Phylogeny, expression patterns and regulation of DNA Methyltransferases in early development of the flatfish, Solea senegalensis

Background

The identification of DNA methyltransferases (Dnmt) expression patterns during development and their regulation is important to understand the epigenetic mechanisms that modulate larval plasticity in marine fish. In this study, dnmt1 and dnmt3 paralogs were identified in the flatfish Solea senegalensis and expression patterns in early developmental stages and juveniles were determined. Additionally, the regulation of Dnmt transcription by a specific inhibitor (5-aza-2′-deoxycytidine) and temperature was evaluated.

Results

Five paralog genes of dnmt3, namely dnmt3aa, dnmt3ab, dnmt3ba, dnmt3bb.1 and dnmt3bb.2 and one gene for dnmt1 were identified. Phylogenetic analysis revealed that the dnmt gene family was highly conserved in teleosts and three fish-specific genes, dnmt3aa, dnmt3ba and dnmt3bb.2 have evolved. The spatio-temporal expression patterns of four dnmts (dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1) were different in early larval stages although all of them reduced expression with the age and were detected in neural organs and dnmt3aa appeared specific to somites. In juveniles, the four dnmt genes were expressed in brain and hematopoietic tissues such as kidney, spleen and gills. Treatment of sole embryos with 5-aza-2′-deoxycytidine down-regulated dntm1 and up-regulated dntm3aa. Moreover, in lecithotrophic larval stages, dnmt3aa and dnmt3ab were temperature sensitive and their expression was higher in larvae incubated at 16 °C relative to 20 °C.

Conclusion

Five dnmt3 and one dnmt1 paralog were identified in sole and their distinct developmental and tissue-specific expression patterns indicate that they may have different roles during development. The inhibitor 5-aza-2′-deoxycytidine modified the transcript abundance of dntm1 and dntm3aa in embryos, which suggests that a regulatory feedback mechanism exists for these genes. The impact of thermal regime on expression levels of dnmt3aa and dnmt3ab in lecithotrophic larval stages suggests that these paralogs might be involved in thermal programing.

DNA methylation is a key regulatory mechanism during embryonic development. Methylation normally occurs at CpG dinucleotides and modulates transcription cascades, genomic imprinting as well as genome stability and chromatin structure [1,2,3,4,5,6,7]. DNA Methylation is catalyzed by DNA methyltransferases (Dnmt) of the Dnmt1 and Dnmt3 families. In mammals, Dnmt1 is the most abundant enzyme and acts mainly as a maintenance methyltransferase to ensure the inheritance of methylation patterns during cell division [8] and it has a direct role on histone methylation [9, 10]. The Dnmt3 enzymes are more diverse (with three genes in mammals Dnmt3a, Dnmt3b and Dnmt3L) and are responsible for de novo DNA methylation in germ cells and in preimplantation embryos [8, 11, 12]. De novo methylation is an essential mechanism of plant and animal development, particularly during tissue differentiation when cells undergo epigenetic reprogramming to adopt a new phenotype [13, 14]. The identification of well-conserved Dnmt1 and Dnmt3 proteins in vertebrates including teleosts suggests that these regulatory pathways may be conserved across vertebrates [15]. However, the teleost specific whole genome duplication has increased the dnmt copy number and six dnmt3 paralogs have been identified in Danio rerio [15,16,17]. The consequences during development of the extra gene copies of dnmt in fish remains to be established.

Although some environmental conditions such as oxygen levels, diets or lighting can modulate DNA methylation patterns, temperature acts as a major epigenetic regulator in embryonic and larval stages of fish [18,19,20]. For example, higher global methylation levels of genomic DNA occur in fish from polar regions relative to those from tropical and temperate regions [21]. Moreover, temperature regime during early development in fish induces epigenetic reprogramming modifying muscle fibre formation and composition, which affects somatic growth in adults [18, 22]. Thermally-dependent programming of muscle growth has been reported in Salmo salar [23, 24], Gadus morhua [25], Dicentrarchus labrax [26, 27], Oncorhynchus mykiss [26], and D. rerio [28]. Recent studies have demonstrated that some of the effects on muscle of thermal programming are linked to changes in the methylation pattern of genes involved in myogenesis [29] establishing DNA methylation as a key regulatory mechanism of muscle development. Moreover, temperature can also affect sex differentiation by modifying methylation patterns of genes that are sexually dimorphic and by influencing endocrine regulation [7, 30,31,32,33]. Thus, the study of Dnmt genes and their regulation by environmental factors may be critical to understand and monitor epigenetic modulation of traits of high relevance for aquaculture.

The Senegalese sole is a flatfish of high interest for aquaculture. The physiological and morphological changes that drive the transition to a benthic mode of life occur early during development (12–20 days post-hatch) and are sensitive to environmental and nutritional factors [34]. Previous studies in sole demonstrated that different temperature regimes during the pelagic larval stage greatly influenced the growth trajectory of post-larval stages [35,36,37]. When premetamorphic larvae were reared at low temperatures (~15 °C), a drop in their digestive capacity occurred and protein metabolism was modified [35]. Muscle cellularity and the expression of genes involved in muscle development such as myogenin (myog) decreased as a consequence of increased promoter methylation [36, 37]. The differential expression of dnmt1 and dnmt3 genes was suggested to be essential for this modulation [37]. Moreover, modified development and skeletal muscle cellularity caused by the temperature regime during embryogenesis was also reported [38]. In addition to the effects on muscle, thermal cycles during larval rearing of fish can also change the sex ratio of the population [39]. All these data indicate the importance of methylation in modulating the plasticity of larval development and the involvement of Dnmts requires further study.

To better understand the role of methylation in the epigenetic regulation of Senegalese sole we: (i) Identified Dnmt-encoding genes in S. senegalensis; (ii) Characterized spatio-temporal expression patterns of Dnmts during larval development and in juvenile tissues; (iii) Used a methyltransferase inhibitor (5-aza-2′-deoxycytidine) to establish the regulation of dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1; and (iv) Evaluated the short-term effects of temperature regimes during larval lecithotrophic stages on dnmt gene expression.

Larval rearing and experimental trials

The samples of juvenile liver, spleen, brain, gills, intestine, head kidney, heart, skeletal muscle, and skin used in this work were obtained in a previously unrelated study [40]. For larval trials, fertilized eggs of Senegalese sole were obtained from CUPIMAR (San Fernando, Cadiz, Spain). Eggs were collected early in the morning (9:00 a.m.) and transferred to a 1000 mL measuring cylinder to separate buoyant (viable) from non-buoyant (non-viable) eggs. The number of eggs in each fraction was estimated using volumetric methods (1100 eggs mL⁻¹). Water temperature and salinity in the broodstock tank (20 animals; ratio 2 M:1F) during spawning were 18 °C and 32 ppt, respectively. Breeders were fed with polychaeta, mussels and squid.

To study the regulation of dnmt gene expression an inhibitor of Dnmt activity, 5-aza-2′-deoxycytidine (5-AzaCdR, Sigma Aldrich, Spain) was used. A stock of 5-AzaCdR was prepared by dissolving it in 0.01% DMSO to a final concentration of 100 mg/mL; it was stored in aliquots at −20 °C until use. Preliminary trials were performed with 5-AzaCdR and the concentration that did not affect the hatching rates was considered to be the optimal treatment dose. Embryos (in gastrula stage) were randomly distributed between fifteen 50 mL sterile-containers (100 embryos per container) and exposed to 10 μM and 50 μM 5-AzaCdR (five replicates per condition) or the vehicle, 0.01% DMSO (control). During 5-AzaCdR exposures, the embryos were incubated at 22 °C for 24 h and 100 rpm in a shaker (INFORS HT Unitron). Larvae were examined at hatching (0 days post-hatch (dph)), fixed in RNA-later for qPCR analysis and stored at −80 °C until use. In addition, some larvae were fixed overnight in 4% paraformaldehyde (PFA) at 4 °C, dehydrated in methanol and stored at −20 °C until used for whole-mount in situ hybridization (WISH) as previously described [41, 42].

To evaluate the effect of temperature on lecithotrophic larval stages (before mouth opening), fertilized eggs in gastrula (50% epiboly stage) were distributed into six 1 L beakers containing 750 ml of sea water (32 ppt) at an initial egg density of 2000 embryos L⁻¹. The incubation temperature was set at 16 °C for half of the beakers (INFORS HT Unitron) and 20 °C for the remaining ones (INFORS HT aerotron) although in the latter case the final average temperature recorded was 20.8 °C. Egg incubation was carried out by gently agitating the beakers at 100 rpm and the sea water was replaced daily by filtering the larvae through a 350 μm mesh net taking care not to damage them. Embryonic stages were classified following the guidelines reported for zebrafish in Kimmel, CB, et al. [43] due to the lack of a detailed staging series in sole. Larvae were sampled at different time points and fixed in RNAlater for gene expression analysis by quantitative PCR or 4% PFA for WISH analysis as indicated above. To compare equivalent larval developmental stages in the two thermal treatment groups, cumulative degree-hours (CDH) was used to establish the sampling times. CDH was calculated as follows: [(average treatment temperature - T₀) × time (in hours)], where T₀ is the threshold temperature (considered to be 13 °C in S. senegalensis) [44] and the average treatment temperatures 16 and 20.8 °C. Moreover, larval growth as determined by total length, total area and yolk sac length were also measured in 25 photographed larvae per condition using ImageJ v1.47 software.

Sequence and phylogenetic analysis

Sequences encoding Senegalese sole dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 were identified after carrying out a search in the databases SoleaDB v3 and v4.1 [34]. The accession number of each transcript is indicated in Additional file 1. Sequences were downloaded and assembled using Seqmanv8.1 (Lasergene, DNASTAR) and edited using EditSeq. Multiple sequence alignments of sole dnmt and orthologues from other teleosts were performed using clustalW in MegAlignv8.1.

For phylogenetic analysis, sequences encoding methyltransferases from other vertebrates encoding for methyltransferases were retrieved from the ENSEMBL (www.ensembl.org) databases (Additional file 1). Maximum likelihood (ML) phylogenetic analysis was carried out using ProtTestv3.2 and the PHYLIP package. The best-fit model for sequence evolution was JTT + I + G + F. For the complete set of dnmts, −lnL was 68,834.14 with a gamma distribution shape parameter (four rate categories) of 0.947 and a proportion of invariable sites of 0.017 (Additional file 2). For the phylogenetic analysis of dnmt3 paralogs (Fig. 1), the lnL was 68,622.37 with a gamma shape of 0.83 and proportion of invariable sites 0.009. The PHYLIP package was then employed to estimate the bootstrap values using SEQBOOT (100 replicates) and the data were analyzed using the software PHYML. The consensus phylogenetic tree was then obtained (CONSENSE). Trees were drawn using Figtree v1.4.2 (http://tree.bio.ed.ac.uk/software/figtree/). Synteny analysis was carried out using Genomicus genome browser (http://www.genomicus.biologie.ens.fr/genomicus-79.01/cgi-bin/search.pl).

Phylogenetic relationships among the predicted amino acid sequences of dnmt3 genes in Senegalese sole and other vertebrates (see Additional file 1 for listed names, accession numbers and abbreviations of each species) using the Maximum Likelihood method. The tree was rooted using the dnmt3L sequence. Only bootstrap values higher than 70% are indicated on each branch. The scale for branch length (1.0 substitutions/site) is shown below the tree

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RNA isolation and RT-qPCR analysis

Pools of embryos (n = 20) and lecithotrophic larvae (n = 15) accounting for ~40 mg wet weight were homogenized using a Fast-prep FG120 instrument (Bio101) and Lysing Matrix D (Q-Bio- Gene) for 40s at speed setting 6. The numbers of embryos/larvae in the pools were always similar between conditions and replicates. Total RNA was isolated using an RNeasy Mini Kit (Qiagen). All RNA isolation procedures were carried out in accordance with the manufacturer’s protocol. In all cases, total RNA was treated twice with DNase I using an RNase-Free DNase kit (Qiagen) to eliminate genomic DNA contamination. RNA sample quality was checked by agarose gel electrophoresis, and quantified using a Nanodrop ND-8000 (Thermo Scientific).

Total RNA (1 μg) from each sample was reverse-transcribed using an iScript™ cDNA Synthesis kit (Bio-Rad) and following the manufacturer’s instructions. Real-time analysis was carried out on a CFX96™ Real-Time System (Bio-Rad) using Senegalese sole specific primers for each transcript (Table 1). Real-time reactions were performed in duplicate 10 μl reaction volumes containing cDNA generated from 10 ng of original RNA template, 300 nM each of specific forward and reverse primers, and 5 μl of SYBR Premix Ex Taq (Takara, Clontech). The amplification protocol used was as follows: initial 7 min denaturation and enzyme activation at 95 °C, then 40 cycles of 30s at 95 °C, 15 s at 68 °C and 30s at 72 °C (95 °C, 40 cycles of 95 °C for 15 s and 70 °C for 30s). After template amplification, a melt curve analysis was performed to confirm that a single PCR amplicon was generated. For larval experiments, all data were normalized using the geometric mean of ubiquitin (ub52) and beta actin (actb1) [45]. For juvenile tissues, 18S rDNA was selected as a suitable reference gene [40, 46]. In embryo experiments, the data were normalized using the geometric mean of 18S rDNA and actb1. Reference genes for normalization were selected according to their expression stability within each experiment. To estimate the PCR efficiency, a standard curve was generated for each primer pair based on 10-fold serial dilutions of cDNA transcribed from 100 to 0.01 ng of total RNA. Estimated efficiencies were 2.06, 2.01, 2.04 and 2.08 for dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1, respectively. Relative mRNA expression was determined using the comparative 2^-(∆∆Ct) method.

Whole-mount in situ hybridization (WISH)

To determine the ontogeny of the expression of the four dnmt genes during development, the larval samples (from 0 to 9 dph) obtained from standard larval rearing procedures, previously collected and described in [41] were used. These samples were designated as the control and were used in WISH analyses for comparison with the results of larval reared under different thermal regimes or treated with 5-AzaCdR.

To synthesize WISH probes for dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1, they were PCR amplified with targeted gene-specific primers. PCR reactions for WISH probe amplification were carried out using cDNA of a larval pool as template. PCR products were cloned into TOPO-TA vector and identity confirmed by cycle sequencing using a BigDye^® Terminator v3.1 kit (Applied Biosystems). Both sense and anti-sense probes were prepared using 20 U T3 or T7 polymerase in transcription buffer (Promega) with 1 μl digoxigenin-RNA labeling mix (Roche Diagnostics, Mannheim, Germany) as described in Campinho et al. [47]. PCR amplification conditions were: 94 °C for 2 min, followed by 30 cycles of 30s at 94 °C, 30s at 60 °C and 90s at 72 °C. Primers were designed using Oligo v6.89 software (Medprobe).

For WISH analyses, samples from chemical or temperature trials were fixed in 4% (wt/vol) paraformaldehyde in 1 × PBS overnight at 4 °C, dehydrated in methanol 100% and conserved at −20 °C until processing. Fixed embryos were depigmented and permeabilized (10 μg/ml proteinase K for 16 min at 37 °C) before being soaked in the digoxigenin-labeled probes as previously described [48]. Excess probe was then removed with successive washes in Hyb(−): 2 × SSC to 2 × SSC + 0.1% Tween-20 (2 × SSCT) and then washed twice for 30 min in 0.2 × SSCT at 68 °C followed by a final last wash in 1 × PBT at room temperature. Samples were pre-incubated for 3 h at RT in MABTr +10% sheep serum (Sigma-Aldrich)/2% Blocking solution (Roche) and then incubated overnight at 4 °C in 1/5000 anti-DIG serum (Roche) diluted in MABTr +10% sheep serum/2% blocking solution. For colour development, samples were washed in MABTr and then incubated in NBT/BCIP for color development. Incubation time was for 60–120 min (depending on the larval stage). For observation and storage, larvae were washed in PBS refixed in 4% PFA/1 × PBS for 20 min, washed in PBT solution and then transferred to glycerol. Twenty animals per experimental condition were used. Digital images were captured using a Leica DFC290 HD digital camera attached to a Leica DMIL LED inverted microscope.

Statistical analysis

Results are expressed as the mean ± standard deviation (SD). All data were checked for normal distribution with the Kolmogorov–Smirnov test as well as for homogeneity of variance with the Levene′s test and when necessary a log transformation was applied. Significant differences during embryonic development and in juvenile tissues were analyzed using one-way ANOVA. To assess if there were significant differences in gene expression and growth between temperature and embryonic or metamorphic stages, a two-way ANOVA was performed using time and treatment as fixed factors. When significant effects of temperature were identified, single ANOVAs were carried out. Statistical analyses were performed using SPSS v21 software (IBM Corp) and Statistix 9 (Analytical Software).

Identification and phylogeny of methyltransferases in S. senegalensis

A search for sequences encoding sole Dnmts in the SoleaDB [34] resulted in 25 putative transcripts, which corresponded to six unique transcripts that were named, dnmt1, dnmt3aa, dnmt3ab, dnmt3ba, dnmt3bb.1 and dnmt3bb.2 in agreement with Ensembl nomenclature for orthologues. Amino acid identity between the sole dntm3a paralogs was 75.1%. Lower amino acid sequence identity was observed between sole dnmt3b paralogs that ranged between 40.2 and 49.6% (Table 2). Amino acid sequence identities between dnmt1 and dnmt3 paralogs were in the range of 11.0–13.7%.

Phylogenetic analysis of the five dnmt3 genes identified two main clusters, referred to as dntm3a and dnmt3b (Fig. 1). The 3a cluster contained two well-supported clades named dnmt3aa and dnmt3ab and the 3b cluster contained three clades with the dnmt3bb.2 closer to dnmt3ba than dntm3bb.1. The dnmt3ba, dnmt3bb.2 and dnmt3aa were fish-specific lineages and dnmt3bb.2 and dnmt3aa were only identified in teleosts. Synteny analysis using the genomicus platform revealed that spotted gar (Lepisosteus oculatus), a basal ray-finned fish, possessed only one dnmt3a gene (identified as dnmt3aa) that clustered in the phylogenetic analysis within the dntm3ab clade close to tetrapods. The dnmt3ba and dntm3bb.1 were arranged in tandem in the spotted gar genome, an organization that was not conserved in teleostei although both paralogs had similar flanking genes (i.e. nol4l paralogs). The dntm3bb.1 and dntm3bb.2 were in tandem in teleostei.

Phylogenetic analysis using both the dnmt1 and dnmt3 sequences clustered the teleost and tetrapod orthologues separately at a large distance as expected based upon amino acid sequence identity (Additional file 2 and Table 2). The five dnmt3 clades remained clearly differentiated in this new analysis.

Expression patterns of dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 during embryonic and larval development

Quantification of mRNA levels for dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 from gastrula to hatching revealed that the transcript abundance of dnmt1 was not significantly modified. Transcripts for the dnmt3aa and dnmt3ab paralogs increased (P < 0.05) and dnmt3bb.1 decreased significantly (P < 0.05) (Fig. 2 and Table 3) from gastrula to hatch.

Expression levels of the dnmt1, dnm3aa, dnmt3ab and dnmt3bb.1 at gastrula, segmentation and hatching in embryos incubated at 16 °C and 20 °C. Data are expressed as the mean fold change (mean + SD, n = 3) from the calibrator group (gastrula). Different letters denote statistically significant differences among developmental stages for each gene (P < 0.05)

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The spatio-temporal expression pattern of dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 in developing embryos was examined by whole-mount in situ hybridization (WISH; Fig. 3, Table 3 and Additional file 3). Expression for dnmt1 was detected in the eyes, brain (mainly in the tectum), spinal cord and intestine at 0 dph (Fig. 3A, A’). At 1 dph, dnmt1 was also detected in the posterior edge of the tectum closely to the midbrain-hindbrain boundary, pharynx and intestine (Fig. 3B, B‘). The dnmt1 signal was weaker at 3 and 5 dph and was located mainly in the brain and spinal cord and at 9 dph a generalized low intensity signal was observed in the brain (Additional file 3). Expression of dnmt3aa was intense in the spinal cord, pronephric duct and somites at 0 dph (Fig. 3C, C‘) and by1 dph its expression was weaker in these organs and and it was also detected in the intestine, hindbrain and pharynx (Fig. 3D, E). As development progressed, dnmt3aa was mainly expressed in the brain, although by 9 dph it was only detected in the anus (Fig. 3F). The paralog dnmt3ab was predominantly observed in the hindbrain, midbrain (and tectum) and forebrain regions as well as in the inner nuclear layer, the inner plexiform layer and the ganglion cell layer of the developing eye at 1 and 3 dph (Fig. 3G,G‘,H,H’). A weak signal was also detected for dnmt3ab in the spinal cord and intestine up to 3 dph (Fig. 3G and Additional file 3). Expression of dnmt3bb.1 at 0 dph was observed in the forebrain-midbrain and midbrain-hindbrain boundaries, in the pectoral fin buds, pronephric duct, eyes and a lower intensity signal was also detected in the intestine and mouth primordium (Fig. 3I, I‘). The dnmt3bb.1 expression in 1 dph larvae was evident in the forebrain-midbrain and midbrain-hindbrain boundaries, pharynx, branchial arches, in the ciliary marginal zone of the eyes and in the intestine (Fig. 3J, J‘).

Temporal and spatial expression of methyltransferases. WISH signals for dnmt1 (A, B), dnm3aa (C-F), dnmt3ab (G, H) and dnmt3bb.1 (I, J) at different ages (0–9 dph) are shown. The ‘indicates the ventral orientation. Structures with an abundant signal are indicated with arrows: (an) anus; (ba) branchial arches; (br) brain; (cmz) ciliary marginal zone; (dm) dorsal midbrain; (ey) eye; (fb) forebrain; (fmb) forebrain-midbrain boundary; (gcl) ganglion cell layer; (hb) hindbrain; (inl) inner nuclear layer; (ipl) inner plexiform layer; (in) intestine; (mb) midbrain; (mhb) midbrain-hindbrain boundary; (mo) mouth; (pd) pronephric duct; (pf) pectoral fin buds; (ph) pharynx; (sc) spinal cord; (so) somite; (te) tectum. Scale bars are indicated (100 and 200 μm)

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Expression levels of dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 in juvenile tissues

The relative gene expression of the four methyltransferase coding genes was quantified by RT-qPCR in nine different tissues of juvenile sole (Fig. 4). The four genes were ubiquitously expressed in tissues although they were low abundance in liver (similar to the muscle that was used as the reference). In the case of dnmt3aa and dnmt3bb.1 transcripts were most abundant in the kidney, spleen, brain and gills.

Relative expression levels of the four dnmts in sole juvenile tissues: muscle, kidney, skin, intestine, heart, brain, spleen, liver and gills. Data were expressed as the mean fold change (mean + SD, n = 4) from the calibrator group (muscle). Different letters denote statistically significant differences among tissues for each gene (P < 0.05)

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Regulation of gene expression by 5-AzaCdR

To explore the transcriptional regulation of the four dnmt transcripts by 5-AzaCdR, embryos in gastrula were exposed to 10 μM and 50 μM of the chemical for 24 h and the expression of dnmts quantified by RT-qPCR (Fig. 5). In larvae from eggs exposed to 50 μM 5-AzaCdR, dnmt3aa mRNA levels increased significantly (P < 0.05). In contrast, a significant reduction in dnmt1 transcripts was detected in larvae exposed to 10 μM and 50 μM 5-AzaCdR relative to the control. No significant changes in the transcript abundance of dnmt3ab and dnmt3bb.1 were detected relative to the control. WISH analysis did not reveal a change in the expression pattern between the control and 5-AzaCdR treated sole (see Additional file 4).

Relative expression levels of the four dnmt genes in sole larvae exposed to 5-AzaCdR (10 μM and 50 μM) for 24 h (at hatch). “C” denotes the control untreated group. Data are expressed as the mean fold change (mean + SD, n = 4) from the calibrator group (control). Different letters denote statistically significant differences among treatments for each gene (P < 0.05)

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Effect of temperature on expression levels of dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 in larval lecithotrophic stages

To assess the effect of temperature on lecithotrophic larval stages (before mouth opening), embryos in gastrula were incubated at 20 °C or 16 °C for 45 and 115 h, respectively. The experimental design and sampling points are depicted in Fig. 6. To compensate for the delayed hatching and slower development and growth caused by lower water temperatures, cumulative-degree hours (CDH) were used to compare larvae at a similar developmental status. Comparison of the CDH values with larval total length, area and yolk sac length confirmed that this index gave a good estimate of developmental status (see Additional file 5). Two-way ANOVA showed that the expression of the four dnmt transcripts changed during development (Fig. 7). The dnmt1, dnmt3aa and dnmt3bb.1 mRNA levels decreased with age whereas dnmt3ab expression levels peaked at 273 CDH. Moreover, temperature had a significant effect on the expression of dnmt3aa and dnmt3ab transcripts that were higher abundance at 16 °C relative to 20 °C. Incubation temperature did not significantly modify the expression of dnmt3bb.1 and dnmt1 transcripts. WISH was also carried out to determine how temperature affected dnmt transcript distribution. Temperature did not affect the expression pattern of the dnmt1 and dnmt3 paralogs in sole larvae and the distribution was the same as described above (Additional file 5).

Experimental design for the evaluation of incubation temperatures during lecithotrophic stages in sole. The sampling points at 16 °C (blue) and 20.8 °C (orange) including the hours after incubation and the estimated CDH are indicated. A picture of the larvae sampled at each point is also shown. H denotes the hatching point

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Expression levels of the four dnmt genes in lecithotrophic stages of sole incubated at 16 and 20 °C. Cumulative-degree hour was used to normalize larval developmental stages between different temperature groups. Data are expressed as the mean fold change (mean + SD, n = 3) from the calibrator group (173 CDH at 20 °C). Asterisks denote significant differences between different temperature treatments for the same CDH (P < 0.05). Different letters denote statistically significant differences due to age for each gene (P < 0.05)

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The Dnmt enzymes play an essential role in the epigenetic regulation of gene expression in early developmental stages of vertebrates. A previous analysis of the zebrafish genome identified up to eight DNA methyltransferase genes belonging to the Dnmt1 (1), Dnmt2 (1), and Dnmt3 (6) families [15] The Dnmt1 and 3 are involved in the maintenance and de novo methylation of DNA, respectively whereas Dnmt2, which was not analyzed in the present study, has been related with RNA methylation. Phylogenetic analysis indicated that Dnmt1 represents a single and highly conserved locus in teleosts and tetrapods suggesting its function has also been conserved during vertebrate evolution. In contrast, Dnmt3 is highly divergent from the Dnmt1 gene and is clustered into two main clades (referred to as dnmt3a and dnmt3b) and five subclades with dnmt3aa, dnmt3ba and dnmt3bb.2 representing fish-specific gene lineages. The phylogenetic models in the present study are in general agreement with previous reports about Dnmt phylogeny [15,16,17]. However, the inclusion in the present study of all the identified Senegalese sole dnmt3 genes and the teleost paralogs available from ENSEMBL refined the analysis of dnmt3 subclades and fish-specific lineages.

The identification of at least five dnmt paralogs in the teleosts indicates that the diversification of the Dnmt3 lineage occurred early during vertebrate evolution during the proposed rounds of genome duplications, 1R, 2R and 3R (or the fish-specific whole duplication) that shaped their genomes [49]. Campos et al. [16] suggested that the dnmt3 genes diverged after the 2R and 3R duplications, however the conservation of dnmt3 in teleosts and the identification of three paralogs in spotted gar, a basal ray-finned fish [50], suggest that dnmt3a and dnmt3b clades might have arisen soon after the first genome duplication (1R). Later, before the tetrapod and teleost divergence, these lineages duplicated again (2R duplication) but only one paralog of each clade was retained in tetrapods. The 3R or fish-specific genome duplication gave rise to new paralogs but only five (two of which (dnmt3aa and dnmt3bb.2) are teleost-specific) were retained. Intriguingly, dnmt3bb.1 shares higher sequence identity and phylogenetic proximity with dnmt3ba than dnmt3bb.2 even though both dnmt3bb-like paralogs are arranged in tandem in the genome of some teleosts (e.g. stickleback, tetraodon, tilapia and zebrafish) suggesting they shared a common origin. The rapid divergence of dnmt3b paralogs in fish could be explained by the acquisition of an N-terminal calponin homology domain in dnmt3ba and dnmt3bb.2 paralogs, as previously suggested, although little is known about its functional significance [15]. Moreover, lineage-specific duplications explain the occurrence of additional methyltransferases in some other species such as zebrafish that has two paralogs (dnmt3 and dnmt5) within the subclade dntm3bb.2.

Methyltransferases are highly regulated during early development in order to tightly control expression cascades. Previous studies in D. rerio and Carassius auratus reported a higher abundance of dnmt1 mRNA levels in early embryonic stages from cleavage to mid-blastula and a reduction close to hatch [51,52,53]. Our expression data reveal a similar expression profile for sole dnmt1 during development although no significant differences were detected. The inverse correlation previously reported between dnmt gene expression and global DNA methylation levels has led to the suggestion that they may be maternal transcripts that direct methylation patterns in early stages [52]. An overview of dnmt expression patterns across teleosts suggests a conserved function in development. For example, dnmt1 has a similar expression pattern in intestine, exocrine pancreas and retina of developing sole and zebrafish (72 h post-fertilization) [10]. A similar situation is observed with dnmt3a and dnmt3b paralogs. Both dnnmt3aa and dnmt3ab increase and dnmt3bb.1 decrease in abundance in sole from gastrula to hatch. In zebrafish embryos RNA-seq data reveals that up to 24 hpf both dnmt3a paralogs increase in expression whereas the four dnmt3b genes gradually decrease [53, 54].

WISH in sole larvae revealed that dnmt’s had a distinct spatio-temporal expression pattern (Table 3) supporting the hypothesis that they play different roles in tissue differentiation. The tissue distribution of dnmt3ab and dnmt3aa during sole development suggests that subfunctionalization of these paralogs probably occurred. In contrast, the zebrafish, dnmt3aa and dnmt3ab had a similar, ubiquitous expression pattern in the brain, pharyngeal arches, pectoral fin buds, intestine, swim bladder and eye, although dnmt3aa expression was specific to the pronephric duct until 96 hpf [6, 14]. Interestingly, this is the first time that of dnmt3aa has been localized in the somites of a teleost fish and suggests it has a direct role in muscle differentiation and could be a putative candidate marker for epigenetic reprograming strategies with impact on growth and flesh quality in aquaculture. The expression pattern of sole dnmt3bb.1 is similar to the ortholog dnmt4 in zebrafish with a notably restricted expression in the lens epithelium and ciliary marginal zone [6, 14, 54] and a possible role in the differentiation and maintenance of the hematopoietic stem and progenitor cells lineages has been proposed [6, 55].

In addition to their role in early fish development, these dnmt genes have also been detected in varying abundance in adult tissues. For example, the dnmt1 and dnmt3b paralogs were detected in a range of organs although they were mainly expressed in the gonads [17, 51, 53]. In contrast, both dnmt3a paralogs were ubiquitously expressed in adult tissues with a higher expression in brain and reduced expression in muscle [17, 53, 54]. The high expression of Dnmt genes in gonads has been linked to their role in maintenance of, and de novo methylation during gametogenesis [17]. In our study, the gonads were not evaluated but the four dnmt genes were expressed in brain and other organs with high levels of proliferation and involved in hematopoiesis such as the kidney, spleen or gills (Table 3). The higher expression of dnmt genes in other tissues than muscle suggests that dnmt1, dnmt3a paralogs and dnmt3bb.1 play an active role in the regulation of cellular differentiation and methylation patterns in these adult tissues. Further research will be necessary to identify the precise role of each paralog.

The Dnmt inhibitors such as 5-azaC, and its deoxy analogue 5-azaCdR have been proposed as a tool to examine the epigenetic regulation of genes by environmental factors in fish [56]. Both inhibitors impose global DNA hypomethylation and DNA damage in cells although they can also exert drug-specific actions on cell viability, protein synthesis, the cell cycle and gene expression [57, 58]. In tumor cell lines, in vitro exposures to 5-azaCdR reduced dnmt1 and dnmt3b mRNA expression and protein levels, and to a lesser extent dnmt3a [58,59,60,61]. The depletion in Dnmt1 was reported to be proteasome-mediated since it started even earlier than the incorporation of 5-azaCdR into DNA and the formation of aza-Dnmt-DNA adducts [62]. Although depletion of Dnmt’s is regularly observed in Dnmt inhibition studies, buffalo skin fibroblast cells exposed to 5-azaC decreased dnmt1 but increased dntm3a and dntm3b mRNA levels at the highest 5-azaC concentrations [63]. Moreover, dnmt1, dnmt3aa and dnmt3bb transcript abundance increased at high doses (2 mM) of 5-azaC in medaka embryos indicating that protein depletion may be associated with transcriptional up-regulation of the genes [64]. In our study, dntm1 was down-regulated and dntm3aa was up-regulated by high concentrations of 5-azaC (50 μM) suggesting that regulatory feedback may compensate for the inhibition of Dnmt activity. Since the dnmt genes exhibit variable spatio-temporal expression patterns in larvae, the impact of 5-azaC on larval reprogramming will likely depend on the timing and dose administered.

The inability of poikilotherms to regulate their temperature explains why changes in environmental temperature can profoundly influence the life cycle, including development of such animals. Temperature modulates larval phenotype by influencing metabolic rate, growth, energy stores, and sex determination and muscle development presumably through epigenetic mechanisms [19]. In this study, fertilized eggs were incubated at two temperatures within the physiological range at which spontaneous spawning occurs in the wild and in captivity [65]. An inverse relationship between the incubation temperature and development was observed as has previously been reported in several fish species including sole [38, 66,67,68,69]. A previous study in S. senegalensis using different incubation temperatures until hatch showed that temperature modified growth and muscle cellularity of benthic post-larvae [38]. Our study revealed that both dnmt3aa and dnmt3ab mRNAs were up-regulated in lecithotrophic larvae maintained at 16 °C relative to those maintained at 20 °C. The observation that somite-specific dnmt3aa was highly responsive to temperature may indicate that this paralog mediates the previously described modifications in methylation and myogenesis in sole cultured at different temperatures [37, 38]. In zebrafish, incubation temperatures also caused stage-dependent modifications in dnmt3 paralog expression during embryonic development although they were not detected specifically in muscle [17]. Further work is required to identify modified gene expression linked to a specific phenotype but the present results on Dnmt have high potential for the aquaculture industry. Manipulation by temperature or other parameters of Dmnt represents a tool that can easily be used to enrich genetic breeding programs, and target muscle reprograming with implications for subsequent generations through the primordial germ cells [19, 32].

This study identified dnmt1 and five dnmt3 paralogous genes in sole. Phylogenetic analysis revealed a high degree of conservation of the dnmt gene family in teleosts, with dnmt3aa, dnmt3ba and dnmt3bb.2 resulting from fish-specific duplications. Clear spatio-temporal differences in dnmt1, dnmt3aa, dnmt3ab and dnmt3bb.1 expression profiles were detected in embryos, early larvae and juveniles. Moreover, expression of all dnmt genes decreased during larval development reinforcing their likely role in controlling cellular differentiation and development of larval tissues and organs. The Dnmt inhibitor 5-azaC modified expression of dntm1 and dntm3aa and revealed as a useful tool to evaluate the impact of methylation during early sole development. Finally, the upregulation of dnmt3aa, the somite-specific isoform, and dnmt3ab at low incubation temperatures, identifies the paralogs as target Dnmt’s for epigenetic reprograming in this species.

5-AzaCdR:

5-aza-2′-deoxycytidine

an:

Anus

BCIP:

Bromo-chloro-indolyl-phosphate

bh:

Branchial arches

br:

Brain

CDH:

Cumulative degree-hours

cmz:

Ciliary marginal zone

dm:

Dorsal midbrain

DMSO:

Dimehtylsulfoxide

dph:

Days post-hatch

ey:

Eye

fb:

Forebrain

fmb:

Forebrain-midbrain boundary

glc:

Ganglion cell layer

hb:

Hindbrain

hpf:

Hours post-fecundation

in:

Intestine

inl:

Inner nuclear layer

ipl:

Inner plexiform layer

MAB:

Malic acid buffer

MABTr:

MAB + 0.1% TritonX-100

mb:

Midbrain

mhb:

Midbrain-hindbrain boundary

mo:

Mouth

NBT:

Nitro blue tetrazolium

pd.:

Pronephric duct

pf:

Pectoral fin buds

PFA:

Paraformaldehyde

ph:

Pharynx

sc:

Spinal cord

so:

Somite

te:

Tectum

WISH:

For whole-mount in situ hybridization

We thank all the bodies that funded this research and the technicians involved in the analysis and running the animal experiments and also CUPIMAR that made the fish trials possible.

Funding

This research has been funded by INIA and EU through the FEDER 2014–2020 “Programa Operativo de Crecimiento Inteligente” project RTA2013–00023-C02–01 and project Algae4A-B from the UE H2020 research and innovation programme under the Marie Skłodowska-Curie grant agreement No 691102. M. A. Campinho is a recipient of a FCT Investigator grant (IF/01274/2014).

Availability of data and materials

The datasets used and/or analysed during the current study are available from the corresponding author on reasonable request.

Authors and Affiliations

1. IFAPA Centro El Toruño, Junta de Andalucía, Camino Tiro Pichón s/n, 11500 El Puerto de Santa María, Cádiz, Spain

   Joana Firmino, Carlos Carballo, Paula Armesto & Manuel Manchado

2. Comparative Molecular Endocrinology Group, Marine Science Centre (CCMAR), Universidade do Algarve, 8005-139, Faro, Portugal

   Joana Firmino, Marco A. Campinho & Deborah M. Power

Contributions

JF, CC, MAC and PA conducted experiments, laboratory analysis and analysed results. MM and DMP designed experiments and conceived the project. All authors read and approved the final manuscript.

Corresponding author

Correspondence to Manuel Manchado.

Ethics approval

All procedures were authorized by the Bioethics and Animal Welfare Committee of IFAPA and given the registration number 06–11–15-337 by the National authorities for regulation of animal care and experimentation.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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