Background

Hemarthria compressa, commonly called whip grass, is a perennial grass in the family Gramineae. It is mainly distributed in tropical and subtropical zones, with a sparse distribution in the temperate-humid zones of the Northern Hemisphere. H. compressa is characterized by its long growing period, high growth rate, strong regenerative capacity, high yield, and strong stress tolerance. In southern China, H. compressa is an important forage grass, and is often used for soil and water conservation as well as ecological management [1, 2]. Most H. compressa studies have focused on agronomic characters, production performance, and genetic diversity. Currently, genetic information about H. compressa is very rare, and no sequence records of this important forage grass have been available in the NCBI GenBank until now. This limits research on functional genes, but transcription factors, as regulatory proteins that regulate signal transduction and gene expression, play an especially important role in exploring gene function. Therefore, identification and characterization of transcription factor will contribute to gene functional studies in H. compressa and other grasses.

Transcription factors are DNA-binding proteins that can specifically bind to one or more cis-acting elements in the promoters of eukaryotic genes, thereby activating or inhibiting transcription. Based on conserved DNA domains, transcription factors are classified into various families such as AP2/ERF, MYB, WRKY, and bZIP. [1, 2]. AP2/ERF is a unique transcription factor family found in plants; it participates in plant development [3-6], hormonal (ABA, ethylene, and others) responses, secondary metabolism, and responses to biotic or abiotic stresses [7, 8]. Based on similarities found in their AP2/ERF domains, Sakuma et al. [9] divided the transcription factors encoding the AP2/ERF domain in Arabidopsis into five groups: four sub-families (AP-2, RAV, DREB, and ERF) and the remaining transcription factors.

The DREB (dehydration responsive element binding protein) subfamily genes play key roles in plant stress responses to low temperatures, drought, and high salinity environments [7, 10, 11]. DREB has a conserved AP2/ERF domain that can specifically bind to the DRE/CRT cis-acting element to activate expression of several stress-tolerance genes, thereby enhancing plant stress tolerance [7, 11, 12]. In Arabidopsis, DREB1A, DREB1B, and DREB1C play significant roles in cold-responsive gene expression. With respect to its AP2/EREBP domain, CBF4/DREB1D displays high homology with DREB1A; however, the expression of CBF4/DREB1D was induced by osmotic stresses instead of cold stress [9, 13]. DREB2A and DREB2B were contained in plants exposed to salinity or drought stresses, while DREB2C, DREB2D, and DREB2F were slightly induced in leaves by salinity treatment while DREB2E was slightly induced in roots by exogenous ABA treatment [9, 10].

In recent years, DREB transcription factors have been identified in a large number of model plant species, including Nicotiana tabacum [14], Arabidopsis thaliana [9], and rice (Oryza sativa) [15],. DREB genes have been studied in forage crops as well. For example, Tang et al. [16] isolated a new DRE-binding protein gene, FaDREB1, from Festuca arundinacea using the rapid amplification of cDNA end-PCR (RACE-PCR) method, which discovered an AP2/ERFBP-type transcription factor and found that the FaDREB1 protein may be involved in the regulation of cold stress via the ABA-independent pathway. Xiong et al. [17] identified a DREB1A/CBF3-like gene LpCBF3 from perennial ryegrass (Lolium perenne L.) and demonstrated that LpCBF3 is similar to DREB/CBF genes in Arabidopsis and is a functional transcription regulator in Arabidopsis. In alfalfa (Medicago falcata L.), two DRE-binding protein genes, MfDREB1s and MfDREB1, which encode AP2/EREBP-type transcription factors, were both found to be inducible by low-temperature stress [18]. Yet, the DREB family of genes in warm-season perennial grasses has been poorly examined so far.

In this study, we used RACE-PCR to clone DREB transcription factor genes from H. compressa. Using to the conserved sequence of the AP2/ERF domain, we successfully cloned a full-length HcDREB2 gene from H. compressa. The HcDREB2 protein bound DRE cis-elements to transactivate the reporter gene in the yeast one-hybrid assay. Moreover, the expression level of HcDREB2 was highly induced by various stress treatments but not by ABA. No DREB genes were identified in H. compressa, and these experimental results provide the first valuable genetic information about the DREB gene family in this species. These results provide a foundation for stress-tolerance breeding in H. compressa through genetic engineering.

Results and discussion

Isolation of HcDREB

A full-length HcDREB gene, HcDREB2 (GenBank ID: KC203598.1), was isolated from cold-treated H. compressa samples. The gene is 1254 bp in length and encodes a putative polypeptide of 264 amino acids (Additional file 1: Table S1). Although the full sequence of HcDREB shared only moderate identity with known DREB proteins in other plant species, it contained a conserved AP2/EREBP domain, including two highly conserved residues (V14 and E19) that are critical to its interaction with the DRE cis-element. This region (between V14 and E19) is unique to DREB2 transcription factors. Besides these conserved residues and domain, we also observed two additional features that are common to DREB proteins: (1) the nucleic localization signal region on the N terminus, which is rich in alkaline amino acids and (2) a transcriptional activation region that is rich in acidic amino acids (Fig. 1). These observations provide additional evidence that the sequence we obtained encoded a DREB family gene. [ Table Omitted - see PDF ]

Expression analysis of HcDREB2

The relative transcription levels of HcDREB2 under low temperature, drought, high salinity, and ABA treatments were determined by qRT-PCR (Fig. 2). HcDREB2 expression was not induced by ABA treatment and remained at a level that was barely detectable by qRT-PCR (Ct value >32). On the contrary, the expression level of HcDREB2 was quickly induced by the other stress treatments. Two peak values were observed during the time course of the treatments; the first and the second peaks were observed after 1 and 8 h, respectively, of cold, drought, and salinity treatments (Fig. 2). After 24 h of treatment, the HcDREB2-expression level declined under cold and drought treatments, but remained at a relatively high level under the salinity treatment (Fig. 2). In brief, the expression of HcDREB2 was independent of ABA but inducible by the three tested abiotic stresses. [ Table Omitted - see PDF ]

It has been suggested that the DREB2 transcription factor participates in stress responses to drought and high NaCl concentration. The expression of DREB2 genes in Arabidopsis and rice were induced by drought and high NaCl concentrations but not low temperatures [10, 19]. Our studies indicate that HcDREB2 gene expression is induced by exposing plants to low temperatures. It is known that the DREB2 gene in some plants can regulate heat-shock response and activate the expression of many abiotic stress genes. The expression of DvDREB2A in chrysanthemum was induced by high temperatures [20]. Over-expression of the ZmDREB2A gene strengthens the tolerance of Arabidopsis for exposure to high temperatures [21]. It has been shown that AtDREB2A, the close homolog of HcDREB2 in Arabidopsis, was induced by drought and high NaCl concentration exposure and was also involved in the penetration stress signal transduction pathway. AtDREB2A went through post-translational modification, and the activated form regulated the expression of a series of down-stream functional genes with DRE elements in their promoters [22, 23]. Despite the similarities, the expression modes of DREB2 genes differed across gene family members and varied across different plant species. The expression mode of DREB genes might also lead to their diversified gene functions by targeting and regulating the downstream functional genes thereby contributing to varied stress tolerances in plants. For examples, TaDREB1 was induced by low temperatures of 0 °C with a photoperiod of 12 h, 20 % PEG6000 for drought stress, 200 mM NaCl for salt stress, and 25 mM ABA for ABA stress in different wheat (Triticum aestivum) cultivars [24]; HvDRF1 was induced by drought achieved by water deprivation of 3-week-old plants grown in small pots containing sandy soil as well as salinity and ABA treatments that were performed by the hydroponic growth of barley seedlings (Hordeum vulgare; 9-day-old plants) in 100 ?m ABA or 250 mm NaCl solution for 6 h [25]. The transcriptional expression of PgDREB2A in Pennisetum laucum is induced by low temperatures and salinity as shown by an experiment conducted with 12-day-old seedlings that were subjected to salt stress (250 mM NaCl) and cold stress (4 °C) for 6, 12, 24, and 48 h, and drought stress that was achieved by drying plants on tissue paper and keeping them wrapped in dry tissue paper for 1 and 2 h [26]. In this study, we showed that HcDREB2 in H. compressa was induced by low temperatures and drought, but not by ABA, which implies that HcDREB2 might play an important role in the stress response of H. compressa and that HcDREB2-mediated stress tolerance might be ABA-independent.

The time course of DREB2 expression in response to abiotic stresses also differed among species. For example, under drought and salinity conditions for merely 10 min, AtDREB2 expression was upregulated quickly in Arabidopsis and reached peak expression after 10 h of treatment [10]. The expression of BeDREB2 in Bermuda grass (Cynodon dactylon) reached its peak when the plant was exposed to salinity for 4 h [27]. In Malus robusta, DREB2 expression peaked when exposed to either low temperatures for 8 h or drought for 1 h [28]. In contrast, in H. compressa, the expression levels of HcDREB2 were lowest under low-temperature, drought, or salinity treatments for 4 h. Specifically, the expression levels of HcDREB2 under low temperatures and drought treatments for 4 h were even below those of the control. The expression of HcDREB2 was induced by low temperatures, drought, and high NaCl concentration and peaked twice (at 1 h and 8 h after treatment) over the 24-h period. This fluctuation of gene expression might reflect adaptation to photoperiod or its circadian rhythm. Fowler et al. [29] found that under low temperatures the expression of CBF3 was regulated by a photo signal, which participated in the related-cell signaling pathway by means of rhythm regulation and energy balance (through photosynthesis). Further studies examining whether the photoperiod regulated the induction of HcDREB2 expression are important for understanding this phenomenon in H. compressa.

Yeast one-hybrid experiment

A yeast one-hybrid assay was conducted to evaluate the transcriptional activation of HcDREB2. We observed that yeast cells transformed with pAbAi-p53?+?pGADT7-Rec-p53 (positive control cells) and pGADT7-Rec-HcDREB?+?pAbAi-DREy were able to grow on SD-screening medium. In contrast, cells transformed with pAbAi?+?pGADT7-Rec, pGADT7-Rec-HcDREB?+?pAbAi-DREt, or pAbAi?+?pGADT7-Rec-HcDREB were unable to grow (Fig. 3). This result suggests that HcDREB2 directly binds DRE cis-elements and trans-activates the transcription of downstream genes. [ Table Omitted - see PDF ]

Compared with DREB1 transcription factors, studies on DREB2 transcription factors are less common, probably because DREB2 transcription factors bind to DRE elements, but only induce low transcription activity. In a transcriptional-activation experiment using Arabidopsis protoplasts, it was found that the transcriptional activation of AtDREB2A was significantly lower than that of AtDREB1A [10]. Furthermore, there was also no significant phenotypic difference between the transgenic Arabidopsis with constitutive expression of DREB2A and wild-type Arabidopsis [10].

DREB transcription factors bind with high specificity to the DRE/CRT cis-acting elements in promoters and thereby trans-activating the expression of these downstream target genes. Thus, DREB genes play an important role in regulating the signal pathways of plant-stress responses. Our experiments using a yeast one-hybrid system show that the HcDREB functioned as a transcriptional activator by specifically binding to a mutant DRE element. There are valine and glutamic acids at amino acid residues 14 and 19, respectively, of the AP2/EREBP domain of the HcDREB2. Both of these residues might play important roles in determining the specificity of the DNA-binding domain [10, 30]. However, as reported in previous studies in rice and barley, the valine at amino acid residue 14 of the AP2/EREBP region may have a decisive effect on the specificity of the DNA-binding domain [31, 32].

Conclusions

We successfully cloned a putative DREB gene (HcDREB2) from H. compressa using the RACE-PCR method. The 1296-bp long HcDREB2 gene encoded a putative protein that consisted of 264 amino acid residues. HcDREB2 shared the highest sequence identity with the DREB2 gene in sorghum. The expression of HcDREB2 was independent of ABA, but was inducible by low temperature as well as drought and salinity (i.e., high NaCl concentration) treatments. The results of a yeast one-hybrid assay showed that HcDREB2 directly bound the DRE cis-acting element to transactivate the expression of the downstream reporter gene. Our study has established a foundation for future research in exploiting stress tolerance mechanisms and molecular breeding of H. compressa and other species.

Methods

Plant material

The H. compressa cultivar 'Guangyi' was used in this study. The plants were maintained and propagated through vegetative cuttings: The mature stems (length >1 m) of H. compressa 'Guangyi' were selected and cut into two cuttings. The cuttings were inserted into 10-cm diameter plastic pots filled with soil, and one node of each cutting was buried in the soil. After shearing the leaves of nodes, one of every three cuttings was put into a conical flask (50 ml) with 25 ml of pure water. The conical flasks were put in a light growth chamber [28 °C/20 °C (day/night),12 h/12 h (day/night)] for 15 days before stress treatments.

Stress treatments

After the cuttings generated new roots and leaves (about 15 days after transplanting), the conical flasks were transferred to another light growth chamber (4 °C). For drought, salinity, and ABA treatments, the culture water was supplemented with 20 % PEG6000, 250 mM NaCl, and 100 ?M ABA, respectively. The tender leaves were sampled at 1, 2, 4, 6, 8, 12, and 24 h after treatments and were frozen in liquid nitrogen. Untreated plants were used as the controls.

cDNA cloning of DREB

The total RNA was extracted from collected samples using the standard TRIzol protocol (Invitrogen, Carlsbad, CA, USA). First-strand cDNA was then synthesized using the PrimeScript(TM) RT reagent (Takara, Shiga, Japan) and a poly(T)-adaptor primer. An alignment of the DREB genes of model plants such as Oryza sativa, Arabidopsis thaliana, Brachypodium distachyon, revealed the AP2/ERF domain was relative conservative. Accordingly, based on the conserved AP2/ERF sequences, a cDNA fragment of DREB from the 'Guangyi' cultivar was then PCR-amplified using the cDNA as template, and a degenerate primer pair (HcDREBF00 and HcDREBR00) was used to amplify the first fragment of the target gene from the cold-treated leaf samples (4 h after treatment; Additional file 2: Table S2). The PCR conditions were as follows: pre-heating at 94 °C for 3 min; 30 cycles at 94 °C for 30 s, 50 °C for 30 s and 72 °C for 1 min; and a final extension at 72 °C for 10 min. PCR products were separated by agarose gel electrophoresis, and the target DNA fragment was recovered using a gel extraction kit (Axygen, Corning, NY, USA). The recovered DNA fragments were then ligated into a pMD19-T vector (Takara). DNA fragments were sequenced at the Beijing Genomics Institute.

The full-length cDNA sequence was isolated using RACE-PCR. The 3'- and 5'- ends of the gene were amplified by using the 3'-Full RACE Core Set Ver.2.0 kit (Takara) and the 5'-Full RACE kit (Takara). For 3'-RACE PCR, the reaction conditions were as follows: pre-heating at 94 °C for 3 min; 30 cycles at 94 °C for 30 s, 50 °C for 30 s, and 72 °C for 1 min; and a final extension at 72 °C for 10 min. For 5'-RACE PCR, the reaction conditions were as follows: pre-heating at 94 °C for 3 min, 30 cycles at 94 °C for 30 s, 50 °C for 30 s, and 72 °C for 1 min; and a final extension at 72 °C for 10 min. DNA recovery and ligation were the same as described above.

Gene transcription analysis

Total RNA extraction and first-strand cDNA synthesis were conducted as described above. The transcription level of the HcDREB2 gene relative to ?-actin was determined by quantitative real-time reverse-transcriptase PCR (qRT-PCR). The qRT-PCR reactions were carried out in 96-well blocks in a BIO-RAD CFX96 Real-Time PCR system (Bio-Rad, Hercules, CA, USA). Each 20-?l reaction contained 2 ?l of cDNA reaction mixture, 0.4 ?l of ROX Reference Dye II, 10 ?l of 2× SYBR® Premix Ex TaqTM (Takara), 0.4 ?l of each primer (10 ?M), and 6.8 ?l of ddH2O. The reaction conditions were 30 s at 95 °C followed by 40 cycles of 95 °C for 5 s and 60 °C for 34 s. The dissociation curve was acquired by heating the amplicon from 60 °C to 95 °C. All qRT-PCR reactions were implemented in both technical and biological triplicates. In order to adjust results for background levels of gene expression, an internal control gene (?-actin) was used (Additional file 3). There are a number of common internal control genes used for qRT-PCR in plants, and these include 25 s ribosomal RNA (25S rRNA), glyceraldehyde 3-phosphate dehydrogenase (GAPDH), ?-actin, and ?-tubulin [33]. We used the 2-??Ct method [34] to calculate relative expression. And then SPSS (version 16.0; SPSS Inc., Chicago, IL USA) was used to conduct a one-way ANOVA, and a Duncan's new multiple range test was used to test for differences in means of the expression data while controlling for multiple comparisons.

Yeast one-hybrid system

We examined the transcriptional activation of HcDREB2 using the yeast one-hybrid system. The putative coding sequence of HcDREB2 was PCR-amplified (see above) and then inserted into a pGADT7-Rec AD cloning vector (Clontech, Mountain View, CA, USA) in order to construct the fusion-expression vector pGADT7-Rec-HcDREB. The wild-type and mutant-type of triple DRE cis-acting elements DREy and DREt, respectively, were separately inserted into the pAbAi vector to construct the fusion expression vectors DREy-pAbAi and DREt-pAbAi. The vectors pGADT7-Rec-HcDREB, DREy-pAbAi, and DREt-pAbAi were then together transformed into Y1H Gold yeast cells. The transformation pAbAi-p53?+?pGADT7-Rec-p53 was used as a positive control, pAbAi?+?pGADT7-Rec was used as a negative control, and pAbAi?+?pGADT7-DREB was used as a blank control. Yeast cells with these vector combinations were inoculated onto SD plates under appropriate selection regimes for at least 48 h at 30 °C.

Abbreviations

25S rRNA:

25 s ribosomal RNA

qRT-PCR:

quantitative real-time reverse-transcriptase PCR

RACE-PCR:

rapid amplification of cDNA end-PCR

Declarations

Acknowledgements

This work was supported by the National Basic Research Program of China (973 Program) (2014CB138705), the National Modern Grass Industry Technology System (No. CARS-35-05), and Sichuan Province Breeding Research grant (2011NZ0098-11).

Open AccessThis article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.

Additional files

Additional file 1: Table S1. Primer used in isolating HcDREB2 gene. (DOCX 16 kb)

Additional file 2: Table S2. Primer used in Real-Time PCR analysis. (DOCX 15 kb)

Additional file 3: Nucleotide sequence and deduced amino-acid sequence of HcDREB cDNA. (DOC 31 kb)

Competing interests

The authors declare that they have no competing interests.

Authors' contributions

X-QZ and XM conceived the project and designed the experiments. Y-XC and L-KH performed the experiments. Y-XC, L-KH, and H-DY wrote the paper. All authors discussed the results and commented on the manuscript. All authors read and approved the final manuscript.