- Research article
- Open Access
The 2HA line of Medicago truncatulahas characteristics of an epigenetic mutant that is weakly ethylene insensitive
- Sergey Kurdyukov1, 4,
- Ulrike Mathesius2,
- Kim E Nolan1,
- Michael B Sheahan^1,
- Nicolas Goffard2, 5,
- Bernard J Carroll3 and
- Ray J Rose1Email author
© Kurdyukov et al.; licensee BioMed Central Ltd. 2014
- Received: 20 February 2014
- Accepted: 12 June 2014
- Published: 21 June 2014
The Medicago truncatula 2HA seed line is highly embryogenic while the parental line Jemalong rarely produces embryos. The 2HA line was developed from one of the rare Jemalong regenerates and this method for obtaining a highly regenerable genotype in M. truncatula is readily reproducible suggesting an epigenetic mechanism. Microarray transcriptomic analysis showed down regulation of an ETHYLENE INSENSITIVE 3-like gene in 2HA callus which provided an approach to investigating epigenetic regulation of genes related to ethylene signalling and the 2HA phenotype. Ethylene is involved in many developmental processes including somatic embryogenesis (SE) and is associated with stress responses.
Microarray transcriptomic analysis showed a significant number of up-regulated transcripts in 2HA tissue culture, including nodule and embryo specific genes and transposon-like genes, while only a few genes were down-regulated, including an EIN3-like gene we called MtEIL1. This reduced expression was associated with ethylene insensitivity of 2HA plants that was further investigated. The weak ethylene insensitivity affected root and nodule development. Sequencing of MtEIL1 found no difference between 2HA and wild-type plants. DNA methylation analysis of MtEIL1 revealed significant difference between 2HA and wild-type plants. Tiling arrays demonstrated an elevated level of miRNA in 2HA plants that hybridised to the antisense strand of the MtEIL1 gene. AFLP-like methylation profiling revealed more differences in DNA methylation between 2HA and wild-type. Segregation analysis demonstrated the recessive nature of the eil1 phenotype and the dominant nature of the SE trait.
We have demonstrated that EIL1 of Medicago truncatula (MtEIL1) is epigenetically silenced in the 2HA seed line. The possible cause is an elevated level of miRNA that targets its 3’UTR and is also associated with DNA methylation of MtEIL1. Down regulation of MtEIL1 makes it possible to form nodules in the presence of ethylene and affects root growth under normal conditions. Segregation analysis showed no association between MtEIL1 expression and SE in culture but the role and mechanism of ethylene signalling in the process of plant regeneration through SE requires further investigation. The work also suggests that epigenetic changes to a particular gene induced in culture can be fixed in regenerated plants.
- 2HA seed line
- Somatic embryogenesis
- Ethylene insensitivity
- Root growth
- Medicago truncatula
- DNA methylation
Forward genetics is a way to gain new knowledge about gene function. However, weak phenotypes are often overlooked. The reverse genetics approach is a way to look more closely at possible phenotypes especially if data about mutated genes are available. The Medicago truncatula seed line, 2HA differs from its wild type (WT) progenitor line, Jemalong, in its ability to produce greatly increased numbers of somatic embryos in tissue culture . Investigation of gene expression points toward candidate genes that are involved in the process of somatic embryogenesis. The ability to produce somatic embryos is often species- and even cultivar-dependent, and the search for key genes in this process has revealed several genes that stimulate or inhibit SE in different plant species [2–8].
Ethylene is a plant hormone that is involved in different developmental processes: root elongation , lateral root emergence , nodulation [11, 12], senescence , fruit ripening  and SE [15, 16]. The ETHYLENE INSENSITIVE3 (EIN3)-like (EIL) gene family in Arabidopsis has been well-characterised using mutants and overexpression experiments. Mutations in EIN3 and EIL1 genes cause strong ethylene insensitivity, whereas mutations of other EIL family members are related to weaker phenotypes, supporting the idea that they are playing an accompanying role during ethylene responses . The triple response test was developed in order to distinguish mutants impaired in response to ethylene. It involves germination of seedlings in the presence of exogenous ethylene or its precursor 1-aminocyclopropane-1-carboxylic acid (ACC). Under these conditions, wild type seedlings display the triple response phenotype of shorter, thicker, and overly-bent hypocotyls. The widely accepted model of ethylene signalling indicates that in the absence of ethylene, EIN3 and other EIL proteins are continuously degraded. The binding of ethylene to its receptor complex leads to stabilisation of these proteins and elicits the downstream ethylene response. EIN3 and EIL1 are transcription factors that bind to promoters of ERF genes and regulate their expression. ERFs are also transcription factors, and they in turn promote ethylene responses by binding to promoters of other genes .
In this study, genes showing differential expression in microarray studies of 2HA and Jemalong four week old cultures were analysed with about 117 genes up-regulated greater than 1.5 times in 2HA. Only a few genes were down-regulated in 2HA. One of these, an EIN3-like gene (MtEIL1) showed a large decrease in expression in 2HA plants. Different aspects of ethylene insensitivity of the 2HA line have been analysed, and weak ethylene insensitivity has been confirmed. Analysis of phenotypic segregation, absence of mutations in its DNA and presence of other phenotypes in 2HA prompted us to further investigate epigenetic differences between 2HA and wild type. Tissue culture is known to be able to induce a number of genomic perturbations and epigenetic mutations . We found many examples of differential DNA methylation between 2HA and the WT plants using an arbitrarily-primed, methylation-sensitive PCR profiling method called Amplified Methylation Polymorphism (AMP) . Differences in methylation of the MtEIL1 gene between the 2HA and WT plants were also found. The methylation of MtEIL1 in 2HA was associated with increased abundance of a small RNA with homology to the 3’ region of MtEIL1. Based on all the data accumulated, we propose that the 2HA seed line is an epigenetic variant of WT Jemalong, and some of its distinctive phenotypes are most likely due to down-regulation of MtEIL1. The proposed epigenetic nature of the phenotypes is discussed.
Comparison of gene expression between embryogenic and non-embryogenic tissue cultures
Transcripts that were up- or down-regulated at least 2 times were analysed in more detail (Additional file 1: Table S1 and Additional file 2: Table S2). The annotation and expression of each of these transcripts was checked against available data on the Medicago truncatula Gene Expression Atlas (http://mtgea.noble.org/v2/index.php) , which shows gene expression in different plant organs and under various experimental conditions. The corresponding TC or EST sequences were retrieved and predicted amino acid sequences from these were used in BlastP searches to find predicted protein domains and matches to other known proteins (Additional file 2: Table S2). Analysis using the M. truncatula Gene Expression Atlas indicated that of the 34 transcripts upregulated in 2HA, 18 were classed as legume-specific, 15 showed high expression in nodules with four of these classed as nodule-specific, ten showed high expression in developing seed and, three were predicted transcription factors. Seven predicted transcripts encoded transposase-like proteins containing either a hAT family dimerisation and/or a BED zinc finger domain. The hAT family dimerisation domain is found in transposases belonging to the hAT superfamily . The BED zinc finger domain is a DNA binding domain also found in transposases and in chromatin-boundary-element binding proteins .
Validation of microarray results by RT- qPCR
Both of the predicted down-regulated transcripts demonstrated nearly identical results in RT- qPCR (probes Mtr.10439.1.S1_at and Mtr.1670.1.S1). PCR amplification with different combinations of primers (F1-F6/R1-R6, Additional file 2: Table S4) followed by sequencing revealed that the two transcripts were part of the same EIN3-like gene (Additional file 3: Figure S1) which we called MtEIL1 and deposited as accession number GQ914771 in NCBI GenBank. This EIN3-like gene was also listed as down-regulated in 2 week 2HA embryogenic calli but was not studied in detail . The 2 week stage is an early callus phase when the induction of SE is starting while week 4 is when the transition from callus to embryogenesis is occurring [25, 26].
Analysis of the EIN3-like gene MtEIL1and its protein
Weak ethylene insensitivity of the 2HA line
Given the down-regulation of MtEIL1, we examined the 2HA line for phenotypes associated with ethylene insensitivity. We also examined sickle mutants of M. truncatula in parallel to WT and 2HA, as these have very strong ethylene-insensitive phenotypes. The sickle mutation in the EIN2 gene, biochemically, is upstream of EIL genes in the ethylene response pathway in M. truncatula.
Ethylene insensitive phenotypes of 2HA line compared to WT Jemalong and strong ethylene insensitive mutant sickle
Ethylene triple response tests
Main root length is increased at 7 days after germination
Nodulation on 1 μM ACC
Callus growth on 10 μM ACC
Additional file 2: Table S3
Increase of short lateral roots (<5 mm) on 1 μm ACC
Increase of long lateral roots (>5 mm) on 1 μm ACC
Segregation analysis of the 2HA phenotypes
The molecular basis of the 2HA phenotypes
Data from AMP PCR, together with the absence of a nucleotide mutation in MtEIL1, prompted a detailed examination of DNA methylation in MtEIL1. We compared methylation of MtEIL1 and its promoter in leaves of 2HA and Jemalong. Genomic DNA was digested by methylation-sensitive endonucleases and used for qPCR with primers surrounding their sites. We found no differences between WT and 2HA in methylation of the promoter of MtEIL1. Methylation of 2HA and WT Jemalong coding regions was different, with strong methylation in the case of 2HA but not Jemalong (Figures 9b,c). Bisulphite sequencing using DNA from Jemalong and 2HA plants confirmed methylation profiling demonstrated in the digestion based assay and showed additional methylation in the 2HA coding region but not in Jemalong (Additional file 3: Figure S7).
Ethylene insensitivity of 2HA plants
Down-regulation of an EIN3-like transcript in 2HA plants was found in all organs checked and led to further investigation of this gene and possible phenotypes caused by the absence of its expression. This transcript, GQ914771, is a homologue of Arabidopsis EIN3 and we called it MtEIL1. The family of EIL genes in Arabidopsis is involved in the ethylene response pathway. Among six EIN3–like genes in Arabidopsis, only two (EIN3 and EIL1) are crucial for the ethylene response and double ein3/eil1 mutants demonstrate complete ethylene insensitivity. At the same time, several other mutants of Arabidopsis were found that demonstrated weak ethylene insensitivity . The EIN3 and EIN3-like gene function in Arabidopsis is mainly regulated through the stability of the corresponding proteins .
The 2HA line demonstrated weak ethylene insensitivity compared to WT plants (Tables 1 and Additional file 2: Table S3, Figures 5 and 6), most probably due to down-regulation of the MtEIL1 gene. Most interesting is the ability to form nodules in the presence of an exogenously added ethylene precursor (Figure 6a). The difference between 2HA and WT is not as pronounced in standard growth conditions except for the increased main root elongation of seven day old seedlings. Similar to Arabidopsis ethylene-insensitive mutant nomenclature, we propose that the 2HA seed line has characteristics of a Medicago eil1 mutant.
Endogenous concentrations of ethylene are low and the whole plant system is well tuned, so small differences (Figure 6) can lead to complete inhibition of nodulation (in the case of 1 μM ACC for WT plants) or to a two times increase in the number of nodules (in the case of 0.1 μM AVG). Ethylene possibly works to control the number of infection sites, so mild attenuation of its action leads to an increased number of nodules without affecting the general system of nodule development [11, 28]. The more pronounced widening of the nodulation zone by AVG in wild type compared to 2HA is reminiscent of the inability of AVG to widen the nodulation zone in the ethylene insensitive sickle mutant . Weak ethylene-insensitivity could be an advantage for plants as they could form nodules even under stress conditions when the ethylene concentration is elevated. The effects of ethylene on lateral root initiation and emergence was less pronounced, but showed significant relative differences between wild type and 2HA. Differential effects of ethylene on lateral root initiation and emergence have been observed in Arabidopsis, where high concentrations of ACC inhibited the initiation of lateral root primordia but promoted their elongation. Low ACC concentration had opposite effects, suggesting a narrow window of optimum ethylene concentration . We found that in wild type plants, a relatively high (1 μM) concentration of ACC caused a significant increase in short lateral roots, but a non-significant increase in longer lateral roots, opposite to the effect in Arabidopsis, suggesting different optimum levels of ethylene between Medicago and Arabidopsis. Surprisingly, AVG had a similar effect to ACC on short lateral numbers, underlining the importance of ethylene acting in a strict concentration window in the root. The 2HA line showed a different response to ACC compared to the wild type, with significant increase in elongated but not short lateral roots. This could indicate a different optimum window of ethylene in 2HA compared to wild type plants.
Gene expression differences between embryogenic calli 2HA and non-embryogenic calli WT
Transcription profiling obtained through microarrays revealed a relatively small number of differentially expressed genes. At the same time there was general up-regulation of transcription in 2HA compared to WT (Figure 1) that could have a cumulative effect on cell fate and mediate further developmental changes . Up-regulation of transposon-like genes with BED and hAT domains that we called BEDHAT1 and BEDHAT 2 (BH1 deposited in NCBI GenBank as accession KF679497, putative transposase), found in 2HA culture (Figure 2), could be an indicator of the general “openness” of chromatin in 2HA tissue cultures . Interestingly, BH2 is active in zygotic embryogenesis and BH1 is up-regulated during nodule formation and zygotic embryogenesis according to the Medicago Gene Expression Atlas . Earlier in culture in the early callus phase (2 weeks) there were more up-regulated and down regulated genes at the 2 times cut-off, but over 99.5% of probe sets were similar in 2HA and Jemalong. However there were transposases and nodulins up-regulated and the EIN3-like gene was down-regulated . It does seem that arrays over weekly periods (as in Figure 2 for individual genes) would provide additional insights.
Among 34 transcripts that showed ≥2 fold up-regulation in 2HA embryogenic 4-week calli we identified several embryo-specific genes, even though their expression is probably limited to a small number of cells. These genes could be good markers for further investigation of SE. Several embryo-specific genes and a number of genes that are preferentially expressed during zygotic embryogenesis as well as during nodule formation (Additional file 1: Tables S1 and Additional file 2: Table S2) were also up-regulated in 2HA tissue cultures or in SE. This suggests a commonality between these three processes: zygotic embryogenesis, somatic embryogenesis and nodule formation. In all these cases, re-differentiation is required and a particular level of pluripotency or “stemness” is necessary.
Relationship between the SE phenotype of 2HA and MtEIL1expression
F2 plants from a cross between 2HA and WT with a high level of MtEIL1 expression are still able to develop somatic embryos (Figure 8). Therefore, low MtEIL1expression does not appear to be an absolute requirement for SE. The development of the 2HA seedline involved regeneration of plants from somatic embryos in tissue culture while the segregation of SE and eil1 traits were limited to tissue culture studies, so the success rate of plant regeneration from somatic embryos is not known. As the original 2HA line has a low level of MtEIL1 expression, there is still a possibility that modified ethylene signalling is playing a role in the process of 2HA development from somatic embryos and further investigations are required in order to find why these two phenotypes co-exist in the 2HA seed line. An interesting observation in B. napus SE , is that from four plant lines which demonstrated SE, the most highly embryogenic was the line that also demonstrated delayed senescence of flowers – an ethylene insensitivity phenotype. We have observed that 2HA has delayed senescence of petals. It has also been shown in Arabidopsis that osmotic stress induces ethylene in leaves, without up-regulation of EIN3, and meristemoids are induced . Ethylene has been shown to be an activator of the transcription factor MtSERF1 that is essential for SE in M. truncatula as well as in soybean and Arabidopsis . As the signalling through MtEIL1 is questionable in 2HA it could occur through the closely related MtEIL2 whose expression is not down-regulated.
Toward molecular characterisation of the 2HA seed line - the MtEIL1gene
The MtEIL1 protein clusters together with MtEIL2 and their closest homologs are two EIL proteins from mung bean (Figure 4). These two proteins are probably equally involved in the ethylene signal transduction pathway as proposed in the original paper . A similar pair is formed by EIN3 and EIL1 from Arabidopsis. In Arabidopsis, EIL1 works co-operatively with, but distinctly from EIN3 to regulate a myriad of ethylene responses . Protein alignment shows that both MtEILs contain the same functional domains that have been previously found (Additional file 3: Figure S2) in mung bean and Arabidopsis . The only difference found between MtEIL1 and MtEIL2 is in the terminal domain where they have nine and six Gln/Asn residues respectively.
The MtEIL1 gene and its promoter were sequenced but no mutations were found. Digestion with methylation-sensitive restriction endonucleases revealed differences in methylation between 2HA and Jemalong plants for the MtEIL1 gene. DNA methylation affected the coding region of MtEIL1 in 2HA but not the promoter. This was associated with increased abundance of a small anti-sense RNA in 2HA as demonstrated by hybridisation to a tiled array of MtEIL1, and RT-qPCR confirmed the existence of this small RNA. It is possible then that the driver of MtEIL1 down regulation is a miRNA that targets the 3’-UTR and causes the down-regulation. To be unequivocal with this latter conclusion an anti-miRNA approach would be required.
DNA methylation analysis and the epigenetic nature of 2HA phenotypes
Differences in DNA methylation between Jemalong and 2HA genomes were obtained in the AMP experiment (Figure 9a). Even though AMP is able to sample only a small part of the genome, it was a good indicator of widespread differences in DNA methylation between WT and 2HA. At the same time, the AMP profiles were consistent with the isogenicity of 2HA and Jemalong genomes because no differences were found in profiles for undigested DNA. DNA methylation changes as a result of in vitro culture are well documented , but there is little work on changes in individual genes resulting in a phenotypic change. Though regions that are hypermethylated in 2HA (such as MtEIL1) are present, hypomethylated regions in 2HA may be responsible for the up-regulation of transposon-like genes (BH1 and BH2) found in 2HA culture. Global hypomethylation changes in reprogramming to somatic embryogenesis in pollen have been documented . Our observations are consistent with the origin of 2HA by selection from a regenerated plant that passed through a cycle of tissue culture [1, 31] and suggests that epigenetic changes in culture directed at specific genes can be fixed in regenerated plants.
Transcriptional gene silencing (TGS) and posttranscriptional gene silencing (PTGS) can interconvert during tissue culture . Their dominance and segregation in progeny are quite different from each other and not simply Mendelian in ratio. Such processes could be responsible for the appearance of the 2HA seed line.
Microarray-based transcription profiling revealed only one gene that was down-regulated >2 times in the 2HA seed line compared to WT but significantly more (34 genes) were up-regulated. Most of them are embryo and nodule specific genes as well as some transposon-like genes. There were no large scale changes observed in the karyotype. The methylation profiling revealed some differences in DNA methylation between 2HA and WT. Furthermore, hypermethylation of the MtEIL1 gene is associated with increased abundance of a small antisense RNA which targets the 3’- UTR region and likely acts to posttranscriptionally silence MtEIL1 expression. MtEIL1 down-regulation impacts on nodulation, root growth, root branching and other phenotypes, consistent with weak ethylene insensitivity. As signalling through MtEIL1 is questionable it could occur through the closely related MtEIL2 whose expression is not down-regulated. These observations are consistent with the origin of 2HA by selection from a regenerated plant that had passed through a cycle of tissue culture [1, 28] suggesting that the epigenetic changes in culture can be fixed in regenerated plants. Finally, segregation analysis indicates that the eil1 trait and SE are not directly linked.
Plant growth and tissue culture
Plant materials were obtained from glasshouse-grown plants. The glasshouse had a 14 h photoperiod and 23/19°C day/night temperature regime. Jemalong 2HA (2HA) was the highly regenerable seed line  and Jemalong and Jemalong A17 (a representative of WT cv Jemalong seed) were WT. The WT Jemalong rarely produce somatic embryos and no embryos were formed in this study. WT Jemalong and WT Jemalong A17 when tested in other studies were interchangeable e.g. Rose et al. . The standard tissue culture procedure was as described . Explants were cultured on P4 10:4 on agar plates for 3 weeks (10 μM NAA, 4 μM BAP) before transfer to P4 10:4:1 (10 μM NAA, 4 μM BAP, 1 μM ABA). Cultures were incubated in the dark. The time course of the developmental sequence of embryogenic calli has been previously documented [25, 26]. Dedifferentiation occurs in the first week and callus is visible at the end of week one and in the second, third and fourth weeks callusing continues and the induction processes for SE occur. At week 4 there is the beginning of transition from calli to embryo formation. This is where morphologically the 2HA and WT start to diverge.
Root growth and the ethylene triple response test
Seeds were soaked in concentrated H2SO4 for two min, washed in water and sterilised in diluted bleach (0.5% (w/v) of sodium hypochlorite) for 6 min, then washed three times in sterile water and spread on filter paper in Petri dishes with P40 media . Sixty to eighty seeds were used for each genotype. Seven days after germination the root length was measured. Tukey-Kramer tests confirmed (p < 0.05) that all three genotypes (Jemalong, 2HA and sickle) were significantly different. For the ethylene triple response measurements were made 4 days after germination. Bending of cotyledons was observed on P40 media and on P40 with 0.5 μm and 1 μm ACC. Cotyledons that formed an angle of < 90° in relation to the stalk were counted as bent. This experiment was repeated three times.
Nodulation and lateral root assays
Seeds of A17 (WT) and 2HA were scarified on sand paper, sterilized in 6% (w/v) sodium hypochlorite on a shaker for 10 min, washed five times in sterile water and plated on water agar plates. The seeds were left at 4°C for two days and then transferred to 25°C overnight for germination. Seeds were then transferred to Fåhreus medium  agar plates, five seedlings per plate, five plates per treatment (i.e. 25 seedlings per treatment). Seedlings were grown in a growth chamber for three days with a day/night cycle of 16 h/8 h, at 25°C with a light intensity of approximately 100 μE. A culture of Sinorhizobium meliloti strain 1021 was grown in Bergensen’s Modified Medium  in a shaking incubator at 28°C overnight on day 3 and adjusted to an OD600 of 0.1. Roots were transferred to Fåhreus medium agar plates containing either 1 μM ACC, 0.1 μM AVG or solvent (methanol at 1 μL/L) as a control on day 3. After a further 24 h incubation in the plant growth chamber to adapt to the altered hormone media, roots were inoculated with 10 μL of a culture of S. meliloti at the zone of emerging root hairs (i.e. on day 4 after germination). Plates were returned to the plant growth chamber (same conditions as above) and left to grow for four weeks.
Nodules were counted under a dissection microscope. Lateral root numbers were counted and classified as either of <5 mm or >5 mm length. The root length covered with nodules (first to last nodule along the root) was measured with a ruler. All data were statistically analysed using InStat version 3.06 for Windows (GraphPad Software). As most data were not normally distributed, comparisons were analysed by Kruskall Wallis tests with Dunn’s multiple comparison post tests.
mRNA microarray analysis
Total RNA was isolated from four weeks culture for three 2HA and three Jemalong samples using the RNAqueous™-4PCR Kit (Ambion, http://www.ambion.com/). Hybridisations were performed according to the Affymetrix manual (Affymetrix, http://www.affymetrix.com/). Data processing was performed as described earlier . Raw data were background corrected, normalized, summarized and log2 transformed using the GCRMA algorithm (ver. 2.2.0) using the affy package of the bioconductor software  with default parameters. Normalised data are provided in Additional file 1: Table S1. Differentially expressed genes were identified by evaluating the log2 ratio between embryogenic and non-embryogenic tissue culture in combination with a standard t-test.
Total RNA was isolated as for microarray analysis. cDNA was synthesised with SuperscriptII (Invitrogen, http://www.invitrogen.com/). PCR master mixes used Platinum Taq polymerase (Invitrogen) with the provided buffer and1.5 μM SYTO9 dye, primers at 0.4 μm and 3 mM dNTPs. A Corbett Rotor-Gene 6000 (Qiagen, http://www.qiagen.com/) machine was used to carry out real-time PCR. The qPCR cycling conditions comprised an initial denaturation at 95°C for 2 min followed by 40 cycles of 95°C for 10 s, 60°C for 30 s and 72°C for 30 s. Dissociation analysis (0.5°C step) was performed in every run and products checked by gel electrophoresis to ensure product uniformity. Analysis of data was performed using Q-Gene software . The GAPDH gene was used as a calibrator. GAPDH is a suitable reference gene for M. truncatula based on geNORM software  and our previous microarray and RT- qPCR studies on SE . Three biological repeats were carried out in triplicate. Sequences of primers are listed in Additional file 2: Table S4.
Amino acid alignment and phylograms
Full length amino acid sequences were aligned using ClustalX 2.0.10 . The phylograms were constructed from aligned sequences using the protein maximum likelihood, proml, programme in PHYLIP [Phylogeny Inference Package Version 3.69;  and drawn with Dendroscope .
Actively growing root tips (2 cm) from germinating seed were collected and placed on ice for 22 h. Root tips were fixed for 3 d in 3:1 ethanol:propionic acid in which 0.2% (w:v) ferric chloride hexahydrate was dissolved as a mordent. After fixation root tips were hydrolysed in 1 N HCl at 60°C for 6 min and stained in aceto orcein (1% (w:v) orcein in 45% (v:v) acetic acid) for 5 d. The 1 mm meristematic region was then treated with 1% (w:v) pectinase at 25°C for 30 min then 5 min in 45% (v:v) acetic acid. Squashes were carried out on a slide with 45% (v:v) acetic acid and the coverslip sealed with paraffin wax. Photgraphs were taken using a Zeiss Axiophot microscope and a Zeiss Axiocam HRc digital camera.
Isolation of the MtEIL1 promoter was performed using a modified gene walking technique (Clontech, http://www.clontech.com) where the first gene-specific primer was biotinylated. After the first round of PCR the resulting product was immobilised on Dynabeads M-280 (Invitrogen), washed with the buffer provided and used for the second round of PCR with nested primers. The sequence of the MtEIL1 promoter was deposited in NCBI GenBank as accession EU499308 (Additional file 3: Figure S1).
Genomic DNA was isolated from leaves of four Jemalong and four 2HA plants using the CTAB method . The Amplified methylation polymorphism (AMP) protocol for arbitrarily detecting DNA methylation variation in genomic DNA was that described in . To test for differential methylation within MtEIL1 in 2HA and Jemalong e.g. , DNA (10 μg) was digested overnight by AciI (New England Biolabs, http://www.neb.com) and cleaned through a PCR clean up column (Promega, http://www.promega.com). The DNA concentration was measured, adjusted and used for subsequent qPCR with primers that surround the digestion site (primer pairs F2/R2 and F4/R4). Normalisation was carried out using part of the MtEIL1 gene that does not have a site for these enzymes. Primers F5 and R5 were used and are closely adjacent to the investigated regions F2/R2 and F4/R4. The whole locus that contains all three fragments is shorter than 2 kb, is surrounded by AciI sites and is readily isolated. Undigested DNA was used in parallel and all products were checked on a gel plus melting curve analysis performed in order to demonstrate specificity of the product. Sequences of primers are listed in Additional file 2: Table S4.
For bisulphite sequencing, DNA was prepared using the MethylEasy™ Bisulphite Kit (Human Genetic Signatures, Australia, http://geneticsignatures.com/) from 3 week-old tissue cultures or from leaves in three biological repeats. Part of the MtEIL1coding region and promoter were amplified using several pairs of primers (Additional file 2: Table S4). PCR products were directly sequenced and methylation as detected by CpG > TpG conversion of CpG sites confirmed in 2HA, but no methylation was detected in Jemalong. The fragment amplified with bFor2 and bRev2 primers demonstrated the most differences in methylation.
Analysis of small RNAs
A 40-nucleotide MtEIL1 tiling array was custom built by LC Sciences (Houston, Texas, USA) with 20-nucleotide steps was hybridised with RNA from 2HA and wild-type callus culture for two weeks. RNA was extracted, labelled with the fluorophore Cy5 and hybridized to the array as previously described . A putative small RNA identified by microarray analysis was amplified by qPCR using an miScript PCR System (Qiagen) with a set of primers (M1 to M7 in Additional file 2: Table S4) that spanned the potential miRNA sequence. Gene specific primers were used together with adaptor primers provided with the miScript PCR System (Qiagen). The M5 primer was used for comparative studies of 2HA and Jemalong RNA isolated from 2 weeks old tissue culture (Figure 10b).
Availability of supporting data
All data sets supporting this article are available within the article and in additional files. The microarray data are deposited in the NCBI GEO repository with GEO accession number GSE58223 at http://0-www.ncbi.nlm.nih.gov.brum.beds.ac.uk/geo/query/acc.cgi?acc=GSE58223.
This work was funded by the Australian Research Council (CEO348212) through the ARC Centre of Excellence for Integrative Legume Research (CILR). We thank Mary Liu and S.J. Sim for technical assistance, Dr. Larry Croft for assistance with the tiling arrays, Dr. Feky Mantiri for assistance with calli growth analysis and Olga Berking for assistance.
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