Abstract
Fruit-specific promoters have been used as genetic engineering tools for studies on molecular mechanism of fruit development and advance in fruit quality and additional value by increasing functional component. Especially fruit-ripening specific promoters have been well utilized and studied in tomato; however, few studies have reported the development of promoters that act at fruit developing stages such as immature green and mature green periods. In this study, we report novel promoters for gene expression during the green to ripening stages of tomato fruit development. Genes specifically expressed at tomato fruit were selected using microarray data. Subsequent to confirmation of the expression of the selected 12 genes, upstream DNA fragments of the genes LA22CD07, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at which specifically expressed at fruit were isolated from tomato genomic DNA as promoter regions. Isolated promoter regions were fused with the GUS gene and the resultant constructs were introduced into tomato by agrobacterium-mediated transformation for evaluation of promoter activity in tomato fruit. The two promoters of LA22CD07, and LesAffx.6852.1.S1_at showed strong activity in the fruit, weak activity in the flower and undetectable activity in other tissues. Unlike well-known fruit-ripening specific promoters, such as the E8 promoter, these promoters exhibited strong activity in green fruit in addition to red-ripening fruit, indicating that the promoters are suitable for transgene expression during green to ripening stages of tomato fruit development.
Key message Novel fruit-specific promoters have been identified and are suitable for transgene expression during green to ripening stages of tomato fruit development.
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Introduction
The tomato (Solanum lycopersicum) is one of the major Solanaceae crops and one of the most widely eaten fruits in the world. Genetic engineering has been used in an effort to improve the quality of the tomato fruit (Butelli et al. 2008; Dharmapuri et al. 2002; Le et al. 2006; Lewinsohn et al. 2001; Mollet et al. 2008; Rosati et al. 2000; Schijlen et al. 2006, 2007; Wang et al. 2008).
The tomato also serves as a vehicle for the production of useful proteins. For example, we reported the overexpression of the miraculin gene and the production of miraculin protein in the tomato fruit (Hirai et al. 2010; Hiwasa-Tanase et al. 2012; Sun et al. 2007; Yano et al. 2010). Chen et al. (2009) reported the production of thymosin alpha1, an immune booster that plays a role in the maturation, differentiation and function of T-cells, in the tomato fruit. Zhang et al. (2007) described the expression of human coagulation Factor IX in the tomato fruit.
The cauliflower mosaic virus 35S promoter (35S promoter) is a constitutive promoter that is widely used for the expression of foreign genes in higher plants. However, in some cases the 35S promoter is not suitable for gene expression because of the possibility that 35S promoter-driven constitutive gene expression could be damaging to plant growth and development.
To overcome the problem of the 35S promoter, tissue-specific promoters have been isolated. Fruit-specific promoters have been isolated as tools for fruit-specific gene expression. In the tomato, promoters from ethylene response genes, such as E8 and E4, have been well studied as fruit-specific promoters (Cordes et al. 1989; Coupe and Deikman 1997; Deikman et al. 1992, 1998; Deikman and Fischer 1988; Kneissl and Deikman 1996; Lincoln et al. 1987; Montgomery et al. 1993a; Xu et al. 1996). Polygalacturonase (Montgomery et al. 1993b; Nicholass et al. 1995) and lipoxygenase promoters (Beaudoin and Rothstein 1997) have also been reported as fruit specific in the tomato. These classical promoters have been reported to act during the late-ripening stage of fruit development. On the other hand, information of promoters that act at fruit expanding stage (immature green), mature green stage and throughout the developmental stage is much less common than the fruit-ripening specific types, although recently Estornell et al. (2009) reported some promoters driving gene expression preferentially in the fruit with different activity ranges.
Many promoter variations expand the capability of intended use depending on the purpose. Therefore, in this study we attempted to isolate novel fruit-specific promoters with different activity from classical promoters. We selected 12 genes which showed high expression in fruit tissues using microarray data obtained from tomato cultivar ‘Micro-Tom’, which has become a model plant of the Solanaceae family (Matsukura et al. 2008). Upon confirmation of the expression of the selected genes, cloning of the promoter regions, and the promoter analysis using GUS gene, we finally identified two promoters with fruit-specific activity. Unlike some classical fruit-specific promoters, these promoters were driven GUS gene expression throughout the fruit development in the green to ripening stages.
Materials and methods
Identification of candidate genes from microarray data
Tomato genes which show fruit-specific expression were selected using gene expression data from following three sources: (1) a dataset available in MiBASE (old version, http://www.kazusa.or.jp/jsol/microtom/) using ‘Micro-Tom’ cDNA array produced by Japan Solanaceae genomics consortium (Yano et al. 2006), (2) a dataset GSE19326 available in Gene Expression Omnibus (http://www.ncbi.nlm.nih.gov/gds) (Ozaki et al. 2010), and (3) datasets ‘Wild type tomato fruit development (set 1 and set 2)’ available in Tomato Functional Genomics Database (http://ted.bti.cornell.edu/cgi-bin/TFGD/miame/home.cgi) (Alba et al. 2005). Sequences of LA15CA04, LA22CD07, LC09AH08, LC04DC11, LA12AA05, LA14AD08 and FB14DB02 were obtained from MiBASE (http://www.pgb.kazusa.or.jp/mibase/). Consensus sequences of unigenes, from which Les.331.1.S1_at, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at probes were designed, were obtained from Affymetrix website (http://www.affymetrix.com). Consensus sequences of TC115787 and TC116003 were obtained from Dana-Farber Cancer Institute Tomato Gene Index (http://compbio.dfci.harvard.edu/cgi-bin/tgi/gimain.pl?gudb=tomato).
RNA isolation and reverse-transcription PCR (RT-PCR) analysis
Total RNA was isolated from the leaves, flowers, stems, roots, and green and red fruits of 3-month-old ‘Micro-Tom’ plants using TRIzol® (Invitrogen, USA) according to the manufacturer’s instructions. One microgram of total RNA from each sample was treated with RQ1 RNase-Free DNase (Promega, USA) and was used for first-strand cDNA synthesis with a poly-T primer and SuperScript II Reverse Transcriptase (Invitrogen, USA) according to the manufacturer’s instructions.
The first-strand cDNA was subsequently used as a template for the expression analysis of the selected genes. RT-PCR was performed with 25–30 cycles for the gene expression analysis using designed gene-specific primers (Table 1). After the PCR, an equal volume of each amplified PCR product was subjected to electrophoresis on a 1 % TAE agarose gel and was visualized using ethidium bromide.
Quantitative real-time RT-PCR (qRT-PCR)
For the analysis of LA22CD07 and LesAffx.6852.1.S1_at expression during fruit development and ripening, total RNA was isolated from the ovary, young (12, 15, and 18 days after flowering) and mature green fruits, orange fruits, and red fruits using the RNeasy plant mini kit (Qiagen, Japan) according to the manufacturer’s instructions. The first-strand cDNA was synthesized from 0.75 μg of total RNA using the Superscript VILO cDNA synthesis kit (Invitrogen, USA). A tenfold dilution of the first-strand cDNA was used as a template for the qRT-PCR using SYBR Premix Ex Taq II (Takara-Bio Inc., Otsu, Japan) in a Thermal Cycler Dice Real-Time System TP800 (Takara-Bio Inc., Otsu, Japan) according to the manufacturer’s instructions. The thermal cycling parameters were set at 95 °C for 10 min to denature, followed by 40 cycles at 95 °C for 5 s and 68 °C for 30 s. The relative quantification of the target gene expression was calculated using the tomato ubiquitin3 gene (X58253) as an internal control. The following primer sequences were used: LA22CD07 forward, 5′-GATCAAACTATTGCTGCCCAG-3′, and reverse, 5′-CTCTTCCTTGCTTCCACTCCAA-3′; LesAffx.6852.1.S1_at forward, 5′-CTGAAATGTCCCGTGATGATGC-3′ and reverse, 5′-CGCTTGCAGGTTCTCTGTTC-3′; E8 forward, 5′-TGGAAAGCCCTAGAGTTGAGGA-3′ and reverse, 5′-GAATCAACAAGTCCTTTAACAC-3′; and ubiquitin3 forward, 5′-CACCAAGCCAAAGAAGATCA-3′ and reverse, 5′-TCAGCATTAGGG CACTCCTT-3′.
Isolation of promoter regions
Genomic DNA was extracted from ‘Moneymaker’ which was cultivated variety for edible use in consideration for prospective various uses such as transformation to cultivated tomato variety using CTAB method (Murray and Thompson 1980). Each 5′-flanking region of LA22CD07 and LesAffx.6852.1.S1_at was isolated from genomic DNA using the GenomeWalkerTM Universal Kit (Clontech, USA) as the putative promoter regions. The promoter regions were obtained from a second PCR using the GenomeWalkerTM Universal Kit, purified using the Wizard(R) SV Gel and PCR Clean-Up System (Promega, USA), and directly sequenced. The ATG start codons were predicted using ORF Finder (http://www.ncbi.nlm.nih.gov/gorf/gorf.html), and the sequences were compared with homologs of other plant species, such as Arabidopsis. Approximately, 2 kb of 5′ upstream regions from the predicted ATG start site were re-amplified from the ‘Moneymaker’ genome using KOD Plus (TOYOBO, Japan). The amplified products were cloned into the pCR®-Blunt II-TOPO® Vector (Invitrogen, USA) and sequenced.
Transient promoter assay
The promoter region in the pCR®-Blunt II-TOPO® Vector was digested with restriction enzymes and ligated in front of the GUS gene in the pBI121 vector to replace the 35S promoter. The constructs containing the promoter region or pBI121 as a control were transformed into Agrobacterium tumefaciens strain GV3101 through electroporation and was used in a transient promoter assay. The assay was performed using green fruit of ‘Micro-Tom’ as previously described (Orzaez et al. 2006). The agrobacterium containing the construct was injected into green fruit and incubated for 4 days at 25 °C under long-day conditions (16 h light and 8 h dark). The total protein from the infected fruit was subjected to a quantitative GUS activity assay using 4-methylumbelliferyl-beta-d-glucuronide (4-MUG) as a substrate.
Production of transgenic tomato
The transformed A. tumefaciens was also used for the production of a transgenic tomato with ‘Micro-Tom’ cultivar. Transformants were produced according to Sun et al. (2006). The presence of the promoter–GUS fusions in the regenerated plants was confirmed by PCR using genomic DNA isolated from the regenerated plants as templates.
GUS assay
For the quantitative analysis, GUS activity was assayed using the substrate 4-MUG according to Jefferson et al. (1987) with slight modifications (Moon and Callahan 2004). Tomato tissue was crushed using liquid nitrogen, and the protein was extracted in extraction buffer (Moon and Callahan 2004). The protein concentration was measured using the Bradford method (Bradford 1976). Approximately 100 μg of protein was used for the GUS assay. The reaction product 4-methylumbelliferone (4-MU) was measured with Safire (Tecan, Switzerland).
The histochemical GUS analysis was performed using 5-bromo-4-chloro-3-indolyl-β-d-glucuronide (X-Gluc) according to Jefferson et al. (1987) with slight modifications to the assay buffer. To reduce the background from GUS staining, 100 mM phosphate (pH 8.0) was used instead of 50 mM phosphate (pH 7.0) in the assay buffer. For the analysis of the red fruit in Fig. 3b, 20 % methanol (final volume) (Kosugi et al. 1990) was added to the assay buffer to further reduce the background staining. The tomato tissues were incubated in an assay buffer at 37 °C for 16 or 6 h. After staining, the sample was washed with 70 % ethanol to terminate the reaction.
Results and discussion
Identification of promotercandidate genes from microarray data for expression in green fruit
To obtain candidates for novel fruit-specific promoters with unique activities compared to classical promoters, such as the E8 promoter, which mainly acts in the fruit late-ripening stage, we employed two strategies. The first strategy was to identify highly expressed genes in green fruit, and the second was to uncover novel fruit-specific genes.
First, we analyzed microarray data using mRNA from ‘Micro-Tom’ green fruit to identify genes that were highly expressed in green fruit and selected seven genes (LA15CA04, LA22CD07, LC09AH08, LC04DC11, LA12AA05, LA14AD08 and FB14DB02). Moreover, microarray database of several ‘Micro-Tom’ tissues was available from the Kazusa DNA Research Institute and Cornell University due to obtaining promoter-candidate genes for fruit-specific expression. Consequently, five genes (Les.331.1.S1_at, Les.3122.2.A1_a_at, LesAffx.6852.1.S1_at, TC115787 and TC116003) were selected. In total, 12 promoter-candidate genes were identified (Table 1).
Expression analysis of the promoter-candidate genes by RT-PCR
To examine whether the promoter-candidate genes uncovered from the microarray data are expressed in tomato fruit and the specificity, we performed RT-PCR analysis using the primer sets listed in Table 1.
We first examined the seven promoter-candidate genes predicted to have high expression levels in green fruit. As shown in Fig. 1, the expression was detected after 25 PCR cycles and was clearly detectable at 27 and 30 cycles using cDNA template derived from green fruits. The expression levels were different among the promoter-candidate genes. Based on the expression levels at 27 and 30 cycles, we selected LA22CD07, LA12AA05 and LA14AD08, which were highly expressed in green fruit, for further studies.
Next, the organ-specific expression patterns were investigated for the five promoter-candidate genes predicted fruit specificity to understand which candidates displayed fruit-specific expression (Fig. 2). In this analysis, the expression of E8 gene was also investigated to compare the expression of promoter-candidate genes with a well-known fruit-specific gene. As a result, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at exhibited fruit-specific expression. However, they also exhibited different expression patterns. Les.3122.2.A1_a_at showed specific and high expression in the both green and red fruit stages, whereas LesAffx.6852.1.S1_at was highly expressed in the green fruit but was only slightly expressed in the red fruit. Les.331.1.S1_at was also highly expressed in the green and red fruits; however, a low level of expression was detected in the flower. TC115787 was expressed in the flower, stem and root in addition to the green and red fruits. TC116003 was expressed throughout the examined organs except the red fruit. The E8 gene was highly expressed in the red fruit but was almost undetectable in the green fruit. This result supports previous studies, which reported that the E8 gene was expressed in a ripening-specific manner (Deikman and Fischer 1988; Kneissl and Deikman 1996; Lincoln et al. 1987).
We uncovered two promoter-candidate genes of Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at with fruit-specific expression and one gene of Les.331.1.S1_at with high expression in the fruit and low expression in the flower. Notably, these three candidates were highly expressed in the green fruit, in which E8 gene expression was almost undetectable. Moreover, the three candidates were also expressed in the red fruit. These results suggest that the promoters of the three candidate genes were active in fruit and have different activities than the E8 promoter.
From these results, six genes, LA22CD07, LA12AA05, LA14AD08, Les.331.1.S1_at, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at, were selected for subsequent analysis.
BLASTN analysis of the candidates
To obtain functional information for the promoter-candidate genes, a BLASTN analysis was performed. The results were summarized in Table 2, which listed the top hits of functionally annotated genes resulting from BLASTN analysis. The BLASTN analysis showed that LA14AD08 returned a hit for a clp-like energy-dependent protease from the tomato and stink bell (Fritillaria agrestis), indicating that LA14AD08 represents a family of Clp proteases. Although LA22CD07 and LA12AA05 hit to the tomato full-length cDNA sequences (Aoki et al. 2010), they did not hit to functionally annotated tomato gene. However, LA22CD07 and LA12AA05 returned hits for the erythroblast macrophage protein emp from Ricinus communis (XM_002525023) with an e value of 5E−39 and the sufD protein from the Ricinus communis (XM_002534741) with an e value of 2E−69, respectively. The result suggest that the two candidates are homologs of the erythroblast macrophage proteins emp or sufD.
Les.331.1.S1_at returned hits for the tomato LOX gene U13681 (Kausch and Handa 1995) and tomloxB (U09025) with e values of 0 (Ferrie et al. 1994). Ferrie et al. (1994) reported the fruit-specific expression of the LOX gene. Beaudoin and Rothstein (1997) reported that the LOX gene promoter activity was active in tobacco and tomato fruits.
Les.3122.2.A1_a_at returned a hit for tomato gene S66607 (Pear et al. 1993), which has been described as a pectin methylesterase-like sequence, indicating that Les.3122.2.A1_a_at is a member of the pectin methylesterases. The expression pattern and promoter analysis of S66607 have not been analyzed; however, it has been reported that some members of the pectin methylesterases exhibited fruit-specific expression (Gaffe et al. 1997; Hall et al. 1994).
LesAffx.6852.1.S1_at returned hits for tomato cDNAs with e values of 0 whose functions have not been reported. LesAffx.6852.1.S1_at also returned a hit for a cysteine protease of Gossypium hirsutum (AY171099) with 69 % identity, suggesting that the LesAffx.6852.1.S1_at is a member of the cysteine proteases.
Isolation and characterization of selected gene promoters
Because the Les.331.1.S1_at promoter had been analyzed previously (Beaudoin and Rothstein 1997), we decided to clone the promoter regions that have not been analyzed: LA22CD07, LA12AA05, LA14AD08, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at.
To clone the promoter regions, we performed genome walking based on the sequence information of the candidates. The PCR fragments obtained from genome walking were directly sequenced. The ATG start codons were predicted using ORF Finder (http://www.ncbi.nlm.nih.gov/gorf/gorf.html), and the sequences were compared with homologs of other plant species. Subsequently, the putative promoter regions, which were approximately 2 kb upstream from the predicted ATG start codon, were re-amplified and sequenced.
To analyze the activities of the isolated promoters, each promoter was cloned to replace the 35S promoter in vector pBI121. We first performed transient assays using ‘Micro-Tom’ green fruit. Significant GUS activity was obtained from the LA22CD07, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at promoters (data not shown). The GUS activities of the LA12AA05 and LA14AD08 promoters were almost the same as that of uninfected green fruit, suggesting that the two promoter fragments do not function in green fruit.
The three promoters from LA22CD07, Les.3122.2.A1_a_at and LesAffx.6852.1.S1_at that exhibited GUS activity in the transient assay were further analyzed using stable transgenic tomatoes. We conducted a GUS histochemical assay of leaves, roots, stems, flowers, green fruits and red fruits in regenerated T0 plants. At least three independent T0 plants per construct were assayed. The GUS staining pattern was almost identical among the tested plants containing the same construct, although the staining intensity varied (data not shown). Figure 3 shows the results of a typical GUS staining of the various tissues of transgenic plants containing promoter–GUS fusion constructs. Unlike the transgenic plants containing the 35S promoter, tissue-specific GUS staining patterns were observed among the transgenic plants containing the LA22CD07 or LesAffx.6852.1.S1_at foreign promoter regions. Figure 3a shows the results from a 16 h GUS staining experiment. The transgenic plants containing the LA22CD07 promoter exhibited strong GUS staining in the green and red fruits, weak staining in the flowers and undetectable staining in the leaves and roots. The transgenic plants containing the LesAffx.6852.1.S1_at promoter also displayed strong staining in the green and red fruits, but the flower staining was stronger than that of LA22CD07. No staining was detected in the tissues from the transgenic plants containing the Les.3122.2.A1_a_at promoter (data not shown). In the case GUS gene driven by 35S promoter, the GUS staining was detected everywhere in tomato plant and the staining levels were relatively high. However, in the green fruit the GUS staining levels were almost same in LA22CD07, LesAffx.6852.1.S1_at and 35S promoters. In the red fruit, the staining levels were also high in these promoters but non-specific staining was observed in the non-transgenic plants. Therefore, the red fruits were further treated with assay buffer containing methanol for 6 h. As shown in Fig. 3b, GUS staining was almost not detected in the wild-type plants and was observed in red fruits of the transgenic plants containing the LA22CD07 and LesAffx.6852.1.S1_at promoters. Moreover, the staining levels were relatively high especially in LesAffx.6852.1.S1_at promoter compared with 35S promoter. These results indicated that these promoters were active in both green and red fruits.
Quantitative real-time PCR analysis of LA22CD07 and LesAffx.6852.1.S1_at was performed to investigate the details of the promoter activities during fruit development and to compare the activity of E8 promoter as known fruit-ripening specific (Fig. 4). The expression of E8 gene was slightly detected in mature green stage and rapidly increased from orange stage. On the other hand, the expression level of LA22CD07 was gradually increased from 12 days after flowering and reached the highest in the red stage. In the LesAffx.6852.1.S1_at the expression was already detected in the ovary and then gradually increased as described for LA22CD07. The result suggested that the two novel promoters had different activation patterns from E8 promoter and were active from small green fruit or ovary stages. Although we have not examined the GUS staining between flowers and green fruits, it might be possible that the two promoters are active at early stages of fruit development (flower to green fruit) because the GUS staining was also observed in the both flowers.
Conclusions
In this study, we isolated novel two fruit-specific promoters from the tomato. These promoters exhibited activities that were different from classical fruit-ripening specific promoters, such as the E8 promoter. The activities are detected throughout during fruit development from ovary to red-ripe fruit. Therefore, the identified two promoters might outperform some fruit-specific promoters that act only at fruit-ripening stage depending on the intended purpose. The two promoters will supply us tools to express genes of interest in fruit regardless of the developmental stage. In this study, we examined only tomato promoters. However, it might be possible to use these promoters in the fruits of other plants because BLAST analysis revealed homologs of LA22CD07 and LesAffx.6852.1.S1_at from many plant species.
Abbreviations
- GUS:
-
Beta-d-glucuronidase gene
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Acknowledgments
We thank the members of the Ezura laboratory for helpful discussions. Micro-Tom seeds (TOMJPF00001) were obtained from the National BioResource Project Tomato (NBRP-Tomato). This research was supported through grants from the “Development of Fundamental Technologies for the Production of High-Value Materials Using Transgenic Plants” project of the Ministry of Economy, Trade, and Industry of Japan to H.E. and K.T.
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Communicated by H. Ebinuma.
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Hiwasa-Tanase, K., Kuroda, H., Hirai, T. et al. Novel promoters that induce specific transgene expression during the green to ripening stages of tomato fruit development. Plant Cell Rep 31, 1415–1424 (2012). https://doi.org/10.1007/s00299-012-1257-5
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DOI: https://doi.org/10.1007/s00299-012-1257-5