Formulation of Novel Liqueurs from Juice Industry Waste: Consumer Acceptance, Phenolic Profile and Preliminary Monitoring of Antioxidant Activity and Colour Changes During Storage

Chemicals and raw materials

Folin-Ciocalteau reagent, sodium carbonate, sodium acetate trihydrate, acetic acid, hydrochloric acid, sodium hydroxide and phenolphthalein were obtained from Merck (Darmstadt, Germany), DPPH (2,2-diphenyl-1-picrylhydrazyl) from Fluka (Buchs, Switzerland), Trolox (6-hydroxy-2,5,7,8-tetramethylchromane-2-carboxylic acid), 2,4,6-tripyridyl-s-triazine (TPTZ) and gallic acid from Sigma-Aldrich, Merck (Munich, Germany), ethanol 96% from Ada Vrenje (Belgrade, Serbia), glycerol from Oleohemija (Belgrade, Serbia), while citric acid was purchased on the local market. Glucose, fructose and sucrose were acquired from Tokyo Chemical Industry, TCI (Zwijndrecht, Belgium). All aqueous solutions were prepared using ultrapure water (Thermo Fisher TKA MicroPure water purification system, ϰ=0.055 µS/cm; Thermo Fisher Scientific, Bremen, Germany). Phenolic standards (protocatechuic, p-hydroxybenzoic, ellagic, chlorogenic, caffeic, p-coumaric, ferulic and sinapic acids, rutin, naringin, pterostilbene, aesculin, quercetin, quercetin-3-O-rhamnoside, quercetin-3-O-galactoside, isorhamnetin and isorhamnetin-3-O-rutinoside) were supplied by Sigma-Aldrich, Merck (Steinheim, Germany).

The company Healthy Organic (Selenča, Serbia) provided apple and beetroot pomace, while chokeberry pomace was acquired from the family farm of D. M. Perić (Belgrade, Serbia). Wet pomace, collected immediately after juice production, was dried at the industrial scale level at 55 °C using the dehydrator Solaris (NTIM Tehnology, Belgrade, Serbia) and ground in an industrial mill to produce a fine powder that is easy to preserve, store, transport and use as a food ingredient (15,16).

Liqueur preparation

For the preparation of the liqueurs, a traditional procedure involving a pilot-scale maceration was used, including two blending tanks with agitation systems (30 L), located at the experimental farm Radmilovac (Faculty of Agriculture, University of Belgrade, Serbia). In the first tank, powdered pomace was macerated in a water-alcohol mixture (φ(alcohol)=40%) for 24 h at (20±2) °C. The pomace to solvent ratio was 1:10 (m/V). Extracts obtained after decanting and filtration through disc filters Fibrafix AF31H (12-5.0 μm retention rate; Filtrox AG, St. Gallen, Switzerland) were transferred into the second tank and commercial sugar (Crvenka a.d., Crvenka, Serbia) and water were added to obtain 150 g/L sugar and a final φ(alcohol)=20%. Citric acid (1 g/L) was added to achieve a sweetness-sourness balance and glycerol (2 mL/L) was used as a body enhancer. Apple pomace liqueur, chokeberry pomace liqueur, a mixture of the two in a 50:50 ratio and a combination of beetroot pomace liqueur with apple pomace liqueur in the 30:70 ratio were formulated. Beetroot was used only in combination to mitigate its pronounced, undesirable earthy flavour.

Physicochemical properties of fresh pomace liqueurs

The turbidity of the analysed liqueurs was determined with a portable turbidimeter (model 2100Q; Hach, Loveland, CO, USA). The results of turbidity measurement are expressed as formazin turbidity with a reading range between 0 and 1000 nephelometric turbidity units (NTU). Non-volatile and volatile acidity (g/L) were determined according to AOAC method 945.08 (17), while the pH was measured by WTW Multi 9310 apparatus (WTW, Weilheim, Germany).

Determination of sugars in fresh pomace liqueurs

The liqueurs were filtered through 0.22-µm filter and the filtrate was analysed using the HPAEC-PAD technique on an ISC 3000 DP liquid chromatograph (Dionex, Sunnyvale, CA, USA) equipped with a quaternary gradient pump (Dionex, Sunnyvale, CA, USA) according to the procedure reported by Vasić et al. (18). The total amount of each sugar compound was calculated from the corresponding calibration curve and expressed in g/L. The linear range was 0.01-0.1 g/L with correlation coefficients over 0.998. The recovery was between 92 and 108%. The limit of detection was from 0.0012 to 0.0034 g/L and the limit of quantification between 0.004 and 0.01 g/L. The precision was lower than 3% and accuracy was around 97%.

Sensory quality rating of fresh pomace liqueurs

The sensory quality of the freshly prepared liqueur samples was assessed in the sensory testing laboratory by a 6-member panel (35-60 years old; 4 male and 2 female) consisting of staff members from the Faculty of Agriculture, University of Belgrade, Serbia, experienced in alcoholic beverage quality judging. The samples were labelled with random 3-digit codes and presented to the panellists monadically in random order. Low sodium bottled water was used for palate cleansing. Overall sensory quality was assessed by evaluating five selected sensory characteristics: colour, clarity, distinction, odour (orthonasal olfaction) and flavour, which were rated using category scales with score ranges 0-1, 0-1, 0-2, 0-6 and 0-10, respectively. The quality of the beverages was rated as follows: excellent quality (quality score>18), very good quality (16-18), good quality (14-16), poor/unsatisfactory quality (12-14) and very poor quality (score≤12). The overall quality score, with a maximum value of 20, was calculated by adding the quality scores of the five individual characteristics. The panel evaluated all of the samples once.

Consumer sensory testing of pomace fresh liqueurs

Consumer acceptance tests were performed in a sensory testing laboratory by 143 students (21-25 years old; 92 female and 51 male) from the Faculty of Agriculture, University of Belgrade. The students were randomly selected, provided that they were relatively frequent (at least occasional) consumers of alcoholic beverages. The samples were labelled with random 3-digit codes and presented to the consumer panel monadically in random order. Low sodium bottled water was used for palate cleansing. Overall acceptance, appearance, odour and flavour acceptance were assessed using the 9-point hedonic scale (1=dislike extremely, 5=neither like nor dislike, 9=like extremely). The just-about-right (JAR) scales (1=too little, 5=JAR, 9=too much) were used to evaluate the intensities of colour (too light/pale – JAR – too dark), sweetness (not sweet enough – JAR – too sweet), sourness (not sour enough – JAR – too sour) and alcoholic strength (too weak – JAR – too strong). In addition, 9-point attribute intensity scales were used to assess consumer perception of fullness of flavour (1=empty, 5=medium, 9=full) and distinctiveness of flavour (1=not at all, 5=medium, 9=completely characteristic).

Identification and quantification of phenolics in fresh pomace liqueurs by HPLC–DAD–MS/MS

After filtration of samples through a 0.22-µm filter, individual phenolic compounds were identified and quantified in the filtrate using a Dionex Ultimate 3000 UHPLC system equipped with a diode array detector connected to a TSQ Quantum Access Max triple quadrupole mass spectrometer (Thermo Fisher Scientific, Basel, Switzerland) with the ion source in the form of electrospray ionisation (200 °C) in the negative mode (from m/z=100 to 1000) using triple quadrupole (UHPLC-DAD-MS/MS), according to previously published procedure (19). The total amount of each compound was calculated from the corresponding calibration curve and expressed in mg/L. The linear range was 0.001-0.1 g/L, whereas the correlation coefficients were from 0.9945 to 0.9996. The recovery of the method was between 85 and 115%. The limit of detection was from 0.00001 to 0.00012 g/L, whereas the limit of quantification was in the range of 0.00005-0.00021 g/L. The precision was less than 5% and accuracy was in the range of 91 to 105%.

Determination of total phenolic concentration and antioxidant activity in fresh and stored pomace liqueurs

The total phenolic concentration of the prepared liqueurs was determined by the Folin-Ciocalteu method described by Singleton et al. (20). Properly diluted samples (0.5 mL) were mixed with 0.1 M Folin-Ciocalteu reagent (2.5 mL), then 2.5 mL sodium carbonate solution (75 g/L) were added after 6 min in the dark, the mixture was left for 2 h in the dark, after which the absorbance at 740 nm was measured using spectrophotometer (Thermo Scientific Evolution 600; Thermo Fisher Scientific Inc., Bremen, Germany), using distilled water as a blank. The results were expressed in gallic acid equivalents (GAE) per litre of liqueur. The antioxidant capacity was determined by DPPH and ferric reducing antioxidant power (FRAP) assays, using procedures described by Blois (21) and Benzie and Strain (22) respectively. Diluted samples (0.2 mL) were mixed with 2.8 mL ethanolic solution of DPPH (0.1 mM) and acetate buffer (0.1 M) in the volume ratio 2:1, and the mixture was allowed to react for 30 min in the dark before absorbance measurement at 517 nm against distilled water (Thermo Scientific Evolution 600; Thermo Fisher Scientific Inc). Diluted samples (0.1 mL) were mixed with distilled water (0.3 mL) and freshly made FRAP reagent (3 mL), incubated for 40 min at 37 °C and the absorbance was measured against the reagent blank at 593 nm. The results of DPPH and FRAP were expressed in mM Trolox equivalent (TE) per litre of the sample. Measurements were performed on the first day (no storage) and upon each month during six months of liqueur storage at (20±2) °C in a dark place and in a refrigerator (4 °C). All measurements were performed in triplicate.

Colour measurements in fresh and stored pomace liqueurs

Colour intensity (CI) and hue (h) were determined according to Glories (23). Liqueurs were diluted to 1:10 with 20% ethanol, centrifuged for 5 min at 3000×g using centrifuge (Tehtnica, Železniki, Slovenia) and absorbance was measured at 420, 520 and 620 nm in a 1-cm cell path using a spectrophotometer (Thermo Scientific Evolution 600; Thermo Fisher Scientific Inc). CI was calculated as:

whereas hue (h) was calculated as:

Measurements were performed on the first day (no storage) and upon each month during six months of liqueur storage at (20±2) °C in a dark place and in a refrigerator (4 °C).

Statistical analysis

The total phenolic content, antioxidant capacity, colour intensity and hue were measured in triplicate and the results are presented as mean value±standard deviation (S.D.). The data related to total phenolic content, antiradical activity (DPPH), total reducing power (FRAP), and analytical colour measurements (colour intensity and hue) were subjected to principal component analysis (PCA). PCA was performed on the unfolded data matrix which included all replicate measurements. Upon dimension reduction, when it was clear that the first extracted principal component (PC1) was sufficient enough to satisfactorily explain the variations in the data matrix, PC1 scores for samples were subjected to 3-way ANOVA (PC-ANOVA) (24) with product/pomace, storage time and storage temperature taken as fixed factors. Also, another PC-ANOVA model, followed by Tukey’s honestly significant difference (HSD) test, was applied in order to separate the mean PC1 scores for samples.

Sensory quality and acceptance (hedonic and attribute intensity) data were subjected to 2-way ANOVA with samples as a fixed factor, and assessors as a random factor. Tukey's HSD test was used to separate the mean values of samples.

Mean drop analysis was performed by combining the JAR data with the overall hedonic data, as described by Rothman and Parker (25), in order to assess the potential impact of being off from just-about-right on the overall acceptability of the liqueurs. Raw JAR scores were grouped into three categories as follows: 1, 2 and 3=below JAR; 4, 5 and 6=JAR; and 7, 8 and 9=above JAR. Mean drop values were calculated by subtracting the overall mean hedonic scores of each below/above JAR category from the hedonic mean of the JAR category. ANOVA and Tukey's HSD test were used in order to compare the overall hedonic mean values of the JAR and non-JAR categories. Minimum percentage skew for ‘not just right’ (the cut-off) was set at 20% of the total consumer panel.

Statistical analyses were performed using SPSS Statistics v. 17.0 (26). The level of statistical significance was set at 0.05.

Physicochemical properties and sugar content of fresh pomace liqueurs

The results of physicochemical analysis (turbidity, pH, non-volatile and volatile acidity) and quantitative sugar profile of liqueurs are summarized inTable 1. The highest value of turbidity was determined in the apple/beetroot pomace liqueur (250.4 NTU), followed by apple pomace liqueur (240.0 NTU) and apple/chokeberry pomace liqueur (229.8 NTU), whereas the lowest value was ascribed to chokeberry pomace liqueur (102.6 NTU). Apple pomace is a rich source of compounds with colloidal properties (i.e. dietary fibre), so as expected, liqueurs produced with this raw material showed higher turbidity (27).

Herein, the obtained pH values of prepared liqueurs were between 3.30 (apple pomace liqueur) and 3.72 (apple/beetroot pomace liqueur). Corroborating the obtained results, the pH values of differently prepared apple wines, reported by Won et al. (28), were lower than 4. Also, pH values of a variety of chokeberry products ranged from 3.31 to 4.28 (29). The pH value of apple/beetroot liqueur (3.72) was similar to the pH of beetroot-based wines (3.56-4.00) reported by Singh et al. (30) and (3.45-3.80) reported by Soibam et al. (31).

No marked difference was evident in the obtained values for non-volatile and volatile acids in all analysed liqueurs. The mass concentration of non-volatile malic acid ranged from 2.48 to 2.84 g/L, whereas the mass concentration of volatile acetic acid was from 0.16 to 0.33 g/L. These results are in line with the values for the total acidity of apple liqueurs (1.16-5.82 g/L) reported by Díez Marqués et al. (32). Liqueurs are alcoholic beverages produced without fermentation, so, expectedly, the volatile acidity is low. On the other hand, acidity regulators such as citric acid, added in the tested samples, in addition to malic and citric acids originating from the apple, also contribute to the pronounced total acidity (32).

As expected, the most abundant sugars in freshly prepared liqueurs detected by HPAEC-PAD technique were glucose, fructose and sucrose. Due to the significant amount of added sugar (150 g/L), the concentration of sucrose was expectedly the highest in all samples when compared to glucose and fructose. As shown inTable 1, there is no significant difference in the total sugar concentration among all analysed liqueurs, which can be explained by the different ratios of individual sugars (glucose, fructose and sucrose) in apple, chokeberry and beetroot pomace. Indeed, the absence of sucrose in cultivated black chokeberries is an important characteristic of its sugar profile (33), while beetroot is a valuable source of sucrose and a scarce source of glucose and fructose (34). In the case of the apple-based samples (apple, apple with chokeberry and apple/beetroot pomace liqueurs), the concentration of fructose was higher than glucose, which is in agreement with a previous study (35). The fresh chokeberry fruit contains a slightly higher concentration of glucose than fructose (8), which is also found in the liqueur prepared with chokeberry pomace.

Sensory properties of fresh pomace liqueurs

According to the results of the sensory quality rating of the liqueurs (Table 2), it seems that selected sensory characteristics were rated in a similar way over the spectrum of the evaluated products. The mean odour quality score for apple/beetroot pomace liqueur (4.4±0.5) was significantly lower (p<0.05) than the other three liqueurs placed within the same homogenous subset. The main defects regarding its odour were the undesirable aroma and flavour linked to an earthy note known to be caused by the volatile bicyclic alcohol geosmin (trans-1,10-dimethyl-trans-9-decalol) (36). The lowest mean overall sensory quality score was obtained for the apple/beetroot liqueur (16.6±0.7), noting that the value differed significantly (p<0.05) from the chokeberry only liqueur, which was the best rated (17.6±0.9). The uniqueness of chokeberry liqueur can be explained by the sensory experts’ additional notes that its flavour and odour were characterised by an appealing and desirable sour cherry aroma. Regardless of the difference, all mean overall quality scores (16.6-17.6) were in the range of ‘very good quality’.

The results of testing the likeability of the liqueurs are shown inTable 3. The overall acceptance, odour and flavour mean hedonic scores of apple/beetroot liqueur (4.5, 4.5 and 4.3, respectively) were in the range of neutral consumer attitude, i.e. ’neither like nor dislike‘ and were significantly lower (p<0.05) than the scores of the other liqueurs that were found in the range of ‘liking’ (≥6.0). On the other hand, by using a 9-point attribute intensity scale, consumers perceived ‘fullness’ and ‘distinctiveness’ of apple/beetroot liqueur flavour at the same intensity level (p>0.05). These results, together with the results of sensory quality testing, indicate that lower hedonic scores for this liqueur were not the result of a lack of flavour, but can most probably be directly linked to the acceptability of the typical earthy, leafy and neutral flavour of beetroot in alcoholic spirits. This conclusion is also supported by the results of mean drop analysis (Fig. 1). There were three large groups of results among consumers (≥20%) for apple/beetroot liqueur tested. Significant mean drops of the overall hedonic scores (p<0.05) were observable, with the opinion that the product was ‘not sweet enough’ (29.4%), ‘not sour enough’ (23.8%), or it was ‘too weak’ (25.2%) in terms of alcohol level. When compared to the other liqueurs, no large consumer groups with significant mean drops were observed for the chokeberry pomace liqueur, whereas for the apple pomace liqueur sample, it can be seen that consumers complained that the product was ‘too sweet’ and ‘not sour enough’.

Fig. 1 Mean drop analysis (N(consumer)=143) for the freshly prepared liqueur samples. A circle in the plot that shows statistically significant mean drop and a large percentage of consumers (above 20% in this case) is a cause for concern and suggests that the product should be modified in the appropriate direction. Liqueurs from the pomace of: a) apple, b) chokeberry, c) apple and beetroot (70:30) and d) apple and chokeberry (50:50), mean drop=the drop of the mean hedonic score calculated as the difference between the ’just-about-right’ consumer group and the ’too much’ or ’not enough of an attribute’ consumer groups

The phenolic profile of fresh pomace liqueurs

The mass concentration of individual phenolics in liqueurs is shown inTable 4. Chokeberry-based liqueurs (chokeberry and apple/chokeberry liqueurs) seem to be the richest source of tested phenolics. In the study of Sokoł-Łȩtowska et al. (37) the amount of phenolic compounds in chokeberry liqueur was also predominant compared to cornelian cherry, black rose, blackcurrant, blackberry, raspberry, mahonia, sloe, strawberry and sour cherry liqueurs. The predominance of ellagic acid in chokeberry, apple/chokeberry and apple/beetroot liqueurs can be easily observed, with chokeberry and apple/chokeberry liqueurs containing by far superior concentrations. A high mass concentration of phlorizin was evident in all liqueurs containing apple pomace, as expected since it was suggested to be used as an apple pomace marker (19). Quercetin and its sugar derivatives were also present in significant amounts in all liqueurs, with chokeberry and apple/chokeberry liqueurs being the most endowed. According to previous studies, quercetin was the predominant flavonol in chokeberry (38). Also, chokeberry wine contained quercetin as the most abundant flavonoid, and represented the richest source of this flavonol, as well, when compared to some fruit wines such as blackberry wine, sour cherry wine, etc. (39). Corroborating the results obtained for apple pomace liqueur, quercetin was one of the major flavonols in apple pomace from several cultivars in which the presence of quercetin glycosides was observed, as well as the prevalence of galactoside over rhamnoside (19). Other phenolic compounds found in liqueurs in notable amounts are ferulic acid, 5-o-caffeoylquinic acid, protocatechuic acid, phloretin, p-hydroxybenzoic acid, rutin, p-coumaric acid and pterostilbene.

Total phenolic content and antioxidant capacity of fresh pomace liqueurs

All produced liqueurs showed notable total phenolic content at the time of preparation, with the following descending order of activities: chokeberry>apple/chokeberry>apple>apple/beetroot liqueur (Table 5). Total phenolic concentration (TPC) for chokeberry liqueur (expressed in gallic acid equivalents (GAE) of (3473±33) mg/L) was in line with the previous findings of Sokoł-Łȩtowska et al. (37), who showed chokeberry liqueur to be among the richest sources of substances reacting with the Folin-Ciocalteu reagent (3292 mg/L). The total phenolic concentration of sour cherry liquor was reported at comparable value (3360 mg/L (40)). In comparison with the total phenolic concentration of commercial Portuguese Terras Madeirenses red wines ((1724-1871) mg/L) (41), chokeberry and apple/chokeberry liqueurs showed almost double concentration, as well as far higher concentrations than those of various red and white wines from the Serbian market (164 to 2314 mg/L) (42). Similarly, when compared to the herbal bitter liqueur based on medicinal plant extracts (43) that contained a conclusively larger concentrations of phenolics (1500 mg/L) than similar commercial herbal spirits, chokeberry and apple/chokeberry liqueurs showed twice as high total phenolic concentration, as well as several times stronger antioxidant activity measured by DPPH and FRAP assays.

It can be noticed that the total phenolic concentration determined by Folin-Ciocalteu assay was higher than the sum of individual phenol concentrations quantified by HPLC. This is in line with previous studies that explained such result by the interference of various substances other than phenols (organic acids, residual sugars, amino acids, proteins and other hydrophilic compounds) in the Folin-Ciocalteu assay, various responses of individual phenols, presence of only low molecular mass phenols in extracts (5,19), as well as missing values of unidentified polyphenols by HPLC/MS.

A similar antioxidant activity of liqueurs measured by DPPH and FRAP assays was obtained as for total phenolic concentration, with chokeberry liqueur being by far the strongest radical scavenger ((28.0±0.7) and (58.9±0.5) mmol/L, respectively). However, in the case of results obtained by FRAP assay, it can be observed that apple/beetroot liqueur had slightly higher antioxidant potential than apple liqueur.

Preliminary evaluation of liqueur storability based on changes of total phenolics and antioxidant activity

The results of total phenolic concentration and antioxidant capacity trends of analysed liqueurs during six months of storage at two different temperatures are presented inTable 5. As evident, total phenolic concentration and antioxidant activity decreased during storage at 20 and 4 °C. However, the decrease differs among liqueurs. After six months, the amount of initial total phenolic content of apple, chokeberry, apple/chokeberry and apple/beetroot liqueurs stored at 4 and 20 °C decreased by about 75, 50, 70 and 80%, and by 70, 50, 70 and 77%, respectively. Throughout the entire storage period, the highest retention of phenolics was observed in chokeberry liqueur, which preserved a much higher concentration at the end of storage than the initial total phenolic concentration of apple and apple/beetroot liqueurs.

In all cases, with the exception of chokeberry liqueur stored at 4 °C, there were no significant differences in total phenolic concentrations after 5 and 6 months of storage, leading to the assumption that the decomposition of phenolic compounds is complete after 5 months.

The decrease of antioxidant activity of chokeberry and apple/chokeberry liqueurs during storage, measured by DPPH, was also the least prominent (by approx. 50%) compared to apple and apple/beetroot liqueur, where drops greater than 60% were observed. At the same time, antioxidant capacity reduction determined by FRAP method was between 65-85% for all analysed liqueurs.

There is scarce literature data on the possibility of utilisation of apple, beetroot and chokeberry pomace in the production of antioxidant-rich alcoholic or non-alcoholic beverages. In a study dealing with antioxidant activity of liqueurs made from ten red fruits, in the majority of samples, the concentration of phenolic compounds decreased over the considered periods (37). The same study demonstrated that chokeberry liqueur was among those with the highest phenolic concentration and antioxidant activity, and when stored at a temperature of 30 °C for 6 months it showed a significant reduction in activity (assayed with the DPPH test) of approx. 50% of the initial value (37). Walkowiak-Tomczak (44) reported that after 20 days under facultative anaerobic conditions, the antioxidant activity of black chokeberry juice concentrate solutions decreased by 7-12% at 10 °C, 12-15% at 20 °C and 16-35% at 30 °C, whereas under aerobic conditions the changes ranged from 63 to 76% after 10 days and from 64 to 79% after 20 days. Furthermore, phenolic compounds in myrtle liqueur showed considerable changes even when stored with constant headspace. The anthocyanins in particular, both total and free, tended to decrease (45).

The majority of spirits, including liqueurs, are commonly stored safely at room temperature since alcohol provides microbiological stability. Studies on a half-year period of sour cherry liqueur storage showed that their characteristic features are almost unchanged if stored at 15 °C and without sugar added, but organoleptic properties were better in samples stored at 30 °C (46). Here, different storage temperatures did not have a significant influence on the total phenolic concentration of chokeberry and apple/chokeberry liqueurs, but the total phenolic concentration of apple and apple/beetroot liqueurs was significantly higher after 6 months of storage at room temperature than in the refrigerator. It seems that the lower temperature might slightly decrease the solubility of phenolics, inducing their precipitation. However, the differences in the obtained values are not so prominent to enable a conclusion that room temperature is the most appropriate condition for storage of analysed liqueurs.

The strong correlation between total phenolic concentration and antioxidant capacity measured by DPPH and FRAP was confirmed by high correlation coefficients (0.978 and 0.966, respectively). Such a result indicates that the potent antioxidant capacity of the liqueurs is highly influenced by phenolics present in apple, beetroot and chokeberry pomace, as well as in the prepared mixtures, which corroborates the previous reports (40,42,47).

Preliminary evaluation of liqueur storability based on colour changes

Colour is one of the most important quality features of liqueurs with a huge influence on consumer preferences. The determination of the optimal storage conditions can prevent colour changes that consumers associate with food spoilage and can thus be crucial in preventing economic losses, especially in sales of new products. According to literature, the intense red colour of chokeberry liqueurs depends on the structure and concentration of anthocyanins (37). Apple skin colour is influenced by chlorophyll and carotenoids, anthocyanins, flavonols and proanthocyanidins, whereas the beetroot pomace is a rich source of red-coloured betacyanins and yellow pigment betaxanthin (48,49).

The colour intensity and hue of the analysed liqueurs are shown inTable 6. The significant difference in the chromatic characteristics of liqueurs is primarily due to the type and quantity of pomace pigment compounds.

The colour intensity of apple/chokeberry, chokeberry and apple/beetroot liqueurs decreased throughout the evaluated storage period, although the reduction was nonlinear. No particular trend of change in CI over time can be observed for apple liqueur, at both tested temperatures. Comparing the results obtained at the two tested temperatures, it can be observed that the lower temperature did not prevent the degradation of colour during storage.

Except in the case of apple liqueur, an increase in hue was observed during the evaluated storage period, indicating the growth in the percentage of the yellow colour and/or loss of the red colour. The colour of myrtle liqueur, evaluated according to the classic spectrophotometric parameters of intensity and hue, showed marked variability during storage in the bottles with increasing headspace, while values remained almost constant in unopened ones (45). The increase in values obtained for the yellow component and hue angle with the ageing time of berry fruit syrup wines with different pH values was previously linked to the formation of anthocyanin-derived yellow-orange pigments like pyranoanthocyanins, as well as to the oxidation of pigments. Also, the red component percentage in these wines decreased after 6 months of storage. The decrease was associated with the possible precipitation of insoluble polymeric anthocyanin-derived pigments, and/or the degradation of free anthocyanins caused by oxidation (50).

Principal component analysis

The results of principal component analysis (PCA) applied to the unfolded data matrix, derived from the antioxidant activity (total phenolic concentration, FRAP and DPPH) and colour measurements (hue and CI), showed that only the first extracted principal component had an eigenvalue larger than one, and according to both the Kaiser criterion and scree plot (51), PC1 was retained for describing objects in the new PC space explaining 87.8% of the variance in the data matrix values. All five initial variables had high PC1 loadings, indicating strong correlations of these attributes with PC1. The antioxidant activity variables (total phenolic concentration, FRAP and DPPH), together with colour intensity (CI), showed strong positive correlations (loading values 0.98, 0.96, 0.99 and 0.96, respectively), while hue showed strong negative correlation (-0.79) with PC1. Therefore, taking into account that greater values for total phenolic concentration, FRAP, DPPH and CI (i.e. greater positive values of PC1) indicated lower levels of the oxidation processes, PC1 was referred to as ‘antioxidant activity’ axis.

The results of ANOVA applied to PC1 scores showed that antioxidant activity was significantly affected (p<0.05) by all examined factors: type of pomace used, storage time and temperature. Also, all interactions among the factors were statistically significant. The plots of factor interactions are shown inFig. 2. The influence of the type of pomace used for liqueur preparation is consistent over different levels of the storage time factor (chokeberry>apple/chokeberry>apple>apple/beetroot liqueur), indicating a stronger influence of chokeberry pomace on the antioxidant potential of the liqueurs over the storage period. Chokeberry is among the richest plant sources of anthocyanins and possesses one of the highest antioxidant activities (8). Sokoł-Łȩtowska et al. (37) reported that the chokeberry liqueur was the richest in anthocyanins (1674 mg/L) among red fruit liqueurs.

Fig. 2 Storage time by type of product/pomace (by storage temperature) interaction profile plots as a result of three-way ANOVA (N=3) applied on PC1 scores, for the liqueur samples produced from apple, chokeberry and beetroot pomace stored for six months at: a) 4 °C or b) 20 °C. PCA included the chemical and objective colour variables. PC1 loading values were 0.98, 0.96, 0.99, -0.79 and 0.96 for total phenolic concentrations, FRAP, DPPH, hue and CI, respectively (the combination of these variables was referred to as ’antioxidant activity’). Values marked with the same lower-case letter within a liqueur sample are not statistically different (α=0.05). PC1 scores for control (freshly prepared) samples were 2.65, 1.29, -0.64 and -0.57 for chokeberry (CL), apple and chokeberry (50:50, ACL), apple (AL) and apple and beetroot (70:30, ABL) liqueurs, respectively

This trend for antioxidant activity over the storage period correlated with the level of antioxidant potential recorded for control (freshly prepared) samples. Mean PC1 scores for the samples after preparation differed significantly (p<0.05) from each other, in the same descending order as observed during the period of storage. Also, regardless of the storage temperature, the curves for chokeberry and apple/chokeberry liqueurs had slightly steeper slopes than apple and apple/beetroot liqueurs, which remained milder (Fig. 2). Although chokeberry and apple/chokeberry liqueurs showed lower total phenolic concentration and antioxidant activity reduction than initial values, according to PC1, the greater initial antioxidant activity expressed through total phenolic concentration, FRAP and DPPH, the greater the rate of their loss during six months of storage at both 4 and 20 °C. Although it has been noticed that sugar moiety stabilises anthocyanins (46), they are unstable pigments, easily oxidised, particularly in the presence of ascorbic acid (the most abundant vitamin in the black chokeberry fruit (8)) and products of its degradation. Polymerisation and condensation of polyphenols are also believed to be involved in these processes during prolonged storage (37). However, due to the variety of compounds interacting simultaneously, it is difficult to establish the exact mechanism of degradation of anthocyanins and other polyphenols.