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Article

Increasing the Safety and Storage of Pre-Packed Fresh-Cut Fruits and Vegetables by Supercritical CO2 Process

by
Alessandro Zambon
1,*,
Víctor González-Alonso
1,
Giovanna Lomolino
2,
Riccardo Zulli
1,
Andreja Rajkovic
3,4 and
Sara Spilimbergo
1
1
Department of Industrial Engineering, University of Padova, 35131 Padova, Italy
2
Department of Agronomy, Food, Natural Resources, Animals and Environment (DAFNAE), University of Padova, 35020 Legnaro, Italy
3
Department of Food Safety and Quality Management, University of Belgrade—Faculty of Agriculture, 11080 Belgrade, Serbia
4
Department of Food Technology, Safety and Health, Faculty of Bioscience Engineering, Ghent University, 9000 Ghent, Belgium
*
Author to whom correspondence should be addressed.
Foods 2023, 12(1), 21; https://doi.org/10.3390/foods12010021
Submission received: 2 November 2022 / Revised: 24 November 2022 / Accepted: 15 December 2022 / Published: 21 December 2022
(This article belongs to the Special Issue Advanced Research in Inactivation Technologies of Foodborne Microorganisms)
Browse Figures
Versions Notes

Abstract

:
This work presents a feasibility lab-scale study for a new preservation method to inactivate microorganisms and increase the shelf life of pre-packed fresh-cut products. Experiments were conducted on coriander leaves and fresh-cut carrots and coconut. The technology used the combination of hydrostatic pressure (<15 MPa), low temperature (≤45 °C), and CO2 modified atmosphere packaging (MAP). The inactivation was achieved for the naturally present microorganisms (total mesophilic bacteria, yeasts and molds, total coliforms) and inoculated E. coli. Yeasts and molds and coliform were under the detection limit in all the treated samples, while mesophiles were strongly reduced, but below the detection limit only in carrots. Inoculated E. coli strains were completely inactivated (>6.0 log CFU/g) on coconut, while a reduction >4.0 log CFU/g was achieved for carrots and coriander. For all the treated products, the texture was similar to the fresh ones, while a small alteration of color was detected. Microbiological stability was achieved for up to 14 days for both fresh-cut carrots and coconut. Overall, the results are promising for the development of a new mild and innovative food preservation technique for fresh food.

1. Introduction

The consumption of fresh fruits and vegetables as ready-to-eat (RTE) products has revolutionized the food industry, and it is expected to grow owing to the changing lifestyle of consumers [1]. However, when fresh-cut products are used as RTE, they usually have a limited shelf life (2–5 days), since they are affected by quick spoilage, mainly caused by oxidative enzymatic deterioration and microorganisms. Moreover, food safety in RTE food is still a challenge because a high risk of cross-contamination by pathogens can occur during the whole food chain. Good handling practices and an improvement in storage conditions and processing technologies are of primary importance to reduce the risk of outbreaks. Current technologies to increase the safety and shelf life of fresh-like products should be improved [2]. Modified atmosphere packaging (MAP) is the most widespread technology used to increase the shelf life of fresh RTE products [3]. By tuning the gas mixtures (usually N2, O2, and CO2) and the specific gas barrier characteristics of the packaging materials, MAP is able to slow down the spoilage process and the microbial growth rate, thus increasing product shelf life [4]. However, MAP technology has almost no impact on the microbial inactivation [5,6]. Preservatives [7] and additional pre-treatments [8] are often used to increase the quality and safety of the products in MAP. Moreover, the possibility of combining MAP with non-thermal technologies has been investigated. For example, MAP was used in combination with gamma irradiation [9,10] and high hydrostatic pressure (HHP) [11,12] to increase the microbial inactivation and the product shelf life. However, irradiation may raise safety concerns and can be negatively perceived by consumers [13], while the very high pressure needed for HHP (<4000 bars) might induce the irreversible transformation of the texture in the fresh products [14].
High-pressure carbon dioxide (HPCO2) was extensively investigated as an alternative low-temperature pasteurization process [15], showing microbial and enzymatic inactivation in both liquid and solid products [16]. In solids, the process has been successfully applied to several food categories, such as vegetables [17,18], fruits [19,20], poultry [21], meat [22], seeds [23], and mushrooms [24]. The process is effective at supercritical conditions, meaning that it can be carried out at mild temperatures because the critical temperature of CO2 is relatively low (31.1 °C), thus enhancing the maintenance of heat-sensitive components [25]. In the HPCO2 process, liquid CO2 is pumped inside a high-pressure chamber where the food is placed until reaching the desired process pressure. Following this, the pressure is maintained until achieving the desired microbial inactivation. At the end of the process, the CO2 is released, and the treated food can be further packaged. Currently, the process itself needs post-processing packaging, which might increase the risk of cross-contamination; thus, it might represent a barrier to industrialization.
Here, we present a preliminary study at the lab scale of a new patented method [26] for the microbial inactivation of fresh and cut RTE solid food. This new process combines the inactivation capacity of high-pressure CO2 within modified atmosphere packaging (HPMAP-CO2). The food is firstly packaged with CO2 as the modified atmosphere, and then the packaged sample is pressurized (pressure <15 MPa) until reaching supercritical CO2 (ScCO2) conditions using a pre-heated hydrostatic pressure vessel. The presented process is able to increase the current inactivation capacity of MAP technologies. Moreover, it avoids post-processing contamination, which might be possible after the HPCO2 process, because the inactivation is achieved after packaging.
The inactivation was evaluated for the naturally present microorganisms (total mesophilic bacteria, total coliforms, and yeasts and molds) and a typical contaminant and food hygiene and safety model organism (Escherichia coli) inoculated on the surface of the product before the treatment. The process was compared with conventional HPCO2 pasteurization for microbial inactivation performance on three products: coriander, carrots, and coconut. Texture and color analyses were used to assess the quality of the treated products.

2. Material and Methods

2.1. Sample Preparation

Fresh carrots, coconut, and coriander were purchased from a local market in Padua, Italy, and prepared according to the literature [27,28,29,30]. All foods were kept refrigerated at 4 °C and used within a few days. Carrots were washed and cut into round pieces of 2.0 ± 0.1 g, with a thickness of 3.0–5.0 mm; coconut was washed and cut into cubes of 2.0 ± 0.1 g; and coriander leaves of similar dimensions were selected and weighed to amount to 2.0 ± 0.1 g. After that, some products were directly treated with the HPCO2 process, while others were packaged as explained in Section 2.2.

2.2. Plastic Pouches Preparation

In total, 10 cm squared pouches were crafted manually using a high gas barrier plastic film (CO2 permeability ≤6.5 cm3/m2/d/bar; PA/EVOH/PA/PE, EuralPack, Shoten, Belgium). Each bag was loaded with 2.0 ± 0.1 g of food products, filled with either air or CO2 (Rivoira, Milan, Italy), and manually closed with a thermal sealer (Impulse sealer PFS-300, Zhejiang, China). The pouch volume was 100 ± 10 mL. Gas composition inside the bags was measured with a gas analyzer (Oxybaby M+I O2/CO2, WITT, Witten, Germany).

2.3. High-Pressure Processes

The HPCO2 processes were carried out within a multi-batch high-pressure apparatus, as explained previously [31,32]. Each product was inserted in a small high-pressure vessel. After the treatment, each reactor was opened under a laminar flow hood. The processed samples were collected in sterile containers and cooled down immediately to 4 °C until further analysis. The HPMAP-CO2 process was carried out using the equipment previously described by Barberi et al. [33]; the packaged products were pressurized by pre-heated water. The products were packaged with 100% CO2 or air (HPMAP-air); HPMAP-air was used as the additional control. At the end of the process, the pouches were removed, dried gently with paper towel, and stored at 4 °C until further analysis.
Process conditions were the same for both processes: 120 bar/40 °C/20 min for carrots, 120 bar/45 °C/30 min for coconut, and 100 bar/40 °C/1 min for coriander. The process conditions were selected from the literature in order to maximize the microbial inactivation [27,28,29,30,34].

2.4. Microbial Count for the Natural Flora

A standard plate count technique was used to analyze the microbial load. Samples were placed in 50 mL falcon tubes in sterility conditions, diluted 1:10 in phosphate-buffered saline solution (PBS; 0.01 M, pH 7.4; Oxoid, Hampshire, UK), and homogenized at 24.0 Hz for 1 min (Stomacher 400, International P.B.I., Milan, Italy). The solution was serially diluted (1:10) in PBS. Next, 100 µL of the appropriate dilutions was spread-plated onto the chosen media: chromogenic agar (Biolife Italiana s.r.l, Monza, Italy) for total coliforms and E. coli, and rose bengal (RB) (Sacco, Cadorago, Italy) for yeasts and molds; 1.0 mL was instead pour-plated into plate count agar (PCA) (Sacco, Cadorago, Italy) for the determination of the total mesophilic count. The incubation conditions were 37 °C and 24 h for E. coli, 30 °C and 48 h for total coliforms, 22 °C and 96 h for yeasts and molds, and 30 °C and 72 h for total mesophiles. At least three independent experiments were carried out for each single treatment condition, and the results were expressed as mean and standard deviation.

2.5. Culture and Inoculation of Escherichia coli

A clinically isolated Escherichia coli (Migula) Castellani and Chalmers (ATCC 25922) strain was used. From a frozen culture at −80 °C, the strain was resuscitated by successive overnight incubation of 100.0 µL culture in 10.0 mL of Luria-Bertani (LB) medium broth (Lennox, L3022, Sigma-Aldrich, St. Louis, MO, USA) at 37 °C. Bacterial culture was incubated at 37 °C with constant shaking (200 rpm), and the growth was carefully monitored spectrophotometrically until the stationary phase. The microbial suspension was centrifuged at 6000 rpm for 8 min; the supernatant was removed, and the pellet re-suspended in PBS reaching a final concentration of 1.0 × 1010 CFU/mL. Inoculated samples were spiked with 20 µL of E. coli suspension to reach a final inoculation level of 1.0 × 108 CFU/g. Spiked samples were dried under laminar flow for 30 min before further processing.

2.6. Texture Measurement

A TA.XTplus Texture analyzer (Stable Micro System, Godalming, UK) was used to measure the firmness of the carrot and coconut samples. A 500.0 N load cell, equipped with a 35.0 mm diameter compression probe, was applied; the compression rate was 2.0 mm/s, 25.0% of the initial height of the sample. For the measurement, carrots were cut into cylinders of 5.0 mm height and 10.0 mm diameter; coconut was cut into pieces and the measurement determined on the height of 10.0 mm. Results were expressed as mean value obtained from 10 different samples. The cutting test was also performed on the samples using a stainless-steel blade of 1.0 mm thickness (Lloyd Instruments LS5, Ametek, Berwyn, PA, USA) with a deformation rate of 2.0 mm/s and 75.0% strain. The cutting test was expressed as the maximum force (Newton) required to cut the sample from the beginning of the test. The parameter was acquired and processed with the Software Texture Exponent (Stable Micro Systems, Godalming, UK).

2.7. pH Measurement

The pH values were measured with an electronic pH meter equipped with a Sension + 5053T penetration pH electrode (Cri-son Instruments Sa, Barcelona, Spain) for food applications, which allowed automatic temperature compensation. At least 10 determinations were executed. The pH was measured 24 h after the process.

2.8. Color Measurement

The color measurement was carried out with a Chroma Meter Minolta CM-600d Sensing colorimeter (Minolta Sensing Inc., Osaka, Japan), on treated and untreated samples (carrot and coconut). The device was set with a CIE (Commission Internationale de l’Éclairage), 8° standard angle observer, and D65 illuminant. The parameters lightness (L*), redness (a*), and yellowness (b*) were recorded and calculated with the CIELAB system (1978) with 400–700 nm reflectance spectrum range. The Hue angle (H*) was calculated as:
H* = tan−1 (b*/a*),
while Chroma (C*) as:
C * = ( a * ) 2 + ( b * ) 2
respectively. For each condition, 10 measurements were carried out.

2.9. Microbiological Storage Test

Samples of carrot and coconut were prepared, packaged, and treated as described in the previous sections, and then stored for 14 days at 4 °C, with monitoring of the microbial growth of the natural flora and the evolution of the gas composition of the pouches. Untreated products packaged in air (MAP-air) and CO2 (MAP-CO2) were used as the controls. Analyses were performed after the treatment (day 0) and after 3, 7, and 14 days of storage.

2.10. Statistical Analysis

Statistical testing was performed in RStudio. Mean values were used to compare differences between treatments. The existence of significant differences (α = 95%) between different treatments was further considered using ANOVA and its subsequent post-hoc analysis (Tukey HSD); the Kruskal–Wallis rank-sum test and Wilcoxon rank-sum tests were used when the assumptions for an ANOVA were not fulfilled.

3. Results and Discussion

3.1. Microbial Inactivation

Figure 1 shows the comparison between the microbial inactivation achieved with the two processes (HPCO2 and HPMAP-CO2) for three food products: coriander (Figure 1a), carrot (Figure 1b), and coconut (Figure 1c).
The inactivation was demonstrated over a range of microbial groups in terms of naturally present microorganisms: total mesophiles, yeasts and molds, and total coliforms. A specific fecal indicator (E. coli) was also investigated by inoculation on the surface at a high concentration (1.0 × 108 CFU/g). The inactivation achieved with HPMAP-CO2 was comparable to the one achieved with the HPCO2 for total mesophilic bacteria, yeasts and molds, and coliforms in all the products. Instead, a slightly higher E. coli inactivation was achieved for coriander and carrots with the HPCO2 process. For coriander, a total inactivation of the mesophiles was not possible for either treatment, while a complete inactivation was achieved for yeasts and molds with the HPCO2, and total coliforms using both processes. These results agree with our previous results achieved with coriander. Indeed, mesophilic bacteria were more resistant to the supercritical CO2 treatment compared with yeasts and molds [27]. Spiked E. coli on coriander was under the detection limit after the HPCO2 process, while almost a 3.0 log CFU/g reduction was achieved with the HPMAP-CO2. Bordeaux et al. showed that a complete inactivation of spiked E. coli was possible after the HPCO2 process [28].
For carrots, a similar inactivation for all naturally present microorganisms was achieved with the two processes. Regarding the inoculated E. coli, a total inactivation was achieved only after the HPCO2 treatment, while 4.66 log CFU/g were reduced with HPMAP-CO2. Tamburini et al. [35] also showed a complete inactivation when spiked carrots were treated with HPCO2 at 120 bar—35 °C—10 min, while Ferrentino et al. [36] showed a complete inactivation also at a lower pressure (100 bar).
For coconut, a total inactivation of total coliforms and E. coli with both processes was observed, but not for the total mesophilic bacteria. Yeasts and molds were under the detection limit only after the HPCO2 process. In the case of mesophilic bacteria, HPCO2 resulted in a slightly higher inactivation compared to HPMAP-CO2, which nevertheless was not found to be significant. Previous studies, with HPCO2 at similar process conditions [30,36], showed a similar inactivation degree; however, a direct comparison might be misleading because the initial load was slightly different. Previous studies with HPCO2 treatment with E. coli on coconut showed a reduction at 60 bar/25 min/35 °C up to 5.0 log CFU/g [34]. These data indicate that E. coli in coconut is easily inactivated by CO2 even at milder conditions.
Overall results demonstrated that at a small scale the inactivation with HPMAP-CO2 and HPCO2 was comparable for the naturally present microorganisms, while the inactivation of inoculated E. coli was different between the two processes in carrots and coriander. The lower inactivation achieved with HPMAP-CO2 for E. coli in carrots and coriander should be further investigated with a wider number of strains and process conditions. The lower inactivation in the case of HPMAP-CO2 might also be explained by the presence of the packaging, which is known to influence the inactivation in the thermal pasteurization [37,38]. It might be possible that the packaging reduces the heat mass transfer, thus reducing the effective process time in which the CO2 is at a supercritical state. However, further studies are needed to confirm any hypothesis.
Two different controls with the HPMAP-CO2 process were carried out (Figure 2) to demonstrate that the microbial inactivation was due to the effect of CO2 at a supercritical state. In the first one, the products were packaged with air instead of CO2, and then processed with HPMAP (HPMAP-air). In the second one, the products were packaged in CO2 and then maintained at the processing temperature for the whole processing time (TMAP-CO2). Microbial inactivation was not achieved when air was used instead of CO2 in the HPMAP process, demonstrating that the pressure itself was not responsible for any microbial reduction. The need for a simultaneous application of pressure, temperature, time, and CO2 was also confirmed by TMAP-CO2. In addition, in this case, the inactivation was negligible for all microorganisms in all the products.
Statistical testing confirmed the significant difference (p-value < 0.05) for all microbial groups (mesophiles, yeasts and molds, and coliforms), in all food products tested, between the samples treated with high-pressure CO2 (HPCO2 and HPMAP-CO2) and the others (untreated control sample, HPMAP-air, and TMAP-CO2).
The gas composition and the volume of the packages were also measured. These values were not significantly different between the treated and untreated samples.

3.2. Texture, pH, and Color Analysis

Traditional HPCO2 and HPMAP-CO2 processes were compared for texture, pH, and color change. As regards the texture, previous works suggested that fruits and vegetables treated with HPCO2 could lose their consistency, and thus becoming useless as an RTE product. Specifically, Valverde et al. [39] reported that pears treated with pressurized CO2 lost their consistency, and this loss was higher as the pressure was increased. Haas et al. [40] reported similar findings for strawberries and melons treated with HPCO2.
The HPMAP-CO2 process induced a consistent change of color and integrity on coriander leaves, similarly to what we reported previously with HPCO2 [41]. A discoloration and a reduction in the firmness were also previously observed on spinach leaves after the HPCO2 [18] and HPP processes [42], suggesting that in general, leaves are not good candidates for high-pressure processes. On the contrary, the visual appearance of coconut and carrots was very similar to the fresh product, demonstrating that firm products could be good food products for both HPCO2 and HPMAP-CO2 processes. For this reason, only carrots and coconuts were further investigated in this study for qualitative analysis.
The cutting force applied with a blade on a food matrix could provide indications of the fracture resistance (using the maximum force during the cutting cycle), and the rubbery behavior of the tissue, as indicated by the increase in both displacement and cutting force. A low cutting force might indicate a food matrix with a fragile structure. The results reported in Table 1 show that the untreated carrots (packaged in air (MAP-air) or CO2 (MAP-CO2)) and the ones treated with HPMAP-CO2 did not show significant differences for the cutting force, indicating that the process did not change the original texture and firmness of the carrots. On the contrary, samples treated with the traditional HPCO2 process presented a lower cutting force value, which was statistically different from the other samples. The low value after the HPCO2 process could be due to the de-structuring effect of the high pressures on the carrots’ tissue that could modify the cellular microstructure with consequent texture alteration [43]. In fact, as reported by Sun et al. [44], the high pressures can cause cell corruption and cell collapse up to destructive damage, cell disruption, cell wall dissolution, and overall texture degradation. These findings suggest that the HPMAP-CO2 process could reduce the de-structuring effect caused by the HPCO2 process, making the treatment more suitable for the development of minimally processed RTE products.
Coconut, on the other hand, did not show significant differences in the cutting force parameter, which was similar in all the samples (treated and untreated). This evidence may be due to the chemical composition and the particular structure of the coconut tissue which were minimally affected by the treatments applied. This finding was already demonstrated by Ferrentino et al. [19], who showed that coconut treated with HPCO2 maintained the same consistency compared to the fresh, untreated one.
Finally, the textural firmness did not show significant differences for all the samples. The stress–strain curves did not present statistically significant differences in the tracings and repetitions for all the trials.
The pH for the untreated products was 6.10 and 6.17 for the carrot and coconut, respectively. These pH values are similar to the literature [19,29,45]. Neither the MAP-CO2 itself nor the high-pressure treatments significantly changed the pH, in contrast to what was reported in the literature for the HPCO2 treatment [19,29], where a slight reduction in the pH was observed after the treatment. In our case, the measurements were performed 24 h after the treatment, allowing the establishment of an equilibrium of the solubilized CO2 with the environment and a subsequent return to the original pH. This observation is important for the development of RTE products and consumers’ acceptance, since small changes in the pH could influence the sensorial perception.
The color measurements are reported in Table 2 for carrots and coconut. The carrots treated with the HPMAP-CO2 and HPCO2 processes had the highest and significantly different b* values compared to the not-treated products (MAP-air and MAP-CO2). Significant differences were observed for the parameter a* (red/green). The highest a* values were present in the untreated products, while the processes induced lower a* values, according to what was reported by Trejo Araya et al. [46]. Based on the colorimetric data, the control samples had a more intense orange color than the treated ones. The non-treated samples did not show significant differences for the L* (lightness) parameter. On the contrary, the treated samples showed significantly lower L* values. The spatial distribution of the color was given by the hue angle (H*) and chroma (C*). The hue angle parameter showed significant differences among the carrot samples. In particular, the treated samples showed the greatest hue angle, i.e., an inclination towards yellow. Additionally, the chroma parameter had higher values for the treated samples rather than for the control.
Furthermore, the coconut showed some significant differences for the parameters a* and L*, which were lower in the treated sample, indicating a variation in the coloring toward green. The parameters b* and C* were not affected by the treatment. On the contrary, the hue angle had significantly higher values in the coconut samples that were subjected to the treatments.
These findings indicate that the process induced a visual change of the original color of the fresh products. For this reason, it has become more and more important to develop and improve methodologies to optimize the process minimizing the change of color, as previously reported by Barberi et al. [33]. A sensorial analysis should also be performed to confirm the perception of the consumers caused by the treatment.

3.3. Microbiological Stability

A storage test at 4 °C for up to 14 days was performed for fresh-cut carrots and coconut as a proof-of-concept for the potentiality of the new HPMAP-CO2 technology at improving the product’s shelf life.
Figure 3 reports the microbial load on fresh-cut carrot for the treated HPMAP-CO2 and two controls (MAP-air and MAP-CO2). The initial microbial load was 4.2, 2.6, and 3.5 log CFU/g for mesophiles (Figure 3a), yeasts and molds (Figure 3b), and coliforms (Figure 3c), respectively. The average gas composition in terms of % CO2 and % O2 was also recorded (Figure 2d).
The results showed that the HPMAP-CO2 treatment was able to reduce the microbial load to undetectable levels of mesophiles, yeasts and molds, and total coliforms, and that microbial counts remained stable over a 14-day storage period. Untreated products showed microbial growth in both CO2 and MAP-air, eventually reaching spoilage levels.
The gas composition of the pouches filled with 100% CO2 (both treated and not treated) remained stable between 95.0 and 98.0% over the storage period, while the packages filled with air underwent a decrease in O2 down to 16.0% by day 14, and a slight increase in CO2 concentration probably caused by the growth of microorganisms and the respiration of the plant tissues.
The bacteriostatic effect of MAP-CO2 in the untreated product was revealed for yeasts and molds and coliforms compared with the MAP-air. Yeasts and molds have been previously reported to be sensitive to high CO2 concentrations during MAP [6]. On the contrary, for total mesophilic bacteria, the load of samples in MAP-CO2 started to be slightly higher than the MAP-air on day 7, reaching a 1.5 log higher load on day 14 compared with the MAP-air sample. This could indicate an overgrowth of lactic acid bacteria in the 100% CO2 samples due to the absence of oxygen [4,6].
Compared to traditional MAP technology, HPMAP-CO2 could extend the shelf life of fresh-cut carrots up to 14 days (or more). Recently, the use of pectin-coating showed the ability to increase the shelf life of fresh-cut carrots up to 12 days [47]. The technology could be potentially coupled with HPMAP-CO2 to obtain a synergistic effect. Microbial inactivation could be increased by tuning pressure, temperature, and treatment time, inducing a higher inactivation. Sensorial studies should be also performed to validate the consumers’ acceptance of the technology.
Figure 4 shows the microbial counts found on fresh-cut coconut for mesophiles (Figure 4a), yeasts and molds (Figure 4b), and coliforms (Figure 4c), as well as the gas composition of the plastic pouches (Figure 4d) during a storage trial of 14 days. The initial microbial load was 6.5, 4.5, and 6.3 log CFU/g for mesophiles, yeasts and molds, and coliforms, respectively. The results showed higher variability compared to the shelf-life trial performed on carrots. On day 0, reductions of 2.2, 2.4, and 3.3 log CFU/g were achieved for mesophiles, yeasts and molds, and coliforms, respectively, compared to the untreated products, which were statistically significant (p < 0.05). In all three microbial groups, the counts of MAP-air at day 14 were higher than 7.0 log CFU/g for mesophiles and coliforms. However, the count up to day 7 did not show a significant increment compared to day 0, which could indicate a higher variability on the initial count due to a random contamination with the shell. However, data on day 14 demonstrated that untreated samples in MAP-CO2 had a lower growth compared to MAP-air, which is consistent with a bacteriostatic effect of high CO2 concentration MAP. The treated bags did not reach spoilage levels during the 14-day storage trial.
The HPMAP-CO2 coconut shelf life at 4 °C could be extended up to 14 days (or longer) in terms of microbial spoilage in comparison to samples stored in air at the same temperature. Our finding is promising for the obtainment of an extension of the shelf life of fresh-cut coconut, which in a previous study by Sinigalli et al. [48] was only 7 days.
The gas composition (Figure 4d) of the pouches loaded with fresh-cut coconut showed a different behavior compared with carrots. The concentration of O2 in MAP-air was reduced from 20.4% on day 0 to 19.0% on day 14. The different O2 consumption can be explained by the different respiration rates of coconut and carrot [49]. The CO2 in the MAP-CO2 was reduced from 95.0% CO2 on day 0, to 87.7% on day 14, while for the HPMAP-CO2, the composition was 79.0% after the treatment, and 58.0% on day 14. It is not very clear how the change in gas permeability observed compared with carrots, and additional experiments with different kinds of products and packaging materials should be performed.

4. Conclusions

This work compared a new HPMAP-CO2 process with the traditional HPCO2 inactivation treatment. Despite its benefit, HPCO2 has never been used industrially to produce RTE foodstuff. Within this work, we proved the potential of HPMAP-CO2 to be used as an alternative technology to increase the safety and the shelf life of fresh RTE food. The comparison between the two technologies was performed at the lab scale on three food categories: fresh-cut carrots, fresh-cut coconut, and coriander leaves. The inactivation degree was similar between the processes, even if a slightly higher inactivation was achieved for mesophilic bacteria and inoculated E. coli in carrots with the HPCO2. The microorganisms in coconut were easily inactivated with both the processes. The microbiological shelf life was achieved up to 14 days with the HPMAP-CO2. HPMAP-CO2 was able to preserve the original texture of the fresh carrots better than HPCO2, while for the coconut, no differences were found after both treatments. The treatments induced a slight change in color compared to the untreated products. A further analysis should be performed to demonstrate the inactivation capacity over a wider group of spiked pathogens and the process scalability by processing bigger amounts of products. Moreover, the enzymatic activity and the retention of the nutritional properties on the treated and untreated products during the storage should be also considered in further studies. Overall, the technology results are promising for the development of a new low-temperature inactivation treatment that could be applied to strong, firm, fresh products.

Author Contributions

Conceptualization, A.Z. and S.S.; methodology, A.Z., V.G.-A., G.L. and S.S.; formal analysis, V.G.-A., G.L.; investigation, V.G.-A.; resources, G.L. and S.S.; data curation, A.Z., V.G.-A. and R.Z.; writing—original draft preparation, A.Z., V.G.-A., G.L., R.Z., A.R. and S.S.; writing—review and editing, A.Z., V.G.-A., G.L., R.Z., A.R. and S.S.; supervision, A.Z., A.R. and S.S.; project administration, A.Z. and S.S.; funding acquisition, A.Z. and S.S. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by “Fondazione Cassa di Risparmio di Padova e Rovigo” through the grant “CARIPARO Visiting Programme 2018”, Innovation Voucher funded by the Interreg ADRION—ADRIATIC-IONIAN Programme “OISAIR” Proof of Concept Call-AREA Science Park; the Department of Industrial Engineering (University of Padova) “Progetto Strategico di Dipartimento” (CoSID) SPIL_SID18_01; the H2020 ERA-NETs SUSFOOD2 and CORE Organic Cofunds, under the Joint SUSFOOD2/CORE Organic Call 2019, project “HO-FOOD, Innovative High pressure process to increase the preservation of ready-to-eat Organic FOOD” CUP C95F20000930001.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

The data are available from the corresponding author.

Acknowledgments

All the authors thank Massimo Vetralla for the support in the experimental activity. G.L. thanks Luciano Magro of the LaCHI Laboratory of the DAFNAE Department (University of Padua), and Fabio Santi for the support for the analytical activity.

Conflicts of Interest

A.Z. and S.S. are co-inventors of the patent describing the new method for food pasteurization: Italian patent n. 10201700009804, European patent application n. 17787252.0, Chinese patent application n. 201780094448.6, and US patent application n. 16/642,401.

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Foods 12 00021 g001 550
Figure 1. Microbial counts of total mesophiles, yeasts and molds, total coliforms, and spiked E. coli, measured on coriander (a), carrot (b), and coconut (c), in the untreated samples (Foods 12 00021 i001), the ones treated directly with high-pressure carbon dioxide (HPCO2, Foods 12 00021 i002) and the ones treated inside the packaging (HPMAP-CO2, Foods 12 00021 i003). Treatment conditions were: 120 bar/40 °C/20 min for carrots, 100 bar/40 °C/1 min for coriander, and 120 bar/45 °C/30 min for coconut. * ND—Not detected. No colonies were found at the lowest dilution possible (<2.0 log CFU/g for yeasts and molds, coliforms, and E. coli, <1.0 log CFU/g for mesophiles).
Figure 1. Microbial counts of total mesophiles, yeasts and molds, total coliforms, and spiked E. coli, measured on coriander (a), carrot (b), and coconut (c), in the untreated samples (Foods 12 00021 i001), the ones treated directly with high-pressure carbon dioxide (HPCO2, Foods 12 00021 i002) and the ones treated inside the packaging (HPMAP-CO2, Foods 12 00021 i003). Treatment conditions were: 120 bar/40 °C/20 min for carrots, 100 bar/40 °C/1 min for coriander, and 120 bar/45 °C/30 min for coconut. * ND—Not detected. No colonies were found at the lowest dilution possible (<2.0 log CFU/g for yeasts and molds, coliforms, and E. coli, <1.0 log CFU/g for mesophiles).
Foods 12 00021 g001
Foods 12 00021 g002 550
Figure 2. Microbial counts of total mesophiles, yeasts and molds, and total coliforms, on coriander (a), carrot (b), and coconut (c), in the untreated samples (Foods 12 00021 i001), the ones treated inside the packaging with air (HPMAP-air, Foods 12 00021 i002), the ones packaged in CO2 and maintained at the processing temperature and time (TMAP-CO2, Foods 12 00021 i004), and the ones treated inside the packaging in CO2 (HPMAP-CO2, Foods 12 00021 i003). Treatment conditions were: 120 bar/40 °C/20 min for carrot, 100 bar/40 °C/1 min for coriander, and 120 bar/45 °C/30 min for coconut. Means with different small superscript letters in the same group of microorganisms are significantly different (p < 0.05). * ND—Not detected. No colonies were found at the lowest dilution possible (<2.0 log CFU/g for yeasts and molds, coliforms, and E. coli, <1.0 log CFU/g for mesophiles).
Figure 2. Microbial counts of total mesophiles, yeasts and molds, and total coliforms, on coriander (a), carrot (b), and coconut (c), in the untreated samples (Foods 12 00021 i001), the ones treated inside the packaging with air (HPMAP-air, Foods 12 00021 i002), the ones packaged in CO2 and maintained at the processing temperature and time (TMAP-CO2, Foods 12 00021 i004), and the ones treated inside the packaging in CO2 (HPMAP-CO2, Foods 12 00021 i003). Treatment conditions were: 120 bar/40 °C/20 min for carrot, 100 bar/40 °C/1 min for coriander, and 120 bar/45 °C/30 min for coconut. Means with different small superscript letters in the same group of microorganisms are significantly different (p < 0.05). * ND—Not detected. No colonies were found at the lowest dilution possible (<2.0 log CFU/g for yeasts and molds, coliforms, and E. coli, <1.0 log CFU/g for mesophiles).
Foods 12 00021 g002
Foods 12 00021 g003 550
Figure 3. Fresh-cut carrot microbial levels of total mesophiles (a), yeasts and molds (b), and total coliforms (c), and gas composition (d), in the control packaged in air (MAP-air) (Foods 12 00021 i005), control packaged in CO2 (MAP-CO2) (Foods 12 00021 i006), and the treated packaged in CO2 (HPMAP-CO2) (Foods 12 00021 i007), during a shelf-life trial at 4 °C. Treatment conditions were 120 bar—40 °C—20 min. Points with different small letters at the same time point represent significantly different values (p < 0.05). * ND—Not detected. No colonies were found at the lowest dilution possible (< 1.0 log CFU/g).
Figure 3. Fresh-cut carrot microbial levels of total mesophiles (a), yeasts and molds (b), and total coliforms (c), and gas composition (d), in the control packaged in air (MAP-air) (Foods 12 00021 i005), control packaged in CO2 (MAP-CO2) (Foods 12 00021 i006), and the treated packaged in CO2 (HPMAP-CO2) (Foods 12 00021 i007), during a shelf-life trial at 4 °C. Treatment conditions were 120 bar—40 °C—20 min. Points with different small letters at the same time point represent significantly different values (p < 0.05). * ND—Not detected. No colonies were found at the lowest dilution possible (< 1.0 log CFU/g).
Foods 12 00021 g003
Foods 12 00021 g004 550
Figure 4. Fresh-cut coconut microbial levels of total mesophiles (a), yeasts and molds (b), and total coliforms (c), and gas composition (d), in the control packaged in air (MAP-air) (Foods 12 00021 i005), control packaged in CO2 (MAP-CO2) (Foods 12 00021 i006), and the treated packaged in CO2 (HPMAP-CO2) (Foods 12 00021 i007), during a shelf-life trial at 4 °C. Treatment conditions were 120 bar—45 °C—30 min. Points with different small letters at the same time point represent significantly different values (p < 0.05). * ND – Not detected. No colonies were found at the lowest dilution possible (<1.0 log CFU/g) in at least one repetition.
Figure 4. Fresh-cut coconut microbial levels of total mesophiles (a), yeasts and molds (b), and total coliforms (c), and gas composition (d), in the control packaged in air (MAP-air) (Foods 12 00021 i005), control packaged in CO2 (MAP-CO2) (Foods 12 00021 i006), and the treated packaged in CO2 (HPMAP-CO2) (Foods 12 00021 i007), during a shelf-life trial at 4 °C. Treatment conditions were 120 bar—45 °C—30 min. Points with different small letters at the same time point represent significantly different values (p < 0.05). * ND – Not detected. No colonies were found at the lowest dilution possible (<1.0 log CFU/g) in at least one repetition.
Foods 12 00021 g004
Table
Table 1. Texture analysis: effect of the different treatments on the cutting test (N) and textural firmness (J), carried out on carrots and coconut. Treatment conditions were the same as detailed in Section 3.1. Values in brackets are SD. Means with different small superscript letters in the same column are significantly different (p < 0.05).
Table 1. Texture analysis: effect of the different treatments on the cutting test (N) and textural firmness (J), carried out on carrots and coconut. Treatment conditions were the same as detailed in Section 3.1. Values in brackets are SD. Means with different small superscript letters in the same column are significantly different (p < 0.05).
TreatmentCarrot (N)Coconut (N)Carrot (J)Coconut (J)
MAP-air77.56 (12.29) a31.34 (3.93) a0.17 (0.02) a0.14 (0.02) a
MAP-CO276.27 (11.48) a31.21 (3.11) a0.16 (0.01) a0.14 (0.02) a
HPMAP-CO279.17 (12.39) a30.81 (4.62) a0.16 (0.03) a0.15 (0.03) a
HPCO261.69 (11.72) b32.23 (6.15) a0.14 (0.02) a0.14 (0.03) a
Table
Table 2. Effect of the different treatments on the color of carrots and coconut, measured by CIELAB system, hue angle (H*), and chroma (C*). Treatment conditions were the same as detailed in Section 3.1. Values in brackets are SD. Means with different small superscript letters in the same column are significantly different (p < 0.05).
Table 2. Effect of the different treatments on the color of carrots and coconut, measured by CIELAB system, hue angle (H*), and chroma (C*). Treatment conditions were the same as detailed in Section 3.1. Values in brackets are SD. Means with different small superscript letters in the same column are significantly different (p < 0.05).
L*a*b*ChromaHue
Carrot
  MAP-air62.46 (1.33) a31.70 (0.86) a42.65 (1.37) a53.15 (1.37) a53.37 (0.94) a
  MAP-CO260.24 (1.67) a33.59 (0.95) a45.74 (3.75) ab56.77 (3.42) ab53.62 (1.88) a
  HPMAP-CO260.44 (3.58) a28.31 (2.10) b49.42 (2.78) b56.98 (2.97) b60.19 (1.87) b
  HPCO257.99 (1.23) b26.90 (1.18) b50.33 (5.91) b57.12 (5.48) b61.68 (2.52) b
Coconut
  MAP-air83.26 (2.48) a−0.65 (0.16) a3.66 (0.60) a3.72 (0.59) a100.47 (3.54) a
  MAP-CO282.86 (2.34) a−0.78 (0.09) ac3.63 (0.63) a3.72 (0.61) a102.40 (2.53) ab
  HPMAP-CO281.70 (1.62) ab−0.87 (0.18) bc3.43 (0.89) a3.55 (0.86) a105.08 (4.07) b
  HPCO279.82 (2.54) b−0.98 (0.17) b4.38 (1.24) a4.49 (1.23) a103.25 (3.06) ab
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Zambon, A.; González-Alonso, V.; Lomolino, G.; Zulli, R.; Rajkovic, A.; Spilimbergo, S. Increasing the Safety and Storage of Pre-Packed Fresh-Cut Fruits and Vegetables by Supercritical CO2 Process. Foods 2023, 12, 21. https://doi.org/10.3390/foods12010021

AMA Style

Zambon A, González-Alonso V, Lomolino G, Zulli R, Rajkovic A, Spilimbergo S. Increasing the Safety and Storage of Pre-Packed Fresh-Cut Fruits and Vegetables by Supercritical CO2 Process. Foods. 2023; 12(1):21. https://doi.org/10.3390/foods12010021

Chicago/Turabian Style

Zambon, Alessandro, Víctor González-Alonso, Giovanna Lomolino, Riccardo Zulli, Andreja Rajkovic, and Sara Spilimbergo. 2023. "Increasing the Safety and Storage of Pre-Packed Fresh-Cut Fruits and Vegetables by Supercritical CO2 Process" Foods 12, no. 1: 21. https://doi.org/10.3390/foods12010021

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