EdibleCoatingBased onRoselle (Hibiscus sabdariffaL.)Mucilage Applied to Soursop Fruits in Postharvest Storage

Programa de Maestŕıa en Ciencias Biológico Agropecuarias, Unidad Académica de Agricultura, Carretera Tepic-Compostela Km 9, Xalisco 63780, Nayarit, Mexico Unidad de Tecnoloǵıa de Alimentos Secretaŕıa de Investigación y Posgrado, Universidad Autónoma de Nayarit, Ciudad de la Cultura s/n Col Centro, Tepic, Nayarit, Mexico Posgrado en Ciencias Agropecuarias y Desarrollo Rural, Universidad Autónoma del Estado de Morelos, Av. Universidad Núm. 1001, Col. Chamilpa, Cuernavaca 62209, Morelos, Mexico


Introduction
Soursop plants are natives of Central America and are grown in some countries in the Southeast of China to Australia as well as in low and warm areas of East and West Africa [1]. Mexico is the main worldwide producer of soursop. In 2018, a production of 29,228.46 T was recorded at national level. In this regard, the state of Nayarit was the largest producer of soursop fruits with 21,810 T [2]. Soursop production contributes to the economic growth of Nayarit; however, a problem in the crop management exits due to the high respiration rate and ethylene production leading to fruit softening, which causes a short postharvest shelf life [3][4][5]. In this context, the storage and commercialization of the fruit are limited; therefore, it is necessary to implement safety storage methods for consumers [6]. Since the initial quality of the fruit cannot be improved, applying technologies during the postharvest period, it is possible to maintain its organoleptic characteristics using storage methods such as the use of packaging, refrigeration systems, and controlled or modified atmospheres [7]. e use of edible coatings stands out among the alternatives for the postharvest storage. Edible coatings from polysaccharides act as a modified atmosphere, creating a semipermeable layer in the fruit that allows gas exchange, reducing metabolic processes, which leads to the increase in the postharvest life of the fruit [8]. Among the polysaccharides used as a coating are chitosan [9], starch [10], alginate [11], and mucilage [12]. Mucilages are classified within hydrocolloids and are complex polymeric macromolecules of hydrocarbon nature that can modify the rheology of a solution due to their highly branched structure [13]. In this regard, they can be considered as a source of raw material for the preparation of edible coatings [14].
e Cactaceae family is one of the main sources of high mucilage content. Bello-Lara et al. [15] applied mucilage (1.5%) extracted from nopal (Opuntia spp.) on Has avocado fruits. e fruits showed a mass loss of 5.9% at 15 days of storage at 6°C and 6.01% at 20 days of storage at the same temperature.
Among the main plant sources that can be extracted from polysaccharides, roselle (Hibiscus sabdariffa L.) calyx is an excellent source of mucilage. Castañeda and Cáceres [16] reported that Hibiscus sabdariffa L. also has high pectin content and, therefore, can be used to make edible coatings applied to fruits and vegetables. However, its effect as a coating on fruit and vegetable products has not been studied.
In the previous context, the roselle mucilage can be used as the preparation material of an edible coating to prolong the shelf life of fruits. Taking this into account, in this study we evaluated the effect of the coating based on roselle mucilage (2%) on the physicochemical changes and biochemical and antioxidant activity during postharvest storage.

Plant Material.
Soursop fruits were harvested at physiological maturity (160 days after the anthesis) according to the recommendations of Balois-Morales et al. [3]. Moreover, we selected four fruits between 700 and 800 g of bright green color, with the absence of mechanical and phytosanitary damage. e fruits were washed with water, subsequently immersed in 1% (v/v) sodium hypochlorite, and allowed to dry until the water evaporated. en, we collected 6 g of pulp from each of the soursop fruits. Next, 1 g of pulp was mixed with 10 mL of distilled water using ULTRA-TURRAX T-25 IKA ® . is mixture was used for the quantification of pH, total soluble solids concentration (TSS), phenols, and antioxidant activity. On the other hand, for the quantification of flavonoids and vitamin C, we used methanol (reactive grade) and trichloroacetic acid (10%) instead of distilled water, respectively. Each independent mixture (24 in total) was centrifuged at 9000 rpm for 25 min at 4°C (Hermle Z 326 K). e supernatant was recovered and used for further analysis.

Development and Application of the Coating.
A 2% solution of mucilage from roselle calyces and water (w/v) was prepared. en, the solution was heated at 50 ± 2°C on a heating plate for 30 min under constant stirring. e temperature helps the solution take a viscous consistency, which will allow better adhesion of the mucilage to the fruits, resulting in the coating. e coating was applied to the soursop fruits by immersion for one min. Once the fruits were coated and left outdoors for the roselle mucilage (2%) to solidify, they were stored in controlled air conditioning chambers (ClimaCell ® , CLC-B2V-M 404).

Experimental Design.
e fruits were grouped into four batches (30 fruits per each). e treatments (T) were as follows: uncoated fruits (T1 and T3), coated fruits (T2 and T4). e fruits of T1 and T2 were stored for 6 days at 22°C and 90% RH. e fruits of T3 and T4 were stored for 8 days (4 days at 15°C, then 4 days at 22°C and 90% RH).

Physicochemical Analysis.
e weight loss was determined by gravimetry using a digital scale (Scout Pro, OHAUS ® ). Color was measured on the soursop peel, brightness or reflected light (L) (0: pure black, 100: pure white), hue angle (°h) (0°: purple-red, 180°: green), and chromaticity (C, intensity from gray to pure color) with a colorimeter (Konica Minolta ® ). Loss of firmness was measured in the equatorial zones of the fruit (with peel) using a penetrometer (Force Gauge model GY-4) with an 8 mm diameter strut. e pH of the pulp was measured with a potentiometer (Hanna Instruments HI22). e total soluble solids concentration (TSS) was determined by placing an aliquot on a digital refractometer (Hanna HI 96801). Titratable acidity was determined according to the official method (AOAC) [17] by volumetric titration with 0.01 N NaOH and phenolphthalein as an indicator.

Total Phenolic Compounds.
We determined total phenolic compounds according to the methodology described by Stintzing et al. [19]. We added 250 μL of Folin-Ciocalteu solution (v/v 1 : 10 in deionized water) to 50 μL of sample, and then 200 μL of sodium carbonate solution (7.5%) was added. Absorbance was measured in a microplate reader (Power Wave XS, Biotek) at a wavelength of 765 nm. e results obtained were expressed in mg equivalent of gallic acid (mg EGA/100 g FW).

DPPH.
e antioxidant activity was determined by the methodology of Morales and Jiménez-Pérez [20]. A DPPH · solution (7.4 mg/100 mL of 80% ethanol) was prepared and then stirred for 60 min. Subsequently, it was diluted with methanol (80%) until reaching an absorbance of 0.70 (±0.02) at 520 nm. An aliquot of 50 μL was added to 250 μL of the DPPH solution and then incubated in dark for 30 min. e absorbance was measured at a wavelength of 520 nm (Power Wave XS, Biotek). e AOX was expressed in mg equivalent of ascorbic acid (mg EAA/100 g FW).

ABTS.
e determination of the inhibitory capacity of the 2,2′-azino-bis-(3-ethylbenzothiazoline-6-sulfonic acid) radical cation (ABTS ·+ ) was quantified according to the methodology of Re et al. [21]. An ABTS (7 mM) and potassium persulfate (2.45 mM) solutions were prepared with distilled water. e solutions were mixed in a 1 : 1 (v/v) ratio, then incubated for 16 h in the dark at 23 ± 1°C, and kept under constant stirring to form the ABTS ·+ radical. e solution was diluted with ethanol (20%) until reaching an absorbance value of 0.70 (±0.02) at 754 nm (maximum absorption wavelength). 10 μL of the sample was taken and reacted with 490 µL of ABTS ·+ for seven min. e absorbance was read at 734 nm. e results were expressed in mg equivalent of ascorbic acid (mg EAA/100 g FW).

FRAP.
is analysis was carried out by the methodology of Benzie and Strain [22] to evaluate the ability of soursop pulp compounds to reduce iron (III) to iron (II). 25 μL of the aqueous solution, 63 μL of phosphate buffer (PBS) (0.2 M, pH 6.6), and 63 μL of potassium hexacyanoferrate (K 3 Fe(CN) 6 ) at 1% were added and then stirred with a vortex. ereafter, the reaction mixture was incubated in the dark for 30 min at 50°C, and 63 μL of trichloroacetic acid (10%) was added and then vortex. Next, a 126 μL aliquot of the supernatant was taken and mixed with 126 μL of distilled water and 25 μL of 0.1% ferric chloride (FeCl 3 ). Finally, the absorbance was measured at 700 nm. e results were expressed in mg equivalent of ascorbic acid (mg EAA/100 g FW).
2.2.7. Flavonoids. It was performed using the protocol established by Zhishen et al. [23]. 50 μL of the sample, 100 μL of deionized water, and 10 μL of NaOH (15%) were mixed, then stirred in a vortex, and kept in dark at 23°C for 6 min. After that time, 15 μL of AlCl 3 (10%) was added, and then briefly vortex. e solution was kept in dark for 6 min at 23°C. Finally, 200 μL of NaOH (4%) was added. e absorbance was measured at 510 nm. e results obtained were expressed in equivalent mg of quercetin (mg EQ/100 g FW).

Vitamin C.
It was evaluated using the method reported by Dürüst et al. [24]. e following solutions were prepared: DCPI (2,6-dichlorophenolindophenol disodium salt) at 24 mg/L in deionized water; acetate buffer composed of 3 g of anhydrous sodium acetate, 7 mL of deionized water, and 10 mL of glacial acetic acid. 50 μL of the samples were mixed with 50 μL of acetate buffer and 400 μL of DCPI. e absorbance was determined at 520 nm in a microplate reader (Power Wave XS, Biotek). e results were expressed in mg equivalent of ascorbic acid (mg EAA/100 g FW).

Statistical Analysis.
e treatments were analyzed under a completely randomized design with a 2 × 2 factorial arrangement.
e factors were the temperature (15°C and 22°C) and the coating (coated and uncoated fruits). e results were analyzed using an ANOVA and the Tukey test with a level of significance P ≤ 0.05 using Statistical Analysis

Weight Loss.
Soursop fruits stored at 15°C showed a daily mass loss of 2.4% (T3) and 2.85% (T4). On the other hand, at four days of storage, an average of 4% was found, while at the end of the storage (8 days) the accumulated mass loss was 9.89 (T3) and 11.43% (T4) (Figure 1(a)). e fruits stored at 22°C showed a daily mass loss of 3.9% (T1) and 4.2% (T2). Further, at the end of the consumption maturity, the accumulated mass loss was 11.8% (T1) and 12.8% (T2). No significant statistical difference between treatments (P ≤ 0.05) was found (Figure 1(a)). Valero and Serrano [26] reported that the weight loss of fruits during postharvest handling is mainly due to their perspiration and respiration. e application of coatings helps to reduce weight loss [27]. Castillo-Ánimas et al. [28] applied candelilla wax on soursop fruits stored at 20°C-22°C and reported losses of an accumulated mass of 3.9%. Moreover, the same authors reported losses of 5% on fruits stored at 12°C-14°C without coating. Tovar-Gómez et al. [29] reported losses around 2.56 and 2.46% in soursop fruits coated with wax emulsions and 1-MCP in soursop fruits stored under similar conditions to those used in this investigation. Jiménez-Zurita et al. [30], in uncoated soursop fruits stored for seven days (four days at 15°C and then three days at 22°C), reported cumulative weight losses of 2.3% and 2.7%, respectively. ese same authors reported a daily mass loss between 1.34 and 1.41% in uncoated soursop fruits stored for six days at 22°C, presenting accumulated mass losses of 6.7 and 7.1%. e results obtained in the present investigation showed lower mass loss in T4 compared with the fruits of T1 and T2. is can be attributed to the effect of the refrigeration temperature and the coating applied [29][30][31].

Firmness.
We observed a gradual decrease in the firmness of the fruits stored at 22°C during storage. According to the statistical analysis, significant differences (P ≤ 0.05) were observed in the treatments, where T1 and T3 showed greater firmness during storage (51.7 and 35.1 N, respectively) ( Figure 1(b)). e loss of firmness in climacteric fruits such as soursop is ascribed to the degradation of the cell wall and the loss of interconnection of pectins and hemicelluloses due to the effects of solubilization and enzymatic depolymerization [32,33]. However, the storage of soursop fruits using refrigeration decreases physiological activities such as softening [34]. e results obtained in this investigation are superior (<22 N) as reported by Montalvo-González et al. [35], who obtained final firmness values of 9.41 N in soursop fruits coated with candelilla wax and beeswax stored at 25°C. Nevertheless, values similar to those obtained by Coêlho de Lima et al. were observed [36]; their firmness values were 19 N in soursop "Morada" fruits without coating stored at 23°C. e results obtained in this investigation were also greater (<22.7 N) than those reported by Márquez et al. [33] indicating firmness values of 4.74 N (five days after harvest) and 7.5 N (seven days after harvest) as the optimum ripeness for the soursop fruit consumption. On the other hand, Ramos-Guerrero et al. [37]

pH.
e pH of the soursop pulp in fruits stored at 22°C decreased during ripening, whose initial values were 5.7 (T1) and 5.4 (T2) up to values of 4.3 and 4.2, respectively. Similar results were obtained in fruits stored at 15°C and 22°C (T3 and T4), with initial values of 5.7 (T3) and 5.8 (T4). Subsequently, these values decreased to 4.7 and 4.5 in consumption maturity, respectively. According to the statistical analysis, significant statistical differences were observed (P ≤ 0.05) (Figure 1(c)). e results obtained in this investigation are in the range established by the Colombian technical standard for commercialization (NTCC) at physiological or commercial maturity, "soursop fruits must have the minimum pH value of 3.38" [38], and agree with those reported by Ramírez et al. [39]. Jiménez-Zurita et al. [40] performed a characterization of soursop fruits in Tepic, Nayarit, at 26°C, obtaining a pH of 3.6 in consumption maturity. Villalba et al. [41] carried out an investigation with soursop fruits from Colombia at consumption maturity, reporting pH values of 3.04. ese results indicate that the fruits of that region of Colombia are more acidic than those analyzed in this investigation.
is characteristic can be explained to different geographical regions, temperature, light intensity, and soil-climatic conditions [42]. González [35] reported similar results of pH � 4.47 in soursop fruits coated with candelilla wax and beeswax stored at 16°C. Furthermore, Jiménez-Zurita et al. [30] coated soursop fruits using wax and 1-MCP emulsions stored at 13 ± 2°C, reaching pH values of 4 ± 0.2. Similar results were obtained in this investigation.

Total Soluble Solids (TSS).
e concentration of TSS in soursop fruits stored for four days at 22°C was 15.7°Bx (T1) and 15.6°Bx (T2), while at the end of storage (six days), values of 13.79 and 14.45°Bx were recorded, respectively. On the other hand, TSS concentration of fruits (T3 and T4) stored at 15°C for four days was 11.8°Bx and when exposed to 22°C was 10.75 and 11.95°Bx, respectively, showing significant differences in the treatments (P ≤ 0.05). Yashoda et al. [43] suggest that changes in the TSS concentration for climacteric fruits are attributed to the reduction of total sugars, starch, and cellulose during ripening, which are converted to oligosaccharides and monosaccharides that confer the texture and flavor characteristics of the fruit. e NTCC states that "soursop fruits must be above 13°Bx," which is the ripeness indicator used for soursop fruits [37].
González et al. [35] reported 18.65°Bx at 10 days after harvest using combinations of 1-MCP and wax emulsions in the conservation of soursop stored at 25°C. Lima et al. [36] reported the final TSS results of 14.4°Bx in soursop fruits stored at 23.4 ± 1.1°C. Tovar-Gómez et al. [29] recorded similar results to those obtained in this investigation at 12 days of storage in soursop fruits treated with 1-MCP stored at 13 ± 2°C. Espinosa et al. [44] indicate that the increase in TSS can be attributed to the hydrolysis of starch, sucrose, pectins, and other soluble compounds such as organic acids or amino acids. e variation in the TSS can be attributed to the type of fruit; the soursop is classified as a multiple fruit derived from several separate individual flowers, whose fertilized ovaries merge to form a single structure, in which each individual fruit corresponds to a berry [45,46]. e pollination of the fruit is not carried out homogeneously, which means that the ripening of the fruit is not uniform.

Titratable
Acidity. Soursop fruits of T1 and T2 had initial values of 0.12 and 0.09% after four days of storage (consumption maturity), respectively. Acidity (%) increased to 0.8 (T1) and 1.0 (T2) (Figure 2(a)). Regarding the fruits of T3 and T4 (stored for four days at 15°C and then four days at 22°C), T3 presented a decreasing behavior from 0.5 to 0.42%, while those of T4 showed an increase from 0.45 to 0.53%, with a significant statistical difference between treatments (P ≤ 0.05) (Figure 2(a)). Tovar-Gómez et al. [29] observed that titratable acidity in soursop fruits increases during the ripening process. However, titratable acidity decreases at the end of storage, indicating that organic acids are used as substrates in the respiration process [47][48][49].
Paull [46] observed that, at room temperature, the decrease in titratable acidity of soursop coincided with the appearance of a slightly unpleasant odor. Jiménez-Zurita et al. [30] have reported values of 0.88 and 0.96% in soursop fruits stored at 22°C after eight days of storage, while Do Sacramento et al. [50], in selections of soursop fruits ("Lisa," "Morada," and "Comum"), obtained values between 0.92 and 1.0% titratable acidity when the fruits ripened. e values obtained in fruits stored at 15°C were lower than the values (0.92-1.00) found in soursop fruits from Brazil [50] but similar to those reported by Márquez et al. [33] for soursop from Colombia. Lima et al. [36] found values of 0.71% titratable acidity after 15 days of storage in soursop fruits coated with 1-MCP and stored at 15°C. Mosca et al. [51] indicate that, during ripening, the titratable acidity of the soursop fruit increases from 0.067 to 0.67% of malic acid while it remains at 0.67% after 10 days at 16°C.

Color (L * C * h ).
e fruits stored at 22°C (T1 and T2) initially presented average brightness values (L) of 44.2 and 44, respectively. On the other hand, a decrease in luminosity was observed once the fruits reached the maturity of consumption, 40.5 (T1) and 41.2 (T2) (Figure 2(b)). Regarding the chromaticity (C) of the fruits of these treatments, the initial value was 16.3 and the final value was 9.2 ( Figure 2(c)). Likewise, the hue angle (°h) presented by these fruits in physiological maturity (T1 and T2) was 109.5 on average and then decreased to 80.49 (Figure 2(d)). e fruits stored for 8 days (4 days at 15°C and then 4 days at 22°C) recorded average initial values of L � 105 (T3) and 113.7 (T4) (Figure 2(b)). e chromaticity (T3 and T4) decreased during storage, registering initial values of 17 (T3) and 13.2 (T4); subsequently, these values reached 11.3 and 5.9 in consumption maturity, respectively (Figure 2(c)). e hue angle of the fruits of T3 and T4 (4 days at 22°C) was 105.2 on average, decreasing to 81.4 (T3) and 78.51 (T4) in the consumption maturity (Figure 2(d)). e fruits stored at 15°C and 22°C presented similar values in color, indicating that the fruits presented an opaque green color with low luminosity.
Significant differences were observed in the treatments evaluated (P ≤ 0.05). e fruits of T3 presented greater luminosity (L � 44.4) and chromaticity (C � 15.8); however, the hue angle was higher in the coated fruits (hue � 102.7). e color changes in the peel of soursop fruits are due to enzymatic oxidation (polyphenol oxidase and peroxidase) and the action of polyphenol oxidases on phenolic compounds that are present in the fruit [52,53]. Balois-Morales et al. [3] observed an increase in the activity of the POD enzyme and reported 83.26 U·mg −1 of protein in soursop fruits after 6 days of storage at 22°C. Lima et al. [36] reported values of L � 50, hue � 118, and C � 24 in uncoated soursop fruits stored at 23°C. Tovar-Gómez et al. [29] reported brightness values of 43 and 45 in soursop fruits coated with wax and 1-MCP emulsions stored at 13 ± 2°C, observing from day 10 a dark peel that caused a decrease in the values of luminosity (43.5).
Lima et al. [47] used 1-MCP as a coating on soursop fruits stored at 15°C and reported final values of 40 for luminosity, 21 for chromaticity, and 130 for hue angle after 15 days of storage. e bright green color of the soursop fruits evaluated in this investigation decreased during ripening to an opaque green with a low luminosity index due to the darkening of the epidermis. is indicates the onset of senescence as a result of the degradation of chlorophyll and the synthesis of pigments, such as carotenoids and anthocyanins [54]. However, the application of edible coatings based on polysaccharides decreases metabolic activities such   as enzymatic browning, which helps to maintain the color of the fruits [55].

Total Phenolic Content (TPC).
e coated and uncoated fruits stored at 22°C (T1 and T2) had initial phenolic values of 66.9 and 35.3 mg EAG/100 gFW, respectively. When the fruits reached the maturity of consumption, the concentration of phenols increased to 107.5 and 67.4 mg EAG/ 100 gFW, respectively (Figure 3(a)). Regarding the fruits stored at 15°C for four days and at 22°C (T3 and T4), a decrease in total phenols was observed during storage. T3 fruits had a phenolic content of 139.6 mg EAG/100 gFW, while the fruits of T4 showed values of 42.94 mg EAG/ 100 gFW. Moreover, when the fruits reached the maturity of consumption, the total phenolic content was 99.75 mg EAG/ 100 gFW (T3) and 74 (T4). Statistically significant differences (P ≤ 0.05) were observed in the treatments evaluated. e increase in the concentration of phenolic compounds can be attributed to the physiological and biochemical process of fruit ripening; therefore, in the maturity of consumption, an increase in phenols is recorded. A decrease in these compounds could be related to oxidative stress due to the low temperature. Soursop fruits show chilling injury in temperatures below 15°C of storage for more than 4 or 6 days. Furthermore, it may be due to the senescence of the fruit which produces the oxidation of phenolic compounds. Phenolic compounds are associated with AOX because of their ability to eliminate free radicals due to the redox properties of their hydroxyl groups attached to the chemical structure of phenolic compounds [56,57]. e decrease in the concentration of the phenols could be influenced by the oxidation of these compounds and by the activity of the enzyme polyphenol oxidase and peroxidase [53,58]. An investigation conducted by Jiménez-Zurita et al. [30], in soursop fruits stored at 22°C, reported 74.20 mg EAG/ 100 gFW, whose values are similar to those found in the present investigation. Silva and Sirasa [59] reported 86.5 mg EAG/100 gFW in fruits of Annona muricata L. and 199.1 mg EAG/100 gFW in the pulp of Annona reticulata fruits from Sri Lanka. Furthermore, Almeida et al. [60] reported a total phenolic content of 54.8 mg EAG/100 gFW in soursop fruits from Brazil. Hassimotto et al. [61] reported values similar to those of our investigation (120.0 mg of GAE/100 gFW.). In addition, Balois-Morales et al. [3] observed that POD activity in soursop fruits increases after storage at 15°C and indicated that the increase of POD could be related to oxidative stress caused by low temperatures.

DPPH.
Uncoated fruits stored at 22°C (T1) showed a decrease in AOX with initial values from 272.5 to 256.2 (mg EAA/100 gFW), while coated fruits (T2) stored under the same conditions showed increased AOX, registering initial values from 181.6 to 234.8 (mg EAA/100 gFW). Uncoated fruits stored at 15°C for four days and 22°C (T3) showed a decrease in antioxidant activity presenting initial values of 290.9 to 255.7 (mg EAA/100 gFW) at the end of storage, while the fruits of T4 stored under the same conditions showed an increase in AOX with initial values of 212.2 mg EAA/100 gFW which then increased to 276.9 mg EAA/ 100 gFW. Significant differences (P ≤ 0.05) were observed in the treatments (Figure 3(b)). e initial differences between treatments in the antioxidant activity could be related to the type of fruit. Soursop is a multiple climacteric fruit, which means that, in a single structure, a large number of fruits are fused and are developed as they are pollinated, which usually is not at the same time. erefore, the soursop fruits might not have a homogeneous maturity. e radical elimination capacity of the soursop fruit pulp could be due to the synergistic effect of several phytochemicals present in total phenolic extracts, as well as the influence of the modified atmosphere in the fruit on the production of phenolic compounds [62,63]. e strong inhibitory effect on the DPPH radical of soursop could be linked to polyphenolic compounds that are able to donate electrons to neutralize free radicals [64]. Fruits stored at 22°C had a higher AOX, which could be related to the high phenolic content found in this investigation. Lower AOX (16.94 mg/100 gFW) has been reported in soursop fruits from Brazil [60]. Chavan et al. [65] suggest that the differences in antioxidant activities can be explained by the variation in the polarities of the solvents used, as well as the weather and soil conditions. e results obtained in this investigation are greater than those reported by Oboh et al. [66], whose values were 102.86 ± 0.215 (μg/ mL) of DPPH radical inhibition in soursop fruits from Nigeria. A study performed in Sri Lanka reported antioxidant activity values of 2.47 ± 0.09 gFW for Annona muricata L. and 3.13 ± 0.07 gFW for A. reticulata fruits [58]. As can be seen, we obtained higher results than the previously mentioned ones. e soursop fruits produced in Nayarit (Mexico) have higher antioxidant activity, possibly due to the edaphoclimatic characteristics (soil and temperature, mainly) and the genetic characteristics that Nayarit has. ese factors contribute to the production of bioactive compounds with antioxidant activity. Furthermore, Berumen-Varela et al. [5] reported a high genetic variability among soursop fruits from different countries, supporting our previous statement.

ABTS.
e AOX of the fruits of T1 and T2 stored at 22°C increased during storage, presenting initial values of 72.5 and 36.6 mg EAA/100 gFW, respectively. en, this activity increased with values of 120.1 (T1) and 72.6 (T2) mg EAA/ 100 gFW six days after storage. Uncoated fruits stored at 15°C (T3) recorded a decrease in AOX, reporting initial values from 113.1 to 111.8 (mg EAA/100 gFW) at the end of storage. Nonetheless, on day eight of storage, T4 fruits stored under the same conditions recorded an increase in AOX with initial values from 37.1 to 98.2 (EAA mg/100 gFW), respectively. Significant differences (P ≤ 0.05) were observed in the treatments (Figure 3(c)). Correa-Gordillo et al. [67] mention that the antioxidant compounds of Annona muricata L. are mainly lipophilic, and the mechanism of action is through the donation of hydrogen. e results obtained are similar to those reported by Beserra et al. [60], who observed an AOX of 91.29 and 93.16 mg EAA/100 gFW in fruits of Annona muricata L. and Annona squamosa L. Kuskoski et al. [68] investigated the AOX in soursop fruit pulp and reported 76.8 mg AA/100 gDW. Singh et al. [69] reported that the difference in AOX is influenced by genotype, fruit maturity status, and edaphic factors.

FRAP.
e uncoated and coated fruits stored at 22°C (T1 and T2) had initial values of 10.5 and 9.9 (mg EAA/ 100 gFW), respectively. Subsequently, this activity increased with values of 17.1 (T1) and 10.5 (T2) mg EAA/100 gFW. e behavior of the fruits stored at 15°C (T3 and T4) recorded an increase from 12.35 to 16.6 (T3) and from 10.26 to 13.29 (T4) mg EAA/100 gFW. Significant differences (P ≤ 0.05) were observed in the treatments (Figure 1(d)). Akomolafe and Ajayi [64] reported that the soursop pulp has electron donor molecules that can react with free radicals to convert them into stable products. ey also reported a reduction capacity of 1.54 mmol EAA/g, indicating a lower AOX compared to this investigation. e results obtained in this study are lower than those reported by Chukwunonso-Agu et al. [70] who found 34.2 mg EAA/100 gDW in pulp stored at 4°C. Sanchez et al. [71] observed that AOX depends on the type of solvent and time and temperature of extraction.
3.11. Flavonoids. Uncoated and coated fruits stored at 22°C (T1 and T2) showed initial flavonoid concentrations of 35   Journal of Food Quality respectively. Further, on day eight of storage, the concentration decreased to 58.7 mg EQ/100 gFW (T3), while in T4 no changes were recorded. Significant differences (P ≤ 0.05) were observed in the treatments (Figure 4(a)). Flavonoids and other polar compounds (saponins, tannins) are phenolic compounds that provide antioxidant properties through an antiradical activity conferred by OH phenolic groups and the double bonds present in their fundamental chemical structure [72][73][74]. An investigation reported by Silva and Sirasa [59] obtained values of 34.4 and 66.5 (mg EQ/100 gFW) in fruits of Annona muricata L. and Annona reticulata L. from Sri Lanka. e variability in flavonoids can be attributed to the cultivar, geographical space of the crop, agricultural practices, harvest and storage, conditions and methods of processing [75].

Vitamin C.
In this investigation, the concentration of vitamin C in fruits stored at 22°C (T1) during storage showed no significant changes (14.7-14.5 mg EAA/100 gFW) from the beginning until the end of storage, respectively. Coated fruits (T2) recorded initial vitamin C values of 18.6 mg EAA/ 100 gFW decreasing on the sixth day of storage (16.36 mg EAA/100 gFW). Uncoated fruits stored at 15°C (T3) showed values of 14.97 mg EAA/100 gFW on the fourth day of storage. However, after eight days of storage, the concentration decreased to 13.92 (mg EAA/100 gFW). T4 fruits recorded 13.25 mg EAA/100 gFW of vitamin C on day four of storage. After that time, the concentration increased to 17.12 mg EAA/ 100 gFW on day eight of storage. Significant differences (P ≤ 0.05) were observed between treatments (Figure 4(b)).
Vitamin C is an enantiomer of L-ascorbic acid; it is recognized as an important antioxidant natural origin compound [76,77]. Agatha et al. [78] report vitamin C values of 22.59 (mg EAA/100 gFW), which coincide with the results found in our research. Moreover, Singh et al. [79] conducted a study on soursop fruits in the Andaman Islands and reported higher concentrations (48 mg EAA/100 gFW) than those obtained in this study. e results obtained in this investigation are superior (<17.12) to those reported by Silva and Sirasa [59] whose values are 12.6 mg EAA/100 gFW in frozen soursop pulp. e difference between vitamin C values may be associated with factors such as storage temperature, fruit ripening stage, agronomic management conditions, and weather [80].

Conclusion
e soursop fruits coated with roselle mucilage (2%) and stored at 15°C for eight days showed the lowest weight loss and titratable acidity. Likewise, the total phenolic content and vitamin C were increased. In the same storage conditions, the antioxidant activity increased during the fruit ripening at the stage of maturity of consumption. No negative effect on the color of the peel was observed due to the application of the mucilage coatings.
Data Availability e statistic analysis data used to support the findings of this study are available from the corresponding author upon request.   Journal of Food Quality 9