Plant materials and treatments

Cherry tomatoes (Lycopersicon esculentum var. cerasiforme ‘XinTaiyang’) were planted in standard culture greenhouses (20–25°C, relative humidity (RH) 70%-85%) of Transfar Agriculture Co Ltd (Xiaoshan, Zhejiang, China). Fruits were harvested at mature green (MG) stage and transported to the laboratory immediately. 600 fruits with uniform size and free from blemishes were selected, and randomly divided into three groups. For each group, either 25 μL of ABA (10 mM) aqueous solution, or NDGA (1 mM) aqueous solution, or distilled water (control) was injected into each fruit from the pedicle with the same depth by microsyringe, respectively. The injection method and chemical concentration were chosen based on preliminary experiments. Fruits were stored at 20°C (90% RH) in the dark for 18 days. Samples of the 9^th day which showed the most observable differences in progress of ripening among three groups were chosen for RNA sequencing. For sampling, fruit calyx and seed were removed, and the pericarps were flash-frozen in liquid nitrogen and stored at -80°C before RNA extraction.

Measurement of Fruit Color and Firmness

Ten fruits per replicate of each treatment were used to determine surface color and firmness, respectively. L*, a*, b* were recorded by a Chroma meter (KONICA MINOLTA, CR-400, Japan), of which, a* was used to depict fruit color variation. Fruits’ firmness was assessed with a digital texture analyzer (TA-XT2i, Stable Micro Systems Ltd.; Godalmin, UK) with a 5 mm diameter probe. The maximum force (N) was recorded during the fruit being penetrated 10 mm at a rate of 1mm/s, and four different points around the equator of the fruit were tested on each fruit. All analyses were conducted in three replicates.

Pigments Quantification

The content of total carotenoids and chlorophyll was measured according to Zhu et al. with a slight modification [34]. Pericarp tissue (1 g) was extracted with 10 ml of 60: 40% (v/v) hexane: acetone at 4°C for 24 h in the dark and then centrifuged at 12000 × g 4°C for 20 min. The optical absorbance of supernatant was measured at 663, 647 and 450 nm against a hexane blank using a UV-VIS spectrophotometer (UV-1750, SHIMADZU, Japan). The total chlorophyll and carotenoids content were calculated with the following equations: total chlorophyll (mg ml^-1) = 8.02 (OD₆₄₃) + 20.2 (OD₆₄₇) and total carotenoids content (mg ml^-1) = (OD₄₅₀)/0.25.

The assay of lycopene and β-carotene contents were conducted by HPLC based on the method of Ronen et al. with minor modifications [35]. Pericarp tissue (1 g) was homogenized with 10 mL cold acetone and incubated in the dark overnight. After centrifugation, the supernatant was collected and then filtered through a 0.45 μm filter. Carotenoids were separated by reverse-phase HPLC using a Zorbax SB-C18 column (silica 5 μm, 4.6 mm × 250 mm) (Agilent, USA). Sample of 20 μL was injected into a Shimadzo LC2012A pump (Shimadzo Corp., Tokyo, Japan). The mobile phase was consisted of acetonitrile: H₂O (9: 1) (solvent A) and 100% ethyl acetate (solvent B), and was used in a linear gradient between A and B for 30 min with a flow of 1 ml min^-1. Lycopene and β-carotene contents were detected at a wavelength of 475 nm. The external standard method was used for quantification.

mRNA-seq Library Construction for Illumina Sequencing

Total RNA extraction, mRNA purification, and cDNA library construction were conducted by LC-BIO (Hangzhou, China). Total RNA samples were prepared using the Total RNA Purification Kit, TRK1001 (LC Science, Houston, TX), treated with RNase-free DNase I following the manufacturer's procedure to remove contaminated genomic DNA. For each group, total RNA was extracted from 10 randomly selected fruits. Then the quantity and purity of total RNA were analyzed with Bioanalyzer 2100 and RNA 6000 Nano LabChip Kit (Agilent, CA, USA). For each treatment sample, equal quantities of high-quality RNA from 10 fruits were pooled for cDNA library construction.

The poly (A) messenger RNA was isolated from the total RNA samples with oligo (dT) attached magnetic beads (Invitrogen). The mRNA was fragmented into short fragments using divalent cations under elevated temperature. The cleaved RNA fragments were reverse-transcribed to the first-strand cDNAs by random hexamer primers. Then the second-strand cDNAs were synthesized to construct the final cDNA library according to the instruction of mRNA-Seq sample preparation kit (Illumina, San Diego, USA). The paired-end cDNAs had a length of 300 bp (± 50 bp). After that, the cDNA libraries were sequenced on the Illumina HiSeq 2000 platform at the LC-BIO (Hangzhou, China) following the manufacturer’s recommendations. The raw sequencing data can be downloaded from NCBI Sequence Read Archive (SRA) under the accession number GSE63521.

RNA-seq Reads Mapping

After removing the low quality reads (i.e. reads containing sequencing adapters; reads containing Ns (unknown sequence) > 5; nucleotide with q quality score lower than 20) from the raw sequencing data, the paired-end reads were aligned to the S. lycopersicum genome (ftp://ftp.jgi-psf.org/pub/compgen/phytozome/v9.0/Slycopersicum/assembly/) by using Tophat version 2.0.9 [36], allowing a maximum of two base mismatches and multiple alignments per read (up to 20 by default).

Transcript Assembly and Abundance Estimation

The mapped reads were then assembled by Cufflinks version 2.1.1 for further annotation and measurement of relative abundances of transcripts [37]. Gene expression level within each sample were normalized with values for fragments per kilobase of exon per million fragments mapped (FPKM). Then Cuffmerge was applied to comerge all transcripts of the three samples to generate unique transcripts, and Cuffdiff reestimated the abundance of the transcripts and concurrently tested for different expression. The genes were considered as significantly differentially expressed between two groups if their absolute value of log₂ fold change > 1 and P value ≤ 0.05. Besides, in order to identify DEGs probably regulated by ABA more comprehensively and objectively, we conducted the comparison of genes expression among three groups (ABA, NDGA and CK). In triadic analysis of differential expression, the genes with P value ≤ 0.05 were identified as the DEGs by the method of Chi-square test. Meanwhile, in the analysis of DEGs, our gene expression level (FPKM value) was normalized by the Z-score determined with the formula: Z = (X- μ) / σ before heat-map plotting, where X represents the FPKM of a gene in a specific sample/time point, and μ and σ are the mean transcript expression and standard deviation of a gene across all samples, respectively [38].

Bioinformatics Analysis

We annotated each tomato gene with Gene Ontology (GO) terms for biological processes, molecular functions, and cellular components by Blast2GO vision 2.2.25 with default parameters (http://www.geneontology.org/) [39]. Meanwhile, the GO enrichment analysis was conducted by performing Fisher’s exact test with P value ≤ 0.05. The information of pathway for each tomato gene was attained from Kyoto Encyclopedia of Genes and Genomes (KEGG) database from the online KEGG Automatic Annotation Server (http://www.genome.jp/kegg/). The differentially expressed genes (DEGs) were also subjected to GO function and KEGG pathway enrichment analysis, and those genes with P-value ≤ 0.05 were defined as significantly enriched GO terms/KEGG pathways. Besides, each gene was aligned to the Cluster of orthologous groups for eukaryotic complete genomes (KOG) database to predict and classify protein functions.

Validation of RNA-seq Results by Quantitative Real-time PCR (qRT-PCR)

In order to verify the transcriptome data, expression level of a randomly selected set of differentially regulated genes was measured by qRT-PCR. The total RNA was extracted from 10 fruits of each treatment by RNAiso Plus (TaKaRa, Japan) and then was pooled at equal quantity. After that, the RNA of three treatments (ABA, NDGA and CK) was reverse-transcribed to cDNA with RNA PCR kit (TaKaRa, Japan), respectively. qRT-PCR was performed with SYBR Premix Ex Taq (TaKaRa, Dalian, China) on ABI Step One RT-PCR system according to the manufacturer’s instructions. Three biological replicates were performed and the primer names and corresponding sequences were listed in S18 Table. Relative expression was normalized to the internal control gene β-actin gene with 2^-ΔΔCT method [40]. The untreated sample (CK) was set as the calibrator for relative expression level. Pearson’s correlation was performed to determine the correlation of genes expression in ABA and NDGA treatments relative to the control between qRT—PCR and sequencing.

Statistical analysis

For all the biochemical measurements, data were analyzed using SPSS software and values were presented as mean ± standard error. The statistical significance of the differences between the samples was analyzed by the least significant difference test (LSD) at a significance level of P = 0.05. Significantly different values evaluated by t test for P value < 0.05 were indicated with asterisks.

General Effects of ABA and Sample Preparation for RNA-seq

To conduct transcriptome analysis of ABA influence on tomato fruit ripening, we selected the samples at specific ripening stage which exhibited the most considerable distinctions among different treatments for high throughput sequencing. During 18 days’ storage, the redness of tomato increased gradually, coinciding with the decline of fruit firmness in all samples (Fig 1a and 1b). In specific, total carotenoids increased as well as chlorophyll degraded during the fruit ripening (Fig 1c and 1d). Besides, lycopene and β-carotene, as the major carotenoids of tomato, accumulated progressively, which contributed to fruit color transition (Fig 1e and 1f). Compared with CK, ABA treatment remarkably promoted fruit ripening, whereas NDGA inhibited the process. Therefore, based on the morphological results, we chose the fruit samples on 9^th day to profile transcription changes via RNA-seq technology.

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Fig 1. Effects of ABA and NDGA applications on tomato ripening-related physiological indexes during storage at 20°C.

(a) The changes of a* value. (b) The changes of fruit firmness (kN). (c) The changes of total carotenoid content during tomato ripening. (d) The changes of chlorophyll content. (e) The changes of lycopene content. (f) The changes of β-carotenoid content. Error bars represented SE of three biological replicates, and asterisks (*) indicates significant difference (P<0.05) between the value in ABA treatment group or NDGA treatment group and that in CK (control).

https://doi.org/10.1371/journal.pone.0129598.g001

Global Analysis of Fruit Transcriptome

The RNA samples from pericarps of ABA/NDGA/CK tomatoes were subjected for high-throughput sequencing performed on an Illumina HiSeq 2000 platform. After trimming low-quality reads, each cDNA library yield 43–51 million sequence reads, representing a total clean database of 14.37 Gb (S1 Table). The qualified sequence reads were mapped against the S. lycopersicum reference genome by TopHat with at most two mismatches tolerance. 3.29–3.82 million reads were mapped to the tomato genome, with an average of 74.81% of total reads aligned to the tomato genomic locations. In addition, 72.27% of CK, 70.41% of ABA and 71.83% of NDGA sequencing reads were uniquely mapped to the reference in each sample (S1 Table). After the assembly of all uniquely aligning reads, we obtained 34054 genes and 47933 transcripts which were identified in the transcriptome. Among those transcripts, 34580 (72.14%) matched completely with the annotated tomato genome, 6012 (12.54%) were unknown transcripts and 11606 (24.21%) were potentially novel isoforms (S2 Table).

Function Classification and KEGG Analysis

Out of all 39690 genes, 11090 (27.94%) were successfully aligned to Gene Ontology (GO) and were classified into 41 functional groups, including 20 groups in biological process, 9 in cellular component and 12 in molecular function (S1a Fig). Within the class of cellular component, “cell” (GO:0005623) with 3254 genes and “cell part” (GO:0044464) with 3254 genes were predominant. In the category related to molecular function, a large amount of genes were involved in the “binding” (GO:0005488, 6190 genes) and “catalytic activity” (GO:0003824, 5521 genes). For the biological process, the assignments were mostly given to the terms of “metabolic process” (GO:0008152, 6022 genes) and “cellular process” (GO:0009987, 5142 genes) (S3 Table).

The total expressed genes were also blasted against the cluster of orthologous groups for eukaryotic complete genomes (KOG) of protein categories. A total of 10194 genes could be assigned to the KOG classification, and clustered into 25 functional categories. Among them, “signal transduction mechanism” (1316 genes, 12.91%) was found to be the major KOG category, followed by “general function prediction only” (1216 genes, 11.93%), “posttranslational modification, protein turnover, chaperones” (1107 genes, 10.86%) and “carbohydrate transport and metabolism” (618 genes, 6.06%). Additionally, only 577 (5.66%) genes were classified into the group of “function unknown” (S1b Fig).

All detected genes were subjected to KEGG pathway enrichment analysis, and 2403 genes were assigned to 144 pathways. The major pathways were “ribosome” (ko03010) (199, 8.28%), “oxidative phosphorylation” (ko00190) (110, 4.58%) and “spliceosome” (ko03040) (105, 4.37%), followed by “purine metabolism” (ko00230) (84, 3.50%), “glycolysis/gluconeogenesis” (ko00010) (82, 3.41%) and “plant-pathogen interaction” (ko04626) (74, 3.08%) (S1c Fig, S4 Table).

Analysis of Differentially Expressed Genes

A total of 25728 genes (75.55% of 34054) were expressed in the tomato fruit transcriptome, and a Venn diagram was adopted to present the number of uniquely or commonly expressed genes in the three analyzed samples (S2a Fig, S5 Table). It was found that 18049 genes expressed commonly across all three samples. CK had 1270 unique genes, while ABA and NDGA had 1518 and 2191 specifically expressed genes, respectively. In addition, 843 common genes were identified in both CK and ABA, and 969 genes were detected in both CK and NDGA (S2a Fig).

In order to evaluate the regulatory role of ABA, differential expression analysis was performed between samples. The expression levels within a given sample were normalized with a value of FPKM (fragments per kilobase of exon per million fragments mapped). 44.68% of all genes were in 10–100 FPKM range, followed by those with expression level of 1–10 FPKM (35.15%), < 1 FPKM (11.7%) and 100–1000 FPKM (7.48%) (S6 Table). The genes with│log₂ (fold change) ≥ 1 and P value ≤ 0.05 were identified as significantly differentially expressed genes in the comparison between two groups. Consequently, there were 10388 (40.38% of 25728) DEGs in total among the three samples (P value ≤ 0.05), and the number of DEGs in exogenous ABA or NDGA treated fruit was counted in S2b Fig.

We grouped all DEGs into GO functional categories in order to identify specific biological processes affected by exogenous ABA and NDGA. In the comparison between ABA and CK, proteins related to “photosynthesis, light harvesting” (GO:0009765, P value = 1.68E-06, regulation: down) were the most significantly enriched term in the biological process category, proteins associated with “photosystem I” (GO:0009522, P value = 7.70E-06, regulation: down) were highly enriched in cellular component and “ribulose- bisphosphate carboxylase activity” (GO:0016984, P value = 0.022, regulation: up, down) were the most highly represented in the category of molecular function. Meanwhile, the differentially expressed genes induced by NDGA were mainly distributed in the “photosynthesis, light harvesting” (GO:0009765, biological process, P value = 2.37E-05), “photosystem I” (GO:0009522, cellular component, P value = 3.50E-05) and “hydrolase activity, acting on ester bonds” (GO:0016788, molecular function, P value = 0.033) (S7, S8 and S9 Tables). These data suggest that the alteration of ABA may influence the expression of genes related to the GO function of “photosynthesis” in tomato fruit.

Next, the DEGs were further subjected to KEGG pathway enrichment analysis. It was found that “photosynthesis-antenna proteins” (ko00196) and “photosynthesis” (ko00195) were the most enriched pathways under the influence of exogenous ABA. The DEGs altered by exogenous NDGA were also involved in the similar KEGG pathways as observed in ABA, indicating a close relationship between photosynthesis and ABA (S10, S11 and S12 Tables).

Analysis of Genes Related to Fruit Color Variation

During tomato ripening, fruit color alters from green to red via the accumulation of carotenoids and a parallel reduction in chlorophyll concentration [41]. Lycopene and β-carotene are the major carotenoids in ripe tomato fruits [42, 43] (Fig 2a). Besides, chlorophyll is an extremely important biomolecule responsible for green color in the early stage of tomato ripening (Fig 2b) [44, 45]. In this study, 34 expressed genes were identified in color alteration process, with 13 DEGs in carotenoids biosynthesis and 2 DEGs in chlorophyll degradation, respectively (S13 and S14 Tables).

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Fig 2. Analysis of DEGs involved in the pathway of carotenoid biosynthesis and chlorophyll degradation.

(a) Schematic diagram of carotenoid biosynthesis (modified from the reference [78]) and the expression profile of 13 DEGs encoding key enzymes in the pathway. (b) Schematic diagram of chlorophyll degradation pathway (referred to reference [78]). The expression profile of 2 DEGs encoding key enzymes in chlorophyll degradation. Analysis of the transcriptional profiles of the relative gene expression values (Z scores) was performed using the heatmap command, Red and green color represent up-regulated and down-regulated genes, respectively. Abbreviations are listed in Supplemental S19 Table.

https://doi.org/10.1371/journal.pone.0129598.g002

To further analyze effects of ABA or NDGA on carotenoids pathway, expression of genes encoding 12 key enzymes involved in the carotenoids biosynthesis were analyzed. DXS is regarded as the rate-limiting enzyme in the MEP (2-C-methyl-D-erythritol 4-phosphate) pathway. We detected two DXS genes expressed in the tomato transcriptome, and one of them was significantly down-regulated by NDGA (Solyc01g067890.2). Compared with CK, the expressed IPI was significantly up-regulated by ABA and down-regulated by NDGA (Solyc04g056390.2). The three expressed GGPSs were all identified as significantly changed, which were specially repressed by NDGA from 1.28 fold to 2.27 fold (Solyc02g085700.1, Solyc02g085710.2 and Solyc04g079960.1). PSY is regarded as a key component in the upstream of carotenoids pathway, which participates in the conversion from GGPP to phytoene. Among the three expressed PSYs, two of them showed obvious increase in expression level after ABA treatment as well as great reduction after NDGA treatment (Solyc03g031860.2, 2277.9 FPKM in CK, 2951.4 FPKM in ABA and 1768.0 in NDGA; Solyc03g115030.2, 204.8 in CK, 232.2 in ABA and 165.9 in NDGA). Some Other important enzymes, PDS, ZDS and CRTISO, which contribute to the production of lycopene were all significantly up-regulated by ABA and evidently suppressed by NDGA in their transcript abundance. However, our data revealed that the transcription of ZEP was repressed by ABA treatment and the enhanced by NDGAtreament (Solyc02g090890.2, 18.0 in CK, 11.2 in ABA and 44.4 FPKM in NDGA).

Chlorophyll degradation is recognized as a pivotal process in fruit degreening [44, 45]. We analyzed major genes involved in chlorophyll breakdown including: Chlase, PPH, PaO and RCCR (S14 Table). Two Chlase genes (Solyc06g053980.2 and Solyc12g005300.1) showed no differences at expression level in ABA or NDGA treatment. One of the expressed PPHs (Solyc01g088090.2) was identified as DEG, which showed increased transcript abundance from 45.8 to 64.1 FPKM upon treatment with ABA. Among three detected PaOs, one of them was elevated by ABA and remarkably suppressed by NDGA (Solyc11g066440.1, 62.3 FPKM in CK, 67.6 in ABA and 51.7 FPKM in NDGA).

Genes Related to Flavonoid Biosynthesis

Flavonoids are ubiquitous plant secondary metabolites with a vast array of biological functions, including coloring, defense against biotic and abiotic stresses and contribution to plant growth and development [46]. Flavonoids are derived from the phenylpropanoid pathway, transforming phenylalanine into 4-coumaroyl-CoA, which demands the involvement of several crucial enzymes like PAL, C4H, and 4CL [47] (Fig 3a). There was only one PAL (Solyc03g078270.1) significantly regulated by exogenous treatments, which exclusively expressed in ABA treated-fruits (not expressed in CK and NDGA treatments) (Fig 3b). Transcription of the C4H (Solyc05g047530.2) was moderately improved by ABA from 24.7 to 33.6 FPKM, and repressed considerably to 7.7 FPKM by NDGA (Fig 3b). Moreover, of five 4CLs, one with high expression level (Solyc03g117870.2) was up-regulated by ABA from 143.2 to 184.9 FPKM, and reduced to 105.7 FPKM by NDGA (S15 Table).

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Fig 3. Analysis of DEGs involved in the pathway of flavonoids biosynthesis.

(a) Schematic diagram of flavonoids biosynthesis (modified from the reference [49]). (b) The expression profile of 16 DEGs encoding key enzymes in the pathway. Abbreviations are listed in Supplemental S19 Table.

https://doi.org/10.1371/journal.pone.0129598.g003

In tomato fruit, flavonoid naringenin chalcone (NarCh) has been reported as a predominant compound of total flavonoids, which was the first intermediate in the biosynthesis of flavonols [48]. It was synthesized from 4-coumarate-CoA by the catalysis of CHS and subsequently converted to naringenin (Nar) with the action of CHI [49]. In our result, the CHS gene (Solyc05g053550.2) expressed significantly higher in ABA treatment and showed a lower abundance in NDGA treated fruits (Fig 3b). However, none of CHIs expressed significantly differentially by either of the exogenous treatments. The expression of F3H was significantly decreased in ABA treatment by almost 2 fold (Solyc02g083860.2, from 130.3 to 67.4 FPKM), but slightly increased in NDGA treatment to 146.2 FPKM. The formed dihydroquercetin and dihydrokaempferol would be converted to kaempferol and quercetin respectively, which were catalyzed by the enzyme of FLS. It was observed that the FLS was suppressed by 1.51 fold in ABA treatment and induced by 1.31 fold in NDGA treatment (Solyc11g013110.1, 714.1 FPKM in CK, 474.8 FPKM in ABA and 932.5 in NDGA).

Many transcription factors have been previously proven to regulate the expression of flavonoids-pathway genes, such as MYB12, AGL8 and PAP1 [48, 50, 51]. We found that the two AGL8s both showed obviously increased expression when treated with exogenous ABA and correspondingly decreased upon NDGA application (Solyc03g114830.2, 165.6 in CK, 203.4 in ABA and 134.0 FPKM in NDGA; Solyc06g069430.2, 625.0 in CK, 772.0 in ABA and 445.7 FPKM in NDGA). Meanwhile, the transcript of PAP1 (Solyc02g081170.2) was also enhanced by ABA, which increased from 174.7 to 203.9 FPKM.

Genes Related to the Reactive Oxygen Species (ROS) Scavenging Enzymes

During fruit maturation, continuously generation of reactive oxygen species (ROS) could cause oxidative damages, initiating a variety of ROS-related disorders or cellular toxicity in plant [52]. ROS include free radicals like superoxide anion (O₂^-), hydroxyl radical (OH^-) and other non-radical molecules such as hydrogen peroxide (H₂O₂), singlet oxygen (¹O₂) [52]. The formation of ROS can be scavenged by a battery of enzymes in the antioxidant system, which was mainly composed of the GSH-ASA cycle (32 detected genes), GPX pathway (99 detected genes), the PrxR/TrX pathway (74 detected genes), SOD (7 detected genes) and the CATs (6 detected genes) [30] (S16 Table).

SODs were antioxidant defense enzymes, catalyzing the dismutation of superoxide radicals (O₂^-) into oxygen and H₂O₂ [53]. Of all seven SODs, five were identified as DEGs, showing remarkably increased expression levels in ABA and decreased levels in NDGA treated samples (Fig 4a). CATs, similar to SOD, were also of great importance to keep the primary products of partial oxygen reduction at steady-state concentrations in cells and tissues [54]. Six expressed CATs were all identified as DEGs, which showed slight alterations upon ABA treatment but noteworthy reductions by NDGA (Fig 4a).

Download:

• PPT
  PowerPoint slide
• PNG
  larger image
• TIFF
  original image

Fig 4. Analysis of DEGs involved in the pathway of ROS-scavenging and photosynthesis, respectively.

(a) Expression profiling of DEGs involved in antioxidant system. Green bar, SODs; yellow bar, CATs; blue bar, genes encoding enzymes of GSH-ASA cycle; pink bar, genes encoding enzymes of GPX pathway; purple bar, genes encoding enzymes of PrxR/TrX pathway. (b) Expression profiling of DEGs encoding key enzymes in different steps of photosynthesis.

https://doi.org/10.1371/journal.pone.0129598.g004

In addition, the GSH-ASA cycle has been proved to be involved in the action of eliminating ROS, which can be stimulated by environmental stress [55]. ASA and GSH were the important elements of GSH-ASA cycle, and the ratios of AsA/DHA (dehydroascorbate) and GSH/GSSG (glutathione disulfide) were considered as signals for modulating antioxidant mechanisms [56]. There were 15 GLRs, 10 APXs, 3 MDARs, 3DHARs and 1 GR in the GSH-ASA cycle. GLRs are small disulphide oxidoreductases with catalytic activity of S-glutathionylated proteins, thus becoming key enzymes in redox signaling and ROS scavenging [57, 58]. Among 15 GLRs, there were 5 genes considered to be altered significantly after exogenous ABA or NDGA applications. The abundances of Solyc06g067960.2, Solyc03g078380.1, Solyc06g005260.2, and Solyc06g082180.1 in NDGA treatment were lower than those in control by 1.39, 1.32, 1.27 and 3.97 fold respectively. APXs were currently reported as the major peroxidase for reducing cellular H₂O₂ into water, by using ASA as electron donor [59]. Almost all APX DEGs exhibited considerably increased abundance with exogenous ABA but were little influenced by NDGA treatment (Fig 4a). Among three MDARs, two of them (Solyc09g009390.2 and Solyc02g086710.2) were both significantly induced by ABA and repressed by NDGA treatment. Moreover, DHARs are also essential enzymes for reducing DHA back to AsA using GSH as reducing substrate [60]. Two DHARs (Solyc06g075520.2 and Solyc11g011250.1) were significantly up-regulated by ABA and down-regulated by NDGA, and the only one detected GR (Solyc09g065900.2), which catalyzed the reduction of GSSG to GSH in conjuction with NADPH, also showed a significantly elevated expression in ABA and a reduction in NDGA samples.

The GPX pathway contained 51GSTs, 6 GPXs and 42 PODs. GSTs are a superfamily of proteins, and there were 31 GSTs showing different expressions upon exogenous ABA or NDGA treatment, most of which were significantly up-regulated by ABA and down-regulated by NDGA (Fig 4a). GPXs also have the catalysis activity of reducing H₂O₂ to water, by using GSH as the reductant [61]. Four GPXs were identified as DEGs, which also showed a similar changing trend like other genes. Eight DEGs were identified among the large family of PODs, and the majority of them were highly expressed in ABA treated fruits.

It has been proposed that TrX/PrX system has a vital role in the removal of H₂O₂ [62, 63]. It has been reported that the Trxs were central players of various signaling cascades including redox homeostasis, and the catalytic activity of oxidized PrxRs could be restored by Trxs [64]. A total of 70 Trxs were expressed in our samples, and almost all of the 29 DEGs were up-regulated by ABA. Prxs are a ubiquitous family of antioxidant enzymes, reducing peroxides by redox-active cysteines [65]. There were four genes encoding PrxRs in the present study, and three of them were in significantly higher abundance in ABA treatment than those in CK (Fig 4a).

Genes Related to Photosynthesis Process

Interestingly, we observed that the GO term and KEGG pathway related to photosynthesis was highly enriched with the treatments of ABA and NDGA, indicating that the photosynthetic system and its components are regulated by phytohormone ABA during postharvest fruit ripening. There was a substantial amount of DEGs associated with different steps of photosynthesis, which showed significantly up-regulation in NDGA-treated fruits and down-regulation in ABA (Fig 4b, S17 Table). The vast majority of DEGs involved in photosystem I and photosystem II had remarkable higher expressions with NDGA application and decreased expressions in ABA treatment. Among 13 genes encoding chlorophyll A/B binding proteins, five of them showed significant differences in expression level. Regarding to photosystem I subunit, 9 DEGs were detected in the tomato transcriptome, all of them were up-regulated by NDGA and down-regulated by ABA. Two of LHCAs were identified as markedly changed in exogenous treatments. In particular, the expression of Solyc10g006230.2 increased from 63.2 to 160.9 FPKM after NDGA application, and dropped to 4.0 FPKM upon ABA treatment. All of four LHCBs were detected as DEGs in our analysis, which also showed the similar expression pattern with exogenous applications. There were 31 genes which encoded the photosystem II reaction center proteins expressed in this study. Of them, only two genes were significantly higher in NDGA and lower in ABA than control. Moreover, most of the genes involved in the generation of oxygen-evolving complex proteins and photosystem II subunit X were found to be induced in NDGA and repressed in ABA treatment as well (S17 Table). Besides, widespread up-regulations by NDGA were also observed in other genes related to light-dependent reactions, such as cytochrome b6f complex, plastocyanins, ATP synthases and NADP reductase (S17 Table).

Apart from that, a large number of DEGs were involved in Calvin cycle and other light-independent reactions of tomato fruit [66]. Notably, RUBPCO, which was one of key enzymes in CO₂ fixation, was strongly activated by NDGA at transcript abundance (32.8 FPKM in CK, 22.0 in ABA and 66.8 in NDGA). In addition, expression of a gene encoding RBCB (Solyc03g034220.2) was significantly increased by 3.64 fold in NDGA treatment and declined by 10.00 fold in ABA treatment. PEPC functions in the formation of oxaloacetate, which was also an important part of Calvin cycle [67]. There are four PEPCs identified as DEGs in this study, and two of them (Solyc07g062530.2 and Solyc04g006970.2) exhibited increased expressions by NDGA along with decreased expressions by ABA. We also observed up-regulation of two FBPs and one FBA in NDGA treatment, the genes participating in light-independent actions.

Real-time Reverse Transcription-PCR (RT-PCR) Validation of Selected DEGs

To validate the gene expression data from RNA-seq, 16 genes having different expression patterns were selected for real-time RT-PCR. Compared with the CK, the expression of all tested genes in ABA and NDGA treatments had a similar tendency between deep sequencing and qRT—PCR, respectively (S3 Fig, S18 Table). Besides, scatterplots by comparing the log2 fold change determined by RNA-seq and RT-PCR were also adopted in our study to confirm the accuracy of the transcriptomic results. Pearson’s correlation test showed that expression of the 16 genes relative to the control exhibited positive correlations between RNA sequencing and qRT—PCR (R² = 0.86 in CK vs ABA; R² = 0.70 in CK vs NDGA), indicating the high reliability of RNA-seq data of tomato transcriptome (S4 Fig). As for the difference of fold change between RNA-seq and qRT-PCR results, it may be caused by the different sensitivity of two different technologies [68]. In addition, the higher fold change observed in some genes by RT-PCR may be due to the exponential amplification in PCR that may boost real mRNA expression [68].