Copper Amine Oxidase (CuAO)-Mediated Polyamine Catabolism Plays Potential Roles in Sweet Cherry (Prunus avium L.) Fruit Development and Ripening

Copper amine oxidases (CuAOs) play important roles in PA catabolism, plant growth and development, and abiotic stress response. In order to better understand how PA affects cherry fruit, four potential PavCuAO genes (PavCuAO1–PavCuAO4) that are dispersed over two chromosomes were identified in the sweet cherry genome. Based on phylogenetic analysis, they were classified into three subclasses. RNA-seq analysis showed that the PavCuAO genes were tissue-specific and mostly highly expressed in flowers and young leaves. Many cis-elements associated with phytohormones and stress responses were predicted in the 2 kb upstream region of the promoter. The PavCuAOs transcript levels were increased in response to abscisic acid (ABA) and gibberellin 3 (GA3) treatments, as well as abiotic stresses (NaCl, PEG, and cold). Quantitative fluorescence analysis and high-performance liquid chromatography confirmed that the Put content fell, and the PavCuAO4 mRNA level rose as the sweet cherry fruit ripened. After genetically transforming Arabidopsis with PavCuAO4, the Put content in transgenic plants decreased significantly, and the expression of the ABA synthesis gene NCED was also significantly increased. At the same time, excessive H2O2 was produced in PavCuAO4 transiently expressed tobacco leaves. The above results strongly proved that PavCuAO4 can decompose Put and may promote fruit ripening by increasing the content of ABA and H2O2 while suppressing total free PA levels in the fruit.


Introduction
Polyamine (PA) is a class of plant growth regulators that are involved in the entire process of plant development, from germination to senescence. The common types of PA are putrescine (Put), spermidine (Spd), and spermine (Spm). The catabolic pathways of PA are mainly mediated by diamine oxidase (DAO) and polyamine oxidase (PAO). In plants, the CuAO can be divided into two groups depending on subcellular localization: the first group is situated in peroxisomes, based on peroxisomal targeting signals, and the other group is located extracellularly, based on N-terminal signal peptides [1]. It has been shown that members of CuAO located to the peroxisome and extracellular compartments are found in several species, including Arabidopsis [2], apple [3], and sweet orange [1]. In most cases, Put can be catabolized by CuAO [4], but Put and Spd can be catalyzed by CuAO in Arabidopsis [2]. However, PAO are involved in the terminal catabolism of Spd and Spm. At the initiation of fruit growth, PA content is at maximum, and it declines as the fruit matures and senescence occurs. Adding exogenous PA or increasing endogenous PA through genetic engineering can effectively delay fruit ripening and senescence [5,6]. Recent reports indicate that the silencing of PpCuAO4 in peach can inhibit Put degradation, slow down  43 5 The corresponding gene structure pattern was obtained by comparing the DNA sequence of the PavCuAO gene with the CDS sequence ( Figure 1). PavCuAO1 and PavCuAO2 had the same gene structure, with 5 exons and 4 introns, respectively, while PavCuAO3 and PavCuAO4 genes both had 4 exons and 3 introns. Unlike other genes, the PavCuAO3 gene only had a 3 untranslated region and no 5 untranslated region structure.
AtNCED was significantly elevated, revealing that PavCuAO4-mediated PA meta might enhance ABA biosynthesis. Our study provided further insight into the PavCuAOs in the catabolism of PAs and fruit ripening.

Identification and Gene Structure Analysis of PavCuAOs
A total of four possible CuAO genes were identified in sweet cherry and PavCuAO1-4 ( Table 1). The ORF length of the four genes ranged from 1944 bp (PavC to 2181 bp (PavCuAO4), with isoelectric points ranging from 5.7 (PavCuAO4) (PavCuAO3) and molecular weights of 72.38 kDa (PavCuAO3) to 81.43 kDa (PavCu All the proteins of the four PavCuAOs were non-hydrophobic proteins, PavCuAO1all localized to chromosome 1, and PavCuAO4 was localized to chromosome 5.  43 5 The corresponding gene structure pattern was obtained by comparing the DN quence of the PavCuAO gene with the CDS sequence ( Figure 1). PavCuAO1 and PavC had the same gene structure, with 5 exons and 4 introns, respectively, while PavC and PavCuAO4 genes both had 4 exons and 3 introns. Unlike other genes, the PavC gene only had a 3' untranslated region and no 5' untranslated region structure.

PavCuAOs Promoter Analysis
Using the online website Plantcare to analyze the promoter of the PavCuAO ge the cis-acting elements of its upstream 2000 bp sequence (Figure 2), we identified response elements in the PavCuAOs promoter that are associated with phytohor and stresses of adversity. The analysis revealed that all PavCuAO genes contained responsive element, anaerobic induction element, and auxin-responsive element, w light-responsive element being the most prevalent. The gibberellin-responsive, A sponsive, and defense-and stress-responsive elements were identified in the reg the PavCuAO1, PavCuAO2, and PavCuAO3 promoters. The promoters of PavCuAO PavCuAO2 also had MeJA-responsive elements, and the PavCuAO2 and PavCuAO moters contained salicylic acid-responsive elements. In addition, PavCuAO4 may volved in low-temperature and wound stress.

PavCuAOs Promoter Analysis
Using the online website Plantcare to analyze the promoter of the PavCuAO gene and the cis-acting elements of its upstream 2000 bp sequence (Figure 2), we identified many response elements in the PavCuAOs promoter that are associated with phytohormones and stresses of adversity. The analysis revealed that all PavCuAO genes contained lightresponsive element, anaerobic induction element, and auxin-responsive element, with the light-responsive element being the most prevalent. The gibberellin-responsive, ABAresponsive, and defense-and stress-responsive elements were identified in the regions of the PavCuAO1, PavCuAO2, and PavCuAO3 promoters. The promoters of PavCuAO1 and PavCuAO2 also had MeJA-responsive elements, and the PavCuAO2 and PavCuAO3 promoters contained salicylic acid-responsive elements. In addition, PavCuAO4 may be involved in low-temperature and wound stress.

PavCuAOs Protein Multiplex Sequence Alignment and Phylogenetic Analysis
The results of the protein sequence alignment for the PavCuAOs revealed that the protein sequences of the group's members were highly conserved ( Figure 3), with PavCuAO1 and PavCuAO2 sharing the maximum similarity (69.79%) and PavCuAO2 and PavCuAO4 having the lowest similarity (46.88%). According to the phylogenetic analysis, the PavCuAO genes were found to be divided into three classes. Among them, PavCuAO1 and PavCuAO2 were clustered into class III, and PavCuAO3 and PavCuAO4 were clustered into class II and class I, respectively. The result of the phylogenetic analysis showed that PavCuAOs and PpeCuAOs were closer ( Figure 4).

PavCuAOs Protein Multiplex Sequence Alignment and Phylogenetic Analysis
The results of the protein sequence alignment for the PavCuAOs revealed that the protein sequences of the group's members were highly conserved ( Figure 3), with PavCuAO1 and PavCuAO2 sharing the maximum similarity (69.79%) and PavCuAO2 and PavCuAO4 having the lowest similarity (46.88%). According to the phylogenetic analysis, the PavCuAO genes were found to be divided into three classes. Among them, PavCuAO1 and PavCuAO2 were clustered into class III, and PavCuAO3 and PavCuAO4 were clustered into class II and class I, respectively. The result of the phylogenetic analysis showed that PavCuAOs and PpeCuAOs were closer ( Figure 4).  I  S  T   S  F  L  R   F  I  I  R   F  T  L  L   T  F  Q  R   F  S  C  D   S  P  C  H   P  A  F  A   T  L  T  S   T  C  A  D   S  L  S  T   S  K  T  P   H  Q  S  H  h   H  H  H  H  p   P  P  P  P  l   L  L  L  L  d   D  D  D  D   P  P  T  P  l   L  L  L  L   T  T  N  T   108  PavCuAO1  113  PavCuAO2  106  PavCuAO3 154 PavCuAO4 Consensus

Expression Analysis of PavCuAOs in Different Tissues and Fruits at Different Developmental Stages
The expression pattern of PavCuAO genes in different tissues of cherry (fruit, flower, stem, leaf) had obvious tissue specificity ( Figure 5). Among them, the expression of PavCuAO1 was the highest at the full flowering stage; PavCuAO2, PavCuAO3, and PavCuAO4 were expressed to the maximum in the pre-flowering buds, young leaves, and color-breaking fruits, respectively.

Expression Analysis of PavCuAOs in Different Tissues and Fruits at Different Developmental Stages
The expression pattern of PavCuAO genes in different tissues of cherry (fruit, flower, stem, leaf) had obvious tissue specificity ( Figure 5). Among them, the expression of PavCuAO1 was the highest at the full flowering stage; PavCuAO2, PavCuAO3, and PavCuAO4 were expressed to the maximum in the pre-flowering buds, young leaves, and color-breaking fruits, respectively.

Expression Analysis of PavCuAOs in Different Tissues and Fruits at Different Developmental Stages
The expression pattern of PavCuAO genes in different tissues of cherry (fruit, flower, stem, leaf) had obvious tissue specificity ( Figure 5). Among them, the expression of PavCuAO1 was the highest at the full flowering stage; PavCuAO2, PavCuAO3, and PavCuAO4 were expressed to the maximum in the pre-flowering buds, young leaves, and color-breaking fruits, respectively. The expression level of PavCuAO1 was low, and the change was not obvious in the fruit development stage. However, PavCuAO3 showed a slow downward trend from G1 to G4. The expression changes of PavCuAO2 and PavCuAO4 were identical, with the expression levels first rising and subsequently falling during the fruit ripening. The PavCuAO2 expression level gradually decreased after reaching the peak in G2, and the expression of PavCuAO4 first increased to the peak and then decreased in G3 ( Figure 5).

Expression Patterns of PavCuAO
Genes under ABA, GA 3, and Abiotic Stress (NaCl, PEG, and Cold) Treatments The expression levels of PavCuAOs under phytohormone treatment and abiotic stress were analyzed. After the ABA treatment ( Figure 6), PavCuAO1-4 all showed a clear tendency to rise and decrease with time, and PavCuAO1, PavCuAO3, and PavCuAO4 all reached a maximum at 3 h and then decreased. In contrast, PavCuAO2 showed a tendency to rise again after decreasing. After the GA 3 treatment, PavCuAO1, PavCuAO2, and PavCuAO3 all displayed the same trend of first increasing, then reducing, and finally increasing again ( Figure 6). Among them, PavCuAO1 and PavCuAO3 both reached the maximum at 2 h, and PavCuAO2 and PavCuAO4 peaked at 3 h. Unlike the remaining three genes, PavCuAO4 did not tend to rise again at 5 h. The expression level of PavCuAO1 was low, and the change was not obvious in the fruit development stage. However, PavCuAO3 showed a slow downward trend from G1 to G4. The expression changes of PavCuAO2 and PavCuAO4 were identical, with the expression levels first rising and subsequently falling during the fruit ripening. The PavCuAO2 expression level gradually decreased after reaching the peak in G2, and the expression of PavCuAO4 first increased to the peak and then decreased in G3 ( Figure 5).

Expression Patterns of PavCuAO Genes under ABA, GA3, and Abiotic Stress (NaCl, PEG, and Cold) Treatments
The expression levels of PavCuAOs under phytohormone treatment and abiotic stress were analyzed. After the ABA treatment ( Figure 6), PavCuAO1-4 all showed a clear tendency to rise and decrease with time, and PavCuAO1, PavCuAO3, and PavCuAO4 all reached a maximum at 3 h and then decreased. In contrast, PavCuAO2 showed a tendency to rise again after decreasing. After the GA3 treatment, PavCuAO1, PavCuAO2, and PavCuAO3 all displayed the same trend of first increasing, then reducing, and finally increasing again ( Figure 6). Among them, PavCuAO1 and PavCuAO3 both reached the maximum at 2 h, and PavCuAO2 and PavCuAO4 peaked at 3 h. Unlike the remaining three genes, PavCuAO4 did not tend to rise again at 5 h. After the NaCl stress treatment (Figure 7), the mRNA abundance of PavCuAO1 was only slightly changed, except for the induction at 4 h. Both PavCuAO1 and PavCuAO2 were up-regulated in expression, while there were no significant changes at 0 h and 8 h. In contrast, PavCuAO3 was not significantly induced throughout the stress. In contrast, PavCuAO4 showed significant down-regulation during this process and reached its lowest value at 8 h. After the NaCl stress treatment (Figure 7), the mRNA abundance of PavCuAO1 was only slightly changed, except for the induction at 4 h. Both PavCuAO1 and PavCuAO2 were up-regulated in expression, while there were no significant changes at 0 h and 8 h. In contrast, PavCuAO3 was not significantly induced throughout the stress. In contrast, PavCuAO4 showed significant down-regulation during this process and reached its lowest value at 8 h.
For the simulated drought conditions (Figure 7), the transcript levels of PavCuAO1 increased significantly at 4 h, with no significant changes at the remaining time points. PavCuAO2 showed a down-regulated trend, but the expression was up-regulated at 8 h. In contrast, both PavCuAO3 and PavCuAO4 showed a significant up-regulated expression trend; however, PavCuAO4 had a reduced transcript level compared to the beginning.
The expression levels of PavCuAO1-4 genes all changed significantly under cold treatment conditions (Figure 7), accompanied by different degrees of up-regulated expression. PavCuAO1, PavCuAO2, and PavCuAO3 all showed an overall increasing trend during cold treatment, while PavCuAO4 showed an overall decreasing trend until 3 d, and then showed a significantly up-regulated expression at 3 d.  For the simulated drought conditions (Figure 7), the transcript levels of PavCuAO1 increased significantly at 4 h, with no significant changes at the remaining time points. PavCuAO2 showed a down-regulated trend, but the expression was up-regulated at 8 h. In contrast, both PavCuAO3 and PavCuAO4 showed a significant up-regulated expression trend; however, PavCuAO4 had a reduced transcript level compared to the beginning.
The expression levels of PavCuAO1-4 genes all changed significantly under cold treatment conditions (Figure 7), accompanied by different degrees of up-regulated expression. PavCuAO1, PavCuAO2, and PavCuAO3 all showed an overall increasing trend during cold treatment, while PavCuAO4 showed an overall decreasing trend until 3 d, and then showed a significantly up-regulated expression at 3 d.

Detection of PA Content in the Ripening Process of Sweet Cherry Fruit
The content of PAs during fruit development was measured, and the results showed Put, Spd, and Spm were higher in the early stage of fruit development and decreased during the whole process. Spd and Spm decreased significantly from G2 to G3 and reached their lowest values in G4. However, the content of Put showed a stable trend after a sharp decrease from G2 to G3, while there was no significant difference between G3 and G4 ( Figure 8).
Put, Spd, and Spm were higher in the early stage of fruit development a during the whole process. Spd and Spm decreased significantly from G reached their lowest values in G4. However, the content of Put showed a sta a sharp decrease from G2 to G3, while there was no significant difference be G4 (Figure 8).

Genetic Transformation of Arabidopsis thaliana with PavCuAO4 and Detectio in Transgenic Plants
To understand the role of PavCuAOs in the catabolism of PAs, PavCuA highly expressed during fruit maturation and development, was selected f transformation of Arabidopsis thaliana. A total of six transgenic lines were the transcription levels of the PavCuAO4 gene in the transgenic line were analyzed. The results showed that the PavCuAO4 expression abundance w in OE2 and the lowest in OE5 (Figure 9). Moreover, the results of the determination of PA content in transgenic that Put content in OE5 plants was significantly lower than WT, while Spd tents were higher than those of WT. The content of PA in OE2 plants was no

Genetic Transformation of Arabidopsis thaliana with PavCuAO4 and Detection of Free PAs in Transgenic Plants
To understand the role of PavCuAOs in the catabolism of PAs, PavCuAO4, which is highly expressed during fruit maturation and development, was selected for the genetic transformation of Arabidopsis thaliana. A total of six transgenic lines were obtained, and the transcription levels of the PavCuAO4 gene in the transgenic line were subsequently analyzed. The results showed that the PavCuAO4 expression abundance was the highest in OE2 and the lowest in OE5 (Figure 9).
The content of PAs during fruit development was measured, and the results showed Put, Spd, and Spm were higher in the early stage of fruit development and decreased during the whole process. Spd and Spm decreased significantly from G2 to G3 and reached their lowest values in G4. However, the content of Put showed a stable trend after a sharp decrease from G2 to G3, while there was no significant difference between G3 and G4 ( Figure 8).

Genetic Transformation of Arabidopsis thaliana with PavCuAO4 and Detection of free PAs in Transgenic Plants
To understand the role of PavCuAOs in the catabolism of PAs, PavCuAO4, which is highly expressed during fruit maturation and development, was selected for the genetic transformation of Arabidopsis thaliana. A total of six transgenic lines were obtained, and the transcription levels of the PavCuAO4 gene in the transgenic line were subsequently analyzed. The results showed that the PavCuAO4 expression abundance was the highest in OE2 and the lowest in OE5 (Figure 9). Moreover, the results of the determination of PA content in transgenic lines showed that Put content in OE5 plants was significantly lower than WT, while Spd and Spm contents were higher than those of WT. The content of PA in OE2 plants was not significantly different from those in the WT. (Figure 10). Moreover, the results of the determination of PA content in transgenic lines showed that Put content in OE5 plants was significantly lower than WT, while Spd and Spm contents were higher than those of WT. The content of PA in OE2 plants was not significantly different from those in the WT. (Figure 10).

Expression Patterns of Genes Related to PA and ABA Synthesis in Overexpressed Plants
The transcript levels of genes related to PA and ABA synthesis showed that the expression of PA synthesis-related genes was not significantly different between the OE2 and WT lines. In comparison to WT, OE5 dramatically increased the transcript levels of AtADC1, AtADC2, and AtSPDS2, and AtSPDS1 expression levels were also enhanced. In addition, the expression level of the ABA synthesis gene AtNCED in OE5 was also significantly higher than that in WT ( Figure 11).

Expression Patterns of Genes Related to PA and ABA Synthesis in Overexpressed Plants
The transcript levels of genes related to PA and ABA synthesis showed that the expression of PA synthesis-related genes was not significantly different between the OE2 and WT lines. In comparison to WT, OE5 dramatically increased the transcript levels of AtADC1, AtADC2, and AtSPDS2, and AtSPDS1 expression levels were also enhanced. In addition, the expression level of the ABA synthesis gene AtNCED in OE5 was also significantly higher than that in WT ( Figure 11).

Expression Patterns of Genes Related to PA and ABA Synthesis in Overexpressed Plants
The transcript levels of genes related to PA and ABA synthesis showed that the expression of PA synthesis-related genes was not significantly different between the OE2 and WT lines. In comparison to WT, OE5 dramatically increased the transcript levels of AtADC1, AtADC2, and AtSPDS2, and AtSPDS1 expression levels were also enhanced. In addition, the expression level of the ABA synthesis gene AtNCED in OE5 was also significantly higher than that in WT ( Figure 11). Figure 11. Transcription levels of PA and ABA synthesis genes in overexpressed plants. Figure 11. Transcription levels of PA and ABA synthesis genes in overexpressed plants.

H 2 O 2 In Situ Histochemical Staining
The H 2 O 2 content was analyzed by DAB staining. The results showed that the leaves on the injected side of the PavCuAO4 gene were darker, indicating that PavCuAO4 accumulated more H 2 O 2 while decomposing polyamines (Figure 12).

H2O2 In Situ Histochemical Staining
The H2O2 content was analyzed by DAB staining. The results showed that the leaves on the injected side of the PavCuAO4 gene were darker, indicating that PavCuAO4 accumulated more H2O2 while decomposing polyamines (Figure 12).

Discussion
The catabolism of PA is mainly catalyzed by PAO and CuAO genes. At present, there are few reports on the regulation of fruit ripening by CuAO-mediated PA metabolism in sweet cherry. Currently, the most research on CuAOs is being conducted in Arabidopsis [28,29] [28,29], followed by studies on grape [25], apple [3], tomato [30], sweet orange [1], strawberry [26], and peach [31], all of which have also been reported successively. During the rapid growth and ripening stages of tomato fruit, transcription levels related to PA biosynthesis and catabolism genes were highly expressed [30]. In peach, PpCuAO4-mediated Put catabolism can induce fruit ripening [31]. After peaches were treated with PA catabolism inhibitors, the fruit appeared to take longer to mature and soften, and less ABA, ethylene, and cell wall-related gene expression were seen [14].
In this study, four PavCuAO genes were identified through the sweet cherry genome, and phylogenetic analysis revealed that PavCuAOs and PpeCuAOs were the closest relatives. Analysis of the transcript levels of PavCuAOs in different tissues and at different stages of fruit development showed that PavCuAOs genes were significantly tissue-specific, a result that was consistent with those in peach and sweet orange [1,32] [1,32], implying that PavCuAOs may function in different tissues. PavCuAO1 and PavCuAO3 were highly expressed in flowers and young leaves, whereas PavCuAO2 and PavCuAO4 had high transcription levels in fruits, flowers, and young leaves, suggesting that PavCuAOs may regulate the development of multiple organs. Both PavCuAO4 and PavCuAO2 displayed the same trend of change during fruit development, indicating the possibility that they may, to some extent, play the same regulatory role in fruit growth, although more research is required to confirm findings. Furthermore, PA catabolism can be induced by hormonal and biological stress responses [9], and in Arabidopsis, Put oxidation by At-CuAOγ1 induced a ROS-dependent SA signaling pathway, which in turn, initiated defense systems in plants [33]. In response to ABA and GA3, we identified that the genes for PavCuAO1-4 were significantly upregulated, indicating that PavCuAOs were implicated in these responses. In addition, most PavCuAO genes were induced by NaCl, PEG, and cold treatments, indicating their ability to function in different stress conditions.
Numerous studies have shown that as the fruit ripens, the PA concentration falls [30,34] [30,34]. In our study, the Put, Spd, and Spm content of sweet cherry fruit decreased significantly in the G2 and G3 stages. Several studies have indicated that CuAO decomposes Put and cadaverine (Cad), albeit less effectively than Spm and Spm [35]. The results of the transgenic plants in this study showed that the Put content of OE5 was significantly lower than that of WT, so PavCuAO4 had the function of catabolism of Put. Ethylene

Discussion
The catabolism of PA is mainly catalyzed by PAO and CuAO genes. At present, there are few reports on the regulation of fruit ripening by CuAO-mediated PA metabolism in sweet cherry. Currently, the most research on CuAOs is being conducted in Arabidopsis [28,29], followed by studies on grape [25], apple [3], tomato [30], sweet orange [1], strawberry [26], and peach [31], all of which have also been reported successively. During the rapid growth and ripening stages of tomato fruit, transcription levels related to PA biosynthesis and catabolism genes were highly expressed [30]. In peach, PpCuAO4mediated Put catabolism can induce fruit ripening [31]. After peaches were treated with PA catabolism inhibitors, the fruit appeared to take longer to mature and soften, and less ABA, ethylene, and cell wall-related gene expression were seen [14].
In this study, four PavCuAO genes were identified through the sweet cherry genome, and phylogenetic analysis revealed that PavCuAOs and PpeCuAOs were the closest relatives. Analysis of the transcript levels of PavCuAOs in different tissues and at different stages of fruit development showed that PavCuAOs genes were significantly tissue-specific, a result that was consistent with those in peach and sweet orange [1,32], implying that PavCuAOs may function in different tissues. PavCuAO1 and PavCuAO3 were highly expressed in flowers and young leaves, whereas PavCuAO2 and PavCuAO4 had high transcription levels in fruits, flowers, and young leaves, suggesting that PavCuAOs may regulate the development of multiple organs. Both PavCuAO4 and PavCuAO2 displayed the same trend of change during fruit development, indicating the possibility that they may, to some extent, play the same regulatory role in fruit growth, although more research is required to confirm findings. Furthermore, PA catabolism can be induced by hormonal and biological stress responses [9], and in Arabidopsis, Put oxidation by AtCuAOγ1 induced a ROS-dependent SA signaling pathway, which in turn, initiated defense systems in plants [33]. In response to ABA and GA 3 , we identified that the genes for PavCuAO1-4 were significantly upregulated, indicating that PavCuAOs were implicated in these responses. In addition, most PavCuAO genes were induced by NaCl, PEG, and cold treatments, indicating their ability to function in different stress conditions.
Numerous studies have shown that as the fruit ripens, the PA concentration falls [30,34]. In our study, the Put, Spd, and Spm content of sweet cherry fruit decreased significantly in the G2 and G3 stages. Several studies have indicated that CuAO decomposes Put and cadaverine (Cad), albeit less effectively than Spm and Spm [35]. The results of the transgenic plants in this study showed that the Put content of OE5 was significantly lower than that of WT, so PavCuAO4 had the function of catabolism of Put. Ethylene induces climacteric fruit ripening, while the regulation of non-climacteric fruit ripening is mainly dominated by ABA [18,20,36]. PA metabolism affects the regulation of various phytohormones such as ABA and ethylene [7], while in most cases, Put and ABA have a positive feedback mechanism that promotes each other's synthesis [37,38]. The expression of AtNCED in overexpressing plants OE5 was significantly higher than that in WT. The results showed that PavCuAO4 could promote ABA synthesis, and PavCuAO4 synthesis was enhanced in the stage of fruit development, thereby promoting ABA synthesis. As per previous studies, CuAO-derived H 2 O 2 may also function as a signaling chemical to speed up the ripening of fruit [38], and H 2 O 2 is essential for ABA-mediated stomatal closure [39]. Furthermore, CuAO has been shown to indirectly alter NO levels by oxidizing PA to produce H 2 O 2 to affect plant development [40], while NO and ABA can also regulate the fruit-ripening senescence process [41,42]. By using a transient expression system to inject PavCuAO4 into tobacco leaves and measuring the H 2 O 2 content using DAB staining, we were able to see that the gene-injected side had a deeper color than the empty side, which meant that PavCuAO4 had acquired more H 2 O 2 throughout the process.
During tomato development, Put content gradually rose to its peak at ripening, while Spd and Spm content declined to their respective lowest levels at this time, resulting in a reduction in the amount of total free PA in the fruit [30]. As the sweet cherry fruit ripened, the concentration of Spd and Spm decreased, which was comparable with the findings for tomato. Elevated PA content was linked to the delayed fruit ripening caused by jasmonic acid in peach fruit [43], whereas transgenic tomato leaves and ripe fruits had increased Spd content but no rise in Spm level, greatly delaying overall fruit ripening and nutritional maturity [6]. The Spm and Spd contents of transgenic plant OE5 were higher than that of WT. In particular, the Spd content was significantly higher than in WT. To explain the increased Spm and Spd contents in transgenic lines, we further analyzed the expression of PA synthesis genes in transgenic lines. The results showed that the expression of AtADC1, AtADC2, AtSPDS1, and AtSPDS2 were higher in OE5 than in WT. Therefore, the genetic transformation of PavCuAO4 enhanced PA synthesis in transgenic lines, and the Spm and Spd contents increased. While the enhanced Put synthesis was also decomposed by the overexpressed PavCuAO4, its content decreased. However, for some reason, the Spm and Spd content decreased during fruit ripening, while PavCuAO4 decomposed the Put, thus reducing the total PA content in the fruit and facilitating fruit ripening. Further evidence that PA catabolism is the primary reason for the decrease in PA content during ripening originated from the upregulation of CuAO and PAO transcriptional levels during grape ripening [7]. Therefore, high levels of Spd and Spm content during fruit development may be detrimental to ripening.
Based on the reported role of PAs in fruit ripening [25,31], and by preventing fruit respiration and thus delaying the loss of soluble solids and titratable acids of fruit hardness, the PA pretreatment can enhance the storage quality of grapes [5]. Similarly, PA treatment of blueberries can also improve quality and extend storage time [44]. The PavCuAO4-mediated PA catabolism can promote fruit ripening, and it can also increase fruit PA accumulation and delay ripening senescence by external application of PAs. This study provides a new theoretical basis for the relationship between PAs and fruit ripening, and also provides new theoretical guidance for fruit breeding and regulation of fruit marketing.

Materials
The experimental materials were collected from a 5-year-old sweet cherry plantation in the Baiyi District, Guizhou Province. The plantation was managed under regular field management. The different tissue samples included fruit (G1 for young fruit, G2 for medium fruit, G3 for color-breaking fruit, and G4 for ripe fruit), flower buds (H1: dormant bud; H2: pre-flowering bud; H3: bellflower; H4: blooming flower), leaves (Y1: young leaf; Y2: mature leaf), and stems (J1). The samples were stored in liquid nitrogen and brought back to store at −80 • C. Five-year-old sweet cherry trees in good growth condition and with healthy branches from the same parts were collected. For NaCl treatment, branches were immersed in 100 mM NaCl solution and leaves were collected at 0, 2, 4, 6, and 8 h after treatment. For cold treatment, branches were inserted into culture bottles containing water and placed in an artificial climate chamber, with a photoperiod set to 14 h of light/10 h of darkness and a temperature set to 4 • C. Samples were taken at 0, 1, 3, 6, 12, 24, 48, and 72 h after treatment. For drought treatment, branches were immersed in 20% PEG 6000 and sampled at 0, 2, 4, 6, and 8 h after treatment. For hormone treatment, cherry leaves were sprayed with 100 mg/L of ABA and GA 3 , at a dosage of 10 mL per branch, and sampled after 0, 1, 2, 3, 4, and 5 h. All treatments were collected from the leaves and stored at −80 • C. The above experiments were set up with three biological replicates.

Determination of PA in Sweet Cherry Fruit and Transgenic Plants
Cherry fruits and leaves of transgenic and wild-type plants were collected to detect PA content. The steps were as follows: grind the material to a powder using liquid nitrogen and weigh 0.5 g of the sample in a 10 mL centrifuge tube; add 1.5 mL of pre-cooled perchloric acid, shake well and mix, then put it into the refrigerator at 4 • C for 1 h; then centrifuge at 4 • C, 15,000 rpm for 30 min; take 1 mL of supernatant and add 10 µL of benzoyl chloride and 1 mL of 2 mol/L sodium hydroxide and mix well, then put it into the water bath at 37 • C for 30 min; add 2 mL of saturated sodium chloride and 2 mL of ether and mix well and centrifuge at 6000 rpm for 5 min; take 2 mL of ether phase, blow dry with a nitrogen blowing instrument; add 2 mL of ether, shake well, and centrifuge for 20 s, then blow dry with nitrogen; add 1000 µL of 60% methanol and shake centrifuge for 30 s; and filter with a 0.45 µm organic filter membrane and fix the volume in a 1.5 mL brown volumetric flask for testing. The determination of polyamines was performed by a high-performance liquid chromatograph (Agilent 1260, Agilent, American) on a chromatographic column (Nova-Pak C18, WATERS, American) with the mobile phase of methanol: water (60:40) at a flow rate of 1 mL·min −1 , column temperature of 30 • C, a wavelength of 254 nm, and experiments were set up with three biological replicates.

Identification of PavCuAO Gene Family Members
Based on the CuAO HMM model (PF01179) in the Pfam database, the CuAO family members of sweet cherry were identified as candidate genes from the whole sweet cherry genome using HMMER3. Then, the Conserved Domain Database of NCBI was used to identify conserved structural domains, and genes containing the structural domain of CuAO were retained. Referring to the method in the reference [45], the evolutionary tree construction and kinship analysis were performed using the maximum likelihood method in MEGA, multiplex protein sequence alignment was performed using DNAman, and gene structure and chromosomal localization were analyzed using TBtools [46]. The cis-acting elements of the promoter were predicted using the PlantCARE online website (http://bioinformatics.psb.ugent.be/webtools/plantcare/html/ (accessed on 10 August 2022)) and mapped using TBtools. Isoelectric points and relative molecular masses were calculated using ExPasy (https://web.exasy.org/protparam/ (accessed on 6 August 2022)).

Gene Expression Analysis
Total RNA was extracted from different tissues, treated samples, and transgenic plants, according to the RNA extraction kit method (SENO, Zhangjiakou, China), and the concentration and purity of the extracted RNA were measured by a spectrophotometer. The cDNA was then synthesized using the RevertAid First Strand cDNA Synthesis Kit (Thermo, Waltham, MA, USA) (see instructions for details) and stored at −80 • C for backup. The PA and ABA synthesis genes (AtADC1, AtADC2, AtSPDS1, AtSPDS2, AtSPMS, and AtNCED) from KEGG and the Arabidopsis Tair database were selected for expression analysis of transgenic Arabidopsis thaliana. PavCuAO1-4 primers were designed by Primer Premier 5, and the PavEF gene was selected as the internal reference gene [47]. The relative expression was calculated by the 2 −∆Ct method [48]. The qPCR system was a 10 µL system, including 5 µL SYBR ® Premix Ex Taq™ II (Bemix, Dongguan, China), 2 µL diluted cDNA, 2 µL ddH 2 O, and 0.5 µL of each primer. They were performed on the qTOWER3G (Analytikjena, Jena, Germany). The reaction procedure was 50 • C for 5 min, 94 • C for 3 min, followed by 94 • C for 20 s and 60 • C for 30 s. Thirty-nine cycles were set up, with three technical replicates for each sample. The gene name and primers were listed in Supplementary Table S1.

Genetic Transformation and Transient Expression
The plant expression vector was selected as pCambia1301-35s-GFP, as shown in Supplementary Figure S1, using the Nco I and Xba I double digestion vector. According to the kit (Ready-to-Use Seamless Cloning Kit, NO. B632219, Sangon Biotech, Shanghai, China) protocol, the ORF full length of PavCuAO3 was cloned, and the recombinant expression vector was constructed using the seamless cloning method.
Thereafter, Arabidopsis thaliana was transformed using the inflorescence infestation approach utilizing the recombinant vector pCambia1301-35s-PavCuAO4, and the transformed seeds were harvested once they had reached maturity. The seeds were spread on MS plates containing thaumatin to screen transgenic plants and identified using PCR. Finally, the transgenic plants were transplanted into soil, and T3 generation transgenic plants were used for subsequent experimental analysis. The primers for gene clone and transgenic line identification are listed in Table S1. In addition, the bacterial solution was injected into tobacco leaves for transient expression, the trans-null was injected as control, and the treated tobacco H 2 O 2 staining reference [49], with slight modifications, was performed as follows: the injected tobacco leaves were immersed in the configured diaminobenzidine (DAB) solution, sealed and placed in an 80 rpm shaker overnight, and then the DAB staining solution was replaced with a bleach solution (ethanol:acetic acid:glycerol = 3:1:1) and placed in boiling water. Following the removal of the chlorophyll in a water bath and changing the bleach solution multiple times to turn the leaves white, the brown precipitate left over from the reaction of DAB and hydrogen peroxide was then photographed against a white background.

Data Analysis
T-tests were performed with SPSS 21.0 software (Chicago, IL, USA) and plotted with Origin 9.0 (Northampton, MA, USA).

Conclusions
In summary, a total of four possible CuAO genes (PavCuAO1-4) were identified in sweet cherry. The majority of PavCuAOs was induced by ABA, GA 3 , and abiotic stress (NaCl, PEG, cold) treatments. The PA content of transgenic plants and transient expression analysis showed that PavCuAO4 was involved in Put catabolism, and it may also promote fruit ripening by increasing ABA and H 2 O 2 content and reducing the total free PA content in the fruit. This data provides a strong basis for understanding the role of the CuAO gene in sweet cherry development, but further experiments are needed to understand its specific role.