Open-access Relationship between volatiles and antioxidant compounds in scald on ‘Alexander Lucas’ pear in different postharvest conditions

ABSTRACT

This study aimed to evaluate the effects of storage conditions on the development of superficial and senescent scald and its relationship with volatiles and antioxidant compounds in ‘Alexander Lucas’ pears (Pyrus communis) harvested at two maturity stages in three orchards. A two-factorial design combined two maturity stages with five storage conditions: standard oxygen plus cold storage (control; 20.9 kPa O2, 0.03 kPa CO2), controlled atmosphere (low O2) ( 2.0 kPa O2, 0.7 kPa CO2), each without and with 1-MCP (300 nl·L-1), and ultra-low O2 atmosphere (0.7 kPa O2, < 0.7 kPa CO2). The fruit were grown in three regions in Germany and stored for seven months (0 °C; 94% relative humidity) plus seven days simulated shelf-life. Scald development was positively correlated to the 6-MHO and α-farnesene (after three months of storage) and negatively correlated to an ascorbate level. The application of 1-MCP led to a reduction in the production of volatile compounds and antioxidants, except by ascorbate, which appeared to be associated with delayed ripening and the less severe development of scald. Ultra-low O2 reduced the scald, but the effects depended on the production region.

Key words ultra-low oxygen; 6-methyl-5-hepten-2-one; 1-methylcyclopropone; α-farnesene; phenolics content; controlled atmosphere

INTRODUCTION

Superficial scald is a physiological disorder that occurs in the absence of preventive treatments during the storage and shelf-life of pears, thus causing economic and quality losses (Isidoro and Almeida 2006, Guerra et al. 2012). The symptoms result in brown or dark colored spots on the fruit epidermis, which often enlarge after removal of the fruit from storage (Whitaker et al. 2009). Superficial scald is associated with oxidation of α-farnesene into conjugated trienols (Gapper et al. 2006, Vanoli et al. 2010) and 6-methyl-5-heptene-2-one (6-MHO), which cause cell damage that leads to the onset of scald symptoms (Pesis et al. 2010).

Senescent scald is the browning of the peel surface that can extend into the underlying flesh and affect European pear fruit during prolonged storage (Lum et al. 2017), and the incidence of senescent scald following storage can be affected by the maturity at harvest (Zhao et al. 2020).

Mitigating actions against ethylene production such storage under low-O2 or ultra-low-O2, controlled atmospheres and application of 1-methylcyclopropene (1-MCP), which delay fruit senescence and/or decrease synthesis and oxidation of α-farnesene, can reduce the scald development (Shang Ma and Chen 2003, Gapper et al. 2006, Isidoro and Almeida 2006, Xie et al. 2014). According to Larrigaudière et al. (2016), the prevention of α-farnesene oxidation can determine the fruit sensitivity to scald. They considered that the oxidation prevention capacity of α-farnesene is determined by the antioxidant potential or the specific antioxidants in the fruit. Thus, the development of this physiological disturbance might depend on the balance between the oxidative processes that are triggered by the products generated from oxidation of α-farnesene (conjugated trienols, 6-MHO) and the presence of antioxidant compounds (phenolic compounds, ascorbate) in the tissue (Guerra et al. 2012).

Furthermore, Lindo-García et al. (2021) found that the regulatory processes triggered by cold stress that leads to the development of scald in pears are complex and cultivar dependent. While the ‘Blanquilla’ pear is related to the fruit’s ability to produce ethylene mediated by cold, the ‘Flor d’Hivern’ pear seems to be mainly associated with a better process of acclimatization to the cold. In ‘Blanquilla’ pears, disorder incidence depended on the initial fruit maturity at harvest and was expressed only after removal from cold storage. In contrast, disorder incidence in ‘Flor d’Hivern’ cultivar developed during cold storage and regardless of initial harvest date (Lindo-García et al. 2020).

According to Whitaker et al. (2009), in addition to post-harvest storage conditions, some factors such as pre-harvest temperatures, fruit maturity levels, and production regions might be important for the development of superficial scald. The maturity stage of fruit affects the incidence of scald (Zhao et al. 2020), but the relationship between maturity stages and superficial scald is still not clear (Whitaker et al. 2009, Hui et al. 2016).

This study aimed to evaluate the effects of 1-MCP and storage conditions on development of scald in ‘Alexander Lucas’ pears harvested at two maturity stages in three orchards, and to define their relationships with the synthesis of α-farnesene, 6-MHO, antioxidant phenolic compounds, and ascorbate.

MATERIALS AND METHODS

Fruit, storage conditions, and tissue sampling

‘Alexander Lucas’ pear (Pyrus communis L.) fruit at two maturity stages MS1 (September 5, 2012) and MS2 (September 18, 2012) were harvested in Baden-Württemberg state, southwest Germany. The orchards are located in the municipalities of Ravensburg (RV; 47°46’N latitude, 9°36’E longitude, average altitude 447 m), Langenargen (LA; 47°35’N latitude, 9°32’E longitude, 402 m average altitude), and Öhringen (OHR; 49°11’N latitude, 9°30’E longitude, 228 m average altitude). The harvest dates were chosen according to indications for the best fruit quality for ‘Alexander Lucas’ pears as evaluated by the Streif index (SI) (Neuwald 2018).

The fruit from both maturity stages were stored for seven months under the following conditions:

  • Control (CS) = 20.9 kPa O2/ 0.03 kPa CO2;

  • Controlled atmosphere (CA) = 2 kPa O2/ 0.7 kPa CO2;

  • Control with 1-MCP = 300 nl·L-1 (CS+MCP);

  • Controlled atmosphere with 1-MCP = 300 nl·L-1 (CA+MCP);

  • Ultra-low O2 atmosphere (ULO) = 0.7 kPa O2/ < 0.7 kPa CO2.

All these treatments were maintained at 0 ± 0.1 °C and 94% ± 2% relative humidity. Following these seven months of storage, the pears were all kept for seven days of shelf-life under ambient conditions (20 ± 2 °C/60% ± 5% relative humidity). The fruit were evaluated for occurrence of superficial and senescence scald (SI), and also for respiration rate, ethylene release, α-farnesene, 6-MHO, phenolic compounds, and ascorbate. α-farnesene and 6-MHO were also evaluated after three months of storage plus seven days of shelf-life under the same conditions.

The experimental design was completely randomized using a factorial scheme (two maturity stages and five storage conditions) as three replicates of 30 fruit to evaluate the severity of scald, four fruit to analyze respiration rate and ethylene release, 10 fruit to analyze α-farnesene and 6-MHO production, and five fruit to analyze antioxidant compounds (phenolic compounds, ascorbate).

Measurements of maturity parameters and ripening index by Streif

Measurements of maturity parameters were made as reported previously by Hendges et al. (2020), and the maturity parameters are given in Table 1.

Table 1
Maturity attributes of the ‘Alexander Lucas’ pears harvested at the two maturity stages from the three production regions.
R I =  flesh firmness  k g c m 2  soluble solids  ( % ) ×  iodine-starch index (1-10)  (1)

Evaluation of scald and measurements of respiration rate and ethylene release

Scald index was determinate by Eq. 2 using scald incidence (number of fruit affected by scald) and the percentage of the fruit epidermis affected by scald (scald severity). The scald severity was evaluated according to the following scale:

  • 0 = no scald;

  • 1 = 1 to 25% surface affected;

  • 2 = 26 to 50% surface affected;

  • 3 = > 50% surface affected.

 Scald index  =  (number of fruit  × 0 ) + (  number of fruit  × 1 ) + (  number of fruit  × 2 ) + (  number of fruit  × 3 ) ( [ (  total number of fruit  × 3 ) ] × 100 (2)

The respiratory rate was determined at 20 °C in a 4.2-L hermetically sealed glass jar in three replicates of four fruit using a continuous-flow gas analyzer. To measure the ethylene release rate, four fruit were placed in a hermetically sealed container for 2 h, and a 10-mL air sample was collected with a syringe. One mL of the container atmosphere was injected into a gas chromatograph (Carlo Erba Strumentazione), with temperatures of 200, 240, and 100 °C for the injector, detector, and column, respectively.

Extraction and quantification of α-farnesene and 6-MHO

To determine the α-farnesene and 6-MHO levels, the method described by Hendges et al. (2018) was applied. Briefly, 30 fruit separated into three replicates were cut longitudinally into wedges. Thirty grams of fruit wedges, including the skin and pulp, were homogenized at 22,413 × g (IKA®, Staufen, Germany) with 30 g of saturated solution of calcium chloride (700 g·L-1 CaCl2) and stored at -28 °C for further studies.

For the analysis, 10 g of sample mix was transferred into 20-mL glass vial, and 50 μL of ethyl nonanoate (internal standard, 0.175 mg·L-1 in ethanol) was added to each sample vial. The vials were flushed with nitrogen and immediately closed with PTFE/silicone septum and sealed with screw caps. A solid phase microextraction fiber (divinylbenzene/ carboxen/ polydimethylsiloxane sorbent length, 1 cm; thickness, 50/30 µm; StableFlex, Supelco, United States of America) was used for volatile extraction. Identification of α-farnesene and 6-MHO was performed by comparisons of their mass spectra with those of available commercial standards and with spectra published in the National Institute of Standards and Technology mass spectral library. Quantification of α-farnesene and 6-MHO was carried out by preparation of calibration curves for each volatile compound. The concentrations of the sample compounds were calculated from the peak areas and the corresponding standards of known concentrations.

Extraction and quantification of ascorbate

For ascorbate determination, the fruit epidermis was removed from the region with the largest fruit diameter. After removal, the epidermis was fragmented, frozen in liquid nitrogen, and stored at -28 °C. Prior to the analysis, the epidermal samples were ground in a coffee mill that was pre-cooled with liquid nitrogen. A total of 15 mL 3% metaphosphoric acid solution (HPO3, 65% purity, 30 g·L-1) was added to 6-g fruit peel powder. The mixture was homogenized (Turrax; 60 s, 22,413 × g), protected from light in a water bath (4 °C, for at least 20 min). After that, the samples were centrifuged (14,000 × g, 20 min), and the supernatant was filtered through a nylon filter (45 μm) coupled to a 13-mm syringe. Forty microliters were injected into the HPLC (Bischof, Germany) manually, of which 20 μL were dispensed into a chamber and then transferred to the column of the HPLC, with 0.8 mL·min-1 eluent flow rate, as 2.5 g tetra-n-butylammonium hydrogen sulfate. The column was incubated at 30 °C. The content of ascorbate was calculated using standards containing 5 mg ascorbate in 100 mL 3% metaphosphoric acid.

Extraction and quantification of phenolic compounds by HPLC-DAD

Fruit epidermis was removed from the region with the largest fruit diameter and immediately frozen in liquid N2. Subsequently, the samples were stored at -80 °C, freeze dried and ground in a ball mill for extraction of phenolic compounds. This was performed by adding 1 mL of methanol and 200-µL methanolic solution of 3-methoxyflavone (c = 0.1 mg·mL-1) as internal standard, to 400 mg dry powder for 30 min in a cooled ultrasound water bath (7 °C). After centrifugation (11,180 × g, 10 min, and 4 °C), the supernatant was evaporated, and the residue was redissolved in 200-µL methanol. A 10 µL sample of these extract was injected into a Kontron HPLC system (Kontron Instruments, Germany) equipped with two pumps, autosampler (model 231, Gilson Abimed Systems) and a diode array detector (DAD). The phenolic compounds were separated on a Nucleosil C18 column (240 × 4 mm i.d., Macherey-Nagel) and eluted with a mixture of water containing 5% formic acid (solvent A) and methanol (solvent B) at a flow rate of 0.5 mL·min-1. The gradient profile was as follows:

  • 0–5 min = 5% B;

  • 5–10 min = 5–10% B;

  • 10–15 min = 10% B;

  • 15–35 min = 10–15% B;

  • 35–55 min = 15% B;

  • 55–70 min = 15–20% B;

  • 70–80 min = 20% B;

  • 80–95 min = 20–25% B;

  • 95–125 min = 25–30% B;

  • 125–145 min = 30–40% BA;

  • 145–160 min = 40–50% B;

  • 160–175 min = 50–90% B;

  • 175–195 min = 90% B.

For selective detection of flavan-3-ols using post-column derivatization with p-dimethyl-aminocinnamic aldehyde, a further Gynkotek HPLC pump (model 300 C, Germering, Germany) and a VIS-detector at 640 nm (Kontron Detector 432, Kontron Instruments) were used. Chlorogenic acid was identified in comparison to a standard solution, and as for the other hydroxycinnamic acids it was measured at 320 nm. The flavonols were detected at 350 nm.

Statistical analysis

The experimental design was completely randomized using a factorial scheme (two maturity stages and five storage conditions). The treatments were composed of three replications and unit experimental of 10 and 30 fruit for the analysis of volatile compounds and scald index, respectively. The scald index (percentage values) was transformed in to “arc sin [(x + 0.5)/100]½” before being subjected to analysis of variance. Tukey’s test was used to compare the means (p < 0.05).

The statistical interactions between treatments were tested, and, when significant, their values (two maturation stages versus five storage conditions) were compared. When the interactions between the treatments were not significant, only the average of the treatments was compared.

The data were analyzed individually for each production region. Principal component analysis was used to summarize the information in the data set of studied parameters. It enables determination of parameters that contribute the most to the classification of the pears and visualization of the classification in a two-dimensional space.

RESULTS AND DISCUSSION

Scald index

The application of 1-MCP diminished the scald index in pears from all three of the orchards. 1-MCP treatment can extend the shelf-life of fruit, maintaining active compounds in peels in addition to reducing superficial scald (Tedeschi et al. 2023). When applied to fruit stored under the standard control CS conditions, 1-MCP reduced the scald index in fruit from LA and OHR, as also for the CA condition for RV (MS2 only) and LA (Table 2). Vanoli et al. (2016) also reported the actions of 1-MCP for the reduction of superficial scald in ‘Abate Fetel’ pears stored under their CS and CA conditions, and Isidoro and Almeida (2006) showed that 1-MCP was effective in further reducing scald in pears stored in controlled atmosphere. Argenta et al. (2002) reported that 1-MCP treatments prevent or reduce superficial and senescent scald in ‘d’Anjou’ pears stored at 1 °C. 1-MCP treatment under CS condition maintains higher level of antioxidant compounds compared to CS, preserving high antioxidant activity even with an early harvest (Tedeschi et al. 2023).

In our study, for the fruit harvested under MS1 in RV and under both maturity stages in LA, the development of scald was completely inhibited by CA+MCP. These results showed that the effects of 1-MCP on scald of ‘Alexander Lucas’ pears that was primarily seen for CS might be dependent on preharvest factors (e.g., pedoclimatic conditions, maturity stage). The reason for the greater control of superficial scald in the fruit under CA+MCP might be related to the joint actions of the two conditions (i.e., low O2, 1-MCP) on the delay of fruit senescence and the reduction in the ethylene release and the synthesis and oxidation of α-farnesene, along with the degradation of the cell membranes.

No effects were seen for the CA condition on the scald index according to maturity stages and production regions (Table 2). In general, CA inhibits the development of superficial scald; however, its effectiveness is influenced as a function of the cultivar and storage period (Lurie and Watkins 2012). The inability of the CA storage on the senescent scald development control found in the present work could be the result of some changes in the metabolism of fruit in function of internal disorders observed. These disorders can lead to changes in ripening and consequently an imbalance on the fruit. In pears, the symptoms of scald-like disorders can result from multiple and different metabolic changes (Lindo-García et al. 2020). The CA stored pears from the LA and OHR orchards showed higher scald indices, and OHR also showed significantly higher values as compared to CS and the other storage conditions.

Table 2
Scald index, α-farnesene, and 6-methyl-5-heptene-2-one levels by ‘Alexander Lucas’ pears harvested at the two maturity stages from the three production regions according to the different storage conditions (0 ± 0.1 °C; 94% ± 2% relative humidity) followed by seven days under ambient conditions (20 ± 2 °C; 60% ± 5% relative humidity)* * values within a column followed by the same lower-case letter are not significantly different, and values within a line followed by the same capital letter are not significantly different (Tukey’s test; .

The storage under ULO reduced the scald in the fruit harvested from RV for MS2 and from LA for both maturity stages, compared to fruit kept under CS. The action of ULO is probably associated with the reduced oxidative processes within the cell membranes that involve α-farnesene. ULO storage atmosphere can inhibit the oxidase enzymes activities, and especially ACC oxidase, that most likely is a key factor determining the action of this storage condition on scald inhibition (Larrigaudière et al. 2019).

As observed in the studies conducted by Giné-Bordonaba et al. (2013) and Larrigaudière et al. (2019), the ULO conditions are more efficient for the reduction of superficial scald as compared to the CA conditions in apples and pears. Despite this, the effect of ULO can be dependent on the fruit production region (Giné-Bordonaba et al. 2013). Differently to 1-MCP, that inhibits ethylene metabolism and fruit ripening, ULO condition only delays this process, as a result of the action of both cold temperature and low O2 partial pressure (Larrigaudière et al. 2019). Larrigaudière et al. (2019) found that inhibition of scald, in part, may be mediated by increased ethanol accumulation, which may act as a weak antioxidant or protect against the effects of cold.

Farnesene production

After three months of storage plus seven of the ambient conditions, fruit treated with 1-MCP (CS or AC) showed lower α-farnesene production, regardless of the orchard and maturity at harvest. After seven months of storage, the treatment with 1-MCP reduced α-farnesene production in the RV pears stored under CS regardless of maturity stage, and in the OHR pears for MS2 only. According to Isidoro and Almeida (2006) and Xie et al. (2014), 1-MCP treatment effectively reduces the accumulation of α-farnesene and conjugated trienes in ‘Rocha’ and ‘d’Anjou’ pear epidermis. Gapper et al. (2006) reported that the application of 1-MCP to ‘d’Anjou’ pears inhibited the expression of the PcAFS1 gene, which encodes α-farnesene synthase, and is positively regulated by ethylene. Thus, 1-MCP would act indirectly through the reduction of the ethylene actions, leading to lower synthesis of α-farnesene, and primarily reducing α-farnesene oxidation and diminishing the α-farnesene metabolites from this process. However, after seven months of storage plus seven days simulating shelf-life, 1-MCP treatment had no effect on fruit harvested from LA for both maturity stages and from OHR (MS1 fruit) (Table 2).

CA (without 1-MCP) treatment did not differ to produce α-farnesene within the fruit, regardless of storage period and production location. There was higher α-farnesene production with the harvest delay in the OHR fruit stored under CS and CA (Table 2).

In this work, ULO had a variable effect, which depended on the production location. According to Larrigaudière et al. (2019), ULO is less effective compared to 1-MCP treatment to prevent α-farnesene accumulation, a result that may be related to the increase in physiological maturity. For fruit harvested from RV, ULO reduced α-farnesene production; however, for the OHR fruit from MS1, an increase in α-farnesene production was seen, as compared to that seen for CS. Larrigaudière et al. (2019) did not find a clear relationship between α-farnesene and conjugated trienes in the development of scald in fruit stored with ULO, as observed in 1-MCP.

Methyl-5-hepten-2-one production

Except for fruit from the OHR (MS2) orchard, the 1-MCP condition (CS or AC) reduced 6-MHO production after three months of storage plus seven days of the ambient conditions, regardless of orchard and maturity at harvest. There was reduction in 6-MHO production in the fruit treated with 1-MCP as a function of the storage conditions and production regions after seven months of storage plus seven days of shelf-life (Table 2).

For the CS+MCP condition, 6-MHO synthesis was reduced in MS1 fruit from LA and OHR. The CA+MCP condition reduced 6-MHO production in the MS1 fruit from RV and OHR, and for both maturity stages from LA. In ‘Dangshansuli’ pears, 1-MCP treatment was reported to inhibit 6-MHO synthesis and prevent the appearance of superficial scald after six months of refrigerated storage (Hui et al. 2016). The oxidation of α-farnesene and the formation of conjugated trienols and 6-MHO are important factors in the development of superficial scald (Pesis et al. 2010). 6-MHO production coincides with the appearance of superficial scald symptoms; in addition, this volatile is more stable than the conjugated trienols, and for this reason, it has been associated with superficial scald (Farneti et al. 2015, Hui et al. 2016). According to Hui et al. (2016), there is an endogenous 6-MHO concentration threshold above which superficial scald occurs. In addition, they reported a positive correlation between the production of conjugated trienols and 6-MHO, and between these compounds and scald incidence.

After seven months of storage, plus seven days at shelf-life, the highest 6-MHO production in the present study was observed in fruit stored under CS and CA, which did not differ significantly from the ULO fruit (from RV) for both maturity stages, and from OHR harvested at MS2 (Table 2).

Compared to CS or CA, ULO reduced 6-MHO production in the LA orchard and when compared to CAin the OHR orchard (MS2 fruit) after three months of storage. ULO also restricted 6-MHO production in the LA fruit harvested at both maturity stages, and in the OHR fruit harvested at MS1 after seven months. These effects on 6-MHO reduction might be the result of increased alcohol dehydrogenase activity under ULO, and the consequent use of 6-MHO as a substrate to detoxify the cells by converting it into 6-methyl-5-hepten-2-ol (Pesis et al. 2010).

Ascorbate production

Ascorbic acid and ascorbate are antioxidants that regulate fruit ripening by eliminating reactive oxygen species and are associated with the control of some physiological disorders such as superficial scald (Arabia et al. 2024). The CA+MCP condition (for both maturity stages) showed positive effects in the maintenance of the ascorbate content in the fruit from OHR, as compared to the control CS treatment. According to to Larrigaudière et al. (2016), the total antioxidant potential did not explain scald sensitivity. However, ascorbate might inhibit the enzyme polyphenol oxidase (PPO) activity and thus have an important role in superficial scald control (Larrigaudière et al. 2016; Arabia et al. 2024). Giné-Bordonaba et al. (2020) mention that 1-MCP can prevent the development of scald through repression of the PPO gene, and also through chloroplast-induced protection.

With the harvest delay, there were reduction in the ascorbate content (as means of all treatments in the RV fruit), and increase in the ascorbate content in the fruit from LA (CS, ULO) and OHR (CS, CA).

Production of phenolic compounds

Treatment with 1-MCP (CS) reduced the contents of catechin, procyanidin B2, epicatechin, and chlorogenic acid in fruit from the RV and LA orchards, and CA+MCP decreased catechin, procyanidin B2, and chlorogenic acid in RV fruit (Table 3). It is possible that 1-MCP acts indirectly in the maintenance of the antioxidant compounds due to its action on ethylene, and consequently on the ripening of the fruit. It is reasonable to suggest that inhibition of ethylene production by 1-MCP may lead to reduce concentrations or interrupt the normal metabolism of phenolic compounds in 1-MCP treated fruit (Hoang et al. 2011). The delay in harvest showed high variability regard to the phenolic compounds according to the storage conditions and production region.

Phenolic compounds are important antioxidant substances and can contribute to the reduction of scald development. However, their accumulation might also influence the appearance of this disorder due to their oxidation by the PPO (Lurie and Watkins 2012). The disintegration of the cell membrane and the process of phenol oxidation in the pear fruit are linked to the onset and development of superficial scald (He et al. 2022). 1-MCP treatment affects several phenolic metabolism related genes (Zhou et al. 2020). Low-temperature storage can compromise the integrity of the internal membranes of cells, promoting the reaction between PPO and chlorogenic acid leading to browning of the peel of the fruit. During the development of scald, the skin of fruit treated by 1-MCP is characterized by the lower polyphenol accumulation than untreated fruit, and the expression of PPO is also strongly inhibited by 1-MCP (Giné-Bordonaba et al. 2020).

Fruit storage under CA condition (without 1-MCP) reduced the contents of phenolics in RV (MS1 and MS2) and LA fruit (MS1) (Table 3). In fruit from OHR, no effects on the content of phenolic compounds were seen for the different storage conditions. Silva et al. (2010) reported little or no effects on the free radical scavenging activity of ‘Rocha’ pears as a function of post-harvest storage conditions. In ‘Cripps Pink’ apples, the storage atmosphere (CA compared to NA) did not significantly affect the concentrations of the total phenolic compounds or individual phenolics (Hoang et al. 2011). According to Hoang et al. (2011), physiological diseases such as superficial scald are not directly related to the levels of antioxidants in whole fruit. The superficial scald development seems to depend on the balance between the oxidative processes initiated by the conjugated trienols and the scavenging capacity of the tissue (Guerra et al. 2012).

Table 3
Ascorbate and phenolic compounds by ‘Alexander Lucas’ pears harvested at the two maturity stages from the three production regions according to the different storage conditions for seven months under refrigeration (0 ± 0.1 °C; 94% ± 2% relative humidity) followed by seven days under ambient conditions (20 ± 2 °C; 60% ± 5% relative humidity)* * values within a column followed by the same lower-case letter are not significantly different, and values within a line followed by the same capital letter are not significantly different (Tukey’s test; .

Multivariate analysis

Principle component analysis was performed to select a subset of variables contributing the most to classify pears regarding the 1-MCP treatment, storage conditions, and maturity stage in the three orchards. It was therefore possible to explain 65.7% of the variability in the studied parameters by the first two principal components (PC). Positive PC1 values were associated with the production of phenolic and volatile compounds, as well as the scald index. Negative PC1 was related to ascorbate production. Positive PC2 values were related to scald index and volatiles compounds, while negative PC2 with production of antioxidants compounds (Fig. 1). A positive correlation was observed between the scald index, α-farnesene (only after three months of storage), 6-MHO, CO2, and ethylene production.

Figure 1
Principal component analysis for the two maturity stages, three production locations and different storage conditions of the ‘Alexander Lucas’ pears, according to scald, volatiles and antioxidante compounds. The extracted principal components accounted for 65.7% of the variability in the data.

The samples are well differentiated into two groups. Principal component analysis effectively classified the samples treated with 1-MCP (CS or CA) and the other storage conditions (CS, CA, and ULO). Except for the RV orchard, the ULO results are positioned in the most central region of Fig. 1 in relation to the other storage conditions, demonstrating a reduction in the production of phenolic and volatile compounds, as well as scalding (PC1 negative). Except for the RV orchard, in which the results from CS storage are positioned in a region with greater production of phenolic compounds, CS and CA, without 1-MCP, presents positive PC1 and PC2, which show a greater production of volatile compounds, as well as scald development. When harvested late, fruit stored in CS from RV orchard showed extreme positive PC1 values (data not shown). The fruit of the 1-MCP treatment showed negative PC1 and PC2, characterizing a lower production of phenolic and volatile compounds, as well as the development of scald.

Some other studies have related superficial scald to α-farnesene content (Gapper et al. 2006, Vanoli et al. 2010); however, the oxidation of α-farnesene, rather than its production, is important for the development of this disorder (Larrigaudière et al. 2016). Farneti et al. (2015) and Hui et al. (2016) reported positive correlations between 6-MHO content and superficial scald in apples and pears. The ascorbate content showed an inverse correlation with the occurrence of scald’s disorder. The result found by Larrigaudière et al. (2016) and Giné-Bordonaba et al. (2020) suggest the protective role that ascorbate may have in controlling the development of this physiological disorder. Ascorbic acid/ascorbate possibly acts as a PPO inhibitor and a scavenger of generated reactive oxygen species inside the cell during superficial scald of pear (Arabia et al. 2024). Zhou et al. (2020) showed that arbutin, chlorogenic acid, catechin, and epicatechin were the main phenolic compounds in the peel, and, except by catechin, 1-MCP treatment significantly inhibited the accumulation of these phenolic compounds.

As verified in this work, 1-MCP in combination with low O2 limits senescent disorders during prolonged low temperature storage and inhibition on scald is evident with a combination of CA and 1-MCP (Lum et al. 2017). However, it is important to keep in mind that this condition can be responsible to lead to an increase in internal browning disorders in ‘Alexander Lucas’ pears (Hendges et al. 2015, Balkees et al. 2022). In addition, CA+1MCP can cause reduction in the production of volatile compounds and ripening delayed (Hendges et al. 2018, Hendges et al. 2020).

As already reported by others (Whitaker et al. 2009, Larrigaudière et al. 2016) and reinforced in the present study, scald is associated with genetic characteristics, pre-harvest and post-harvest factors, and the interactions between them. These factors had significant influences on the scald appearance of ‘Alexander Lucas’ pears here, and therefore new studies should be carried out to relate pre-harvest conditions (maturity stage, production region, and others) to the biochemical processes involved in the development of scald during and after storage.

CONCLUSION

Fruit treatments that combined controlled atmosphere or cold storage plus 1-MCP reduced scald, but the effects varied between orchards.

1-MCP treatment decreased the production of volatiles and antioxidant compounds, excepted by ascorbate, which appeared to be associated with delayed ripening and the less severe development of scald.

Use of ultra-low O2 reduced the scald, but the effects depended on the production region. Storage under controlled atmosphere without 1-MCP application did not reduce the appearance of scald in these pears stored for seven consecutive months plus seven days of exposure to ambient conditions.

There were positive correlations between the development of scald and the production of 6-MHO and α-farnesene (after three months of storage). Ascorbate was negatively correlated with scald.

ACKNOWLEDGMENTS

We acknowledge Prof. Dr. Dieter Treutter (in memoriam) for his support on this research. Prof. Dr. Treutter’s, as well as work group, Dr. Lonela Regos, and Dr. Johannes Hadersdorfer, contributions and technical supervision were invaluable for this work. The authors would like to acknowledge Berenice Vollmar for technical assistance with the ripening parameters, ascorbate, and senescent and superficial scald analysis. We acknowledge Prof. Dr. Donnchadh Mac Carthaigh, Felix Büchele, and Kiran Dhuraji Hivare for the revision and improvement of the manuscript.

  • How to cite: Hendges, M. V., Steffens, C. A., Amarante, C. V. T., Vidrih, R., Zlatic, E., Balkees, B., Kittemann, D. and Neuwald, D. A. (2024). Relationship between volatiles and antioxidant compounds in scald on ‘Alexander Lucas’ pear in different postharvest conditions. Bragantia, 83, e20230226. https://doi.org/10.1590/1678-4499.20230226
  • FUNDING
    Coordenação de Aperfeiçoamento de Pessoal de Nível Superior
    Finance Code 001

DATA AVAILABILITY STATEMENT

The datasets generated and/or analyzed during the current study are available from the corresponding author.

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Edited by

Publication Dates

  • Publication in this collection
    28 June 2024
  • Date of issue
    2024

History

  • Received
    13 Oct 2023
  • Accepted
    01 Apr 2024
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