Protein characterisation and antioxidant potential of fresh cheese obtained by kombucha inoculum

Materials

For the production of fresh cheese, pasteurized milk was used with milk fat content of 2.8%, manufactured by Mlekoprodukt AD from Zrenjanin. Milk inoculation was performed using different starter cultures: FD-DVS XPL-1 (Chr. Hansen A/S, Denmark) containing Lactococcus lactis subsp. cremoris, Lactococcus lactis subsp. lactis, Lactococcus lactis subsp. lactis biovar diacetylactis, Leuconostoc and Streptococcus thermophilus; and kombucha inoculum produced in laboratory conditions, cultivated on black tea (Camellia sinesis - 1.5 g/L) with the addition of saccharose concentration 70 g/L. 10% (v/v) of the inoculum from the previous fermentation was added to the tea cooled to room temperature. Incubation was performed at 25 °C during 7 days. The pH value of the kombucha inoculum was 4.72. Coagulation enzyme CHY-MAX®Powder Extra NB enzyme manufactured by Chr Hansen A/S from Denmark, (composition: sodium chloride, chymosin and casein peptone). Pepsin (with declared activity minimum 0.7 FIP U/mg) and pancreatin enzyme (with declared activity of 4 × USP specifications of units (0.03 N-benzoyl-L-tyrosine ethyl ester, BTEE (N-benzoyl-L-tyrosine ethyl ester) units/mg), were obtained from AppliChem (Darmstadt, Germany) and Sigma (St. Louis MO, USA), respectively. Reagents and solutions used in the analysis are: solution A (2% Na₂CO₃; 0.02% K, Na tartrate in 0.1M NaOH), solution B (0.5% copper sulphate), solution C: mix A and B in a ratio of 50:1 and Folin-Ciocalteu reagent (dilute 1:2 with distilled water).

Fresh cheese manufacture

Fresh cheese was produced in laboratory conditions at the Faculty of Technology in Novi Sad. Two types of fresh cheese were prepared: with XPL-1 culture (a concentration of 0.02 g/L) and kombucha inoculum (a concentration of 100 mL/L). Starter culture and kombucha inoculum were added to milk heated to 35 °C. After 30 minutes, a coagulation enzyme CHY-MAX^®Powder Extra NB enzyme, EC 3.4.23.4, was added to both cheese samples (with starter culture and with kombucha inoculum) at 35 °C and at a concentration of 0.5% (1% solution of enzyme, Chr Hansen, Denmark). Coagulation at 35 °C lasted until a pH of ~4.5-4.6 was reached. After that, the coagulum was cut, pasteurized at 60 °C with gentle stirring for 5 minutes and cooled (to 25 °C). Whey was separated through a cloth. All cheese samples were homogenized using a mixer, packed in cups with lids and stored in the refrigerator at temperature 4 °C. Fresh cheese sample produced with kombucha inoculum (KFC) and fresh cheese produced with XPL-1 starter culture (XFC) were analysed immediately after production.

Chemical analyses of milk and fresh cheese

Chemical analysis of milk composition and fresh cheese samples was performed by employing standard methods: dry matter content after drying at 105 °C (SRPS EN ISO 5534:2007), fat according to Van Gulik (SRPS ISO 3433:2013), total nitrogen according to Kjeldahl (SRPS EN ISO 8968-1:2016) and ash after mineralization at 550 °C (Carić et al., 2000). The content of non-casein nitrogen (NCN) in milk and cheese was determined by treating the sample with a 10% solution of acetic acid and then with a solution of 1 mol/L sodium acetate, whereby casein precipitation occurs. Non-casein nitrogen is determined in the filtrate by the standard Kjeldahl method. Non-protein nitrogen (NPN) was determined by the addition of 24% trichloroacetic acid with intensive mixing that causes precipitation of protein fractions in milk and cheese sample, and then the content of non-protein nitrogen is determined in the filtrate by Kjeldahl method. Based on the obtained results, casein, whey protein content and real proteins were calculated (Carić et al., 2000, SRPS EN ISO 8968 - 4: 2016). All chemical analyses and assays were performed in triplicate for all produced samples (n) and values were expressed as average value. pH was measured by an electric pH-meter (pH Spear, Eutech Instruments, Oakton, England) and pH-meter Mettler Toledo, Switzerland.

Protein digestion

Digestion was performed in a glass laboratory beaker using a combination of two enzymes: pepsin and pancreatin. Fresh cheese sample with starter culture XPL-1 was diluted with water in the ratio 1:5, while cheese sample with kombucha was dissolved in the ratio 1:10 and heated to temperature of 37 °C on an electric stirrer. The first aliquot (1-1.5 mL) is then taken and the pH is measured. The aliquot was centrifuged for 5 minutes, the solution was separated and labelled. The rest of the solution on the electric mixer is still maintained at a temperature of 37 °C. HCl was added until a pH of ~2.5-3 was reached and then 0.05 g of pepsin was added. After 60 minutes, the aliquot (1-1.5 mL) was heated for 5 minutes at 100 °C, centrifuged (Eppendorf, Centrifuge 5424) and the solution separated and labelled. The rest of the solution was further maintained on an electric stirrer at 37 °C, NaOH was added until a pH of ~7.5 was reached and then 0.05 g of pancreatin was added. After 120 minutes, the aliquot (1-1.5 mL), was heated for 5 minutes at 100 °C, centrifuged, the solution separated and labelled. The collected supernatants were further analysed.

Determination of protein concentration and the degree of hydrolysis

Fresh cheese suspension and trihloracetic acid (0.44 mol/dm³) were mixed in 1:1 volume ratio and incubated in the fridge, for 30 min. Thereafter, the mixture was centrifuged (Eppendorf, Centrifuge 5424). Soluble proteins were determined by the method ofLowry et al. (1951). The bovine serum albumin as the standard protein (0.5 mg/mL) was used for calibration. The measurement is based on the spectrophotometric (colorimetric) method, where the concentration of soluble proteins from the calibration line is determined on the basis of the absorption value of the coloured solution. The colour intensity is proportional to the protein content of the sample, and absorbance was measured spectrophotometrically at 660 nm (SP6-550 UV/VIS, spectrophotometer, Pye Unicam, England). The degree of hydrolyses (DH) was calculated as the ratio of 0.22 mol/dm³ trichloroacetic acid (TCA) soluble proteins to total proteins in the hydrolysate, and expressed as a percentage.

Capillary electrophoresis

Protein characterization was performed by electrophoretic separation by automatic capillary chip electrophoresis on an Agilent 2100 Bioanalyzer (Agilent Technologies, Santa Clara, CA, USA) using the Protein 80 Plus LabChip kit. Data analyses were performed with the Agilent 2100 Expert software. Before applying the samples to the chip, they were prepared according to the method proposed byTidona et al. (2011) with some modifications. Applied method for preparation of milk samples: in 100 μl of milk was added 400 μL of deionized water, vortex treatment was applied for a few seconds, the sample was mixed with buffer in a ratio of 1: 1.5 (buffer 2 x treatment buffer (0.125 M tris-HCl pH 6.8, 4% SDS, 2% glycerol, 5% 2-mercaptoethanol). After that, we applied a vortex treatment (for a few seconds), heat denaturation (100 °C, 5 min) and centrifugation of the samples (20 min, 14.000 rpm). Applied method for preparation of cheese samples: in 20 mg of cheese sample was added 250 μL of buffer (2 x treatment buffer (0.125 M tris-HCl pH 6.8, 4% SDS, 2% glycerol, 5% 2-mercaptoethanol) and vortex treatment was applied for a few seconds. After heat denaturation (100 °C, 5 min), dissolved samples were diluted with 750 μL buffer and centrifuged (20 min, 14.000 rpm). The results of chip electrophoresis analysis are presented in software in two different ways in the form of quantitative profiles (electropherograms) and in the form of simulated gel images.

Total phenolic content

Total phenolic content in cheese samples and cheese hydrolysates was done by the Folin-Ciocalteu spectrophotometric method (Singleton and Rosi, 1965;Kähkönen et al., 1999). The values for absorbance of the samples were measured at 750 nm (6300 Spectrophotometer, Jenway, UK). Results are expressed as mg of gallic acid equivalents (GAE) per g of cheese sample (mg GAE/g), and in hydrolysates was expressed as mg of gallic acid equivalents (GAE) per mL of sample (mg GAE/mL).

DPPH assay

The ability to neutralize 2,2-diphenyl-1-picrylhydrazyl free radicals (DPPH) was measured using a modified method byBrand-Williams et al. (1995). DPPH reagent and diluted cheese sample were added to a glass cuvette (2.9 mL + 0.1 mL) and incubated at room temperature for 60 min. Absorbance was measured at 517 nm using a UV-VIS spectrophotometer (6300 Spectrophotometer, Jenway, UK). Results were reported as μM of Trolox equivalent per g of cheese sample (μM TE/g). Measurements in cheese hydrolysates were performed according to the same principle. Results were reported as μM equivalent of Trolox per mL of cheese hydrolysate (μM TE/mL).

FRAP assay

The ability to reduce Fe³⁺ was determined by the FRAP assay (Benzie and Strain, 1996). Properly diluted cheese samples and FRAP reagent were mixed (0.1 mL + 2.9 mL) and incubated in the dark at 37 °C for 10 min. Absorbance measurements were performed at 593 nm with UV - VIS spectrophotometer (6300 Spectrophotometer, Jenway, UK). Results were expressed as μM of Fe²⁺ equivalents per g of cheese sample (μM Fe²⁺/g). Reduction capacity of the cheese hydrolysate was determined in the same way, and the results were expressed as μM of Fe²⁺ equivalent per mL of cheese hydrolysate (μM Fe ²⁺/mL).

ABTS assay

The ability to neutralize ABTS free radicals was determined using a modified spectrophotometric method reported byRe et al. (1999). Properly diluted cheese samples and ABTS reagent were mixed (0.1 + 2.9 mL) and incubated at room temperature for 5 h in the dark. Absorbance was measured at 734 nm with UV – VIS spectrophotometer (6300 Spectrophotometer, Jenway, UK). Results were expressed as μM of Trolox equivalents per gram of cheese sample (μM TE/g), and for cheese hydrolysate samples as μM Trolox equivalents per mL of sample (μM TE/mL).

Statistical analysis of results

Statistical analysis was performed in order to determine the influence of kombucha inoculum on the quality of fresh cheese. Each experiment was repeated at least three times. Analysis of variance (ANOVA) was performed using Statistica software program. The difference between the mean values was determined at the level of 5% statistical significance using Duncan's test.

Acidification process

Milk fermentation process by kombucha inoculum and traditional starter culture XPL-1 at temperature 35 °C was followed through measuring of pH value. Selected starter cultures had different acidification rate (Fig. 1a). It is evident that the fermentation process was faster in sample made with kombucha inoculum than in the sample produced by traditional starter culture (XPL-1). Acidification time of kombucha fresh cheese was 78 minutes shorter than traditional fresh cheese. Milk with kombucha inoculum reached a maximum acidification rate at 650 min (pH 5.00), while sample with tradition culture XPL-1 had maximum at 400 min (pH 5.25). Different acidification times are the result of different metabolic activity of the applied starter cultures. Decrease of pH during milk fermentation is a result of lactose fermentation. Consequently, the content of L-lactic acid increased in kombucha fermented milk samples (Vukić et al., 2014). Also,Ozyurt (2020) studied the fermentation process of beverages produced by kombucha cultivated on goat, cow and soya milk. The author found that using kombucha inoculum, the fermentation time of cow's milk to reach pH 4.4, is significantly shorter and it amounts to 6 hours.Malbaša et al. (2014) investigated fermentation process of milk with 0.8, 1.6 and 2.8% fat content at 37, 40 and 43 °C using wild thyme kombucha starter. These authors revealed that the fermentation time of milk at 43 °C ranged from 10 to 14 hours. Also, they concluded that fermentation was significantly shorter at higher fermentation temperature regardless of milk fat content. Evidently, different factors, such as starter culture type, milk composition, fermentation temperature, macromolecules interaction contribute to decrease pH value of gel and different rates of coagulum formation during fresh cheese production.

Figure 1 a) Acidification rate of milk by applying of kombucha inoculum and traditional starter culture b) Changes of the pH during milk fermentation by applying of kombucha inoculum and traditional starter culture

Chemical composition of fresh cheese samples

The process of milk fermentation using kombucha inoculum and conventional (traditional) starter culture (XPL-1) significantly affects the chemical composition and profile of individual protein fractions in fresh cheese samples. Composition of fresh cheese samples are compared inTable 1. There are significant differences in chemical composition and protein contents between fresh cheese fermented by kombucha and fresh cheese produced by traditional starter culture. Dry matter of fresh cheese produced with XPL-1 starter culture (37.40%) was significantly lower than in kombucha fresh cheese (49.83%). These results are in accordance with the Serbian Regulation (2014). In this Standard, fresh cheeses are required to have the total solids content higher than 20%. Also, our results of fresh cheese produced with XPL-1 showed similar chemical composition with literature data (Miloradović et al. 2018), while dry matter of kombucha fresh cheese was 45% higher compared to cows´ Quark type cheese. Traditional fresh cheese contained 13.23% protein and 19.0% fat, while kombucha fresh cheese contained 21.33% protein and 26.75% fat. Casein content was 58% higher in the sample of cheese with kombucha compared to cheese with traditional starter culture. It is evident that fresh cheese with kombucha contains a significant amount of milk proteins in which casein fractions are predominantly present and whey proteins in a much smaller amount. The content of casein in cheese obtained by kombucha represents 86.31% of total solids non-fat, while fresh cheese with traditional culture contained 62.77%.

Hydrolysis of fresh cheese protein

Milk proteins are nutritionally very important because they have numerous beneficially effects on the gastrointestinal (GI) and immune systems. Milk proteins are the important source of bioactive peptides. Bioactive peptides can be released by hydrolysis (e.g. pepsin, trypsin and chymotrypsin) during gastrointestinal digestion or by activity of proteases and peptidases released by lactic acid bacteria (LAB) (Santiago-Lopez et al., 2018). The solubilized protein content in supernatant related to protein content in undigested matrix represents the amount of soluble proteins in supernatant of digestion mixtures (Rinaldi et al., 2014). Soluble proteins and changes in hydrolysis degree (DH) at steps of the simulated gastrointestinal digestion are shown inFig 2. Due to the presence of digestive enzymes the amount of soluble proteins increased during in vitro GI digestion for both fresh cheese samples. The content of soluble proteins during protein digestion was significantly higher in the sample of fresh cheese with kombucha than in cheese with traditional starter culture. The low amount of soluble proteins measured in both of samples after first initial phase (before addition of enzymes). The content of soluble proteins in XFC ranges from 20 mg/g in the initial phase to 90 mg/g after digestion with pancreatin. In kombucha fresh cheese, the content of soluble proteins after the third phase (decomposition by pancreatin) is 100% higher in relation to the solubility of proteins in the XFC sample. The highest increase was observed in kombucha fresh cheese after digestion with pancreatin (180 mg/g sample).

Figure 2 Soluble proteins and degree of proteolysis in fresh cheese sample after gastric and duodenal phases of in vitro digestion

The degree of proteolysis was calculated based on the content of soluble proteins and total proteins in the samples. The initial value of the degree of proteolysis in both cheese samples was less than 5% and was slightly higher in the XFC sample (Fig 2b). The results of the degree of hydrolysis in cheese samples before digestion are higher compared to the data from the literature (Hrnjez et al., 2014;Tagliazucchi et al., 2017).Hrnjez et al. (2014) investigated the degree of proteolysis in fermented dairy products with starter culture and kombucha during storage. They concluded that at the end of fermentation the highest degree of proteolysis (compared to milk - 1.7 ± 0.02) had a sample with kombucha inoculum K (2.56 ± 0.151%), a slightly lower value of the sample with probiotic starter culture P (2.35 ± 0.041%), and the lowest value for the sample with yogurt starter culture Y (2.25 ± 0.034%). Maximum proteolysis in fresh cheese samples was achieved in gastric phase with pancreatin. DH in gastric phase was higher in the KFC sample (53.60%) than in XFC sample (50.8%). Kombucha fresh cheese has 22.35% less water and 27.27% higher casein content in dry matter without fat than fresh cheese produced with XPL-1 culture, which contributed to higher protein solubility and a higher degree of proteolysis during the digestion of the kombucha fresh cheese. Our results can be correlated with results ofFang et al. (2016) who found that in vitro GI digestion depends on the chemical composition and texture of the sample, as well as on enzyme treatment. These authors concluded that water content negatively affect cheese disintegration suggesting that the disintegration in increased in low moisture and MNFS (moisture in the non-fat substance) cheese.Fang et al. (2016) found that cheese with high casein density are firmer and harder to disintegrate, but the composition has a stronger influence on cheese disintegration than the textural properties. Also, the addition of enzymes enabled 72% of cheese disintegration to be achieved at the end of duodenal digestion, while it reached 30% when no enzymes were added.

Protein characterisation during in vitro GI digestion

Lab on chip gel images of milk, undigested samples and digested fresh cheese samples during in vitro GI digestion are shown inFig.3a. The first image shows comparison of the intensity of the bands of milk and fresh cheese samples. It is evident that casein fractions are predominantly present in kombucha fresh cheese, while fractions with molecular weights less than 10 kDa are more present in the fresh cheese obtained with traditional culture. Based on this results, a relative amount of protein fractions in undigested milk and fresh cheese samples was calculated (Fig.3b). The obtained relative amount of α-casein in tested milk was 34.81%, whereas relative concentration of β-casein was 24.46% (Fig. 3a). The α-casein (31.08%) and β-casein (47.53%) were detected in kombucha fresh cheese. During in vitro GI digestion, for XFC fresh cheese sample both fractions of casein are degraded more rapidly by pepsin than protein fraction in kombucha fresh cheese (Fig.3a). At the end of simulated duodenal digestion, the bands of caseins were not visible, while the band of whey proteins was still intense, that it has not been totally solubilized and digested. It means that the present whey protein aggregates may be also resistant to duodenal digestion. This is in accordance with other studies that have confirmed resistance of β-lactoglobulin to digestion with pepsin (Hodkinson et al., 2018). In digested cheese samples, whey proteins were detected in low relative amount, but it was higher in fresh cheese with XPL-1 culture than in kombucha fresh cheese. Since these proteins are one of the main milk allergens, it can be assumed that cheese with kombucha inoculum is a smaller allergen than traditional fresh cheese and can be used for a special diet for people with protein allergies.

Figure 3 a) Comparison of gel images of undigested (milk and fresh cheese samples) and digested samples b) Relative amount of selected protein fraction in digested fresh cheese samples; (1) first lane undigested fresh cheese, (2) second lane at the beginning of GI digestion, after the addition of pepsin and (3) third lane - after the addition of pancreatin

Antioxidant capacity of fresh cheese samples

Fermentation process, protein profile, content of soluble proteins and degree of proteolysis significantly influence antioxidant potential of fresh cheese samples. The results of antioxidant activity and total phenol content in milk, kombucha inoculum, fresh cheese samples and their hydrolysates are shown inTable 2. Antioxidant activity of milk and kombucha inoculum (0.0287 μM Fe²⁺/g and 0.0056 μM Fe²⁺/g, respectively) was lower than in cheese samples. Considering antioxidant capacity (AC), the obtained results showed higher antioxidant capacity (AC) of fresh cheese with traditional culture (XFC) (1.24 μM Fe²⁺/g) than kombucha fresh cheese (0.93 μM Fe²⁺/g). The results of DPPH assay showed different ability for milk, kombucha and fresh cheese samples. DPPH value of milk and kombucha inoculum were 0.0014 and 0.007 μM TE/g, respectively. Statistically significant increase (p<0.05) in antioxidant activity was found in both fresh cheese samples. Maximum DPPH value (0.95 μM TE/g) was observed in kombucha fresh cheese, while DPPH of cheese sample XFC was 0.93 μM TE/g. Among all samples, the best sample which showed the highest ABTS was fresh cheese produced by a traditional starter culture (XPL-1). The ABTS radical scavenging abilities of kombucha fresh cheese (1.2203 μM TE/g) was significantly lower than in control sample (2.0148 μM TE/g). These results are in accordance with literature data.Hrnjez et al. (2014) investigated biological potential of fermented milks produced by application probiotic (P), yoghurt (Y) and non conventional starter culture kombucha (K). They found that the highest ABTS value had the sample Y (50.6542), slightly lower value the sample P (47.4733) and finally the lowest value the sample K (41.0446). The DPPH value after production was the highest in sample kombucha fermented milk product (17.8832), lower in probiotic sample (13.2299) and in yoghurt (9.4586). The antioxidant activities of fresh cheese hydrolysates is also presented inTable 2. It is evident that FRAP, DPPH and ABTS of radical scavenging abilities of kombucha fresh cheese hydrolysate are higher than in hydrolysates of fresh cheese produced with traditional starter culture (XPL-1), but DPPH and ABTS not statistically significant. The higher antioxidant potential of the hydrolysate prepared from fresh kombucha cheese can be explained by the fact that this cheese sample has a higher protein content (casein fraction) as well as a higher content of phenols which significantly contribute to the biological potential of the product. The share of casein in fat free dry matter in the kombucha cheese sample is 27.26% higher compared to fresh cheese produced by traditional culture (XPL-1).Rival et al. (2001) found that the antioxidant potential of casein fractions ranges from β-casein> αs1-casein> αs2-casein> α lactalbumin> β lactglobulin. Since the relative proportion of β-casein is predominantly present in kombucha cheese, the hydrolysate of kombucha fresh cheese had greater antioxidant potential compared to traditional fresh cheese (XFC).

In addition to the significant protein content, the phenol content in kombucha fresh cheese significantly affected the antioxidant potential of the cheese samples. Total phenolic content of kombucha inoculum was 0.1252 mg GAE/g and in milk sample 1.203 mg GAE/g, respectively. Phenolic contents of the inoculum have influenced the total phenolic content of fresh cheese. Kombucha fresh cheese sample showed a higher total phenol content than fresh cheese produced by traditional starter culture. Total phenols determined in kombucha fresh cheese sample was 5.81 mg/GAE/g, while in traditional fresh cheese content of phenol was 0.98 mg/GAE/g. Application of kombucha contributed the increase in phenolic components in fresh cheese sample. These results are in accordance with literature data (Ozyurt 2020,Cardoso et al., 2020).Ozyurt (2020) concluded that total phenolic contents of black tea –based beverages increased with fermentation time and ranged from 227.78 to 312.26 μg/GAE/g. Also,Cardoso et al. (2020) found high concentrations of most phenolic concentration and catechin in kombucha. Black tea kombucha had a total phenolic content of 1.09 mg GAE/mL, which was approximately 55.7% higher than that of green tea kombucha with 0.70 mg GAE/mL. According toCardoso et al. (2020), 127 phenolic components have been identified in green and black kombucha tea that contribute to higher antioxidant capacity. Antioxidant activity is associated with the formation of low molecular weight components and the degradation of polyphenols present in tea by enzymes produced by bacteria and yeasts during fermentation (Cardoso et al., 2020;Coelho et al., 2020). Total phenolic components and content of some components in milk and kombucha inoculum which possess strong antioxidant activity are expected to be directly related to fresh cheese antioxidant capacity. The higher antioxidant potential of fresh cheese hydrolysate produced using kombucha compared to the sample of cheese produced by traditional culture can be related to higher content of soluble proteins and the degree of proteolysis of cheese samples during digestion. Given the results of the biological potential of the analysed cheese samples, it can be concluded that the kombucha cheese sample provides better protein bioavailability. Due to the content of phenolic components and antioxidant ability, kombucha has a positive effect on health and it is recommended for people who are exposed to oxidative stress (Cardoso et al., 2020;Coelho et al., 2020).