epsilon viniferin (≥95%) and resveratrol (≥99%) were purchased from Sigma-Aldrich and Extrasynhtese. Their stock solutions were prepared in methanol at concentration levels ranging from 1 to 5 g/L and stored at −20°C.
Dimethylsulfoxide (DMSO), Triton X-100, 2,2′-Azinobis-(3-ethylbenzothiazoline-6-sulfonic acid) cation radical (ABTS˙+), Trolox (6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid), Butylated hydroxytoluene (BHT), EDTA, Folin–Ciocalteau reagent, Tyrosinase from mushroom, kojic acid, L-tyrosine, xanthine oxidase from bovine milk, xanthine, nitroblue tetrazolium chloride (NBT), phenazine methosulphate (PMS), β-nicotinamide adenine dinucleotide (NADH), dihydrorhodamine 123 (DHR), and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) were purchased from Sigma-Aldrich (St. Louis, MO, USA). Other chemicals were obtained from local commercial sources, and were of analytical-grade quality.
Caco-2 cells (clone type C2Bbe1) were acquired from the American Type Culture Collection (ATCC, USA), and HT29-MTX was offered from Dr. T. Lesuffleur (INSER-MU178, Villejuif, France). Dulbecco’s Modified Eagle Medium (DMEM), Fetal Bovine Serum (FBS), Hank’s Balanced Salt Solution (HBSS), non-essential amino acids, penicillin, streptomycin, and trypsin–EDTA were obtained from Invitrogen Corporation (Life Technologies, S.A., Madrid, Spain).

2.2. Material Collection

Samples of Malbec and Torrontés grape pomace were gathered from Albarossa Winery, situated in Tafí del Valle, Tucumán, Argentina, during the 2019 and 2020 harvests. Notably, the vineyard cultivation practices at this winery refrain from the use of chemical substances. The grapes exhibited robust health, with no signs of Botrytis cinerea detected. Assessment for the presence of B. cinerea was conducted visually, and its absence can be attributed to the windy and arid conditions characteristic of the Calchaquí Valleys region.
The Calchaquí Valleys, located in the northwest region of Argentina, have a temperate climate with notable thermal amplitudes and, occasionally, experience prolonged late frosts in spring. Its high-altitude vineyards range from 1700 meters to 2400 meters. The grapes were grown on soils characterized as sandy loam or sandy with a high proportion of fine sand. The soil profile is deep, with a somewhat rocky subsoil ensuring excellent permeability and leaching of salts [15].
The regional white wines correspond to the Torrontés varietal (Vitis vinifera L.), which has become the emblematic variety of the region. This grape is optimal to produce aromatic wines and adapts very well to the entire area, becoming the most cultivated one in the region [16]. On the other hand, the Malbec wine varietal (Argentina’s most exploited purple grape variety) from the Calchaquí Valleys shows different particularities from other country wine regions due to the terroir characteristics described above.
Notably, Torrontés pomace was obtained from a white wine making process, meaning that grapes were not subjected to ethanolic fermentation. In contrast, Malbec pomace was acquired from red wine making process, where grapes are entirely involved in fermentation. The collected specimens were stored at -80 °C before being oven-dried at temperature below 45°C for 48 h, ensuring the preservation of phenolic compounds until a constant weight was attained. Moisture was calculated by weight difference before and after drying. The dried material was crushed with a grinder until reaching a particle size < 250 µm (sieve mesh 60). The extract was prepared from this pomace powder.

2.3. Preparation of Extracts

The active principles were extracted by hydroalcoholic maceration (ethanol: water, 50:50 v/v) in a solid-liquid ratio of 1/4, w/v. Two successive extractions were performed by shaking at room temperature (150 rpm/min) for 3h. The extracts were vacuum filtered using Whatman No. 4 filters and evaporated to dryness by vacuum evaporation and subsequent lyophilization. The extracts obtained during the processes were stored in the dark at 4ºC until use. The extraction yields were expressed in mg of soluble principle per gram of dry pomace (mg/g DP) and was calculated as follows: Weight of extract obtained (mg)/Initial weight of the plant matter to be extracted (mg)/

2.4. Phytochemical Analysis

2.4.1. Quantification of Different Phenolic Groups

For this assay, stock solutions of 2.5 mg/mL of each extract were used. Total extractable phenols and nonflavonoid compounds were determined colorimetrically using Folin Ciocalteu’s reagent at 765 nm [17]. A standard curve was performed with gallic acid (2-20 µg/mL) as standard, and the results were expressed in mg of gallic acid equivalents (GAE) per g of dry pomace extract (DPE) (mg GAE/g DPE) and g of dry pomace (mg GAE/g DP) (R2 = 0.9965, p≤0.05). To eliminate the potential sugar interference, the Torrontés extract was purified by solid-phase extraction previous to Folin Ciocalteu’s analysis. C18 cartridge (Waters’ Sep-Pak Cartridges) was activated with 2 mL of methanol and then 5 mL of deionized water. Then, 9 mL of the extract (2.5 mg/mL) was injected and eluted using 9 mL of acidic deionized water (0.1% formic acid). Finally, 9 mL of acidic methanol (0.1% formic acid) was used to recover the polyphenols compounds [18].
The total flavonoid content was determined using sodium nitrite (5%) and aluminum chloride (10%). The technique is based on the formation of specific colored complexes between flavonoids and the reagents (NaNO2 and AlCl3), with the color intensity measured spectrophotometrically at 510 nm [19]. For quantification, a quercetin standard curve (4-80 µg/mL) was used and the results were expressed as mg quercetin equivalents (QE) per g of extract (mg QE/g DPE) (R2 = 0.9939, p≤0.05)
The flavone and flavonol content was evaluated spectrophotometrically at 425 nm with aluminum chloride (5%) [17,20]. This technique is based on the formation of a complex between the aluminum ion, Al (III), and the carbonyl and hydroxyl groups of the flavonoid. The standard curve was performed with quercetin (5-40 µg/mL), and the results were expressed in mg of quercetin equivalents (QE) per g of extract (mg QE/g DPE) (R2 = 0.9941, p≤0.05).
Flavanone and dihydroflavonol content was measured at 495 nm [17,20]. This technique is based on the reaction of these compounds with 2,4-dinitrophenylhydrazine (DNP) in an acidic medium to form colored phenylhydrazones. The standard curve was performed with naringenin (20-200 µg/mL), and the results were ex-pressed in mg of naringenin equivalents (NE) per g of extract (mg NE/g DPE) (R2 = 0.9998, p≤0.05).
Orthodiphenols were assessed by UV-Visible spectrophotometry using the sodium molybdate method at a wavelength of 370 nm [21]. A standard curve was performed with caffeic acid (2-20 µg/mL), and the results were expressed as mg of caffeic acid equivalents (CAE) per g of extract (mg CAE/g DPE) (R2 = 0.9981, p≤0.05).
Hydroxycinnamic derivates were evaluated at 320 nm using caffeic acid (0.5-5 µg/mL) as standard, and the results were expressed as mg of caffeic acid equivalents (CAE) per g of ex-tract (mg CAE/g DPE) (R2 = 0.9972, p≤0.05) [22].
The assessment of total anthocyanin content was carried out by the pH differential method, and the results were expressed as mg cyanidin-3-glucoside equivalents per g of extract (mg C3GLE/g DPE) according to Carullo et al. [23]. Results were determined by means of the following formula
m g C 3 G L E / L D P E = A M W D F 1000 ε 1
where:
A = (A520nm – A700nm)pH=1 – (A520nm – A700 nm)pH=4.5; MW (molecular weights of cyanidin-3-glucoside) =449.2 g/mol; DF = dilution factor; ε= (molar extinction coefficient) = 26900 L/mol cm and 1000 = conversion factor from g to mg.
Determination of the tannin content of the extracts was performed as reported previously by Bouabid et al. [24] using the vanillin assay. A standard curve was performed with catechin (5-25 µg/mL), and the results were expressed as mg catechin equivalents per g of extract (mg CE/g DPE).

2.4.2. Identification of Phenolic Compounds by HPLC-DAD Analysis

The HPLC analyses were carried out in a Shimadzu HPLC system equipped with a LC-20AD prominence pump, a DGU-20AS prominence degasser, a CTO-10AS VP col-umn oven, a SIL-20A HT prominence autosampler, and an SPD-M20A photodiode array detector (Kyoto, Japan).
The phenolic profile of obtained extracts was analyzed according to the method described by Moreira et al. [25] with slight modifications. Chromatographic analyses were performed using a Shimadzu HPLC system, and polyphenols separation was achieved on a Gemini C18 column (250 × 4.6 mm, 5 μm) from Phenomenex at 25°C. The solvent system used, pumped at a flow rate of 1 mL/min, was methanol (eluent A) and water (eluent B) both acidulated with formic acid (0.1%) and the following gradient was employed: 0–5 min: 20–24% A; 5–7 min: 24-25% A; 7–10 min: 25–26% A; 10–11 min: 26–26.5% A; 11–18 min: 26.5% A; 18–25 min: 26.5–30% A; 25–50 min: 30–45% A; 50–60 min: 45–50% A; 60–70 min: 50–55% A; 70–90 min: 55–70% A; 90–100 min: 70–100% A, followed by 100% A for 5 min and back to 20% A in 10 min and 5 min of reconditioning before the next injection. The individual phenolic compounds were identified by comparing the samples’ retention time and UV-Vis spectra with those from pure standards. Chromatograms were recorded at 280, 320, and 360 nm depending on the maximum absorption of the phenolic compound identified. Before injection, the dried extract was resuspended in methanol/water (20:80) and filtered through a 0.22 μm PTFE syringe filter. The quantification of phenolic compounds was made based on calibration curves of the pure standards, and results were expressed as mg of compound per 100 g of DPE.

2.5. Antioxidant Capacity Assays

At least three independent experiments were performed for each method. For sample and positive controls, six concentrations were analyzed in duplicate. Prior to the assays, the absorption of the extract was studied at the proper wavelengths. GraphPad Prism 7 software (GraphPad, La Jolla, CA, USA) was used to calculate the results based on the curves of inhibition percentage versus antioxidant concentration. For chelating, scavenging and reducing capacities, the concentration of the extracts necessary to chelate, scavenge or reduce 50% of the radicals or iron ions (IC50) was determined through linear regression analysis. If the IC50 was not reached, the results were expressed as the percentage of inhibition at the highest concentration tested.

2.5.1. Phosphomolybdenum Reducing Capacity

The phosphomolybdenum method described by Carullo et al. was used [23]. The absorbance of the green-colored complex was measured spectrophotometrically at 695 nm. The standard curve was performed with ascorbic acid (5-50 µg/mL) as standard, and the results were expressed in μg of ascorbic acid equivalents (AAE) per mg of DPE (μg AAE/mg).

2.5.2. Metal Chelating Capacity

Metal chelating capacity is based on the formation of colored Fe+2 complexes whose concentration can be determined spectrophotometrically. Molecules present in a sample that can chelate iron will compete with ferrozine, decreasing the reaction’s coloration (absorbance) [17]. The absorbance was measured at 562 nm. EDTA (5-20 μg/mL) was the positive control used.

2.5.3. ABTS Cation Radical Scavenging Capacity

The assay to determine the ability of the extracts to scavenge the 2,2′-Azinobis-(3-ethylbenzothiazoline-6-sulfonic acid) cation radical (ABTS˙+) was carried out according to a method previously described [17]. The absorbance was measured at 750 nm, and the percent purification was calculated at 6 min. Trolox (2-7 μg/mL) was used as a positive control.

2.5.4. Nitric Oxide Scavenging Capacity

The method described by Torres-Carro et al. [17] was used to determine the nitric oxide depurating capacity of the extracts. This technique uses Griess reagent to give a pink-colored azo complex with a maximum absorption at 550 nm. Ascorbic acid (25-200 μg/mL) was used as positive control.

2.5.5. Iron Reducing Power

The ability of the residue extracts to reduce potassium ferricyanide (Fe+3) to potassium ferrocyanide (Fe+2), which forms a Prussian blue complex, was detected spectrophotometrically at 700 nm. The absorbance values were used to determine the concentration required to reduce 50% of Fe+3 (RC50). BHT (3-13 μg/mL) was used as a positive control [17].

2.5.6. Copper Reducing Power

The CUPRAC assay was performed utilizing the copper(II)-neocuproine (Cu(II)-Nc) reagent as the chromogenic oxidant [26]. The standard curve was performed with gallic acid (0.5-5 μg/mL), and the results were expressed in μg of gallic acid equivalents (GAE) per mg of DPE (μg GAE/mg).

2.5.7. Superoxide Anion Radical Scavenging Assay

The quenching ability of superoxide anion radical (O2●-) was assessed based on the NBT reduction into purple-coloured diformazan [27]. O2●- was produced by the non-enzymatic NADH/PMS/O2 system. The absorbance was measured at 560 nm at 37 °C for 5 min. Results were expressed as the inhibition, in IC50, of the NBT reduction to diformazan. As positive controls, catechin (10-100 μg/mL) and gallic acid (10-100 μg/mL were employed.

2.5.8. Hypochlorous Acid Scavenging Assay

The quenching abilities of the samples and positive controls against hypochlorous acid (HOCl) were determined through a procedure previously described. [27]. DHR, used as a fluorescence probe, was oxidized to rhodamine by HOCl. A 1% (m/v) NaOCl solution was used after adjusting the pH to 6.2. The inhibition of HOCl-induced oxidation of DHR was determined. Catechin (0.05-0.5 μg/mL) and gallic acid (0.5-2.0 μg/mL) were employed as positive controls.

2.5.9. Saccharomyces cerevisiae Survival Assay

Yeast cells were exposed to oxidative stress induced by 2 mM H2O2 in the presence and absence of extract. Two controls were used: yeast exposed to the vehicle of extract (DMSO) and yeast exposed to extracts without the addition of H2O2. Cell viability was analyzed by determining the CFU/mL in a solid medium [28]. The results are expressed as a percentage of survival. One hundred percent survival is defined as the CFU/mL observed on the control plate, which contains yeast exposed to extract vehicle, without extracts or hydrogen peroxide.

2.6. Totoxicity Trials

2.6.1. Artemia Salina Test

The acute toxicity levels of Torrontés and Malbec pomace extracts, concentrations from 250 to 500 μg/mL, were evaluated using the brine shrimp lethality test [17]. The experiments for each concentration were conducted in triplicate. The negative control wells contained DMSO to a final concentration lower than 0.3%, and the positive control potassium dichromate (10-40 μg/mL). Survival percentages were calculated by comparing the number of survivors in the test wells with respect to the negative control.

2.6.2. Hemolysis

The hemolytic impact of the pomace extracts was assessed spectrophotometrically at 550 nm following the method described by Torres-Carro et al. [17]. Extracts ranging from 200 to 1000 μg DPE/mL, or the vehicle (serving as a 0% hemolysis control), were brought into contact with a 10% suspension of human red blood cells (HRBC). A 100% hemolysis controls were established by exposing the 10% HRBC suspension to deionized water and to 1% (w/v) Triton X-100.

2.6.3. Cell Viability Assay

The 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay was performed to evaluate the effect of the different extract concentrations (0.1–1000 µg DPE/mL) on the intestinal cell lines. Passages 69-71 and 31-32 were used for Caco-2 and HT29-MTX, respectively. Briefly, cells (25 × 103 cells/mL) were incubated during 24 h with fresh medium in the absence or presence of the extracts dissolved in cell culture medium.
Following the extracts removal from each well, cells were washed with HBSS. The number of viable cells was determined by adding MTT reagent and incubating for 3 h at 37 °C. DMSO was used to solubilize the crystals. The positive control was DMEM, and the negative control was 1% (w/v) Triton X-100. Cells were grown according to the methodology described by Pinto et al. [27]. The absorbance was read at 590 nm with background subtraction at 630 nm. Results were expressed as percentages of cell viability.

2.7. Enzyme Inhibitions

The enzyme inhibition was calculated percent as follows: % inhibition= [(Abs control – Abs sample)/Abs control] x 100, where Abs control is the absorbance of the control solution and Abs sample is the absorbance of the sample solution. When possible, the concentration responsible for inhibiting 50% of enzyme activity (IC50) was established through regression analysis, employing a concentration-inhibition response curve.

2.7.1. Tyrosinase

The tyrosinase inhibitory capacity of Torrontés and Malbec pomace extracts was performed as previously described Matos et al. [6]. The absorbance was measured at 475 nm after 20 min incubation. Kojic acid (0.1-5 µg/mL) was used as a positive control agent.

2.7.2. Xanthine Oxidase

The assay was conducted as previously described Quy & Xuan [29]. The absorbance was measured at 290 nm in a spectrophotometer. The reference inhibitor Allopurinol (0.05-5 µg/mL) was used as a positive control.

2.7.3. Lipoxygenase

The assessment of LOX activity followed the methodology outlined by Torres-Carro et al. [17]. Soybean LOX was exposed to different concentrations of the extracts or vehicle and its substrate, linoleic acid. The inhibitory potential was gauged by computing the percentage of hydroperoxide production inhibition at 234 nm. Quercetin (40-70 µg/mL) and gallic acid (30-80 µg/mL) were used as positive controls.

2.8. Statistical Analysis

All data were expressed as the mean ± standard deviation from at least three independent experiments. The HPLC statistical analysis was conducted using IBM SPSS Statistics 26.0 software (SPSS Inc., Chicago, IL, USA). For the other assays, the statistical analysis was performed using INFOSTAT Analytical Software (Universidad Nacional de Córdoba, Córdoba, Argentina). Differences in mean values were evaluated using Student’s t-test for independent samples. In all analyses, p-values < 0.05 were considered statistically significant.

3. Results and Discussion

3.1. Chemical Composition

Vitis vinifera byproducts are an important source of phytochemicals with potential health-promoting properties and biotechnological interest. The chemical composition and health benefits of several grape pomaces have been previously reported [5]. However, little is known about the phytochemical profiles of wine pomace Malbec and Torrontés from Calchaquí Valleys.
In the present study, the Malbec and Torrontés pomace samples had moistures between 65 and 70%, the oven drying over freeze-drying was selected due to its potential applicability within the wine industry and cost-effectiveness [30]. After drying and milling into flour, the grape pomaces were extracted with the use of non-toxic solvents (ethanol/water) and dried. Green solvents were used to acquire and characterize polyphenolic extracts suitable for human consumption or utilization in medical, cosmetic, or pharmaceutical sectors. Additionally, it is noteworthy that ethanol is a byproduct of wine industry. The extraction yields of soluble compounds from Malbec and Torrontés pomace were 161.6 ± 16.7 and 735.2 ± 51.2 mg extract/g flour, respectively (16% and 73%). The extraction yields, and the total phenolic content align with the results obtained using the same solvent (ethanol 50%) for other red wine pomaces, with values ranging between 5.3% and 16.1% [31,32]. Furthermore, the Torrontés pomace yields were significantly higher than those reported for other white wine pomaces, which ranged between 4.9% and 7.4% [32], having probably a higher content of extractable compounds than polyphenols. It is worth noting that this yields discrepancy may be attributed to the fact that, in the cited study, the authors chose to wash the pomace with water before drying to eliminate residual sugar, a step that was not carried out in the present work.
The analysis of the phenolic metabolites identified in the pomace extracts is detailed in Table 1. A comparison between the two analyzed pomace varieties reveals that the red Malbec variety exhibited a total phenol content 6.5 times higher than that of Torrontés. Non-flavonoid phenolic compounds accounted for 19.5% of the total polyphenol content in the Malbec pomace extract, while in Torrontés, these compounds represent 40.2%. The total flavonoid compound content in the Malbec extract surpassed that of Torrontés 7.5 times. Interestingly, the tannin content was almost similar in both varieties. It should be noted that no anthocyanins were detected in the Torrontés extract (<LOQ).
The concentration of total polyphenols in the Malbec dry extract (156.01 mg GAE/g DPE) was very similar to the findings in a Malbec pomace from Mendoza, Argentina (Cuyo region), which reported 196.2 mg GAE/g DPE) [31]. The present findings align with the total polyphenol levels (ranging between 127 and 298 mg/g DPE) and the total flavonoid content (ranging between 137 and 322 mg/g DPE) observed in four other red skin pomaces derived from Italian cultivars (Barbera, Grignolino, Pinot Noir, and Nebbiolo). Nevertheless, in the present study, the tannin content was lower [32]. Furthermore, the results achieved exceed those reported for Merlot pomace from Brazil [33] in terms of total polyphenols, total flavonoids, and anthocyanins. It is worth noting that all these studies utilized extraction conditions like the present research. Higher values of total polyphenols (523 mg/g DPE), but lower levels of anthocyanins (1.67 mg/g DPE), were reported for Cabernet Sauvignon grape pomace (Mexico) that was defatted with hexane prior to extraction with ethanol at 60% [30].
Likewise, Torrontés pomace from Galicia (extracted with 65% methanol) exhibited a lower concentration of total phenolic compounds (22 mg GAE/g DPE) as reported by Alvarez-Casas et al. [34], being consistent with the present findings (19.9 mg GAE/g DPE). The sugars present in phenolic-extracted Torrontés grape marc, lead to a reduced polyphenol richness per mass of extract when compared to the red pomace extract. Guaita et al. [32] documented higher values of total phenolics (144-208 mg/g DPE), total flavonoids (108-206 mg/g DPE), and tannins (64-108 mg/g DPE) for three other white-skinned pomaces of Italy (Muscat blanc, Arneis, Cortese) extracted with 50% ethanol. Variations in extraction methods, grape types, and agroclimatic conditions contribute to disparities in the measured total polyphenols, explaining the divergent values reported in literature. Moreover, the genotype is the main factor that influence the relative concentrations of the different phenolic compounds [35].
By HPLC-DAD analysis 35 individual phenolic compounds were identified in the extracts, including 14 phenolic acids, 18 flavonoids, and 3 stilbenoids (Table 2). Most of the compounds identified were found in both pomaces. In the Torrontés extract, the main polyphenols were: 4,5-di-O-caffeoylquinic acid ˃ 4-O-caffeyolquinic acid ˃ kaempferol-3-O-glucoside ˃ isorhamnetin-3-O-glucoside ˃ caftaric acid ˃ sinapic acid ˃ gallic acid ˃ ferulic acid ˃ protocatechuic acid ˃ (+)-catechin. Regarding the Malbec extract, the main phenolic compounds were: protocatechuic acid ˃ (+)-catechin ˃ gallic acid ˃ 4-O-caffeyolquinic acid ˃ sinapic acid ˃ 4,5-di-O-caffeoylquinic acid.
The phenolic patterns among the varieties exhibited notable quantitative differences. For instance, in the Torrontés extract, the content of 4,5-di-O-caffeoylquinic acid is 5 times higher compared to that of the Malbec extract. Conversely, the Malbec extract displayed significantly elevated levels of (+)-catechin, protocatechuic acid, and gallic acid, which were 8.8, 9.8, and 2.7 times higher, respectively, than those found in the Torrontés extract. Additionally, in pomace of another red grape variety, Cabernet Sauvignon, quercetin, catechin, epicatechin, and syringic acid emerged as dominant phenolic compounds [36].
To contextualize our findings against other published data for red and white whole pomaces (skin and seeds) extracted with hydroalcoholic solvents, the results were exsented in milligrams of the compound per gram of dry pomace extract (mg/g DPE) or per gram of dry pomace (mg/g DP) (Table 2). The results attested that gallic acid (2.74-73 mg/g DPE and 6.4-14.07 mg/g DP), protocatechuic acid (≤0.29 mg/g DPE and 0.6-2.03 mg/g DP), chlorogenic acid (≤0.06 mg/g DPE and ≤0.13-0.23 mg/g DP), and ferulic acid (2.4 mg/g DPE and <0.13 mg/g DP) are present in concentrations much higher than the values reported for red wine pomaces [14,30,31,33,37,38,39]. Furthermore, the phenolic acids: gallic (3.3-11.12 mg/g DP), protocatechuic (0.39-7 mg/g DP), caffeic (falling within the range of 0.15 mg/g DP), caftaric (1.9-7.9 mg/g DP), and ferulic (0.13-0.22 mg/g DP); and the flavonoids quercetin-3-O-galactoside (approx. 0.96 mg/g DP) and kaempferol-3-O-glucoside (approx. 0.21 mg/g DP) are found in much higher concentrations than those reported in literature for white wine pomaces [14,34,39]. Although resveratrol has not been identified, the presence of derivatives such as polydatin, also known as piceid (resveratrol derivative with improved bioavailability), and trans-epsilon viniferin (a resveratrol dimer) has been detected. To the best of our knowledge, this study reports for the first time the presence of neochlorogenic acid, 4-O-caffeoylquinic acid, 3,5-di-O-caffeoylquinic acid, 4,5-di-O-caffeoylquinic acid, sinapic acid, and isorhamnetin-3-O-rutinoside in hydroalcoholic extracts of wine pomace.
Malbec wine pomace from Argentina’s Cuyo region exhibited lower levels of catechin (338 mg/100 g DPE) and gallic acid (25 mg/100 g DPE) comparatively to the present findings for Malbec pomace from the Calchaquí valleys. In contrast, Cuyo’s Malbec wine pomace displayed higher concentrations of epicatechin (176 mg/100 g DPE) and syringic acid (173 mg/100 g DPE). It is interesting to note that protocatechuic acid, the main phenolis acid observed in this study, was not reported in Malbec pomace from Cuyo [31]. In another study [14] that assessed the polyphenol content in a concentrated chromatographic fraction obtained from a methanolic extract of red pomace from the Calchaquí Valleys (unknown variety), the C6-C1 phenolic acids, gallic acid and syringic acid were identified as the main phenolics. In agreement with the present results, Teixeira et al. [35] reported protocatechuic acid as the most abundant hydroxybenzoic acid in pomace from red varieties.
Regarding white wine pomace from the Calchaquí Valleys (unknown variety), Salazar et al. [14] highlighted gallic acid as the predominant phenolic acid. In contrast, the results obtained in this work reveal a distinct composition, with an emphasis on the prevalence of derivatives of caffeoylquinic acid, contrasting with Salazar’s observations. In Galician Torrontés pomace, phenolic acids such as gallic, protocatechuic, and caftaric, and the flavonoids epicatechin, quercetin, and quercetin derivatives were identified [34]. In the present work, a greater diversity of phenolic compounds was explored, which explains why other authors do not report the caffeoylquinic acid-derived compounds, which quantitatively were one of the most important in the present research.
A literature review [35] described notable distinctions in the hydroxycinnamic acid content between red and white grape skins. Specifically, white grape skins exhibited elevated levels of cis-coutaric acid and trans-caftaric acid, whereas red grape skins were predominantly composed of chlorogenic acid (3-O-caffeoylquinic acid). This study observed similar chlorogenic acid content in both varietals, while caftaric acid was only present in the Torrontés pomace.

3.2. Biological Activity

3.2.1. Antioxidant

Reactive species, particularly reactive oxygen species (ROS) and reactive nitrogen species (RNS) play a significant role in various physiological processes, including cell signaling, inflammatory cascade, and homeostasis. Consequently, the evaluation of the scavenging capacity of an extract against ROS and RNS becomes more intriguing due to their pivotal functions in living tissues. The antioxidant and antiradical activities of hydroalcoholic extracts was evaluated in nine different assays (Table 3 and Figure 1). In the ABTS cation radical, nitric oxide, superoxide anion, and hypochlorite assays, the Malbec extract demonstrated the best scavenging efficiency, as indicated by lower IC50 values. In the iron-chelating assay, the Malbec extract could chelate 42% of the metal at 1000 µg/mL (Table 3). Additionally, the Malbec extract exhibited superior Fe3+ and Cu2+ reducing power when compared to the Torrontés extract (Table 3). To assess the bioactivity of wine pomace in safeguarding Saccharomyces cerevisiae cells from induced oxidative damage, cell viability was measured in the presence or absence of extracts as chemoprotectors. As depicted in Figure 1, selected concentrations from the samples (12.5-150 µg/mL) exhibited non-cytotoxicity to S. cerevisiae. Upon the induction of oxidative stress, yeast cells demonstrated sensitivity to H2O2, with only 50% surviving the oxidative insult. Malbec grape pomace extract (12.5 µg/mL) rescues 24% of yeast from oxidative stress induced by H2O2, while the Torrontés pomace did not show a protective effect.
In summary, Malbec grape pomace demonstrated significant scavenging activity against ROS and RNS, potentially attributed to its higher phenolic content when compared to Torrontés grape pomace, particularly in what concerns to catechin, epicatechin, gallic acid, and protocatechuic acid whose free radical scavenging potential has been extensively demonstrated [2]. This distinction could account for the heightened antioxidant activity observed in this particular varietal.
The divergence in the antioxidant and antiradical activities between red and white pomace extracts is attributed to their distinct phenolic profiles, significantly influenced by the grape variety and extraction methods [40]. The free radical scavenging activity and the ferric-reducing power of grape pomace are correlated with specific phenolic acids (gallic and caffeic), flavan-3-ols (catechin, epicatechin, galloylcatechin), and flavonols (quercetin) [38].
The antioxidant activity results obtained in this study surpassed those reported by other authors for hydroalcoholic extracts of red wine pomace (Syrah, Petit Verdot, and Romy) and white wine pomace (Chenin Blanc and Banaty): ABTS scavenging (IC50 56.22 µg/mL for Romy and 78.47 µg/mL for Banaty), iron-reducing ability (RC50 160.97 µg/mL for Romy and 141.5 µg/mL for Banaty), iron-chelating capacity (CC50 262.67 µg/mL for Romy and 248.35 µg/mL for Banaty), superoxide anion scavenging (IC50 190 µg/mL for Petit Verdot, 240 µg/mL for Syrah, and 2160 µg/mL for Chenin Blanc), hypochlorite scavenging (IC50 17 µg/mL for Petit Verdot, 31 µg/mL for Syrah, and 128 µg/mL for Chenin Blanc) [41,42]. No reports were found regarding nitric oxide scavenging capacity. Pomace extracts from Syrah, Merlot, and Cabernet Sauvignon boosted the S. cerevisiae survival rate by 8% to 16% compared to cells exposed to H2O2 [28].
Protocatechuic acid, catechin, gallic acid, ferulic acid, and chlorogenic acid, present in the Calchaquíes Valleys wine pomaces, exhibit various pharmacological activities. These include antioxidant, anti-inflammatory, neuroprotective, antibacterial, antiviral, anticancer, antiosteoporotic, analgesic, antiaging, antihypertensive, anti-diabetic, antihyperlipidemic, anticoagulant, antiulcer, cardioprotective, and hepatoprotective properties [43,44,45,46,47,48]. The antioxidant properties of the pomace extracts observed, particularly Malbec, are partially attributed to the high content of these phenolic compounds.
Additionally, accumulated evidence demonstrated that caffeoylquinic acids present in high concentration in the Torrontés pomace extract have a wide range of biological activities, such as antiparasitic, antioxidation, antiviral, antibacterial, anti-inflammatory, anticancer, neuroprotective, and anti-diabetic effects [48]. Di-O-caffeoylquinic acids protect bone marrow-derived mesenchymal stem cells from •OH-induced damage and the antioxidant mechanisms include electron-transfer, H+-transfer, and Fe2+-chelation [50].
Likewise, polydatin has demonstrated a countless of pharmacological properties, primarily including anticancer, cardioprotective, anti-diabetic, gastroprotective, hepatoprotective, neuroprotective, and antimicrobial effects, along with health-promoting roles in the renal system, respiratory system, rheumatoid diseases, the skeletal system, and women’s health. This resveratrol derivative has a higher antioxidant and anti-inflammatory activity than resveratrol [51].
The proven antioxidant capacity of the hydroalcoholic extracts derived from Malbec and Torrontés pomace, coupled with their demonstrated antivirulence activity against pathogenic bacteria (P. aeruginosa and S. aureus) as indicated by other authors [12,13], implies a promising prospect for their use as natural preservatives in the food industry. This potential application could play a crucial role in mitigating oxidative processes.
This collective evidence elucidates the biological activity of the Calchaquíes Valleys wine pomaces, underscoring the substantial health-promoting benefits associated with the presence of these diverse and potent phenolic compounds.

3.2.2. Cytotoxicity

The cytotoxic assay performed on HT29 and Caco-2 colon cancer cells is shown in Table 4. The Torrontés extract significantly reduced cell viability in a dose-dependent manner, achieving 67% and 48% viability for HT29 and Caco-2 cells, respectively, at the highest tested concentration (1 mg/mL). In contrast, Malbec pomace at the same concentration reduced the viability of Caco-2 cells by 20%. These findings align with previous research indicating that grape pomace can inhibit the proliferation of colon adenocarcinoma cells (Caco-2, HT-29) in a dose-dependent manner, and that white grape pomace is more active than red [52].
The anti-proliferative effects of Zalema (white grape) pomace hydroalcoholic extract (methanol 75%), as well as specific phenolic standards like catechin, epicatechin, quercetin, and gallic acid on Caco-2 cells, have been previously documented [53]. Additionally, the anti-proliferative impact of caffeoylquinic acids on human colon cancer cells has been established [49,54]. The observed effects in this study could be attributed, at least in part, to the high content of these acids in the Torrontés pomace. On the other hand, the synergistic effect of different polyphenolic compounds as chemopreventive agents is well-documented [53].
This study represents the first report on the cytotoxic evaluation of pomace from the Calchaquí Valleys on human colon carcinoma cells and the first description of the anti-proliferative capacity of Torrontés wine pomace.
This study represents the first report on the cytotoxic evaluation of pomace from the Calchaquí Valleys on human colon carcinoma cells and the first description of the anti-proliferative capacity of Torrontés wine pomace.

3.2.3. Toxicity

Considering that the analyzed extracts are derived from by-products of the wine industry and may harbor potential health benefits, it becomes crucial to assess their toxicity. This assessment employs two distinct experimental models: a holistic organism model utilizing Artemia salina and a eukaryotic cell model involving human red blood cells. Notably, at concentrations up to 1000 μg/mL, none of the extracts demonstrated toxicity towards red blood cells (data not shown). In the brine shrimp test, the Malbec and Torrontés pomace extracts exhibited no toxicity up to 500 μg/mL (Figure 2). Aligning with these results, polar extracts (both aqueous and alcoholic) from red grape pomace of Malbec and Syrah varieties in the Cuyo region of Argentina (Mendoza) did not induce toxicity in fish (Danio rerio) and crustaceans (Artemia salina) up to a concentration of 500 μg/mL. Similarly, no toxicity was observed in a murine macrophage cell line (RAW 264.7) up to a concentration of 1000 μg/mL [55]. In the case of hydroalcoholic extracts derived from white grape pomace (Falanghina) and red grape pomace (Tintilia and Vernaccia Nera di Serrapetrona) from Italy, the toxicity limits surpassed 40 mg/mL. In contrast, for the Sagrantino red variety, the toxic threshold was determined to be greater than 2 mg/mL in the brine shrimp test [56].

3.2.4. Enzyme Inhibition

Skin aging often leads to pigmentation disorders, prompting the cosmetic industry to seek anti-hyperpigmentation compounds. These disorders occur due to the melanin accumulation, which is influenced by various factors. Therefore, inhibiting the melanin production by blocking the enzyme tyrosinase is a key strategy for skin-whitening products, being flavonoids promising compounds for this field [57]. Exploiting the bioactives contained in grape pomaces to obtain high-value cosmetics may support the growth of innovative start-ups and expand the value chain of grapes [9]. In this study, Torrontés demonstrated no impact on this enzyme activity up to 200 µg/mL concentration. Conversely, Malbec pomace displayed a dose-dependent inhibitory effect, leading to an approximately 90% decrease in tyrosinase activity at the same concentration (200 µg/mL) (Figure 3). The IC50 value for the Malbec extract was 89.9 ± 2.1 µg/mL. For kojic acid, a well-established tyrosinase inhibitor used as a reference, the IC50 was 0.37 ± 0.03 µg/mL. In comparison, the IC50 reported for Tempranillo (red variety) pomace extract (ethanol 50%) from Valladolid (Spain) was 4000 µg/mL [6]. Additionally, an ethanol extract (0.3 mL aliquots) of a mixture of white grapes (Trebbiano and Verdicchio) pomaces demonstrated a 79% reduction of the tyrosinase activity [58]. Extracts from red grape stems of six grape varieties (1 mg/mL) inhibited the tyrosinase enzyme activity from 41.47% to 53.83%, with the Syrah variety exhibiting the highest activity [59]. Furthermore, it is noteworthy that certain flavonoids, including kaempferol, catechin, myricetin, and quercetin, among others, have been identified as inhibitors of tyrosinase in previous studies [6,58]. The higher content of flavonoid-type compounds in the Malbec extract could elucidate its superior ability to inhibit this enzyme. These results suggest that Malbec pomace from the Calchaquí Valleys is a valuable source of natural ingredients for cosmeceutical applications.
5-lipoxygenase (5-LOX) governs a critical biosynthetic pathway in generating eicosanoids. The ultimate product of the 5-LOX pathway, leukotriene B4 (LTB4), is a mediator in several diseases. Inhibitors of 5-LOX exhibit therapeutic potential for various inflammatory conditions, including asthma, allergy, and atherosclerosis [60]. The pivotal role of LOX and its derivatives in tumor initiation and cancer metastasis is well-established. Heightened levels of 5-LOX have been discerned in diverse cancer cell lines, encompassing those linked to prostate, lung, colon, breast, and other cancers [61]. Thus, identifying compounds capable of inhibiting the LOX enzyme is a compelling focal point in the quest for bioactive natural products with potential anticancer properties.
Figure 4 illustrates the kinetics of hydroperoxide production by the LOX enzyme varying concentrations of pomace extracts. Both compounds exhibit a dose-dependent inhibition of LOX activity. Based on dose-response curves, the extract concentration resulting in a 50% activity reduction (IC50) was estimated to be 154.7 ± 4.1 and 784.7 ± 18.2 µg DPE/mL for Malbec and Torrontés, respectively, indicating that the Malbec extract is a more potent inhibitor of LOX than Torrontés extract. The IC50 values for the positive control employed, namely quercetin and gallic acid, were 48.4 ± 1.9 and 54.1 ± 0.5 µg/mL, respectively. Grape pomace extracts from Montepulciano d’Abruzzo (Italy) red wine displayed dose-dependent LOX inhibition ranging from 23% to 47% at tested concentrations of 10 and 100 µg/mL, respectively [62]. Previous studies have indicated a positive correlation between LOX inhibition and the concentrations of gallic acid, vanillic acid, p-coumaric acid, catechin, epicatechin, and rutin in pomace [63]. In the present work it was observed that Malbec pomace exhibited higher levels of most of these compounds, potentially accounting for its fivefold greater capacity to inhibit this enzyme.
The xanthine oxidase inhibitors have potential as anti-gout agents. Hyperuricemia, a metabolic anomaly characterized by the excess production of uric acid or its insufficient excretion, often leads to gout, marked by elevated serum urate and the simultaneous accumulation of urate crystals in bones or joints. Xanthine oxidase converts hypoxanthine to xanthine and, subsequently, produces uric acid. Effective strategies for gout prevention and recovery include xanthine oxidase inhibitors. Grape polyphenols, including cinnamic acid derivatives, syringic acid, ellagic acid, caffeic acid, and ferulic acid, are considered to contribute to the inhibition of xanthine oxidase activity, as mentioned in a review of several in vitro studies [64]. Despite the potential of phenolic compounds and flavonoids in mitigating the conditions associated with hyperuricemia, in the trials performed none of the pomace extracts was able to inhibit the enzyme up to a concentration of 250 µg/mL. This study marks the first report on the evaluation of wine pomace from the Calchaquí Valleys concerning LOX, tyrosinase, and xanthine oxidase enzymes.

4. Conclusion

In this study, we identified 35 phenolic compounds in the hydroalcoholic extracts derived from the pomace of Malbec and Torrontés wines from the Calchaquí Valleys of Argentina. Both extracts exhibited significant antioxidant activity, with Malbec showing superior antiradical activity, reducing power, hypochlorite scavenging, and iron-chelating capacity. Additionally, Malbec extract demonstrated the ability to inhibit tyrosinase, an enzyme affecting the skin, and the pro-inflammatory enzyme lipoxygenase. However, the Torrontés pomace extract was more effective against colon cancer cells.
These findings support the idea that both extracts could be considered potential functional ingredients with preventive properties against diseases. These extracts have potential applications in pharmacology, cosmetics, and the food industry. Therefore, it is imperative to conduct further comprehensive studies to validate their practical utilization. The exploitation of this byproduct has the potential to impact the local economy significantly.

Author Contributions

Pablo Ezequiel Tapia: Performed the experiments, Analyzed the data, Wrote the paper. Ana Margarida Silva: Performed the experiments, Analyzed the data. Cristina Delerue-Matos: Performed the experiments, Analyzed the data. Manuela Moreira: Performed the experiments, Analyzed the data. Francisca Rodrigues: Conceived and designed the experiments, Analyzed the data, Wrote the paper. Romina Torres Carro: Performed the experiments; María Daniela Santi: Analyzed the data, María Gabriela Ortega: Conceived and designed the experiments, Analyzed the data; María Amparo Blázquez: Analyzed the data. Mario Eduardo Arena: Conceived and designed the experiments, Analyzed the data, Wrote the paper, María Rosa Alberto: Conceived and designed the experiments, Analyzed the data, Wrote the paper, Conceived and initiated the project.

Funding

The authors acknowledge the financial support from the SCAIT-UNT (PIUNT D702 y D708), the Agencia Nacional de Promoción Científica y Técnica ANPCyT (PICT 2018-02071 and 02514, PICT 2021-0060, PICT-2021-I-A-00439 I), The Consejo Nacional de Investigaciones Científicas y Técnicas, CONICET (PUE 0021), ANPCyT BID-PICT 1576 and 2417 and SECYT-Universidad Nacional de Córdoba (05/C375). This work also received financial support from project UIDB/50006/2020 and UIDP/50006/2020 through national funds.

Data Availability Statement

The datasets used and/or analyzed during the current study are available on reasonable request.
Ethics declarations.

Ethics approval

Not applicable.

Consent to participate

All the authors have approved the final version of the manuscript for publication.

Consent for publication

All the authors have approved the final version for publication.

Acknowledgments

Ana Margarida Silva is thankful for the Ph.D. grant (SFRH/BD/144994/2019) financed by POPH–QREN and subsidized by the European Science Foundation and Ministério da Ciência, Tecnologia e Ensino Superior. Manuela M. Moreira (CEECIND/02702/2017) and Francisca Rodrigues (CEECIND/01886/2020) are thankful for their contracts financed by FCT/MCTES – CEEC Individual Program Contract. The authors also are grateful to Albarossa cellar for providing the wine pomace.

Competing interests

The authors declare no competing interests.

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Figure 1. Saccharomyces cerevisiae survival in presence of different pomace extract concentrations (from 12.5 to 150 µg DPE/mL). Different letters indicate significant differences between treatments (p < 0.05), according to Tukey’s test.
Figure 1. Saccharomyces cerevisiae survival in presence of different pomace extract concentrations (from 12.5 to 150 µg DPE/mL). Different letters indicate significant differences between treatments (p < 0.05), according to Tukey’s test.
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Figure 2. Artemia salina survival in absence and presence of different pomace hydroalcoholic extract concentrations (µg DPE/mL). Results are expressed as mean ± standard deviations. Different letters indicate significant differences between samples (p < 0.05) according to Student’s t test.
Figure 2. Artemia salina survival in absence and presence of different pomace hydroalcoholic extract concentrations (µg DPE/mL). Results are expressed as mean ± standard deviations. Different letters indicate significant differences between samples (p < 0.05) according to Student’s t test.
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Figure 3. Tyrosinase inhibition by Malbec pomace hydroalcoholic extract. Results are expressed as mean ± standard deviations. Different letters mean significant differences between concentrations (p<0.05), according to Tukey’s test.
Figure 3. Tyrosinase inhibition by Malbec pomace hydroalcoholic extract. Results are expressed as mean ± standard deviations. Different letters mean significant differences between concentrations (p<0.05), according to Tukey’s test.
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Figure 4. Lipoxygenase inhibition by different concentrations (µg DPE/mL) of hydroalcoholic extracts of Malbec and Torrontés pomace. Results are expressed as mean ± standard deviations.
Figure 4. Lipoxygenase inhibition by different concentrations (µg DPE/mL) of hydroalcoholic extracts of Malbec and Torrontés pomace. Results are expressed as mean ± standard deviations.
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Table 1. Polyphenol composition of the extracts.
Table 1. Polyphenol composition of the extracts.
Phytochemical group Malbec Torrontés
mg/g DPE mg/g DPE
Total Phenolics (GAE) 156.01 ± 3.49a 19.91 ± 1.21b
Hydroxycinnamic acids (CAE) 11.39 ± 0.32a 0.47 ± 0.01b
Orthodiphenols (CAE) 31.79 ± 0.62a 4.71 ± 0.28b
Anthocyanins (C3GE) 6.30 ± 0.49a <LOQ
Non-flavonoid phenolics (GAE) 30.49 ± 1.15a 8.01 ± 0.94b
Tannins (CE) 23.20 ± 1.30a 17.37 ± 0.47b
Total flavonoids (QE) 327.25 ± 6.30a 43.67 ± 1.39b
Flavones/Flavonols (QE) 73.56 ± 1.41a 1.17 ± 0.07b
Flavanones/Dihydroflavonols (NE) 63.65 ± 5.56a 10.10 ± 0.85b
DPE: dry pomace extract. DP: dry pomace. GAE: Gallic Acid Equivalents. CAE: Caffeic Acid Equivalents. QE: Quercetin equivalents. NE: Naringenin equivalents. CE: Catechin Equivalents C3GE: Cyanidin-3-glucoside Equivalents. LOQ: Limit of quantification. Results are expressed as mean ± standard deviations. Different letters in the same row indicate significant differences between samples (p < 0.05) according to Student’s t test.
Table 2. Phenolic compounds quantified in wine pomace samples through HPLC-DAD.
Table 2. Phenolic compounds quantified in wine pomace samples through HPLC-DAD.
Phenolic compound Retention time mg/100 g DPE mg/100 g DP
(min) Malbec Torrontés Malbec Torrontés
Phenolic acids
Gallic acid 5.618 245.0 ± 12.0a 89.3 ± 4.5b 39.2 ± 1.9a 65.2 ± 3.3b
Protocatechuic acid 9.935 700.0 ± 35.0a 71.2 ± 3.6b 112.0 ± 5.6a 51.9 ± 2.6b
Neochlorogenic acid 10.219 6.1 ± 0.3a 1.9 ± 0.1b 0.9 ± 0.1a 1.4 ± 0.1b
Caftaric acid 15.436 <LOQ 90.6 ± 4.5 <LOQ 66.1 ± 3.3b
Chlorogenic acid 17.869 6.6 ± 0.3a 6.8 ± 0.3a 1.1 ± 0.1a 5.0 ± 0.2b
4-O-caffeoylquinic acid 19.897 130.0 ± 6.0a 118.0 ± 6.0a 20.8 ± 1.0a 86.1 ± 4.4b
Vanillic acid 20.748 ND ND ND ND
Caffeic acid 21.224 6.7 ± 0.31a 18.7 ± 0.9b 0.9 ± 0.1a 13.7 ± 0.7b
Syringic acid 22.283 38.6 ± 1.9a 27.6 ± 1.4b 6.2 ± 0.3a 20.2 ± 1.0b
p-Coumaric acid 33.758 28.2 ± 1.4a 36.7 ± 1.8b 4.5 ± 0.2a 26.8 ± 1.3b
trans-Ferulic acid 37.289 45.7 ± 2.3a 74.2 ± 3.7b 7.3 ± 0.4a 54.2 ± 2.7b
Sinapic acid 37.662 108.0 ± 5.0a 89.6 ± 4.5b 17.3 ± 0.8a 65.4 ± 3.3b
3,5-di-O-caffeoylquinic acid 50.127 7.2 ± 0.4a 45.0 ± 2.2b 1.2 ± 0.1a 32.9 ± 1.6b
Ellagic acid 55.284 33.4 ± 1.7 ND 5.3 ± 0.3 ND
4,5-di-O-caffeoylquinic acid 56.781 50.7 ± 2.5a 258.0 ± 13.0b 8.1 ± 0.4a 188.3 ± 9.5b
Cinnamic acid 58.47 ND ND ND ND
Flavonoids
(+)-Catechin 14.143 618.0 ± 31.0a 70.1 ± 3.5b 98.9 ± 5.0a 51.2 ± 2.6b
(-)-Epicatechin 23.294 43.2 ± 2.2a 17.2 ± 0.9b 6.9 ± 0.4a 12.6 ± 0.7b
Naringin 49.847 31.9 ± 1.6a 54.6 ± 2.7b 5.1 ± 0.3a 39.9 ± 2.0b
Quercetin-3-O-galactoside 52.177 25.2 ± 1.3a 43.8 ± 2.2b 4.0 ± 0.2a 32.0 ± 1.6b
Quercetin-3-O-glucopyranoside 52.735 ND ND ND ND
Rutin 53.284 19.1 ± 1.0a 16.4 ± 0.8b 3.1 ± 0.2a 12.0 ± 0.6b
Phloridzin 54.355 32.3 ± 1.6a ND 5.2 ± 0.3 ND
Myricetin 57.943 17.6 ± 0.9a 18.9 ± 0.9a 2.8 ± 0.1a 13.8 ± 0.7b
Quercitrin 59.07 ND ND ND ND
Kaempferol-3-O-glucoside 59.466 ND 116.0 ± 6.0 ND 84.7 ± 4.4
Kaempferol-3-O-rutinoside 60.01 <LOD 66.6 ± 3.3 <LOD 48.6 ± 2.4
Isorhamnetin-3-O-glucoside 60.277 ND 95.6 ± 4.8 ND 69.8 ± 3.5
Isorhamnetin-3-O-rutinoside 61.568 24.2 ± 1.2a 10.2 ± 0.5b 3.9 ± 0.2a 7.4 ± 0.4b
Naringenin 68.149 <LOD <LOD <LOD <LOD
Quercetin 71.031 18.6 ± 0.9a 11.4 ± 0.6b 3.0 ± 0.1a 8.3 ± 0.4b
Phloretin 72.269 <LOQ <LOD <LOQ <LOD
Tiliroside 76.233 22.7 ± 1.1 <LOQ 3.6 ± 0.2 <LOQ
Kaempferol 79.854 3.4 ± 0.2a 4.4 ± 0.2b 0.6 ± 0.1a 3.2 ± 0.2b
Apigenin 81.44 <LOD <LOD <LOD <LOD
Chrysin 90.832 <LOD <LOD <LOD <LOD
Stilbenoids and others
trans-Polydatin 39.182 18.9 ± 0.9a 3.6 ± 0.2b 3.0 ± 0.1a 2.6 ± 0.1b
Resveratrol 52.507 ND ND ND ND
trans-Epsilon viniferin 69.158 6.5 ± 0.3a 6.2 ± 0.3a 1.0 ± 0.1a 4.5 ± 0.2b
DPE: dry pomace extract. DP: dry pomace. Results are expressed as mean ± standard deviations. LOQ: limit of quantification; LOD: limit of detection; ND: not detected. Different letters in the same row indicate significant differences between samples (p < 0.05) according to Student’s t test.
Table 3. Antioxidant capacity of wine pomace hydroalcoholic extracts.
Table 3. Antioxidant capacity of wine pomace hydroalcoholic extracts.
Sample Phosphomolybdenum reducing capacity
(μgAAE/mg DPE)		 Cupric reducing capacity
(μgGAE/mg DPE)		 ABTS•+
scavenging
IC50 (μg/mL)		 NO
scavenging IC50 (μg/mL)		 Fe+3
reducing RC50 (μg/mL)		 Iron
chelating
CC50 (μg/mL)		 O2●-
scavenging
IC50 (µg/mL)		 HOCl
scavenging
IC50 (µg/mL)
Malbec 178.57 ± 4.99a 171,18 ± 2,2a 7.79 ± 0.17a 414.19 ± 5.79b 10.22 ± 0.16a 41.82% ± 0.48%* 74.17 ± 4.12a,b 6.71 ± 0.36b
Torrontés 4.74 ± 0.16b 26,12 ± 0,52b 49.5 ± 1.46b 15.34% ± 0.78%** 84.62 ± 0.95b 11.28% ± 1.05%* 874.61 ± 15.71c 27.40 ± 0.19c
Controls
BHT - - - - 11.37 ± 0.13a - - -
Trolox - - 3.74 ± 0.06a - - - - -
Ascorbic acid - - - 36.13 ± 6.01a - - - -
EDTA - - - - - 13.97 ± 0.06 - -
Catechin - - - - - - 99.21 ± 0.85b 0.095 ± 0.006a
Gallic acid - - - - - - 52.49 ± 1.58a 0.82 ± 0.06a
Different letters in the same column show significant differences among each treated group, according to Tukey test (p≤0.05). IC50 = Concentration required to decrease in 50% the reactivity of the reactive species in the tested media (mean ± standard error of the mean). Phosphomolybdenum reducing capacity expressed as micrograms of Ascorbic acid Equivalentes per milligram of DPE (dry pomace extract) (µg AAE/mg DPE). Cupric reducing antioxidant capacity expressed as micrograms of Gallic acid Equivalents (μg GAE/mg DPE). Fe3+ Reducing Capacity (RC), ABTS radical cation (ABTS∙+), Nitric oxide (NO), Superoxide anion radical (O2●-) and hypochlorous acid (HOCl) Scavenging Capacities (IC). Iron Chelating capacity (CC) determined by linear regression analysis. *Inhibition percentage with the concentration of 1000 µg/mL. **Inhibition percentage with the concentration of 250 µg/mL.
Table 4. Effects of wine pomace samples, exposure on the viability of HT29-MTX and Caco-2 cells at different concentrations as measured by the MTT assay (n = 3).
Table 4. Effects of wine pomace samples, exposure on the viability of HT29-MTX and Caco-2 cells at different concentrations as measured by the MTT assay (n = 3).
Cell Viability (%)
Concentration
(µg DPE/mL)		 HT29-MTX cells Caco-2 cells
Malbec Torrontés Malbec Torrontés
0.1 132.25 ± 10.18a 109.33 ± 19.90a 120.67 ± 6.92a 70.29 ± 10.03b
1.0 133.03 ± 12.93a 110.34 ± 9.63a 79.08 ± 6.94b 65.14 ± 14.27b
10 131.85 ± 14.80a 103.57 ± 16.69a 82.82 ± 11.80b 66.85 ± 7.36b
100 122.19 ± 16.94a 66.87 ± 13.06b 88.48 ± 12.45b 66.85 ± 10.52b
1000 104.75 ± 23.03b 33.56 ± 4.38c 81.26 ± 12.83b 52.51 ± 1.53c
Medium 100.00 ± 8.86a
Triton X-100 0.00 ± 0.00
Different letters mean significant differences between concentrations of the same extract (p<0.05), according to Tukey’s test.
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