Plant material, treatments and experimental design

‘Tommy Atkins’ mangoes were obtained from an orchard located in Culiacan, Sinaloa, Mexico (24° 46’ 23’’ N and 107° 32’ 56’’ W, at 26 m a. s. l.). The fruits were harvested from trees 15 and 20 years old located in sandy or clay soils, warm weather (30-34 °C). The plants were maintained with drip irrigation before the rainy season. The fruits were selected in stage 2 (8-11 °Brix) (^{Crisosto et al., 2009}) with absence of physical damage and a weight range of approximately 350 to 420 g, and transferred to the Physiology and Technology Postharvest laboratory at the Autonomous University of Sinaloa, Mexico.

Fruits were cleaned by dipping in a solution of 300 (L·L^-1 sodium hypochlorite for 3 min, air dried and randomly divided into four groups. Each group received one of the following treatments: control (immersed in water at room temperature), HWT₁ (dipping in water at 46.1 °C for 75 [^{USDA-APHIS, 2014]}), HWT₂ (dipping in water at 55 °C for 5 min [^{Ghasemnezhad et al., 2008}]), and HWT₁ + HWT₂ (sequential treatment under the same aforementioned conditions, applied one after the other).

The HWT were carried out using a water bath (1266-02, Cole-Parmer®, Thermo Scientific, USA) with continuous hot water recirculation. Untreated mangoes (immersed in water at room temperature) were used as the control. Fruits of each treatment were stored at 5 °C (85-90 % relative humidity) for 15 and 30 days. After storage for 30 days at 5 °C, the fruits were exposed to ripening for 4 and 8 days at 21 °C ± 1 °C.

Parameters evaluated

Statistical analysis

Data were subjected to a two-way analysis of variance (ANOVA) using Stat-graphics Plus 5.1 software (Statistical Graphics, Rockville, MD). The effect of treatments (control, HWT₁, HWT₂ and HWT₁+HWT₂) and days of storage (0, 15, 30, 30+4 and 30+8 days) were the factors analyzed. Significant differences (P < 0.05) between means were established using Fisher’s least significant difference (LSD) test. Unless another number is indicated, three replicates with five repetitions were used for the analysis.

Chilling injury index

The application of HWT and storage time had a significant effect on the presence of CI symptoms like pitting, uneven color development and decay in “Tommy Atkins” mango (Figure 1). The application of HWT₁, HWT₂ or HWT₁ + HWT₂ significantly reduced the susceptibility to CI compared with the control after 30 days at 5 °C (Figure 1a). When fruits were transferred at ripening, the presence of symptoms increased as the storage period progressed (30+8 days) (Figure 1b). Mangoes treated with HWT₂ and HWT₁ + HWT₂ resulted in a lower CII (1.72). When doing a linear regression analysis, HWT₂ showed the lowest rate in the appearance of symptoms during storage at 5 °C (linear term coefficient of 0.053, coefficient of determination of R² 0.999), while HWT₁ + HWT₂ presented this behavior during storage at 21 °C (linear term coefficient of 0.080, coefficient of determination of R² 0.955). This result is related to postharvest heat treatment, since it generates physiological and biochemical changes in the fruit. These changes are related to factors such as the type of heat treatment, the exposure time and the fruit genotype (^{Ummarat, Matsumoto, Wall, & Seraypheap, 2011}).

Figure 1 a) Chilling injury index (CII) of “Tommy Atkins” mango during storage at 5 °C plus 4 and 8 days at 21 °C, and b) representative images of mango from each treatment after 30 days at 5 °C plus 8 days at 21 °C. HWT = hot water treatments. Data are the mean of five replicates with Fisher’s least significant difference (LSD = 0.17) as vertical bars. Different letters show significant differences among treatments (Fisher, P < 0.05). 

The increase in CI tolerance favored by an individual short or long heat treatment has been previously reported in “Tuu Shien” and ‘Keitt’ mango (^{Le et al., 2010}; ^{Díaz-Corona et al., 2020}), “Hom Thong” banana (^{Ummarat et al., 2011}) and “Hongyang” kiwifruit (^{Ma et al., 2014}). Also, this tolerance was observed when sequential heat treatment was applied in “Frangi” papaya (^{Shadmani et al., 2015}). The ability of HWT₂ and sequential treatment to reduce CII can be attributed to the maintenance of cell membrane integrity (less MDA content) and a reduction in membrane permeability (less EL; Figure 2a), as well as an increase in the enzymatic antioxidant system that protects cells from oxidative stress in fruit subjected to HWT₁ + HWT₂.

Figure 2 a) Electrolyte leakage and b) malondialdehyde (MDA) content in “Tommy Atkins” mango during storage at 5 °C plus 4 and 8 days of ripening at 21 °C. HWT = hot water treatments. Data are the mean of five replicates with Fisher’s least significant difference (LSD = 0.17) as vertical bars. Different letters show significant differences among treatments (Fisher, P < 0.05). 

Also, the reduction in CI susceptibility in HWT₁ fruit with respect to the control was related to higher enzymatic activity, but not to a reduction in cell membrane damage, since HWT₁ presented higher MDA and EL values than the control. Thus, the use of sequential heat stress allows a greater activation of the antioxidant system in the fruit, priming it for greater stress such as long-term cold stress (30 days at 5 °C).

Electrolyte leakage and malondialdehyde

The EL increased in different proportions during storage at 5 °C and room temperature for all treatments. At day 15, mango treated with HWT₂ and HWT₁ + HWT₂ presented lower EL than HWT₁ and the control, while after 30 days of cold storage, only the HWT₁ + HWT₂ treatment maintained the lowest EL. However, during storage at 21 °C, all treatments presented similar EL (Figure 2a). In regression analysis at 5 °C, HWT₁ + HWT₂ showed the lowest rate of electrolyte release, obtaining a linear term coefficient of 0.437 (coefficient of determination of 0.983), while, contrary to what was observed in the analysis of variance at 21 °C, HWT₁ presented the lowest rate in EL (linear term coefficient of 0.141, coefficient of determination of R² 0.826).

On the other hand, MDA content increased with storage time at both storage temperatures (Figure 2b). Fruit treated with HWT₂ showed the lowest MDA content at the end of storage at 5 °C, followed by fruit of the sequential treatment, while the application of HWT₁ promoted a higher MDA content, even over the control. During ripening, fruit treated with different HWTs presented higher MDA content than the control, but the use of HWT₁ + HWT₂ allowed lower lipid peroxidation. Similar behavior was observed in linear regression analysis, as HWT₂ presented the lowest MDA production rate with a regression coefficient of 0.052 and coefficient of determination of R² 0.989 at 5 °C. On the other hand, at 21 °C, this analysis showed that HWT₁ presented the lowest MDA production rate with a regression coefficient of 0.398 and coefficient of determination of R² 0.999, which differs from the analysis of variance possibly due to variability in MDA production.

The abiotic stress produced by low temperatures promotes oxidative damage in fruit and fast senescence. Therefore, accumulation of reactive oxygen species (ROS) in cells due to stress can result in membrane deterioration and an increase in EL and MDA content (^{Nasef, 2018}). The use of HWT₂ and HWT₁ + HWT₂ protected the cell membrane, reducing the levels of EL and MDA during cold storage. However, after removing from 5 °C, HWT fruit showed significant increases in these parameters. Similar results were previously reported in different fruits (pomegranate, mandarin, banana, and cucumber) treated with HW for a short time (40 to 55 °C, 4 to 10 min), where heat treatment reduced membrane damage (^{Mirdehghan et al., 2007}; ^{Ghasemnezhad et al., 2008}; ^{Ummarat et al., 2011}; Nasef, 2018).

^{Nasef (2018}) reported that heat treatment (55 °C for 5 min) alleviated CI in cucumbers due to a reduction in EL and retention of membrane integrity. Likewise, the behavior of the sequential treatment of the present study was similar to that of the combination of two HWTs (36.5 °C for 75 min plus 46.5 °C for 61 min) in “Tommy Atkins” mango stored at 4 and 9 °C, because the sequential heat treatment may delay ripening and softening, and thus reduce EL (^{Nyanjage et al., 1999}). The individual application of heat treatments presented similar EL to the control. This increase in cell membrane permeability is attributed to the effects of heat stress, as it induces the activation of heat shock proteins, the arginine pathway, and glucose metabolism. Furthermore, it increases antioxidant enzymes and antioxidant compounds such as ascorbic acid and glutathione, which inhibit peroxidative damage (^{Zhang et al., 2019}).

Weight loss

All treatments presented an increase in WL during storage at 5 °C, reaching values ranging from 2.98 % for HWT₁ + HWT₂ up to 3.92 % for HWT₁ at the end of storage (Figure 3). Mango treated with a sequential treatment resulted in the lowest WL (2.98 %), showing significant differences (P < 0.05) with the fruit of the other treatments after 36 days at 5 °C. Interestingly, HWT₁ and control fruit had similar values and resulted in the highest WL percentages. Likewise, this study revealed that HWT₁ + HWT₂ was more effective in reducing WL than the individual application of each heat treatment, which suggests that sequential heat treatment could reduce alterations in fruit peel, transpiration and respiration during cold storage, without inhibiting ripening when transferred to room temperatures (^{Shadmani et al., 2015}).

Figure 3 Weight loss of Tommy Atkins mango during storage at 5 °C. Data are the mean of nine replicates. Vertical bars represent Fisher’s least significant difference (LSD) = 0.33. 

The application of sequential heat treatment in mango could increase the barrier properties of cuticle and epicuticular wax, maintaining the integrity of the tissue (^{Shadmani et al., 2015}). Contrary to these results, “Kensington” mango subjected to sequential treatment for a long time (vapor heat, 40 °C for 8 h plus HWT, 47 °C for 15 min) and stored at ripening temperature showed increased WL (2.29 %), a higher respiration rate, accelerated ripening (11.43 N in firmness, 13.92 °Brix, 0.96 titratable acidity), and increased transpiration and dehydration, compared to control fruit (^{Jacobi, Macrae, & Hetherington, 2000}). On the other hand, ^{Nasef (2018}) reported that WL of cuccumbers was affected by treatment temperature (45 or 55 °C for 5 min), storage period (7, 14, 21 days at 5 °C plus 2 and 4 days at 20 °C), and their interaction. The use of 55 °C for 5 min could increase the barrier functions of the cell membrane and cell wall, including during ripening. The use of quarantine treatment plus short-term heat treatment has not been previously reported.

Color

Color parameters (L* and Hue angle) are presented in Table 1. Fruit showed an initial bright red and green coloration with average values of 41.18 and 18.23 for L* and °Hue, respectively. Storage time had a significant effect on loss of luminosity (-9.67 % on average), regardless of the treatment, which was maintained when the fruits were transferred to ripening at 21 °C in HWT₁ + HWT₂ and the control. HWT₂ showed the lowest reduction in L* values after 30 days of cold storage, and after 8 days of ripening with respect to the other treatments. The treatments HWT₁ and HWT₁ + HWT₂ showed the highest loss in L* values during cold storage (-13.91 %) and ripening (-16.51 %), respectively.

On the other hand, a significant reduction (P < 0.05) in °Hue values was observed during cold storage in HWT₁ fruit, while the values in the other treatments remained nearly constant. After an additional 8 days at 21 °C, only the control presented a significant reduction in °Hue (-13.42 %). The HWT₂ and HWT₁ + HWT₂ preserved mango quality and maintained good appearance and color (luminosity and °Hue). This behavior can be associated with a reduction in CI symptoms and WL, stabilization of the cell membrane and a delay in ripening that in combination reduced the changes in peel color (^{López-López et al., 2018}).

Similar results were previously observed in “Dahshan” cucumber, because the use of HWT for 5 min maintained a good color and appearance which was attributed to a delay in chlorophyll degradation by reduction of chlorophyll oxidase and peroxidase activities, induction of heat shock protein, stabilization of cellular membrane, and reduction of WL (^{Nasef, 2018}). Likewise, the peel color index did not change significantly in mango immersed in heat treatments for a long time (75 min, 20 min) (^{Dea et al., 2010}; ^{Alvindia & Acda, 2015}) or sequential heat treatment (3 min, plus 40 min) (^{Le et al., 2010}), but they do when exposed to irradiation (^{Cruz, Soares, Fabbri, Cordenunsi, & Sabato, 2012}).

Firmness

In relation to firmness, all treatments presented a significant reduction during storage at 5 and 21 °C (Table 1). Initial firmness values ranged from 123 to 137 N, and after 30 days of cold storage varied from 112.95 to 97.67 N. Interestingly, control fruit showed the lowest decrease in firmness (-16.75 %). The application of HWT₁ in mango promoted the highest loss of firmness (-24.08 %), followed by HWT₂ (-23.80 %) and the sequential treatment (-20.93 %). However, when the fruits were transferred to ripening, those of HWT₂ showed the lowest loss of firmness, followed by HWT₁ + HWT₂, while the control and HWT₁ fruits showed higher loss of firmness without significant differences (P > 0.05) between them.

The use of HWT₁ + HWT₂ caused a significant reduction in firmness compared with the treatments separately at the beginning of the study, which could be due to an increase in respiration rate and ethylene synthesis that cause degradation of starch into sugars, or to an activation of degradative enzymes that affect the cell wall (^{Hossain, Rana, Kimura, & Roslan, 2014}). Although the HWT₁ + HWT₂ treatment had the lowest firmness values at the end of the storage period at 5 °C, it also presented the least change with respect to the initial day. Therefore, when sequential heat treatment is combined with storage at cold temperatures, cell wall degradation is reduced. According to ^{Mirdehghan et al. (2007}), a double stress could cause less depolymerization and solubilization of pectic substances (polyuronide) leading to reduce soluble pectin and ripening, as well as a decrease in the compression strength and enzymatic activity maintaining cell integrity and lower loss of firmness and cell decay (^{Le et al., 2010}; ^{Mahto & Das, 2013}).

During ripening, the immersion of fruit in HWT₂ reduced softening at day 30 at 5 °C plus 8 days at 21 °C, which could be associated with the short immersion time that had no effect on the activity of the enzymes polygalacturonase and (-galactosidase (^{Chávez-Sánchez, Carrillo-López, Vega-García, & Yahia, 2013}). Similar results with sequential treatments were reported by ^{Jacobi et al. (2000}) in “Tuu Shein” mango treated with hot air for 8 h plus HW for 15 min, and ^{Le et al. (2010}) in mango treated with HW plus vapor heat for 40 min, where the authors observed reduced softening due to less cell wall degradation and changes in soluble pectin content.

Oxidative metabolism (enzymatic activity)

SOD activity increased for all treatments during storage at 5 °C. At day 30, the sequential treatment showed the highest activity followed by HWT₁, while HWT₂ and the control showed lower SOD activity without significant differences (P > 0.05) between them (Figure 4a). At day 30+8, all treatments presented a significant reduction in SOD activity; however, HWT₁ + HWT₂ maintained the highest activity with significant differences with respect to the other treatments. SOD enzyme contributes in the initial step of eliminating ROS and catalyzes the transformation of superoxide ion (O₂ ^-) to H₂O₂ (^{Alscher, Erturk, & Heat, 2002}; ^{Soleimani-Aghdam, Jannatizadeh, Sheikh-Assadi, & Malekzadeh, 2016}). In this study, the application of HW for a long time (HWT₁ and HWT₁ + HWT₂) enhanced SOD activity, however, the sequential treatment presented higher activity at both storage temperatures (5 and 21 °C).

Figure 4 Antioxidant enzymatic activity in mango “Tommy Atkins” during storage at 5 °C (continuous lines) plus 4 and 8 days at 21 °C (dotted lines): a) superoxidase dismutase (SOD), b) catalase (CAT), and c) ascorbate peroxidase (APX). Data are the mean of five replicates with Fisher’s least significant difference (LSD) as vertical bars.  

The HWT₂ did not show any effect on SOD activity due to low membrane damage and reduced ROS content. These results suggest that the effect of HWT₁ + HWT₂ on the reduction of CI can be associated with an increase in SOD activity which prevented the accumulation of O₂ ^- and therefore oxidative damage, decreasing EL and MDA content during cold storage. No significant differences were observed in SOD activity between HWT₂ and control fruit. Contrary to this result, ^{Fogelman, Kaplan, Tanami, and Ginzberg (2011}) and ^{Wang et al. (2016}) reported that the increase in SOD activity in “Hami” melon was due to the effect of immersion in HW at 59 °C for 30 s plus 55 °C for 3 min; however, SOD activity did not have an effect on CI reduction, since it increased the content of O₂ ^- and H₂O₂ which led to lipid peroxidation and membrane damages.

On the other hand, the results obtained in this study were similar to those reported by ^{López-López et al. (2018}) in “Keitt” mango immersed in quarantine treatment and stored at 5 °C, since an increase in SOD activity was related to CI tolerance and reduced membrane damage. Moreover, the use of sequential HWT (42 °C for 30 min plus 49 °C for 20 min) in “Frangi” papaya did not significantly increase SOD activity during storage at 6 °C; therefore, it did not correlate with CI tolerance (^{Shadmani et al., 2015}). This is contrary to our results with sequential treatment, and can be associated with the differences in exposure time at both temperatures.

In a similar mode, HWT₁ + HWT₂ and HWT₁ presented higher CAT activities during cold storage, showing increases of 38.80 and 27.67 %, respectively, at day 30 (Figure 4b). HWT₂ and the control showed lower activity (19.80 and 11.68 %, respectively). When the fruits were transferred at 21 °C, those treated with HWT₁ had the maximum reduction in CAT activity at day 30+4, while the fruit treated with HWT₁ + HWT₂ maintained the highest activity with significant differences with respect to the other treatments. At the end of ripening storage, CAT activity was reduced in all treatments and no significant differences were observed among them. CAT reduces H₂O₂ to water and oxygen, protecting the cell membrane of oxidative damage (^{Nasef, 2018}).

CAT activity showed similar behavior to SOD activity. HWT₁ and HWT₁ + HWT₂ treatments presented a significant increase in CAT activity at the end of storage at 5 °C; the quarantine treatment can induce oxidative stress, but it also induces oxidative stress defense (^{López-López et al., 2018}). HWT₂ induced minimum CAT activity, similar to the control, but with the difference that HWT₂ reduces membrane damage and ROS production. During ripening, the increase in CI symptoms was associated with reduced CAT activity and accumulation of H₂O₂, a molecule that easily passes through the cell membrane and reacts with intracellular metal ions, producing hydroxyl radicals that cause damage in protein and DNA structure and also loss of membrane integrity (^{Sala & Lafuente, 2000}).

HWT₁ + HWT₂ maintained the highest activity during the first four days at ripening as observed for SOD activity. Both enzymes help to reduce H₂O₂ and O₂ ^- production limiting hydroxyl radical intracellular and CI symptoms. In agreement with this, different authors indicate that heat treatment increases CAT activity and reduces the accumulation of H₂O₂ protecting the cell from damage and CI symptoms, with even CAT presenting higher antioxidant effect than APX, an enzyme that competes for H₂O₂ during cold storage (^{Fogelman et al., 2011}; ^{Nasef, 2018}). On the other hand, ^{Shadmani et al. (2015}) report that sequential HW in papaya promoted less CAT activity than the control at 6 °C, especially after two weeks. They observed that H₂O₂ accumulation in control fruit was correlated with higher CAT activity, and hence, it was not observed that higher CAT activity correlated with CI tolerance in HWT fruit (Shadmani et al., 2015).

Regarding APX activity, this increased during cold storage in fruit with different HWTs, while control fruit did not show significant changes (Figure 4c). After 30 days at 5 °C, sequential treatment presented higher APX activity with significant differences with respect to HWT₂ and the control. After 4 days at 21 °C, APX activity was reduced for all HWTs, but HWT₁ + HWT₂ maintained the highest values with respect to the other treatments. After 8 days at 21 °C, no significant differences in APX activity were observed between the control and all HWTs. In this work, the use of different HWTs increased APX activity, especially at the end of storage at 5 °C. During ripening, all treatments reduced APX activity in a similar way to the other enzymes (SOD and CAT), showing the highest activity with the sequential treatment.

^{Chongchatuporn et al. (2013}) indicate that a reduction in CI susceptibility is related to a reduction in ROS and an increase in CAT and APX activities during cold storage. Similar results were previously observed in strawberry (^{Vicente, Martínez, Chaves, & Civello, 2006}), broccoli (^{Zhang et al.,2009}), banana (^{Ummarat et al., 2011}), and mango (^{López-López et al., 2018}), where a higher transcription and activity of APX were observed with respect to the control, reducing ROS accumulation and cell damage and increasing CI tolerance. A coordinated increase in the activities of antioxidant enzymes such as SOD, CAT, and APX promoted by sequential treatment is very important for scavenging ROS to protect the cell membrane, to induce CI tolerance and to maintain quality during cold storage.

Thus, the use of heat treatment for balance between antioxidant enzymes is critical for cell survival during cold stress (^{Zhang et al., 2013}; ^{López-López et al., 2018}). It is important to highlight that the observed effect for sequential treatment (quarantine plus short-term) has not been previously reported for SOD, CAT and APX activities and CI tolerance in mango.