Storability and Linear Regression Models of Pericarp Browning and Decay in Fifty Litchi (Litchi chinensis Sonn.) Cultivars at Room Temperature Storage

The primary cause for the limited shelf life of litchi fruit is rapid pericarp browning and decay. This study aims to evaluate the storability of 50 litchi varieties and establish a linear regression model for pericarp browning and decay based on 11 postharvest physical and chemical indices after 9 days of storage at room temperature. The results indicated that the average value of the browning index and decay rate significantly increased to 3.29% and 63.84% of 50 litchi varieties at day 9, respectively. Different litchi varieties showed different variations in appearance indicators, quality indicators, and physiological indicators. Furthermore, principal component analysis and cluster analysis revealed that Liu Li 2 Hao exhibited the highest resistance to storage, whereas Dong Long Mi Li, Jiao Pan Li, E Dan Li 2 Hao, and Ren Shan Li were not resistant. Stepwise multiple regression analysis further demonstrated that the factors were highly correlated with the decay index, with a partial correlation coefficient of 0.437 between the effective index and the decay index. Therefore, pericarp thickness, relative conductivity, pericarp laccase activity, and total soluble solids were significant indicators for the comprehensive evaluation of litchi browning and decay, and relative conductivity was the significant determinant causing fruit browning. These findings provide a new perspective on the sustainable development of the litchi industry.


Introduction
Litchi (Litchi chinensis Sonn.) is a tropical fruit with high commercial value in the international fruit market [1]. As typical tropical fruit, litchi exhibits many disadvantageous after postharvest storage. The litchi fruit has a high respiration rate while being stored at room temperature, and the pericarp oxidizes rapidly within 2 to 3 days, resulting in severe quality degradation and a decline in market value [2]. The browning of litchi fruit is primarily caused by desiccation of the pericarp. For example, pericarp moisture loss usually occurs through the micro-cracks of pericarp tissues. In addition, litchi fruit internal and external quality conditions, along with postharvest losses, directly affect fruit quality parameters such as color, quality indicators, and physiological indicators [3]. However, the objective traits, including yield, quality, and storability, are quantitative and show a highly complex relationship, resulting in lower heritability. Moreover, the postharvest physiochemical indicators of fruit also exhibit different characteristics and unclear interrelationships. Based on these effects, the correlation between different indicators of litchi fruit and fruit browning can be explored to effectively screen and identify more storage After air drying, the fruit were packed in sealed polyethylene film (0.02 mm thick) bags (30 fruit per bag; 15 bags of each replicate and treatment) and held in a room at 25 ± 1 • C for 9 days. Three bags of the fruit were removed for the analysis of the indicators at 0, 3, 5, 7, and 9 days of storage. The indicators measured included apparent indicators (color, browning index, decay rate, peel thickness, peel water content), quality indicators (total soluble solids, titratable acid, Vc), and physiological indicators (peel relative conductivity, laccase activity, POD activity). All analyses were conducted in triplicate ( Figure 1). iprodione solution and 500 mg·L −1 prochloraz solution for 1 min to eliminate potentia microbes.
After air drying, the fruit were packed in sealed polyethylene film (0.02 mm thick bags (30 fruit per bag; 15 bags of each replicate and treatment) and held in a room at 25 1 °C for 9 days. Three bags of the fruit were removed for the analysis of the indicators a 0, 3, 5, 7, and 9 days of storage. The indicators measured included apparent indicator (color, browning index, decay rate, peel thickness, peel water content), quality indicator (total soluble solids, titratable acid, Vc), and physiological indicators (peel relative con ductivity, laccase activity, POD activity). All analyses were conducted in triplicate (Figur 1).

Appearance Indicators
Pericarp thickness was measured using a Vernier caliper in each replication for eac

Appearance Indicators
Pericarp thickness was measured using a Vernier caliper in each replication for each treatment.
Pericarp moisture content was quantified as relative mass loss by weighing (±1 mg). The pericarp of five fruits per sample was weighed before and after oven drying for 4 h at 105 • C and re-cooling in a desiccator.

Quality Indicators
A set of 15 fruits per replicate was homogenized and filtered. The supernatant was collected for the analysis of total soluble solids, titratable acidity, and ascorbic acid. Total soluble solids were measured with a digital refractometer [22].
Titratable acidity was determined by titration of juice with 0.1 mol·L −1 NaOH [24]. Specifically, pipette 2 mL of the juice into a triangular flask and titrate with 0.025 mol L −1 NaOH solution; 1% phenolphthalein was used as an indicator. Each experiment was repeated in triplicate at least three times. The equation given below was used to calculate the titratable acidity: where V1 represents the volume of NaOH consumed for titration (mL); V2 represents the volume of juice taken for titration (mL); C represents the concentration of NaOH (mol L −1 ); K represents the conversion factor of acid. Ascorbic acid was determined by titrating 10 g of mixed pulp sample with the standard 2,6-dichlorophenol dye [25]. Specifically, after juice extraction, 1 mL of juice was quickly drawn in a triangular flask, and 4 mL of 2% oxalic acid solution was added and titrated with 2,6-dichloroindophenol solution until pink; the endpoint was no fading within 15 s, and the volume of consumed dye was noted. The 2,6-dichloroindophenol solution was calibrated with standard Vc.
where T represents the amount of 1 mL of 2,6-dichloroindophenol solution equivalent to the ascorbic acid standard solution (mg mL −1 ); V1 represents the volume of standard ascorbic acid (mL); V2 represents the volume of 2,6-dichloroindophenol solution consumed for the titration of standard ascorbic acid (mL); V represents the volume of 2,6-dichloroindophenol solution consumed for the titration of the blank (mL). The equation given below was used to calculate the Vc content: where V3 represents the volume of 2,6-dichloroindophenol solution consumed during the titration of the sample solution (mL); V4 represents the volume of juice taken during the titration (mL).

Physiological Indicator
Pericarp relative conductivity was determined using other researchers [26] method. Pericarp discs with a 5 mm diameter were removed from 10 fruit at the equatorial region (three discs per fruit), then rinsed and incubated in 25 mL of distilled water for 30 min. Next, initial electrolyte leakage was monitored with a conductivity meter (DDS-11A, Shanghai, China). Total electrolyte leakage was determined after boiling for 30 min and cooling to 25 ± 1 • C. Relative conductivity was expressed as a proportion of total electrolyte leakage.
Litchi peroxidase activity (POD) was extracted by homogenizing the pericarp (1 g) with 5 mL of 0.05 mol·L −1 phosphate buffer (pH 7.0). The homogenate was centrifuged for 20 min at 13,000× g and 4 • C, and the supernatant was collected as the crude enzyme extract. POD activity was assayed using the method as follows: in a 3 mL reaction mixture that contained 0.05 mL enzyme extract, 2.75 mL 0.05 mol·L −1 phosphate buffer (pH 7.0), 0.1 mL of 0.46% H 2 O 2 , and 0.1 mL of 4% guaiacol. The increase in absorbance at 470 nm due to guaiacol oxidation was recorded for 2 min using a spectrophotometer (Z 2000, HITACHI, Japan). One unit of enzyme activity was defined as the quantity of the enzyme that caused a change of 0.001 in absorbance per minute.
Litchi laccase activity was extracted by homogenizing the pericarp (8 g) with 20 mL of 0.05 mol·L −1 phosphate buffer (pH = 7.0) with Polyclar AT (insoluble polyvinylpyrrolidone; 10% of pericarp by weight). The homogenate was centrifuged for 20 min at 13,000× g and 4 • C. Then, the supernatant was collected as the crude enzyme extract. In a 3 mL reaction mixture that contained 0.05 mL enzyme extract, 2.35 mL MUB (modified universal buffer) (pH 4.0), and 0.6 mL of 0.02 M ABTS (2,2 -azinobis-(3-ethylbenzthiazoline-6-sulphonate)). The increase in absorbance at 420 nm was recorded for 2 min using a spectrophotometer (Z 2000, HITACHI, Tokyo, Japan). One unit of enzyme activity was defined as the quantity of the enzyme that caused a change of 0.001 in absorbance per minute.

Statistical Analysis
All the treatments and measurements were set up in a completely randomized factorial design with three replicates. All data were subjected to analysis of variance (ANOVA) with SPSS 27.0 (IBM SPSS 27; SPSS Inc., Armonk, NY, USA). The samples consisted of fifty litchi varieties under various storage times at room temperature. The eleven indexes under the various storage times were the variables. Correlation analysis, factor analysis, multiple linear stepwise regression, and clustering analysis were used as the analysis method. Factor analysis was performed using the Kaise standardized orthogonal rotation method. The variable load values in the rotating component matrix were used to select the explanation of the variables with the common factor. In addition, data were plotted using ORIGIN 2022 (Origin Laboratories, Northampton, MA, USA) software.

The Change in Pericarp Browning and Apparent Indicators of Harvested Litchi Fruit
One of the major factors that affect the commercial value of litchi fruit is pericarp browning [27]. As storage time increases, the browning index of the fruits significantly increases, resulting in the fruits turning brown ( Figure 2c). Therefore, a colorimeter was used to measure the rind color of the litchi fruit after harvest (Figure 2e-g). The L* and b* values showed no difference between day 0 and day 3; however, the fruit values began to decrease significantly by the fifth day, and the L* and b* values decreased by 20.84% and 27.62%, respectively, on the ninth day. On the other hand, the a* value did not significantly differ within the first 5 days and then began to decrease significantly by the seventh day, and the lowest value was reached on the ninth day, with a decrease of 19.76%. It is worth noting that the a* value represents the degree of redness of the Litchi fruit [23], which suggests that the fruit's redness can be effectively maintained within the first 5 days after harvest.
To further evaluate the postharvest phenological characteristics of litchi fruits during storage at room temperature, the pericarp thickness (Figure 2a), moisture content (Figure 2b), and decay rate (Figure 2d) were measured. As the storage time prolonged, the pericarp thickness of litchi fruits significantly reduced, and the decay rate of litchi fruit began to increase significantly by the fifth day and decreased by 17.89% by the ninth day, while the moisture content of the fruit remained mostly unchanged. Overall, these results suggest that the best storage period for litchi fruit is within 5 days after harvesting at room temperature. (g) b*. Different letters above groups represent significant differences; shared letters represent no significant differences. The error bars represent standard deviation.

The Change in Quality Indicators of Harvested Litchi Fruit
This study aims to evaluate the quality of litchi fruits stored at room temperature for different time periods by determining total soluble solids, Vc content, and titratable acidity. As the storage time increased, a significant decrease in total soluble solids was observed in litchi fruits, namely, they decreased by 14.38% compared with day 0 (Figure 3a). The Vc Foods 2023, 12, 1725 7 of 17 content decreased, but the change was not significant (Figure 3b). However, the titratable acidity significantly decreased on the third day (decreased by 36.35%) and then remained stable from day 3 to day 7 and increased significantly on the ninth day ( Figure 3c). nificant differences. The error bars represent standard deviation.

The Change in Quality Indicators of Harvested Litchi Fruit
This study aims to evaluate the quality of litchi fruits stored at room temperature for different time periods by determining total soluble solids, Vc content, and titratable acidity. As the storage time increased, a significant decrease in total soluble solids was observed in litchi fruits, namely, they decreased by 14.38% compared with day 0 (Figure 3a). The Vc content decreased, but the change was not significant (Figure 3b). However, the titratable acidity significantly decreased on the third day (decreased by 36.35%) and then remained stable from day 3 to day 7 and increased significantly on the ninth day ( Figure  3c).

The Change in Physiological Indicators of Harvested Litchi Fruit
The relative conductivity of the fruit pericarp represents the cell membrane permeability or degree of cell membrane injury, and its value increases with the degree of cell aging and damage [28]. The research results indicated that there is no difference in relative conductivity within the first 5 days of room temperature storage, a significant increase was observed starting from day 7, and the maximum value was reached at day 9, with an increase of 52.22% compared to day 0 ( Figure 4), indicating that the integrity of litchi fruit pericarp cell membranes can be well maintained within 5 days after harvest. Laccase is a degradation enzyme for epicatechin-mediated anthocyanin in litchi fruit tissue [29], the activity of which directly affects fruit pericarp browning. The results of this study show that laccase activity remained stable within the first 5 days of room temperature storage, with no significant upward trend, and a significant increase in laccase activity was observed on the seventh and ninth days, by 25.60% and 34.29%, respectively (Figure 4), indicating that the epicatechin-mediated anthocyanin in the fruit tissue began to degrade significantly on the 7th day, which increased the browning index of the litchi fruit pericarp. In order to further evaluate changes in the antioxidant system, this study has measured the activity of peroxidase (POD) in litchi fruit, which can effectively remove peroxides. Surprisingly, the activity of POD did not show significant changes during the room temperature storage of litchi fruit, possibly due to the fact that the antioxidant system is easily influenced by multiple factors and is itself a complex nonlinear system.

The Change in Physiological Indicators of Harvested Litchi Fruit
The relative conductivity of the fruit pericarp represents the cell membrane permeability or degree of cell membrane injury, and its value increases with the degree of cell aging and damage [28]. The research results indicated that there is no difference in relative conductivity within the first 5 days of room temperature storage, a significant increase was observed starting from day 7, and the maximum value was reached at day 9, with an increase of 52.22% compared to day 0 ( Figure 4), indicating that the integrity of litchi fruit pericarp cell membranes can be well maintained within 5 days after harvest. Laccase is a degradation enzyme for epicatechin-mediated anthocyanin in litchi fruit tissue [29], the activity of which directly affects fruit pericarp browning. The results of this study show that laccase activity remained stable within the first 5 days of room temperature storage, with no significant upward trend, and a significant increase in laccase activity was observed on the seventh and ninth days, by 25.60% and 34.29%, respectively (Figure 4), indicating that the epicatechin-mediated anthocyanin in the fruit tissue began to degrade significantly on the 7th day, which increased the browning index of the litchi fruit pericarp. In order to further evaluate changes in the antioxidant system, this study has measured the activity of peroxidase (POD) in litchi fruit, which can effectively remove peroxides. Surprisingly, the activity of POD did not show significant changes during the room temperature storage of litchi fruit, possibly due to the fact that the antioxidant system is easily influenced by multiple factors and is itself a complex nonlinear system.

Correlation Analysis of Indicators at Room Temperature Storage
In this research, a correlation analysis was conducted on various indices associated with the browning index and decay rate of litchi fruits, including pericarp thickness, moisture content, total soluble solids, Vc, relative conductivity, L*, a*, b*, and POD activity. The results revealed significant correlations between the browning index and decay rate and

Correlation Analysis of Indicators at Room Temperature Storage
In this research, a correlation analysis was conducted on various indices associated with the browning index and decay rate of litchi fruits, including pericarp thickness, moisture content, total soluble solids, Vc, relative conductivity, L*, a*, b*, and POD activity. The results revealed significant correlations between the browning index and decay rate and physicochemical indicators during room temperature storage, as shown in Figure 5. Specifically, the browning index and decay rate exhibited highly significant positive correlations with relative conductivity and laccase activity. Moreover, the browning index and decay rate showed highly significant negative correlations with pericarp thickness, total soluble solids, Vc, L*, and a*, which is the most visual response to fruit browning, indicating the result obtained was reliable. In addition, L*, a*, and b* showed a significant negative correlation with relative conductivity. Therefore, the factors that significantly affected the browning index and decay rate of litchi fruit were initially screened by correlation analysis, and the potential association of these indicators with the browning index and decay rate was initially verified to lay the foundation for the subsequent analysis.

Principal Component Analysis and Cluster Analysis
Moisture content, titratable acidity, b*, and POD were excluded from the analysis due to variance values below 0.6. The remaining seven physicochemical indicators were considered for PCA analysis, with a measure of sample adequacy greater than 0.8. The five principal components, with eigenvalues >0.7, accounted for 85.21% of the total variance among the accessions (Table 2). PC1, which explained 30.375% of the total variance, was primarily influenced by pericarp thickness and total soluble solids. PC2, which accounted for 20.92% of the variance, was primarily associated with Vc and a*. The eleven variables were categorized into five principal factors based on high loads, and these five factors provided plausible explanations for the browning and decay metabolism of litchi fruit. The following model was developed based on principal component analysis:

Principal Component Analysis and Cluster Analysis
Moisture content, titratable acidity, b*, and POD were excluded from the analysis due to variance values below 0.6. The remaining seven physicochemical indicators were considered for PCA analysis, with a measure of sample adequacy greater than 0.8. The five principal components, with eigenvalues >0.7, accounted for 85.21% of the total variance among the accessions (Table 2). PC1, which explained 30.375% of the total variance, was primarily influenced by pericarp thickness and total soluble solids. PC2, which accounted for 20.92% of the variance, was primarily associated with Vc and a*. The eleven variables were categorized into five principal factors based on high loads, and these five factors provided plausible explanations for the browning and decay metabolism of litchi fruit. The following model was developed based on principal component analysis: Total scores for browning and rotting were calculated using the indicators obtained at 0, 3, 5, 7, and 9 days, and the correlations of these indicators with the browning index and decay rate were analyzed (Table 3). Cluster analysis was performed based on

Stepwise Multiple Regression Analysis
A summary of the browning index model showed that the R 2 value was 0.669, indicating that 66.9% (R = 0.823) of the difference in response variables is attributable to the change in control variables. According to the results above, the relevant indices of litchi fruit, such as relative conductivity, total soluble solids, pericarp thickness, laccase, L*, a*, and Vc, were found to be major factors contributing to changes in the browning index. Therefore, a stepwise regression procedure involving seven steps was employed to select the controlled variables ( Table 4). The results indicated that step 7, which included the controlled variables relative conductivity, total soluble solids, pericarp thickness, laccase, L*, a*, and Vc, achieved the best fit to the data. Thus, the final model included seven controlled variables, and based on these variables, the regression model was constructed: After performing a t-test, the results showed that the standardized coefficients for relative conductivity, total soluble solids, pericarp thickness, laccase activity, L*, a*, and Vc were statistically significant. These factors were considered to be highly correlated with the browning index, which was found to have a partial correlation coefficient of 0.318. The order of these factors in terms of absolute values, from highest to lowest, was as follows: relative conductivity > laccase activity > Vc > pericarp thickness > total soluble solids > a* value > L* value. These findings suggest that lower relative conductivity and lower laccase activity, as well as higher values of pericarp thickness, Vc, a*, and L*, contribute to a reduction in the browning index. Moreover, the theoretical browning index calculated by the model exhibited a positive correlation with the measured value (R = 0.886 **), which indicates a high degree of agreement between the theoretical and measured values.
The summary of the disease index model revealed an R 2 value of 0.573, indicating that there were 57.3% (R = 0.757) changes in the response variable. Four controlled variables were identified in the final model, including relative conductivity, total soluble solids, pericarp thickness, and laccase activity; based on these variables, a regression model was constructed, and four steps were taken to select the controlled variables, as presented in Table 4. The statistical procedures indicated that step 4, which included the controlled variables of relative conductivity, total soluble solids, pericarp thickness, and laccase activity, resulted in a better fit to the data. Consequently, the final model included the four controlled variables, and the regression model was constructed accordingly: After conducting a t-test, it was shown that the standardized coefficients for relative conductivity, total soluble solids, pericarp thickness, and laccase activity were statistically significant. Further analysis of the data revealed that these factors were highly correlated with the decay index, with a partial correlation coefficient of 0.437 between the effective index and the decay index. The order of absolute values for these factors, from highest to lowest, was as follows: relative conductivity > laccase activity > pericarp thickness > total soluble solids. These results suggested that a lower relative conductivity and lower laccase activity, in addition to higher values of pericarp thickness and total soluble solids, decreased the decay index. Moreover, the theoretical decay index calculated by the model showed a positive correlation with the measured value (R = 0.923 **), indicating a high degree of consistency between the theoretical and measured values. These seven phenotypic traits can be used as comprehensive evaluation indices for predicting the browning index and decay rate.

Differences in Storability in Litchi Varieties
This study has evaluated the storage performance of 50 litchi cultivars at room temperature and further screened out litchi cultivars with better storage tolerance. The browning index and decay rate of the fruit were the most direct indicators to evaluate storage perfor-mance. As expected, with the extension of room temperature storage time, the browning index and decay rate of all cultivars increased significantly ( Figure 6). The apparent indicators (such as pericarp thickness, moisture content, L*, a*, and b*), quality indicators (such as total soluble solids, Vc, and titratable acid), and physiological indicators (such as relative conductivity, laccase activity, and POD activity) of different cultivars also showed varying degrees of change (Figures 2-4). From the apparent indices of 50 litchi varieties measured at different time periods, we can draw the conclusion that the best storage period is 5 days at normal temperature after harvest. However, because of varietal differences, the 50 litchi varieties will likely exhibit significant differences in browning and decay. Based on the results, the most obvious finding to emerge from the principal component and cluster analysis was that Liu Li 2 Hao exhibited the strongest resistance to browning and decay at room temperature and can be considered the variety with the strongest storability among the 50 litchi varieties (Tables 2 and 3). In comparison with other researchers' results, which used postharvest treatments such as ascorbic acid treatment [30], melatonin treatment [31], and apple polyphenol treatment [32], the Liu Li 2 Hao variety still exhibited a lower browning index and better storage performance during the same time period. Moreover, the results from the stepwise multiple regression analysis indicated that the strength of Liu Li 2 Hao lies in the fact that it can maintain a higher level of total soluble solids and pericarp thickness and lower relative conductivity during room temperature storage. In addition, Dong Long Mi Li showed the worst storability at room temperature. The primary reason for this discrepancy may be attributed to its lower level of pericarp thickness and higher relative conductivity (Figures 2 and 4). The classification results of the different litchi fruit varieties obtained in this study were generally consistent with the conventional understanding of their storability. As a result, these findings could serve as a foundation for selecting suitable litchi breeding parents.
ds 2023, 12, x FOR PEER REVIEW 13 of 1 differences, the 50 litchi varieties will likely exhibit significant differences in browning an decay. Based on the results, the most obvious finding to emerge from the principal com ponent and cluster analysis was that Liu Li 2 Hao exhibited the strongest resistance t browning and decay at room temperature and can be considered the variety with th strongest storability among the 50 litchi varieties (Tables 2 and 3). In comparison wit other researchers' results, which used postharvest treatments such as ascorbic acid trea ment [30], melatonin treatment [31], and apple polyphenol treatment [32], the Liu Li 2 Ha variety still exhibited a lower browning index and better storage performance during th same time period. Moreover, the results from the stepwise multiple regression analys indicated that the strength of Liu Li 2 Hao lies in the fact that it can maintain a higher lev of total soluble solids and pericarp thickness and lower relative conductivity during room temperature storage. In addition, Dong Long Mi Li showed the worst storability at room temperature. The primary reason for this discrepancy may be attributed to its lower lev of pericarp thickness and higher relative conductivity (Figures 2 and 4). The classificatio results of the different litchi fruit varieties obtained in this study were generally consisten with the conventional understanding of their storability. As a result, these findings coul serve as a foundation for selecting suitable litchi breeding parents.

Impact Factors for Pericarp Browning
Under the conditions of postharvest storage at room temperature, in addition to th apparent indicators of fruit, the quality and corresponding physiological changes of th fruit should be the secondary key indicators that need to be focused on. The overall tren of total soluble solids in the fruit of 50 litchi varieties showed a significant decrease, ind

Impact Factors for Pericarp Browning
Under the conditions of postharvest storage at room temperature, in addition to the apparent indicators of fruit, the quality and corresponding physiological changes of the fruit should be the secondary key indicators that need to be focused on. The overall trend of total soluble solids in the fruit of 50 litchi varieties showed a significant decrease, indicating a decrease in edible quality [33]. The titratable acidity of litchi fruits also showed a similar trend, mainly due to the aging and oxidation reactions of the fruit during postharvest storage [34,35]. The accumulation of reactive oxygen species (ROS) during fruit storage reduces the storage quality of litchi fruit. Vc, usually as an antioxidant, can prevent plants from oxidative damage [36]. The significant increase in Vc content in litchi fruit on the ninth day may be related to the plant's self-regulation mechanism. The above indicators affected the color of the litchi pericarp to a great extent, thus affecting the commercial value.
Furthermore, the accumulation of ROS depends on the plant's antioxidant system [37]. As a result, POD has the ability to effectively regulate ROS concentrations, preventing ROS damage [38,39]. Despite its exclusion through component analysis and clustering analysis, its role in antioxidant defense is worth discussing. The results of this study suggest that the activity of POD in litchi fruit remains stable and does not show a significant increase or decrease with prolonged storage time at room temperature, indicating that litchi fruit tissue maintains a certain degree of antioxidant activity at normal temperature and does not lose its protein function, which also contributes to the prolongation of litchi storage time. Additionally, the color of the litchi fruit pericarp is due to the abundant anthocyanins present [40]. Polyphenol oxidase (PPO) is an enzyme highly correlated with the browning of fruit pericarp, which forms brown polymers through the oxidation of phenolic compounds, flavonoids, and ascorbic acid substrates in the pericarp, resulting in pericarp browning [40]. In addition, it is noteworthy that compared with PPO, laccase has a wider substrate range [41] and stronger oxidation characteristics for phenolic substances [40]. The results showed that the laccase activity gradually increased under normal temperature storage conditions (Figure 4), which kept the anthocyanin in plant tissue at a low level and caused the litchi fruit browning. In addition, the integrity of the fruit tissue cell membrane system is closely related to its browning degree and decay rate [42]. In this study, the relative conductivity of 50 litchi varieties increased significantly from the seventh day (Figure 4), resulting in the severe browning of litchi fruit at that time ( Figure 2). This result may be explained by the fact that the damage of cell membranes during the postharvest storage of litchi fruit may lead to the direct contact of enzymes and phenolic substrates to produce brown or brown substances, causing fruit browning. A stepwise multiple regression analysis can also confirm these discussions. Based on the results, the following conclusion can be drawn: among the 50 litchi varieties, Liu Li 2 Hao has the best storage capacity, mainly due to lower relative conductivity and lower POD and laccase activities.

Evaluation Model for Pericarp Browning
In this study, principal component analysis was used to condense a vast number of interrelated traits into a limited number of principal factor trait groups to replicate the correlation between the primary traits and the principal factor groups [43][44][45]. In summary, the results show that relative conductivity, pericarp thickness, and fruit quality are responsible for the browning of litchi fruit at room temperature and all changes that could cause the browning or decay of the pericarp. Specifically on the index of relative conductivity, the result showed that the pericarp relative conductivity had the strongest positive correlation with the fruit browning index and decay rate ( Figure 5) and had the highest contribution rate to fruit browning and decay (Table 4). These results were in accord with recent studies indicating that the maintenance of membrane integrity is the key issue in prolonging the shelf life of litchi fruit [6]. After constructing a browning index evaluation model using the stepwise regression method, all predictors in the model were found to be highly representative and originating from different common factors. There was high credibility in the calculated theoretical values, which were consistent with the measured values. The effective index selected to explain browning had a high credibility of 82%. According to linear regression analysis, the higher levels of total soluble solids, pericarp thickness, L*, a*, and Vc, as well as lower relative conductivity and lower laccase activity, were conducive to improving fruit browning resistance.

The Application of the Linear Regression Models
The linear regression models in this study presented several advantages. In this study, the indicators of the evaluation models were the conventional physical and chemical indices of litchi storage, which was simple and easy to obtain, and the features extracted from the evaluation model were conducive to simplifying the types of indicators. The seven traits obtained from the integration and screening by principal component analysis, cluster analysis, and stepwise regression analysis can reflect more information and can be used as the main form of future litchi browning evaluation. The greatest strength of this model is that the models more accurately evaluate the storability of the fruit and avoid errors caused by subjective evaluation. Furthermore, based on the senescence characteristics of litchi fruit at room temperature, the model can be used to determine the objective of senescence regulation according to the characteristics of different varieties and to design personalized fresh-keeping technology and storage methods to extend the postharvest life of fruits as much as possible. Additionally, this study provides new insights into the genetic breeding of litchi germplasm resources. The model can be used to select parameters suitable for breeders, growers, and processors and objectively quantify the quality differences between cultivars with breeding lines. For the different varieties or sources of fruit, researchers only need to measure the relevant characteristic indices during storage and use the predictive model to calculate the browning index and decay rate. The indicators in this study can be used not only as evaluation indicators of litchi storage tolerance but also for litchi breeding patents and the natural hybridization of progeny selection. Additionally, we measured the browning degree and decay rate of 50 litchi varieties and screened out the most storable litchi variety at room temperature, Liu Li 2 Hao, and the more storable litchi varieties Wu Jun 2 Hao, Shang Shu Huai, Qiong Shan 31 Hao, Zu Shan 4 Hao, Jian Ye Li, Jing Xing, Hai Guo 4 Hao, Xue Huai Zi, Jia Yuan Mi Li, Zhuang Yuan 1 Hao, Cheng Tuo, Huai Zhi, and Yuan Duan Li. The practical significance of this study is obvious; in Guangxi, for example, more than 90% of litchi planting is small retail planting. Most fruit farmers do not know how to prolong the storage time of fruit after harvest, leading to the problem of "high yield and slow sales". Choosing a more storage-tolerant litchi variety can alleviate this phenomenon to some extent. The selection of litchi varieties that are more resistant to storage at normal temperatures and the combination of fresh-keeping treatment technology can further extend the shelf life of fruits and effectively avoid waste.

Conclusions
The senescence and deterioration of harvested litchi fruits are rapidly reflected on pericarp browning and disease development. The browning index of 50 litchi varieties is significantly decreased and the decay rate significantly increased during storage at room temperature. In addition, storage at room temperature caused a series of changes in the appearance index, physiological index, and quality index of litchi fruit. We screened out the most storage-resistant litchi variety, Liu Li 2 Hao, using principal component analysis and cluster analysis. The stepwise multiple regression analysis further confirmed that relative conductivity, laccase activity, Vc content, pericarp thickness, total soluble solids, and a* and L* total soluble solids can be used as comprehensive evaluation factors to predict fruit decay rates and browning indices in litchi. The most important significance to emerge from this study is that the characteristic extracted from the liner regression model contributes to simplifying the indicator types, which contribute to predicting the browning index and decay rate by only measuring the appearance-quality-related indicators of fruits during storage. The main strength of this study is that the relevant characteristic indices during storage can be used in the predictive model to calculate the browning index and decay rate and provide guidance for the selection of the varieties of litchi planting and the development of litchi postharvest preservation technology. With regard to the research methods, some limitations need to be acknowledged, namely, the model needs to be further validated and optimized through numerous experiments. Therefore, further studies could evaluate the limitations.