We hypothesised that daily food availability times serve as an ‘epigenetic’ factor and affect reproductive physiology in continuously reproducing species. This we tested by measuring mRNA expression of genes coding for enzymes involved in DNA methylation–demethylation (dnmt, tet) and histone modification (hat1, hdac) in the hypothalamus, liver and gonads of male and female zebra finches that were paired for a year under 12 h light:12 h dark conditions with food availability restricted to 4 h in the morning (morning FA group) or evening (evening FA group), with controls provided with food ad libitum. The overall hypothalamic and hepatic expression patterns of hat1 and hdac were similar but those of dnmt and tet were different between males and females. Irrespective of the timing of food availability, both hat1 and hdac mRNA levels were increased in the hypothalamus, but not in the liver, in which hat1 mRNA levels were increased in the morning FA group. While hypothalamic tet levels were higher in evening FA males, hepatic tet levels were higher in morning FA birds (tet1, only males). Gonadal expression levels similarly varied and showed sex differences. Histone-modifying genes did not show food availability effects, except for elevated testicular hdac3 levels. Similarly, testicular dnmt3b and tet2 mRNA levels were increased and decreased in morning and evening FA groups, respectively, whereas ovarian dnmt1 and tet2 levels were reduced in morning FA and tet1 levels were reduced in evening FA groups. The present results suggest that an enforced daily feeding schedule in the long term could serve as a conditioning environment that shapes overall hypothalamic regulation, and liver and gonadal function at the epigenetic level in diurnal vertebrates.

DNA methylation and histone modification (=epigenetic marks) modify local chromatin and affect DNA accessibility and DNA template processes during gene transcription (Allis et al., 2014). DNA methylation, which involves DNA methyltransferase (DNMT)-catalysed methylation of CpG dinucleotides, is an important mechanism of transcriptional repression (Moore et al., 2013). The functionality of DNA methylation remains ambiguous and debated, however (Bewick et al., 2016). As a counter-regulatory step to DNMT-mediated methylation, the ten–eleven translocase (TET) enzymes catalyse DNA demethylation (Ito et al., 2010). The complementary epigenetic modifier system includes processes that involve the acetylation and deacetylation of histone proteins by histone acetyltransferases (HATs) and de-acetyltransferases (HDACs), respectively. HATs promote transcription by chromatin unfolding, whilst HDACs repress transcription by chromatin condensation (Allis et al., 2014). The acetylated open-chromatin structure may also allow access to gene transcription repressors (Verdone et al., 2006).

Epigenetic marks, unlike fixed DNA sequences, are not stable and can undergo changes in response to exogenous stimuli, including diet (Zhang and Kutateladze, 2018), photoperiod (Stevenson and Prendergast, 2013), temperature (Vinoth et al., 2018; Yan et al., 2015), maternal effects (Bentz et al., 2016) and social interactions (Alvarado et al., 2014). In turn, epigenetic modification can influence the expression of genes without changing nucleotide sequences, and contribute to an altered phenotype. Much of the evidence for epigenetic modification among vertebrates comes from mammals and has been frequently reviewed (see especially Bohacek and Mansuy, 2015; Chen et al., 2017; Klemm et al., 2019). However, increasing evidence also suggests epigenetic changes as an important mechanism for phenotypic diversity in the face of environmental changes among birds (Sepers et al., 2019). DNA methylation levels of glucocorticoid receptor gene correlated with rainfall variation during the pre-breeding period, and with adult male reproductive behaviour in superb starlings (Lamprotornis superbus; Rubenstein et al., 2016). Similarly, DNA methylation levels of several loci positively correlated with the brood size of zebra finch (Taeniopygia guttata) nestlings (Sheldon et al., 2018).

Accumulated evidence from several taxa suggests a role of nutritional cues in epigenetic modification. DNA methylation reversibly marked the behavioural sub-castes of workers that forage and nurse in bees (Herb et al., 2012). Both food quality and quantity affected epigenetic modifications in rodents (Dunn and Bale, 2009; Zheng and Pan, 2010; Zheng et al., 2012). The maternal exposure of rat pups to a low-protein diet down-regulated the expression of the p16 cell cycle gene through histone modification, and predisposed offspring towards certain diseases when adult (Zheng and Pan, 2010; Zheng et al., 2012). However, the functional linkage of time-restricted feeding with epigenetic control of physiology and behaviour is only beginning to emerge. A recent study showed a time-restricted feeding-induced reduction in HDAC activity, and hence increased histone H3 acetylation, in mouse hippocampus (Landgrave-Gómez et al., 2016). The question that we addressed here is: what is the consequence of long-term time-restricted feeding on epigenetic modification in a continuously reproducing diurnal vertebrate? We investigated this in diurnal zebra finches (Taeniopygia guttata) in which a previous study has shown time-restricted feeding-induced effects on reproductive performance, and the quality and quantity of offspring survivors, as assessed at multiple levels including circulating levels of hormones (sex steroids and mesotocin), egg laying latency and egg quality, reproductive fecundity, and offspring growth and size when adult (Mishra and Kumar, 2019). Importantly, time-restricted feeding adversely affected reproductive health, as suggested by reduced sex steroids and mesotocin levels compared with levels in birds that were fed ad libitum (Mishra and Kumar, 2019). Here, we examined whether time-restricted feeding affected the mRNA expression of epigenetic modifier genes, and whether the expression pattern differed between morning and evening FA groups. In particular, we measured the mRNA expression of genes involved in DNA methylation and demethylation (dnmt1, dnmt3a, dnmt3b, tet1, tet2), and histone modification (hat1, hdac2, hdac3 and hdac4) in the hypothalamus (the overall regulatory centre), liver (the site of metabolic homoeostasis) and gonads (the reproductive gland involved in gamete production and sex hormone secretion, which hence represented the endpoint of reproductive activity).

Animals and experiment

The Institutional Animal Ethics Committee, IAEC (DU/ZOOL/IAEC-R/2015/02) of the Department of Zoology, University of Delhi, India, approved the study. We used tissues harvested from our previous study (Mishra and Kumar, 2019), described in detail therein. Briefly, we used 36 adult birds of each sex (1–1.5 years of age with similar body mass: 12.4±0.1 g), born and raised in our indoor aviary and maintained at constant temperature (24±2°C) and photoperiod (12 h light:12 h dark; light 200±10 lx, dark 0 lx). Birds were housed in same-sex cages (54 cm×42 cm×30 cm; n=4 per cage) and kept on a 12 h light:12 h dark photoperiod, as before, for 3 weeks, during which they had no visual or acoustic contact with the opposite sex. This was done to break any pair bonds that were established in the aviary; we removed any eggs laid during this period to discount the carry-over effect of previous co-habitation. Birds had ad libitum access to food and water, and were fed daily on Setaria italica (Kakuni; 3.64 kcal g−1) seeds as the primary diet, supplemented with hard-boiled eggs (1.47 kcal g−1) mashed with crushed egg shell. Thereafter, for 24/36 birds of each sex, the food availability period was restricted by step-wise reduction of food availability times over 3 days to 8, 6 and 4 h, aligned with lights on (hour 0; morning FA) or lights off (hour 12; evening FA). Thus, time-restricted feeding deprived all birds of food for the same period of time but with a difference in the direction of food deprivation in relation to 4 h food availability. The remaining 12 birds of each sex continued to be given food ad libitum, and served as controls. Each day, we provided a food-filled cup at hour 0 to ad libitum-fed birds and the morning FA group, and at hour 8 to the evening FA group, and the cup was replaced by an empty food cup at hours 4 and 12 for the morning and evening FA group, respectively, and with another food-filled cup the next day at hour 0 for ad libitum-fed birds.

After a week of acclimation to the particular feeding condition, separately housed males and females were randomly paired, so each feeding condition had 12 breeding pairs. Each bird lived with the same partner for about a year, during which we assessed time-restricted feeding-induced effects on reproductive health and performance, as reported by Mishra and Kumar (2019). Thereafter, pairs were separated and returned to the same-sex groupings and maintained on identical lighting and feeding regimes to those during the breeding protocol, to minimise the influence of co-habitation. After 8 weeks, five randomly chosen birds from each group (n=5 per sex and food condition) were decapitated under dim red light half an hour before lights on so that they were ‘starved’ for the almost the entire night period, irrespective of the feeding regime (zebra finches do not eat during the period of darkness; I.M. and V.K., unpublished observations). Thus, in the current study, we performed gene expression analyses on a subset of animals from the larger year-long experiment. We preferred decapitation (an unanticipated quick procedure that lasts only ∼10 s from removal of the bird from its cage to its decapitation) over anaesthesia usage, as anaesthesia can influence mRNA expression levels in tissues (Hamaya et al., 2000; Staib-Lasarzik et al., 2014). The brain, liver and gonads were removed, the hypothalamus was quickly excised from the brain (Mishra et al., 2018), and all tissues were stored at −80°C until processed for gene expression assays.

Analysis of mRNA expression of epigenes in different tissues by qPCR

From each tissue, a 1 μg aliquot of total RNA extracted using Tri reagent (AM9738; Ambion, Austin, TX, USA) and treated with RQ1 RNase-free DNase (M6101, Promega, Madison, WI, USA) was reverse transcribed using Revert-Aid first strand cDNA synthesis Kit (K1622, Thermo Fisher Scientific, Waltham, MA, USA). The mRNA expression of hat1, hdac2, hdac3, hdac4, dnmt1, dnmt3a, dnmt3b, tet1 and tet2 genes was measured in the hypothalamus, liver and gonads using gene-specific primers (Table 1) and SYBR green chemistry, using protocols standardised and routinely used in our laboratory (Majumdar et al., 2015; Mishra et al., 2018; Sharma et al., 2018). We performed 2-step qPCR with an Applied Biosystems ViiA7 thermal cycler using 10 μl reaction mixture, with 1 μl each of cDNA (10 ng ml−1) and forward and reverse primers (500 nmol l−1; Table 1), 5 μl Power Syber Green PCR Mastermix (ABI 4387669; 1× in total reaction volume) and 2 μl of nuclease-free water, for a total of 40 cycles, each lasting for 75 s (15 s melting at 95°C+60 s annealing at 60°C). We used β-actin as the endogenous control (reference) gene, which was found to have high stability and low inter- and intra-group variability (Sharma et al., 2018). Here also, we assessed the stability of the β-actin gene using Best-Keeper (Pfaffl et al., 2004), and found that its values were stable and did not vary much between the treatment groups (s.d.±crossover threshold, Ct<1.0; hypothalamus: 0.99, liver: 0.86, testis: 0.88, ovary: 0.92). Both sample and reference genes were run in duplicate, and the relative mRNA expression level was determined as 2–ddCt (Livak and Schmittgen, 2001). Briefly, we first calculated ΔCt by subtracting the crossover threshold (Ct) of the reference gene from the target gene (Cttarget gene−Ctreference gene). ΔCt value was then normalised against the Ct value of a pooled sample containing an equal quantity of cDNA from all samples; this gave the ΔΔCt value (Mishra et al., 2017; Sharma et al., 2018). For better visual resolution and presentation, data on mRNA expression were further transformed to define the sample with the lowest mRNA levels as a relative quantity of 1, which amounts to a log2 value of 0. On this scale, a difference of 1 unit reflects a 2-fold difference in the respective mRNA expression level (Mishra et al., 2018). The expression of hdac2 was found to be below the detection limit in both the testes and ovary, and that of dnmt3a was below the detection limit the hypothalamus, liver and gonads and hence was excluded from the presentation.

Table 1.

Gene-specific primers used for qPCR

Gene-specific primers used for qPCR
Gene-specific primers used for qPCR

Statistical analysis

Statistical analyses were performed using Graph Pad Prism (version 6, San Diego, CA, USA) or SPSS Statistics software (version 20, IBM), as appropriate. All tests were two-tailed, and we report the results as means±s.e.m. We used generalised linear model (GLM, 2-factor analysis) followed by pairwise sequential Bonferroni post hoc test to test the effects of the feeding regime (factor 1), sex (factor 2) and their interaction (factor 1×factor 2) on mRNA expressions in the hypothalamus and liver, as values were not repeated measures. However, we did not compare the mRNA levels in the testes with those in the ovary, so we used Kruskal–Wallis (KW, 1-factor analysis) test followed by Dunn's post hoc test to test the effect of feeding regime on gene expression separately in the testes and ovary. We also calculated effect size estimates as ε2=KW value/(N2−1/N+1) for 1-factor analysis (Kruskal–Wallis test) and η2partial=SSeffect/(SSeffect+SSerror) (where SS is sum of squares) for 2-factor analysis (GLM). We used log-transformed values for the statistics, and P<0.05 was considered a statistically significant difference.

Effects of time-restricted feeding on epigene expression

Hypothalamus

Time-restricted feeding significantly altered the hypothalamic expression of epigenetic modifier genes. There was a significant effect of feeding regime on all the measured epigenetic markers (hat1: Wald's χ2=66.95, P<0.0001; hdac2: Wald's χ2=53.85, P<0.0001; hdac3: Wald's χ2=59.92, P<0.0001; hdac4: Wald's χ2=164.49, P<0.0001; dnmt1: Wald's χ2=25.53, P<0.0001; dnmt3b: Wald's χ2=19.49, P<0.0001; tet1: Wald's χ2=11.29, P=0.004; tet2: Wald's χ2=29.11, P<0.0001; GLM; Table 2). We also found a significant sex effect on dnmt3b (Wald's χ2=6.60, P=0.010; GLM; Table 2) and tet2 (Wald's χ2=3.91, P=0.048; GLM; Table 2) expression, and of the feeding regime×sex interaction on hdac4 expression only (Wald's χ2=6.59, P=0.037; GLM; Table 2). In particular, the mRNA level of histone modifiers (hat1, hdac2, hdac3 and hdac4) was significantly increased in both sexes in time-restricted feeding groups, except for hat1 levels in morning FA females (P<0.05; Bonferroni post hoc test; Fig. 1A–D). However, there were sex differences in the expression pattern of dnmt and tet genes. Whereas dnmt1 mRNA expression was unaffected in males, the levels were significantly reduced in morning FA females (P<0.05; Bonferroni post hoc test; Fig. 1E). Similarly, we found significantly increased dnmt3b, tet1 and tet2 mRNA expression in males, but not in females, subjected to morning FA (dnmt3b alone) and evening FA regimes (P<0.05; Bonferroni post hoc test; Fig. 1F–H).

Table 2.

Results of generalised linear model analysis presented as Wald's χ2, alpha (P-value) and effect size estimate

Results of generalised linear model analysis presented as Wald's χ2, alpha (P-value) and effect size estimate
Results of generalised linear model analysis presented as Wald's χ2, alpha (P-value) and effect size estimate
Fig. 1.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the hypothalamus of adult male and female zebra finches. (A–D) Histone modification genes hat1, hdac2, hdac3 and hdac4. (E–H) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference between food restriction groups as determined by generalised linear model (GLM) test followed by Bonferroni post hoc test. P<0.05 was considered statistically significant.

Fig. 1.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the hypothalamus of adult male and female zebra finches. (A–D) Histone modification genes hat1, hdac2, hdac3 and hdac4. (E–H) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference between food restriction groups as determined by generalised linear model (GLM) test followed by Bonferroni post hoc test. P<0.05 was considered statistically significant.

Liver

mRNA expression patterns in the liver showed a significant effect of feeding regime (hat1: Wald's χ2=41.98, P<0.0001; hdac2: Wald's χ2=9.27, P=0.010; hdac4: Wald's χ2=93.20, P<0.0001; dnmt1: Wald's χ2=47.27, P<0.0001; dnmt3b: Wald's χ2=14.96, P=0.001; tet1: Wald's χ2=16.57, P<0.0001; tet2: Wald's χ2=69.02, P<0.0001; GLM; Table 2) and sex (hdac3: Wald's χ2=4.40, P=0.036; hdac4: Wald's χ2=4.02, P=0.045; dnmt1: Wald's χ2=9.58, P=0.002; dnmt3b: Wald's χ2=8.68, P=0.003; tet1: Wald's χ2=18.20, P<0.0001; GLM; Table 2), and a feeding regime×sex interaction for hdac3 mRNA expression alone (Wald's χ2=7.51, P=0.023; GLM; Table 2). In both sexes, hat1 mRNA levels were significantly higher in the morning FA group than in the evening FA or ad libitum-fed group (P<0.05; Bonferroni post hoc test; Fig. 2A). There was no difference in mRNA expression of hdac3, but hdac4 mRNA levels in both sexes were significantly higher in time-restricted feeding groups (P<0.05; Bonferroni post hoc test; Fig. 2C,D). Similarly, in both sexes, dnmt1 mRNA levels were significantly higher in time-restricted feeding groups, as compared with the ad libitum-fed group (P<0.05; Bonferroni post hoc test; Fig. 2E). However, dnmt3b mRNA levels were significantly higher in morning FA males and evening FA females, as compared with the ad libitum-fed birds (P<0.05; Bonferroni post hoc test; Fig. 2F). Within the time-restricted feeding groups, dnmt1 and dnmt3b mRNA expression showed sex-dependent differences. For example, both dnmt1 and dnmt3b mRNA levels were significantly higher in males than in females in the morning FA group (P<0.05; Bonferroni post hoc test; Fig. 2E,F). We also found that tet1 mRNA levels in male birds were significantly higher in morning FA birds than in evening FA and ad libitum-fed birds; mRNA levels were also higher in males than in females in the ad libitum-fed and morning FA groups (P<0.05; Bonferroni post hoc test; Fig. 2G). Likewise, tet2 mRNA levels in both sexes were significantly higher in morning FA birds than in ad libitum-fed and evening FA birds (P<0.05; Bonferroni post hoc test; Fig. 2H).

Fig. 2.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the liver of adult male and female zebra finches. (A–D) Histone modification genes hat1, hdac2, hdac3 and hdac4. (E–H) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference between food restriction groups and asterisks indicate differences between male and female zebra finches as determined by GLM test followed by Bonferroni post hoc test. P<0.05 was considered statistically significant.

Fig. 2.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the liver of adult male and female zebra finches. (A–D) Histone modification genes hat1, hdac2, hdac3 and hdac4. (E–H) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference between food restriction groups and asterisks indicate differences between male and female zebra finches as determined by GLM test followed by Bonferroni post hoc test. P<0.05 was considered statistically significant.

Gonads

We found a significant time-restricted feeding-induced effect on testicular mRNA expression of hdac3 (KW statistic: 9.50, P=0.002, N=15, ε2=0.68, Kruskal–Wallis; Fig. 3B), dnmt1 (KW statistic: 6.62, P=0.028, N=15, ε2=0.47, Kruskal–Wallis; Fig. 3D), dnmt3b (KW statistic: 9.14, P=0.0035, N=15, ε2=0.65, Kruskal–Wallis; Fig. 3E) and tet2 genes (KW statistic: 7.46, P=0.014, N=15, ε2=0.53, Kruskal–Wallis; Fig. 3G). In the ovary, however, there were significant time-restricted feeding-induced effects on dnmt1 (KW statistic: 6.14, P=0.038, N=15, ε2=0.44, Kruskal–Wallis; Fig. 4D), tet1 (KW statistic: 7.46, P=0.014, N=15, ε2=0.53, Kruskal–Wallis; Fig. 4F) and tet2 (KW statistic: 9.62, P=0.001, N=15, ε2=0.69, Kruskal–Wallis; Fig. 4G), but not on hdac3 and dnmt3b mRNA expression. Further, testicular hdac3 mRNA levels were significantly higher in evening FA and those of dnmt3b were higher in morning FA groups than in the ad libitum-fed group (P<0.05, Dunn's post hoc test; Fig. 3B,E). However, testicular tet2 mRNA levels were significantly higher in ad libitum-fed than in evening FA birds (P<0.05, Dunn's post hoc test; Fig. 3G). In the ovary, dnmt1 and tet2 mRNA levels were significantly lower in the morning FA group and tet1 levels were significantly lowed in evening FA birds, as compared with levels in the ad libitum-fed group (P<0.05, Dunn's post hoc test; Fig. 4D,F,G).

Fig. 3.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in testes of adult male zebra finches. (A–C) Histone modification genes hat1, hdac3 and hdac4. (D–G) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference as determined by Kruskal–Wallis test followed by Dunn's post hoc test. P<0.05 was considered statistically significant.

Fig. 3.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in testes of adult male zebra finches. (A–C) Histone modification genes hat1, hdac3 and hdac4. (D–G) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e.m. Different letters indicate a significant difference as determined by Kruskal–Wallis test followed by Dunn's post hoc test. P<0.05 was considered statistically significant.

Fig. 4.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the ovary of adult female zebra finches. (A–C) Histone modification genes hat1, hdac3 and hdac4. (D–G) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e. Different letters indicate a significant difference as determined by Kruskal–Wallis test followed by Dunn's post hoc test. P<0.05 was considered statistically significant.

Fig. 4.

Effects of daily food restriction on mRNA expression of genes involved in histone modification and DNA methylation in the ovary of adult female zebra finches. (A–C) Histone modification genes hat1, hdac3 and hdac4. (D–G) DNA methylation genes dnmt1, dnmt3b, tet1 and tet2. Birds were subjected to 4 h of food availability in the morning (morning FA group, FA-M) or evening (evening FA group, FA-E), with controls provided with food ad libitum (FAL). Data are means±s.e. Different letters indicate a significant difference as determined by Kruskal–Wallis test followed by Dunn's post hoc test. P<0.05 was considered statistically significant.

We show differential effects of time-restricted feeding on the mRNA expression of genes coding for histone-modifying enzymes and DNA methyltransferases/translocases in tissues that are involved in the neuroendocrine regulation (hypothalamus), metabolic homeostasis (liver) and reproduction (gonad) in diurnal zebra finches. Intriguingly, we found tissue-specific sex-dependent genetic responses to time-restricted feeding and its timing during the day. For example, the overall hypothalamic and hepatic expression patterns of hat1 and hdac were similar but those of dnmt and tet were different between males and females. More specifically, irrespective of the timing of food restriction, both hat1 and hdac mRNA levels were increased in the hypothalamus but not in the liver, in which hat1 mRNA levels were increased only in the morning FA group. Increased hypothalamic expression of hdac under the time-restricted feeding regime in zebra finches was consistent with its expression in the medial hypothalamus of adult mice in response to fasting or a high fat diet (Funato et al., 2011). Likewise, hypothalamic dnmt1 mRNA levels were decreased in morning FA females, but those of dnmt3b, tet1 and tet2 were increased in morning FA and/or evening FA male zebra finches. This is inconsistent with the reported increase in dnmt1 and dnmt3b expression in response to 12 h food deprivation in chickens, which was reversed after 36 h of food deprivation (Kang et al., 2017). However, DNA methylation was significantly decreased in pregnant rats subjected to a reduced protein diet, suggesting the hypomethylation of specific genes (Lillycrop et al., 2005). We speculate that differences in the epigene expression pattern were linked to the daily food times and tissue-specific regulatory mechanism(s) in zebra finches. We would not discount that the diet-induced effects on epigenetic modification also affected the egg components, and resulted in a time-restricted feeding-dependent effect on reproductive performance (Groothuis et al., 2005). Indeed, time-restricted feeding significantly affected egg quality, as assessed in the measures of primary maternal investment and other parameters, egg mass and volume, and the percentage lipid and yolk testosterone content (Mishra and Kumar, 2019). In particular, eggs were significantly smaller in size and lower in mass in time-restricted feeding than in ad libitum-fed pairs, and eggs from morning FA pairs had a significantly higher percentage of lipid and lower yolk testosterone content, as compared with eggs from the evening FA or ad libitum-fed pairs (Mishra and Kumar, 2019).

Interestingly, we found clear differences in the mRNA expression pattern of genes in gonads, as compared with that in the hypothalamus and liver. This was particularly evidenced by the non-detection hadc2 mRNA and no-difference in hat1 and hdac4 mRNA levels in gonads between the three feeding regimes. There were also differences in the mRNA expression pattern of genes between the testes and ovary. In response to time-restricted feeding, there was increased testicular expression of hdac3 and dnmt3b in the evening and morning, respectively, and decreased expression of tet2 in the evening; however, mRNA levels of dnmt3b and tet2 were relatively high and low in evening FA and morning FA birds, respectively, compared with those in ad libitum-fed birds. In ovary, in contrast, we found decreased dnmt1 in morning FA birds, decreased tet1 in evening FA birds, and decreased tet2 in both morning and evening FA birds. We suggest a differential time-restricted feeding-induced effect at the gonadal level in male and female zebra finches. Perhaps, testicular hdac3 was associated with delayed reproductive performance, as reported by the delayed egg laying onset and reduced reproductive success in response to evening FA in zebra finches (Mishra and Kumar (2019). A direct functional link between histone deacetylase activity and testicular function has indeed been suggested by an adverse effect of the histone deacetylase inhibitor Trichostatin A in murine spermatogenesis (Fenic et al., 2004). A linkage of hdac3 to the local inhibition of reproductive function has also been suggested in the Siberian hamster, Phodopus sungorus (Lynch et al., 2016). The lack of change in ovarian hdac expression in zebra finches is also consistent with results in Siberian hamsters (Lynch et al., 2016). We interpret that high dnmt3b and low tet1 and tet2 mRNA levels indicate an elevated methylation state in response to time-restricted feeding in zebra finches. At the same time, reduced tet2 expression in both testes and ovary might suggest a commonality in time-restricted feeding-induced effects on reproductive tissues in zebra finches, as suggested by studies in Siberian hamsters (Lynch et al., 2016).

In conclusion, we suggest that time-restricted feeding could potentially modulate overall hypothalamic regulation, liver functions and gonadal activity at the genetic level in diurnal zebra finches. Probably, the food availability and its timing served as an ‘epigenetic’ factor in the regulation of gene expression and, in turn, affected reproductive physiology via the hypothalamus–liver–gonad axis in zebra finches. However, this is purely speculative and needs further investigation. A role for diet via its effects on DNA methylation has been suggested in the regulation of reproductive performance in mammals, including humans (Cisneros, 2004). Although we have shown changes in the mRNA expression of genes involved in the epigenetic modification in response to restricted food availability, the mechanism(s) of epigenetic modification may need to be further confirmed in a future study. The overall implication of the present results is that an enforced daily feeding schedule in the long term could serve as a conditioning environment that shapes the activity of the genome by chromatin activation/silencing, which in turn could affect reproductive physiology and performance in vertebrates.

Author contributions

Conceptualization: V.K.; Methodology: I. Mishra, A.P., V.K.; Formal analysis: I. Mishra, A.S., T.B., I. Malik; Investigation: I. Mishra, A.P., T.B., I. Malik, V.K.; Data curation: I. Mishra, A.S.; Writing - original draft: A.S., V.K.; Writing - review & editing: A.S., V.K.; Visualization: V.K.; Supervision: V.K.; Project administration: V.K.; Funding acquisition: V.K.

Funding

A research grant (EMR/2015/002158) from Science and Engineering Research Board (SERB) to V.K. provided funding. The experimental facility used for this study was built under Intensification of Research in High Priority Area (IRHPA) grant support (IR/SO/LU-2005) by the Department of Science and Technology and SERB.

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Competing interests

The authors declare no competing or financial interests.