Microbial Decontamination of Red Wine by Pulsed Electric Fields (PEF) after Alcoholic and Malolactic Fermentation: Effect on Saccharomyces cerevisiae, Oenococcus oeni, and Oenological Parameters during Storage

New techniques are required to replace the use of sulfur dioxide (SO2) or of sterilizing filtration in wineries, due to those methods’ drawbacks. Pulsed electric fields (PEF) is a technology capable of inactivating microorganisms at low temperatures in a continuous flow with no detrimental effect on food properties. In the present study, PEF technology was evaluated for purposes of microbial decontamination of red wines after alcoholic and malolactic fermentation, respectively. PEF combined with SO2 was evaluated in terms of microbial stability and physicochemical parameters over a period of four months. Furthermore, the effect of PEF on the sensory properties of red wine was compared with the sterilizing filtration method. Results showed that up to 4.0 Log10 cycles of S. cerevisiae and O. oeni could be eradicated by PEF and sublethal damages and a synergetic effect with SO2 were also observed, respectively. After 4 months, wine treated by PEF after alcoholic fermentation was free of viable yeasts; and less than 100 CFU/mL of O. oeni cells were viable in PEF-treated wine added with 20 ppm of SO2 after malolactic fermentation. No detrimental qualities were found, neither in terms of oenological parameters, nor in the sensory parameters of wines subjected to PEF after storage time.


Introduction
Wine is a fermented beverage with particular characteristics, such as a low pH (3.0-3.9) and the presence of ethanol (8-16% v/v), which thereby restrain the proliferation of foodborne pathogenic microorganisms and spore-forming bacteria. However, certain groups of microorganisms are able to grow in wines and spoil them in different stages of the winemaking process [1]. Such spoilage microorganisms are usually either the endogenous microbiota of grape skins, or microorganisms stemming from contact surfaces and equipment in wineries [2]. On the other hand, microorganisms that are essential in wine production, such as Saccharomyces cerevisiae and lactic acid bacteria (LAB), responsible for alcoholic and malolactic fermentation, respectively, may likewise be involved in wine spoilage. These microorganisms therefore need to be controlled after fermentation to avoid undesired re-fermentation, which, in turn, may lead to off-flavors, increments in volatile acidity, or even the production of biogenic amines [3].
To obtain quality wines and avoid economic losses, it is essential to control all of the involved spoiling microorganisms in grapes, must, and wine, as well as on surfaces in wineries. Apart from rigorous standard cleaning and disinfection plans, the conventional method for microbial control in wineries is the application of sulfur dioxide (SO 2 ) [4]. Sulfur dioxide has bacteriostatic and antifungal activity but also plays an essential role as an antioxidant: all of these functions make it a thoroughly convenient compound for wine Values represent mean with standard deviation. * Color intensity. ** Total polyphenol index. *** Total anthocyanin content. A.U.: absorbance units. a : expressed as tartaric acid. b : expressed as acetic acid. c : expressed as the mean ± the deviation of the analytical method. d : expressed as tartaric acid. e : expressed as malvidin-3-glucoside.

PEF Processing
PEF treatments were applied in a continuous flow by means of a commercial generator (Vitave, Prague, Czech Republic) able to deliver pulses of up to 20 kV. Square waveform monopolar pulses were delivered in a parallel titanium electrode chamber with a 0.4 cm gap (3.0 × 0.5 cm). Wines tempered at 20 • C in a heat exchanger placed prior to the treatment chamber were pumped by a peristaltic pump (BVP, Ismatec, Wertheim, Germany) at different flow rates into the chamber. After the treatments, wines were cooled down in less than 5 s to under 20 • C in a second heat exchanger located after the treatment chamber. The actual voltage during treatments was measured by a high voltage probe (Tektronik, P6015A, Wilsonville, OR, USA) connected to an oscilloscope (Tektronik, TDS 220). Inlet and outlet temperatures were measured by a type K thermocouple inserted in the circuit (Ahlborn, Holzkirchen, Germany).
In preliminary studies, a matrix of different PEF parameters was tested with the aim of identifying optimal conditions for microbial decontamination. Wines after AF (1.9 mS/cm) and MLF (2.0 mS/cm) were pumped at 10 L/h, resulting in a residence time of 0.22 s in the chamber. Pulses of 10 µs were delivered at electric field strengths of 15, 20, and 25 kV/cm, and at a repetition rate ranging from 8.0 to 80 Hz, corresponding to effective treatment times ranging from 20 to 175 µs. These treatments corresponded to total specific energies of 35 to 120 kJ/kg, thereby implying an exit temperature in the range of 30 to 50 • C ± 2 • C. For the storage study, the two PEF treatments selected for each red wine were applied at 15 kV/cm. Wine after AF was treated with total specific energies of 39 and 97.2 kJ/kg (exit temperatures of 30 and 45 • C, respectively), whereas for wine after MLF, energies were 77.8 and 116.7 kJ/kg (exit temperatures of 40 and 50 • C, respectively).

Sulfite Addition
Immediately after PEF treatments, wine samples were added with the corresponding amount of SO 2 . A stock solution of 25 g/L of SO 2 was prepared from potassium bisulfite (Sigma, Burlington, MA, USA). PEF-treated and untreated wines were dosed with 0, 20, and 30 ppm of SO 2 . The total free SO 2 content at the starting point of the storage study was the sum of the initial free SO 2 content in wine after AF (19 ppm) and after MLF (10 ppm) plus the corresponding doses of SO 2 added in this step.

Microbial Analysis
Microbial survivors were measured by the corresponding plating of aliquots of wine samples diluted in peptone water (Oxoid, Basingtok, Hampshire, UK) and plated onto the appropriate agar medium. For yeast enumeration, Potato Dextroxe Agar (Oxoid) was used, and plates were incubated at 25 • C for 48 h. Lactic acid bacteria (LAB) survivors were enumerated in Mann Rogosa Sharpe (MRS) Agar (Oxoid) and the plates were incubated in anaerobic conditions (<1% O 2 ) at 30 • C for 24 to 72 h. After the plate incubation, the number of counted colonies corresponds with the number of viable microorganisms expressed as a colony form unit per milliliter (CFU/mL) or its decimal logarithm (Log 10 CFU/mL). The survival fraction was calculated by dividing the number of microorganisms that survived the treatment (N t ) by the initial number of viable cells (N 0 ).

Analysis of Oenological Parameters
The initial and final oenological parameters of all of the wine samples were measured. The pH, glucose-fructose, % ethanol, and total and volatile acidity were analyzed by FTIR spectroscopy using MIURA 200 and BACCHUS 3 MultiSpec models (TDI, Barcelona Spain). Absorbance measurements were performed after centrifuging wine samples in an Eppendorf AG centrifuge for 15 min at 3000 rpm (Eppendorf, Hamburg, Germany). All spectrophotometric determinations were measured by spectrophotometer (DS-11, DeNovix, Wilmington, DE, USA). The color index (CI) was determined as the sum of absorbance at 420, 520, and 620 nm. The total polyphenol index (TPI) was determined by measuring the direct absorbance at 280 nm. Total anthocyanins (TAC) expressed in malvidin-3-glucoside (mg/L) were calculated by determining the absorbance at 520 nm of samples diluted 1/10 (v/v) in 1% (v/v) of HCl, adapted from Maza et al., (2019) [22].
The determination of total and free sulfur dioxide (SO 2 ) was performed by the Ripper method, which is based on an oxidation-reduction titration using iodine as a reagent in an acid medium in the presence of starch. Briefly, 1 mL of starch (1%) and 2 mL of sulfuric acid 1/3 w/v vinikit (PanReac, Barcelona, Spain) were added to 15 mL of wine. This solution was titrated with an iodine solution (0.01 N) until a blue color appeared.

Sensory Evaluation of PEF Treatments in a Commercial Wine
To evaluate the impact of PEF on sensory properties, independent experiments were performed in a finished red wine prior to being bottled. This red wine was treated by PEF at two different intensities and compared with the same wine after sterilizing filtration in the facilities of the winery. A total amount of 50 L of red wine (1.5 mS/cm) was processed by PEF at a flow rate of 25 L/h. Pulses of 5 µs were applied at 107 and 190 Hz at 15 kV/cm at the total specific energies of 77.8 of 155.6 kJ/kg that corresponded to exit temperatures of 40 and 60 ± 2.0 • C, respectively. The cooling exchanger placed immediately after the PEF chamber reduced the wine's temperature to under 20 • C in less than 5 s before bottling. After 1 month of storage, physicochemical and sensory analyses were performed. Oenological parameters were measured as previously described (Section 2.5), and a sensory evaluation was carried out by a complete sensory triangle discrimination test, performed by 16 panelists from the Campo de Borja Appellation of Origin (nine men/six women ages 26 to 58). Panelists were distributed in individual booths and were given no information regarding the testing samples. Comparisons performed in the triangle test were between the sterilized filtered wine and the PEF-treated wines, using a completely randomized design. Samples were previously tempered to room temperature and 20 mL were served in clear wine glasses (ISO NORM 3591) [23]. Panelists had to distinguish the one different sample among the three samples presented in each batch, by taste and/or aroma.

Statistical Analysis
Samples were analyzed in three independent replicates and data are expressed as the mean ± the standard deviation. When called for, one-way analysis of variance (ANOVA) and Tukey tests using GraphPad Prism (Graph-Pad Software, San Diego, CA, USA) were performed to evaluate the significance of differences among the mean values. Differences were considered significant at p ≤ 0.05. The significant difference for the triangular test was determined using statistical tables reported by Roessler et al., (1948) [24].

PEF-Resistance of Saccharomyces cerevisiae and Oenococcus oeni
Preliminary experiments were conducted to determine the resistance of S. cerevisiae to PEF treatments of Grenache red wine after alcoholic fermentation, and of O. oeni after malolactic fermentation. The ultimate objective of these experiments was to select PEF processing conditions for subsequent study, aiming to evaluate the evolution of these microbial populations in each wine during storage.
Survival curves corresponding to the inactivation of S. cerevisiae and O. oeni at different electric fields (15,20, and 25 kV/cm) are shown in Figure 1A,B, respectively. The numbers next to the symbols indicate the outlet temperature of wine attained during PEF processing. Due to the wine's short residence time in the treatment chamber (0.22 s), no heat is exchanged with the surroundings. Consequently, all of the electrical energy delivered to the treatment chamber to generate the electric field is transformed into heat, thereby increasing the wine's temperature. However, in the experimental approach used in this study, wine was cooled below 20 • C within 5 s after the PEF treatment, independently of the outlet temperature. As can be observed in the two graphs, the temperature increased with the treatment time (number of pulses × pulse width). Figure 1 shows that the inactivation kinetics of the two microorganisms is different. In the case of S. cervisiae, the survival curve's shape is concave upwards, whereas in the case of O. oeni a linear behavior can be observed. The shape of the survival curves of S. cerevisiae could be explained by the effect of temperature on the membrane's stability as a consequence of the phase transition of the phospholipids from gel to the liquidcrystalline phase. A sudden change in inactivation kinetics can be observed when the output temperature of the wine was over 40 • C. This change would indicate that above 40 • C the cytoplasmic membrane of S. cerevisiae is more vulnerable to the pore formation caused by PEF [25]. The positive effect of treatment medium temperature on microbial inactivation has been previously reported by several authors [10,26]. However, in the case of O. oeni, no radical changes in the inactivation kinetics were observed in the same range of outlet temperatures. This might indicate differences in the cytoplasmic membrane composition of both microorganisms, which could vary in terms of the manner in which the temperature affects the phase transition of the phospholipids.  Figure 1 shows that the inactivation kinetics of the two microorganisms is different. In the case of S. cervisiae, the survival curve's shape is concave upwards, whereas in the case of O. oeni a linear behavior can be observed. The shape of the survival curves of S. cerevisiae could be explained by the effect of temperature on the membrane's stability as a consequence of the phase transition of the phospholipids from gel to the liquid-crystalline phase. A sudden change in inactivation kinetics can be observed when the output temperature of the wine was over 40 °C. This change would indicate that above 40 °C the cytoplasmic membrane of S. cerevisiae is more vulnerable to the pore formation caused by The inactivation of the two microorganisms increased with the electric field, whereby shorter treatments at higher electric fields strengths were required to achieve a given level of inactivation. For example, to inactivate 2.0 Log 10 cycles of the population of S. cerevisiae, the treatment time decreased from 140 to 52 µs when the electric field was increased from 15 to 25 kV/cm. The same electric field increment reduced the treatment time from 180 to 40 µs to achieve a similar inactivation in O. oeni. In the case of S. cerevisiae, the outlet temperature for both treatments applied at different electric field strengths was the same (45 • C), thereby indicating that the total specific energy of the treatments applied at different electric fields was equivalent (97 kJ/kg). Huang [18,27] also reported that the electric field did not modify PEF lethality on different Saccharomyces strains suspended in must or wine when treatments of the same specific energy were applied. However, in the case of O. oeni, the total specific energy required for achieving an equivalent lethality was lower when the electric field strength was increased. For example, in order to obtain 2.0 Log 10 cycles, the total specific energy decreased from 117 to 49 kJ/kg when the electric field was increased from 15 to 25 kV/cm. Consequently, whereas the outlet temperature of the treatment applied at 15 kV/cm was around 50 • C, the outlet temperature of the treatment applied at 25 kV/cm lay in the range of 30.4 to 34.8 • C. The total specific energy of a PEF treatment depends on the applied voltage, total treatment time, and the electrical resistance of the treatment chamber. Since total specific energy is an integrate parameter that involves electric field strength and treatment time, it has been proposed as a single parameter to define the intensity of a PEF treatment [28]. This approach could be considered in the case of the strain of S. cerevisiae used in this study, upon which equivalent total specific energy delivered at different electric field strengths had the same lethal effect. However, in most microorganisms observed in the O. oeni strain, treatments of the same specific energy are more effective in terms of microbial inactivation when the applied electric field strength is higher [29]. Therefore, in this case, to define the intensity of a given PEF treatment, it is necessary to report both the electric field strength and total delivered specific energy.
It has generally been reported that yeasts are more sensitive to PEF than bacteria [30][31][32]. The high PEF sensitivity of yeast has been associated with the fact that larger cells require a lower critical electric field to achieve the transmembrane potential threshold for the manifestation of electroporation. However, other intrinsic microbial factors in addition to cell size seem to play a role in microbial resistance to PEF. Whereas at 15 kV/cm the resistance of the two microorganisms to PEF treatments of different duration was similar, at higher electric field strength O. oeni was slightly more sensitive than S. cerevisiae. For example, a treatment of 20 kV/cm for 70 µs that corresponded with an exit temperature of 40 • C inactivated around 1.5 Log 10 cycles of S. cerevisiae, and around 2.5 Log 10 of O. oeni. The higher resistance of S. cerevisiae to PEF might be explained by the fact that, in contrast to other studies in which the wine was contaminated with yeast previously grown in laboratory media, our investigation was conducted with the cells that had performed the alcoholic fermentation. The presence of ethanol during the growth of those cells could provoke changes in the composition or structure of their cytoplasmic membrane [33,34], which, in turn, could lead to a cross-protection against the electroporation brought about by PEF.
It is difficult to compare the PEF resistance of the strains used in this investigation with reported data in view of the widely varying protocols employed for PEF application, the differences among the investigated strains, their physiological state, and the variabilities in the composition of wines. The PEF resistance of yeast and lactic acid bacteria in wine has been reported in previous studies. Treatments at an electric field above 17 kV/cm and 90 kJ/kg were required to achieve between 2.0 and 3.0 Log 10 cycles of the inactivation of the Saccharomyces population [18,19]. After alcoholic fermentation, intense PEF treatments (33 kV/cm; 158 kJ/kg; 105 µs) inactivated between 3.7 and 7.2 Log 10 cycles of the population of yeast cells involved in the fermentation process [35]. Meanwhile, lethality reported for O. oeni ranged from 1.5 to 3.2 Log 10 when PEF treatments of 17-23 kV/cm and 60-100 kJ/kg were applied [19,20].

Inactivation of Saccharomyces cerevisiae and Oenococcus oeni by Combining Moderate PEF Treatments with SO 2
Several authors have reported that when PEF treatments are applied to a microbial population, a proportion of cells is sublethally injured, and this is more evident when moderate conditions are applied [36]. The final recovery or death of that injured population is directly dependent on either optimal or adverse recovery conditions [37,38]. Preventing the reparation of sublethal injuries caused by PEF by adding preservatives is a strategy that can increase the lethality of moderate PEF treatments [39][40][41][42]. Figure 2 illustrates the inactivation of S. cerevisiae (Figure 2A) and O. oeni ( Figure 2B) in the respective wines after fermentation by combining PEF treatments of different durations at 15 kV/cm with the addition of 20 ppm of SO 2 evaluated 24 h after processing. The lethal effects of the individual treatments are also shown in order to identify if the effect of the combined treatments was additive or synergic. Figure 2A,B show that the added SO 2 scarcely affected the viability of the untreated cells of S. cerevisiae and O. oeni. On the other hand, the inactivation of PEF-treated cells of S. cerevisiae maintained for 24 h in wine without added SO 2 increased significantly. For example, the inactivation detected just after the 140 µs PEF treatment increased from 2.0 to 4.0 Log 10 cycles after 24 h. This effect could be explained by the supposition that the presence of ethanol and the content of free sulfites in the wine (14.7%; 19.2 ppm, see Table 1) prevented the recovery of a proportion of the yeast cells that had been sublethally injured as a consequence of the PEF treatment. The addition of 20 ppm of SO 2 barely increased lethality compared with wines treated solely with PEF; the difference is not statistically significant (p > 0.05). The yeast cells that survived in PEFtreated wine during 24 h were thus unaffected by the addition of 20 ppm of extra sulfites.

Inactivation of Saccharomyces Cerevisiae and Oenococcus Oeni by Combining Moderate PEF Treatments with SO2
Several authors have reported that when PEF treatments are applied to a microbial population, a proportion of cells is sublethally injured, and this is more evident when moderate conditions are applied [36]. The final recovery or death of that injured population is directly dependent on either optimal or adverse recovery conditions [37,38]. Preventing the reparation of sublethal injuries caused by PEF by adding preservatives is a strategy that can increase the lethality of moderate PEF treatments [39][40][41][42]. Figure 2 illustrates the inactivation of S. cerevisiae (Figure 2A) and O. oeni ( Figure 2B) in the respective wines after fermentation by combining PEF treatments of different durations at 15 kV/cm with the addition of 20 ppm of SO2 evaluated 24 h after processing. The lethal effects of the individual treatments are also shown in order to identify if the effect of the combined treatments was additive or synergic. Figure 2A,B show that the added SO2 scarcely affected the viability of the untreated cells of S. cerevisiae and O. oeni. On the other hand, the inactivation of PEF-treated cells of S. cerevisiae maintained for 24 h in wine without added SO2 increased significantly. For example, the inactivation detected just after the 140 µs PEF treatment increased from 2.0 to 4.0 Log10 cycles after 24 h. This effect could be explained by the supposition that the presence of ethanol and the content of free sulfites in the wine (14.7%; 19.2 ppm, see Table 1) prevented the recovery of a proportion of the yeast cells that had been sublethally injured as a consequence of the PEF treatment. The addition of 20 ppm of SO2 barely increased lethality compared with wines treated solely with PEF; the difference is not statistically significant (p > 0.05). The yeast cells that survived in PEF-treated wine during 24 h were thus unaffected by the addition of 20 ppm of extra sulfites.  The incubation of PEF-treated O. oeni cells for 24 h in wine without added SO 2 did not significantly increase the lethality of the treatments applied over different time intervals. This observation confirms results obtained by other authors who reported that sublethal injury did not occur when Gram-positive bacteria, such as O. oeni, were treated by PEF in media of low pH [43,44]. Regarding the combination of PEF with SO 2 , the most effective combination was observed 24 h after mixing 20 ppm of SO 2 with wine treated for 173 µs. The PEF treatment thus sensitized a proportion of the surviving population to SO 2 , whereby the lethality of the combined treatment was over 2.0 Log 10 cycles more than the sum of the single treatments. The main mechanism involved in the antimicrobial effect of SO 2 on yeast is related to the diffusion of SO 2 into the cytoplasm and the subsequent disturbance of metabolic processes by the binding of SO 2 to essential molecules (proteins, nucleic acids, coenzymes, cofactors, vitamins, etc.). Although the activity of SO 2 against bacteria is still unclear, the electroporation phenomenon triggered by PEF could enhance the diffusion of SO 2 into the cytoplasm of O. oeni, thereby exerting an effect similar to the one described for yeast [4].

Evolution of the Microbial Population in Wine Treated by PEF after Alcoholic and Malolactic Fermentation during 4 Months of Storage
Based on preliminary results obtained on the resistance of S. cerevisiae and O. oeni to PEF treatments of different intensities and their combination with SO 2 , treatment conditions with the aim of evaluating the evolution of the microbial population in wines during 4 months of storage were chosen.
Treatments at 15 kV/cm of a shorter (62 µs) and longer (140 µs) duration that corresponded to a total specific energy of 39 and 97.2 kJ/kg and an outlet temperature of 30 and 45 • C, respectively, were selected for wine obtained after alcoholic fermentation. Table 2 shows the evolution of yeast populations in wine treated by the two selected PEF treatments after alcoholic fermentation without adding SO 2 or with the addition of 20 ppm of SO 2 . For comparative purposes, the evolution of the yeast populations in the untreated wines with and without 20 ppm of added SO 2 is also included. The initial number of viable yeast cells in the untreated wines was 3 × 10 6 CFU/mL. This initial number was maintained during the first month of storage, even in the untreated wine dosed with 20 ppm of sulfites. After 4 months of storage, the yeast cell population decreased by about 3.0 logarithmic units. These results indicate that the addition of 20 ppm of SO 2 did not compromise the viability of yeast cells that fermented a wine which already had 19 ppm of free SO 2 by the end of fermentation. The reduction of the yeast cell population observed between 1 and 4 months might be the loss of viability that occurs in a microbial population when it is maintained under conditions in which multiplication does not occur. In the case of PEF-treated wines, a similar reduction in yeast viability as in the control wine after 4 months was achieved just after the application of the most intense PEF 2 treatment (97.2 kJ/kg; 171 µs), or after 1 day of incubation in the wine treated at lower intensity PEF 1 (39 kJ/kg; 83 µs). After 4 months of incubation, no viable yeasts were detected in the two wines, even when SO 2 was not added to them. In the case of the wine that had undergone malolactic fermentation, as sublethal injury was not detected in O. oeni cells after PEF treatment, the two longer treatments (132 and 173 µs) that correspond to a total specific energy of 77.8 and 116.7 kJ/kg, respectively (outlet temperatures of 40 and 50 • C), were selected. Moreover, in order to obtain synergetic effects, the low-intensity treatment (PEF 3 ) was combined with the addition of 30 ppm of sulfites, and the high-intensity treatment (PEF 4 ) was combined with the addition of 20 ppm of sulfites.
As the presence of yeast in addition to O. oeni was detected in the wine obtained after malolactic fermentation, the evolution of the two microorganisms under the different assayed conditions is shown in Table 3. It shows that the initial concentration of O. oeni after malolactic fermentation (≈10 5 CFU/mL) slowly decreased during storage in untreated wines with no added SO 2 , as well as in those with 20 or 30 ppm of SO 2 added; the decrease was slightly higher in the latter ones. After 4 months of storage, the differences in concentration of viable cells between the untreated wine without added SO 2 and with 30 ppm added was lower than 1.0 Log 10 cycle. On the other hand, as had been observed in the case of the yeast after alcoholic fermentation, the population of O. oeni decreased more rapidly in wines treated by PEF. After 4 months of storage, the concentration of viable cells was around 2 × 10 3 and 6 × 10 2 CFU/mL in wines without added SO 2 but treated with low and high intensity PEF, respectively. However, in wines with 20 or 30 ppm of SO 2 , the number of viable cells of O. oeni was lower than 1 × 10 2 CFU/mL, independently of the intensity of the PEF treatment applied. It is remarkable that in both PEF-treated wines combined with added SO 2 , a pronounced synergetic effect could be observed, obtaining a reduction of 2.0-3.0 Log 10 cycles of the initial O. oeni population within just 24 h. Values represent mean with standard deviation. Different letters within the same column indicate significant differences (p ≤ 0.05). n.d. = not detected. <1.5 Log 10 CFU/mL = below the quantification limit (30 CFU/mL).
Regarding the evolution of yeast, Table 3 shows that the concentration of yeast populations in wine after malolactic fermentation was around 0.5 log cycles lower than in wine after alcoholic fermentation (Table 2). This confirms that yeast viability after alcoholic fermentation decreases along time. Untreated yeast populations in wine after malolactic fermentation decreased along storage time: the number of viable yeasts after 4 month of storage was less than 1 × 10 2 CFU/mL. As occurred in the case of wine after alcoholic fermentation, the addition of 20 ppm of SO 2 did not significantly affect the yeasts' viability along storage as compared to the wine without added SO 2 that contained 10 ppm of free SO 2 at the moment of the trial. After 15 days of incubation, viable yeast cells were not detected in the wines treated by PEF at the two assayed intensities, independently of whether SO 2 had been added or not.
These results thus evidence the capacity of PEF, even applied at quite moderate intensities, as a potential alternative alone or in combination with sulfites, for microbial control at different steps of the red wine production process. The inactivation of yeast by means of PEF after alcoholic fermentation would allow for the achievement of a lower free SO 2 content, thereby facilitating the implementation of LAB for further malolactic fermentation. González-Arenzana et al., (2018) [35] reported a shortening of the malolactic fermentation time for wines pre-treated by PEF, attributing this reduction of fermentation time to the decrease in competitive pressure for lactic acid bacteria. Furthermore, the complete decontamination of yeasts after alcoholic fermentation would be of special interest for sweet or semi-sweet wines with residual sugars, in order to prevent re-fermentation [45]. On the other hand, in addition to preventing re-fermentation by yeast, PEF alone, or in combination with SO 2 after malolactic fermentation, could contribute to the prevention spoilage caused by lactic acid bacteria during storage in bottles, which generally leads to phenomena such as a slimy appearance, undesirable off-flavors, and/or the production of biogenic amines [3].

Effect of PEF Treatments on the Oenological Parameters of Wine after 4 Months of Storage
Any new technique that might be potentially introduced in wineries should guarantee zero drawbacks in terms of physicochemical parameters of wine. Furthermore, as a potential alternative to SO 2 , which acts as an antioxidant, PEF technology should not trigger oxidative reactions that compromise wine quality. Thus, once the effectivity of PEF treatments for controlling different microbial populations along the winemaking process had been observed, the effect of PEF on the oenological parameters of wines was evaluated. After 4 months of storage, the oenological parameters of the untreated and PEF-treated wines, with and without the addition of SO 2 after alcoholic and malolactic fermentation, are shown in Tables 4 and 5, respectively.  The results in Tables 4 and 5 show no significant differences between the PEF-treated wines and the untreated wines from a practical point of view in terms of pH, glucosefructose, % ethanol, and total and volatile acidity. Neither did PEF treatments significantly affect indexes related to polyphenol content, such as color index, total polyphenol index, and total anthocyanin content. These results support previous studies which reported that PEF treatments applied at moderate intensities did not impair wine properties [20,46].

Evaluation of the Effect of PEF Versus the Sterilizing Filtration Method on the Oenological and Sensory Properties of a Commercial Red Wine
Red wine is a valuable product in which, in addition to physicochemical properties, it is especially vital to maintain sensory characteristics. Color, flavor, and aroma characteristics are essential in wine quality. In order to prevent undesirable effects on the sensory properties of wine, thermal treatments have traditionally been avoided in the wine industry for microbial decontamination in comparison with other food industries. Consequently, before bottling, wine frequently undergoes a sterilizing filtration treatment to avoid microbial spoilage during its subsequent shelf life.
As pointed out above, when a liquid food is processed by PEF in a continuous flow, a temperature increment in the food occurs because all of the electrical energy required to generate the electric field is transformed into heat. In order to ascertain whether that temperature increment affected the oenological and sensory properties of wine, we compared a commercial wine ready for bottling after sterilizing filtration with the same wine treated by PEF at two different intensities that corresponded to outlet temperatures of 40 and 60 • C. The oenological parameters of wines either untreated, PEF-treated, or sterilized by filtration after 1 month of storage are presented in Table 6. In comparison to the untreated wine, PEF treatments did not affect oenological parameters, even in the case of the more intense treatment applied (155.6 kJ/kg; 60 • C). In contrast, the only difference found in Table 6 corresponds with the color index (CI) of the wine treated by means of sterilizing filtration, which was significantly lower (p ≤ 0.05). This finding confirms that microbial sterilization by means of a filtration process is a harsh procedure that affects wine color [47,48]. Regarding the effect of PEF on sensory properties of wine, Table 7 shows the results of the triangle test comparing the aroma and taste of wines sterilized by filtration and treated by PEF at two intensities. Results shown in Table 7 indicate that panelists were not able to detect differences in aroma and taste between wine after sterilizing filtration and the PEF-treated wines, even those treated at the highest intensity. More than 56% of correct responses are required for differences to be considered statistically significant (p < 0.05) [24]. Therefore, results obtained in the sensory study demonstrated that the rapid, brief temperature increment that occurred in a red wine as a consequence of the application of a PEF treatment did not negatively impair its oenological and sensory properties, even when the wine's outlet temperature was 60 • C. This result is particularly relevant and underscores PEF's potential for implementation as a microbial control method in the wine industry.

Conclusions
This study reinforces the growing evidence that PEF is a technology that can be potentially successful in helping to reduce the number of sulfites used in wineries, not only due to its effectivity in inactivating different microorganisms, but also due to its zero detrimental effect on wine quality.