Please cite this paper as:
Sinesio-Jr, J., Bargi-Souza, P., Matos, R., Leite, E., Buonfiglio, D., Andrade-Silva, J., Motta-Teixeira, L., Curi, R., Young, M., Cipolla-Neto, J. and Peliciari-Garcia, R.A. 2019. Melatonin and the heart circadian clock of euglycemic and type 2 diabetic male rats: a transcriptional evaluation. Melatonin Research. 2, 3 (Aug. 2019), 139-151. DOI:https://doi.org/https://doi.org/10.32794/11250035.
Melatonin and the heart circadian clock of euglycemic and type 2 diabetic male rats: a transcriptional evaluation
José Sinésio-Jr1^, Paula Bargi-Souza1,2^, Raphael Afonso Matos1, Eduardo de Almeida Leite1, Daniella do Carmo Buonfiglio1, Jéssica Andrade-Silva1, Lívia Clemente Motta-Teixeira1, Rui Curi1,3, Martin Elliot Young4, José Cipolla-Neto1, Rodrigo Antonio Peliciari-Garcia5*.
1Department of Physiology and Biophysics, Institute of Biomedical Sciences-I, University of São Paulo, São Paulo, SP, Brazil.
2Department of Physiology and Biophysics, Institute of Biological Sciences, Federal University of Minas Gerais, MG, Brazil.
3Post-graduate Interdisciplinary Program in Health Sciences, Institute of Physical Activity and Sports Sciences, Cruzeiro do Sul University, São Paulo, Brazil.
4Division of Cardiovascular Diseases, Department of Medicine, University of Alabama at Birmingham, Birmingham, Alabama, USA.
5Morphophysiology & Pathology sector, Department of Biological Sciences, Federal University of São Paulo, Diadema, SP, Brazil.
^Authors have the equal contributions.
*Correspondence: peliciari.garcia@unifesp.br; Tel: +55 11 3385-4137, ext. 3431.
Running Title: Transcriptional effects of melatonin in the rat heart
Received: May 13, 2019; Accepted: August 19, 2019
ABSTRACT
Diabetes increases risk of various comorbidities, including retinopathy, neuropathy, and cardiovascular disease, comprising both ischemic and non-ischemic cardiomyopathy. Cardiac dysfunction during diabetes is associated with perturbations at histologic, metabolic, biochemical and molecular levels. The circadian clock is misaligned in multiple organs during diabetes, including the heart. Such alterations in clock function have been postulated to play a causal role in cardiac dysfunction even though the mechanisms leading to circadian misalignment are currently unknown. Melatonin has been reported to alter heart circadian clock components and its circulating levels are decreased during diabetes. These observations led to the hypothesis that decreased melatonin levels during diabetes could be related to misalignment of the heart clock. To evaluate this hypothesis, in the current study male Wistar and non-obese type 2 diabetic Goto-Kakizaki (GK) rats were given melatonin supplementation in their drinking water during the dark phase (for 12-wks), followed by assessment of clock component and the mRNA expression of the clock-controlled genes in the hearts of these animals. Melatonin supplementation significantly altered mRNA expression of targeted genes in both euglycemic and diabetic rat hearts. Collectively, under the condition of diabetes, the jeopardized pineal melatonin synthesis with misalignment of cardiac circadian clock components may likely mediate heart metabolic dysfunction, and/or even cause cardiovascular diseases.
Keywords: Melatonin, pineal gland, cardiac tissue, clock gene, metabolism, Goto-Kakizaki rats.
__________________________________________________________________________________________
1. INTRODUCTION
The prevalence of diabetes mellitus (DM) is increasing at alarming rates worldwide. According to the International Diabetes Federation (IDF – 2017), the number of people aging between 20-79 years old that developed diabetes corresponds to 424.9 millions, while the projection for 2045 could reach up to 628.6 million (1). The diabetes is a primary risk factor for development of cardiovascular disease (2-4). During diabetes, some events are directly interlinked to precipitation of diabetic cardiomyopathy, such as: hyperglycemia, insulin resistance, hyperinsulinemia, oxidative stress as well as inflammatory processes (5).
Melatonin is one of the most versatile hormones within the organisms. It can interact with G protein-coupled membrane receptors or nuclear receptors (6-8). This molecule exhibits an amphiphilic property (9) and thus, it presents in any compartment of the cell to act directly as a potent antioxidant molecule and also to activate antioxidative enzymes (10). In addition, Melatonin has been reported to reduce blood pressure, decrease cardiac arrhythmias, attenuate cardiac ischemia-reperfusion injury, and protects against cardiac infarction (11-20).
It has been reported by our group that pineal melatonin synthesis can be further induced by insulin (21, 22), while streptozotocin (STZ)-induced diabetes leads to impairment of pineal melatonin synthesis, highlighting a possible role the rat pineal gland on hyperglycemic condition (23). Zhou and colleagues (2018) also reported that melatonin exerted the beneficial effects that counterbalance the diabetic cardiomyopathy through a mechanism that involves the Syk-mitochondrial complex I-SERCA pathway (24).
Cardiomyocyte circadian clock controls the heart expression of genes associated with metabolism and function (25, 26). The cardiac tissue exhibits a time-of-day dependency of many physiological events throughout the period of 24 h, including adequate response to fatty acid availability, hypertrophic stimuli, prevalence of heart attack in the early hours of the morning, myocardial infarction, and sudden death (27-30). Furthermore, the incidence of cardiovascular disease has been associated with conditions where the heart clock is in constant dyssynchrony (e.g. shift workers) (31, 32).
As an internal zeitgeber, melatonin signals to the cellular circadian clock, as described for suprachiasmatic nucleus (SCN), pars tuberalis, adipose tissue, liver, skeletal muscle, and the heart (33-39). In the cultured adult rat cardiomyocyte, melatonin treatment did not alter the expression pattern of Bmal1, Nr1d1 and Dbp. However, 16 h after the coupling of circadian clock rhythmicity in the cell cultures, a challenge with melatonin avoids the reduction of Nr1d1 mRNA expression, an effect that seems to be mediated by its interaction to nuclear receptors (8).
Considering the chronobiotic and cardioprotective effects of melatonin, its reduced synthesis during diabetes, and the major role of the heart circadian clock in cardiac physiology, the aim of this investigation is to evaluate whether melatonin supplementation affects the heart circadian clock gene expression in euglycemic (Wistar) and non-obese type 2 diabetic, Goto-Kakizaki (GK) rats, a reliable model in the study of type 2 DM (40).
2. MATERIAL AND METHODS
2.1. Animals.
GK male rats were obtained from Charles River Laboratories International, Inc. (Wilmington, MA, USA), and Wistar male rats from the animal facility of the Institute of Biomedical Sciences at University of São Paulo (ICB-USP), (São Paulo, SP, Brazil). The rodents were housed at the Institute’s animal facility, maintained at 25 ± 2˚C under a light-dark cycle of 12 h/12 h (lights on 06:00 am= ZT0), being allowed free access to water and standard rodent chow (Nuvilab1, Curitiba, PR, Brazil) until the 10th week of age. The Committee of Ethics in Animal Experimentation of the ICB-USP (protocol # 86/2016) approved all experimental procedures of this study.
2.1.2. Experimental design.
The animals were then randomly divided into four groups: Wistar: Vehicle (W), Wistar:Melatonin (WMel), GK:Vehicle (GK), and GK:Melatonin (GKMel), in a total of 5-7 animals/ZT/group. Melatonin supplementation was given as previously described (41). In brief, melatonin (Sigma, St Louis, MO, USA) [3 mg/kg body weight] or Vehicle was supplemented in the drinking water of the rats during the dark phase in a daily basis for 12 weeks. At the end of the study, the rats were euthanized by decapitation and the heart ventricles were collected at ZTs 0, 4, 8, 12,16, and 20, respectively. The samples were frozen in liquid nitrogen and stored at -80˚C until further analysis.
2.1.3. RNA extraction and Real-Time qPCR (RT-PCR).
The total RNA extraction from rat heart ventricles using Trizol was performed according to the manufacturer’s instruction. Single-strand DNA synthesis was accomplished by the use of MMLV-RT (Promega) from 1 μg total RNA. Gene expression analysis was performed by RT- qPCR using SYBR GREEN (Invitrogen) as fluorescent dye. The 2(-Delta Ct) method was applied as described by Livak and Schmittgen (2001) (42); the Ct value is the calculated cycle number where the fluorescence signal was emitted significantly above background levels. The efficiency/slope obtained values of all investigated genes were close to the optimal values required for the 2(-Delta Ct) analysis (43). The RT-qPCR data are normalized by the housekeeping gene Peptidylprolyl isomerase A (Ppia). The primer assays for Adiponectin (Adpn), Peroxisome proliferator activated receptor alpha (Ppara), and Peptidylprolyl isomerase A (Ppia) were designed from rat sequences available in the GenBank (Table 1). The primer sequences for all the other investigated genes have been published elsewhere (8, 26, 44-46).
Table1. Rat primer sequences used in RT-qPCR.
Gene/GenBank# |
Primers |
Sequences |
Amp length (bp) |
Adipoq (Adpn) NM_144744.3 |
Forward Reverse |
5'-CTCCTGCTTCATTCCTCTCTTC-3' 5'-GTTGTCACTCACTCCTCCATC-3' |
85 |
Ppara NM_013196.1 |
Forward Reverse |
5'–ACTATGGAGTCCACGCATGTGA-3' 5'–GTACGCCAGCTTTAGCCGAA-3' |
70 |
Ppia NM_017101.1 |
Forward Reverse |
5'–AAGACTGAGTGGCTGGATGG-3' 5'–GGCTTCCACAATGCTCATGC-3' |
72 |
2.1.4. Statistical analysis.
The data are plotted as the means ± SEM. One, two or three-way ANOVA was appropriately applied to evaluate the influence of variables such as time, melatonin treatment (referenced as treatment per se) and genotype, followed by Bonferroni’s post-hoc analyses for pair-wise comparisons, using both GraphPad Prism (GraphPad Prism, version 7.0, San Diego, CA, USA) and Statgraphics Centurion (Statgraphics Centurion, version 17.1.06, Warrenton, VA, USA) software. The null hypothesis of no time, treatment, and genotype effect was rejected at P < 0.05. A second mathematical and statistical procedure was applied to investigate the presence of a daily 24 h rhythm (47). The method consists of adjusting a cosine curve to the actual 24 h time series (Cosinor method). The theoretical cosine curve fit was applied to each temporal series using the least-square calculation. The goodness of the fit using the F statistics was then estimated. The null hypothesis tested was that of zero amplitude, that is, no rhythmicity at the assumed frequency (24 h). A significant periodic fit was considered when the P value was <0.05. In addition, for each significant cosine fitted data series, the rhythmic parameters as acrophase (time of the peak), mesor (medium value of the adjusted curve) and amplitude (difference between peak value and mesor) of the adjusted curve were calculated (48, 49). When appropriate, Student’s t-test was also applied to these parameters.
3. RESULTS
3.1 Effects of melatonin in the heart core circadian clock expression.
The mRNA expression of positive elements from the clockwork machinery presented time main effect for Bmal1, Clock and Npas2 (Figs. 1A-C); genotype and time main effect for both Clock and Npas2, with interactions between these factors. In addition, Npas2 exhibited a treatment-genotype interaction and two pair-wise differences at ZT20, related to genotype (Figures 1B-C). The cosinor analysis revealed an acrophase delay of Bmal1 in type 2 diabetic (GK) versus euglycemic (W) rats. A phase advance was also observed in melatonin-treated diabetic animals (GKMel) compared to the GK group (Figure 2A, Table 2). As Bmal1, the cosinor curve adjustment of the gene Clock showed a 24-h rhythmic pattern for all groups, except for the melatonin treatment of Wistar animals (WMel), which had no rhythmicity. Both mesor and acrophase of type 2 diabetic animals of Clock had significant differences compared to euglycemic rats (increase and phase delay, respectively). The same pattern was observed for Npas2, except that in the latter case, GK had a reduction of the mesor instead an increase. Moreover, a phase delay was found for the acrophase of melatonin treated GK animals (GKMel) compared to euglycemic rats subjected to melatonin treatment (WMel) (Figures 2B-C, Table 2).
Three-way ANOVA of the core clock negative components analyzed in this study has shown a time main effect for expression of all genes, a genotype main effect for Cry1 and Cry2 expression and a treatment main effect only for Nr1d1. Genotype-time interaction was observed for Per2 and Cry1 expression, and treatment-genotype interaction was detected for Per1 and Cry1, whereas interaction between treatment-time was observed for Per2 and Nr1d1. The interaction between the three factors treatment-genotype-time was found only for Per1 (Figures. 1D-H). Genotype pair-wise comparison for Per1 at ZT12, and melatonin treatment in GK groups for Per2 at ZT16 were observed (Figures 1D-E). For Cry2 mRNA expression, pair-wise differences were found at ZT8 for melatonin treatment in GK (GKMel vs GK) and for genotype (GKMel vs WMel and W vs GK) at ZT12, whereas Nr1d1 presented a melatonin-induced increase at ZT4 observed in the euglycemic rats (W vs WMel) (Figures 1G-H).
Cosinor analysis depicted the loss of circadian rhythmicity of Per1 expression in GK animals challenged with melatonin (GKMel), while Per2 expression exhibited a phase advance in the acrophase in both melatonin-treated groups (WMel and GKMel) compared to their respective controls (W and GK, respectively). The acrophase of Cry1 expression was phase delayed in GK melatonin-treated rats compared to WMel rats. In addition, both melatonin-treated groups presented no circadian rhythmicity for Cry2. No statistical differences were observed in the cosinor analysis of Nr1d1 mRNA expression (Figures 2D-H, Table 2).
Figure 1. Effects of melatonin on circadian core clock components mRNA expression in euglycemic and type 2 diabetic rat hearts.
ZT24 was double plotted as ZT0. A-H) mRNA expression of Bmal1, Clock, Npas2, Per1, Per2, Cry1, Cry2 and Nr1d1, respectively, normalized by Ppia mRNA molecules and presented as absolute values of means ± SEM. Three-way ANOVA (P value, time, treatment and interactions are reported within respective graphs). Bonferroni’s post hoc test for pair-wise comparisons (respective ZTs) *,@,&,#P<0.05 for W vs WMel, W vs GK, WMel vs GKMel and GK vs GK Mel, respectively. n=5/ZT/group. ZT=Zeitgeber Time. Wistar (W); Melatonin (Mel); Goto-Kakizaki (GK).
Figure 2. Cosinor analysis of melatonin-mediated effects on circadian core clock components mRNA expression in euglycemic and type 2 diabetic rat hearts.
ZT24 was double plotted as ZT0. A-H) Cosinor curve fit of Bmal1, Clock, Npas2, Per1, Per2, Cry1, Cry2 and Nr1d1, respectively. One-way ANOVA and Cosinor were independently calculated for the experimental groups. Each of the cosinor parameters (mesor, amplitude and acrophase) was compared by Two-way ANOVA or Student’s t-test (when appropriate). Mesor (dashed horizontal lines) and acrophase (dashed vertical lines). Bonferroni’s post hoc test, *,@,&,#P<0.05 for W vs WMel, W vs GK, WMel vs GKMel and GK vs GK Mel, respectively. ZT=Zeitgeber Time. Wistar (W); Melatonin (Mel); Goto-Kakizaki (GK).
Table 2. Cosinor analysis (plotted as means ± SEM), periodicity of 24 h.
W |
WMel |
GK |
GKMel |
|||||||||
Mesor |
Amplitude |
Acrophase |
Mesor |
Amplitude |
Acrophase |
Mesor |
Amplitude |
Acrophase |
Mesor |
Amplitude |
Acrophase |
|
Bmal1c |
1.96±0.15 |
2.20±0.20 |
23.27±0.23 |
1.94±0.19 |
2.31±0.25 |
23.20±0.28 |
2.01±0.23 |
2.38±0.30 |
0.12±0.33@ |
2.09±0.15 |
2.31±0.19 |
23.53±0.22# |
Clocka,c |
0.74±0.04 |
0.24±0.06 |
22.59±1.04 |
- |
- |
- |
0.88±0.02@ |
0.23±0.03 |
0.49±0.32@ |
0.89±0.02 |
0.28±0.03 |
0.23±0.25 |
Npas2a,c |
0.48±0.03 |
0.38±0.04 |
23.47±0.26 |
0.45±0.03 |
0.37±0.04 |
23.04±0.26 |
0.37±0.02@ |
0.30±0.03 |
0.31±0.27@ |
0.45±0.02 |
0.32±0.02 |
0.56±0.20& |
Per1 |
2.74±0.27 |
1.46±0.36 |
12.46±1.04 |
3.10±0.29 |
1.72±0.39 |
11.53±0.58 |
3.04±0.27 |
1.56±0.36 |
12.48±1.00 |
- |
- |
- |
Per2b,c |
0.80±0.01 |
0.65±0.02 |
13.54±0.08 |
0.82±0.05 |
0.62±0.07 |
12.33±0.27* |
0.80±0.01 |
0.53±0.02 |
14.41±0.09 |
0.75±0.06 |
0.45±0.08 |
12.38±0.47# |
Cry1c |
1.22±0.08 |
0.68±0.11 |
18.03±0.34 |
1.26±0.07 |
0.64±0.10 |
17.31±0.31 |
1.19±0.01 |
0.59±0.02 |
18.54±0.06 |
1.09±0.04 |
0.49±0.05 |
18.54±0.22& |
Cry2 |
0.08±0.01 |
0.04±0.01 |
16.37±0.56 |
- |
- |
- |
0.10±0.00 |
0.04±0.01 |
15.34±0.38 |
- |
- |
- |
Nr1d1 |
13.32±1.92 |
15.33±2.82 |
7.38±0.39 |
15.32±1.26 |
16.77±1.88 |
7.13±0.23 |
13.06±0.89 |
13.92±1.30 |
8.04±0.20 |
13.16±1.32 |
14.66±1.96 |
7.14±0.28 |
Pdk4a,b |
23.59±0.58 |
13.65±0.86 |
17.03±0.13 |
- |
- |
- |
20.53±0.78@ |
15.96±1.17 |
17.29±0.15 |
15.65±0.35# |
8.66±0.52# |
17.20±0.12 |
Ucp3a,b |
0.83±0.05 |
0.49±0.08 |
19.06±0.34 |
- |
- |
- |
0.98±0.02@ |
0.82±0.06@ |
19.21±0.16 |
0.98±0.02 |
0.67±0.03 |
19.26±0.10 |
Pparα |
- |
- |
- |
x |
x |
x |
x |
x |
x |
x |
x |
x |
Acot1 |
0.43±0.07 |
0.37±0.10 |
18.30±0.54 |
x |
x |
x |
0.45±0.03 |
0.19±0.04 |
19.00±0.48 |
- |
- |
- |
Cd36 |
x |
x |
x |
x |
x |
x |
x |
x |
x |
x |
x |
x |
Adpna,b |
0.22±0.03 |
0.14±0.03 |
22.11±1.02 |
0.31±0.02* |
0.17±0.03 |
21.43±0.44 |
0.12±0.01@ |
0.05±0.01 |
21.53±0.51 |
0.13±0.00& |
0.05±0.01& |
22.25±0.31 |
Two-way ANOVA or Student’s t-test (when appropriated), P<0.05 for each of the parameters: mesor (a), amplitude (b) and acrophase (c). Bonferroni’s post hoc test, *P<0.05 vs W, @P<0.05 vs W, &P<0.05 vs WMel, #P<0.05 vs GK. (x) no period variation of the means in One-way ANOVA. (-) no circadian rhythmicity in the cosinor analysis. Wistar (W); Melatonin (Mel); Goto-Kakizaki (GK). For optimization of cosinor statistical analysis, the mesor and amplitude values of all groups are multiplied by 100. n=5.
3.2 Melatonin-induced alterations in metabolism clock-controlled gene expression in the heart.
The mRNA content of clock-controlled genes involved in glucose and fatty acid metabolism, and uncoupling of ADP oxidative phosphorylation in the heart was also investigated in euglycemic and non-obese type 2 diabetic animals treated or not with melatonin (Figure 3). Pdk4, Acot1, and Adpn showed treatment, genotype and time main effects in the three-way ANOVA with interactions of treatment-time for Pdk4, genotype-time, treatment-time and treatment-genotype-time for Acot1 and genotype-time and treatment-genotype for Adpn expression (Figures 3A-C). Moreover, Pdk4 mRNA expression also revealed melatonin treatment induced pair-wise differences at ZT16 regardless the genotype, and at ZT20 for GK animals (GKMel vs GK). Ucp3 and Cd36 expression presented genotype and time main effects, with treatment-time and genotype-time interactions for Ucp3, whereas Cd36 showed a treatment-genotype interaction. The pair-wise comparison revealed genotype differences for both genes (ZT 16 for Ucp3 and ZTs 4 and 12 for Cd36), but only in the euglycemic rats (Figures 3D-E). The content of Pparα mRNA presented time main effect and treatment-genotype-time interaction (Figure 3F).
The cosinor analysis of metabolic clock-controlled genes showed a melatonin-induced arrhythmic circadian expression of Pdk4, Acot1 and Ucp3 in the hearts of euglycemic rats (WMel) (Figures 4A-B, and D, Table 2). Melatonin also induced a loss of the circadian rhythmicity of Acot1 in the hearts of type 2 diabetic rats (GKMel) (Figure 4B, Table 2). The melatonin supplementation evoked significant alterations in the mesor values of Adpn (increase, Figure 4C, Table 2) and Pdk4 (reduction, Figure 4A, Table 2) expression in euglycemic and GK rats (WMel and GKMel), respectively. In the latter, the altered amplitude in cosine curve was observed for GK animals supplemented with melatonin (GKMel) (Figure 4A, Table 2). Genotype-induced alteration of mesor was also seen in Pdk4 and Adpn, as well as, mesor and amplitude of Ucp3 (Figure 4, Table 2). Pparα and Cd36 mRNA expression did not present a circadian pattern of oscillation in the heart of animals subjected to the experimental conditions (Table 2).
Figure 3. Effects of melatonin on clock-controlled genes mRNA expression in euglycemic and type 2 diabetic rat hearts.
ZT24 was double plotted as ZT0. A-F) mRNA expression of Pdk4, Acot1, Adpn, Ucp3, Cd36 and Ppara, respectively, normalized by Ppia mRNA molecules and presented as absolute values of means ± SEM. Three-way ANOVA (P value, time, treatment and interactions are reported within respective graphs). Bonferroni’s post hoc test for pair-wise comparisons (respective ZTs) *,@,&,#P<0.05 for W vs WMel, W vs GK, WMel vs GKMel and GK vs GK Mel, respectively. n=5/ZT/group. ZT=Zeitgeber Time. Wistar (W); Melatonin (Mel); Goto-Kakizaki (GK).
Figure 4. Cosinor analysis of melatonin-mediated effects on clock-controlled genes mRNA expression in euglycemic and type 2 diabetic rat hearts.
ZT24 was double plotted as ZT0. A-D) Cosinor curve fit of Pdk4, Acot1, Adpn, Ucp3, respectively. One-way ANOVA and Cosinor were independently calculated for the experimental groups. Each of the cosinor parameters (mesor, amplitude and acrophase) was compared by Two-way ANOVA or Student’s t-test (when appropriate). Mesor (dashed horizontal lines), amplitude (vertical line interval) and acrophase (dashed vertical lines). Bonferroni’s post hoc test, *,@,&,#P<0.05 for W vs WMel, W vs GK, WMel vs GKMel and GK vs GK Mel, respectively. ZT=Zeitgeber Time. Wistar (W); Melatonin (Mel); Goto-Kakizaki (GK).
4. DISCUSSION
Several studies reported the effects of melatonin in the cardiovascular system ranging from reduction of blood pressure to protective effects of the heart after ischemia-reperfusion events (17-20, 50). The therapeutic benefits of melatonin in pathological conditions as the diabetic cardiomyopathy have also been described (24). During diabetes, the pineal melatonin synthesis is reduced as demonstrated in STZ-induced diabetic rats (23), as well as, in type 2 diabetic Goto-Kakizaki rats (51). This reduction might directly impair the systemic effects of melatonin, including signaling to the heart, which could lead to dyssynchrony of the cardiac clockwork machinery.
Indeed, a phase advance of core clock and metabolic clock-controlled genes were reported in STZ-induced diabetes rat heart (52). Moreover, an increase in the mRNA expression of fatty acid and glucose-related metabolic genes as Acot1, Cd36, Pdk4, and Ucp3 has been also reported in STZ-induced diabetic mice hearts (53). The few data related to the heart circadian clock and type 2 DM was obtained by a transcriptome analysis, which revealed significant alterations of core clock and clock-controlled genes in the heart of GK rats including Bmal1, Npas2, Per2, Dbp and Tef (54). Our results partially reinforce the correlation between type 2 diabetes and core clock/clock-regulated genes mRNA expression in the heart, since genotype main effects or genotype interactions between time and/or treatment were significant for all targeted genes, except Bmal1 and Nr1d1. These data contrast the overexpression of Ucp3, Pdk4, Acot1 and the acrophase alteration of core clock components observed in type 1 DM (52, 53), suggesting a differential metabolic adaptation of the heart according to the diabetes features of type 1 or 2.
The effects of melatonin in the heart and cardiovascular system circadian clocks of hypertensive rats induced a phase-shift of Per2 and Bmal1 mRNA expression (37, 38). In cultured rat cardiomyocytes, we reported that administration of melatonin did not alter the mRNA expression of Bmal1, Nr1d1 and Dbp, but specifically at time 16 h of the culture it avoided the decrease of Nr1d1 and induced its expression for up to 12 h after the melatonin challenge. The blockage of melatonin membrane receptors (MT1 and MT2) did not alter the melatonin-induced alterations mentioned above, suggesting the non participation of melatonin membrane receptors in this response (8). The differences between whole heart and cell type-specific melatonin effects might be associated with cell types (cardiomyocytes, fibroblasts and endothelial cells) and by 3D structure interaction of the organ, which is not the case when cells are in the culture. In fact, the 3D dependence in organ function was already reported in central nervous system structures, as the pituitary (55, 56). However, the relationship between heart function and its cellular organization for the melatonin effects requires further investigation.
Melatonin supplementation abolished or altered the rhythmic expression pattern of core clock components (observed through cosinor analysis) including Clock, Cry2 and Per2, metabolic clock-controlled genes involved in glucose, fatty acid metabolism and energy generation through the electron transport chain oxidative phosphorylation including Pdk4, Ucp3 and Acot1, and increased the mesor of Adpn in the heart of euglycemic (W) rats. Although Nr1d1 did not present any significant alteration in the cosinor analysis, an obvious effect of melatonin treatment was observed for this gene. Once again, cellular and whole heart responses to melatonin should be taken into consideration. The type 2 diabetic animals also reflected the effects of melatonin supplementation observed in the core circadian clock and clock-controlled metabolic genes. GKMel group showed a phase advance for Bmal1 and Per2, an abolishment of Per1 and Cry2 circadian rhythmicities, whereas Pdk4 mesor had a significant reduction. Collectively, these data suggest that at least some of the heart circadian clock components as well as relevant glucose and fatty acid clock-related genes are independent targets for melatonin, which corroborates the literature (cell and heart), either in euglycemic or type 2 DM conditions.
As already mentioned, the heart circadian clock has a crucial role on the regulation of the heart metabolism and function (57, 58). The elevated fatty acid availability found in diabetes can modulate the heart metabolism, which in turn is regulated by the heart circadian clock (53). Thus, misalignment of heart metabolism and circadian clock, additionally influenced by melatonin reduction, might be partially related to development of cardiac dysfunction, which is often observed during diabetes.
In summary, melatonin-mediated alterations in the mRNA expression of some core clock and metabolic clock-related genes in hearts of euglycemic and type 2 diabetic rats were observed in the current study. Melatonin treatment altered or even evoked loss of the transcript’s circadian rhythmicity. Genotype-related differences in mRNA expression of genes in the cardiac tissue of both Wistar and Goto-Kakizaki rats were also identified with or without melatonin supplementation. The results provide additional information on the potential associations of melatonin and diabetic cardiomyopathy, particularly related to the circadian genes as well as their regulatory genes expression in heart locally. This information is valuable to use melatonin as a potential therapeutic agent for increased cases of diabetes.
ACKNOWLEDGEMENTS
This work was supported by São Paulo Research Foundation (FAPESP - JCN# 2014/50457-0, and RC# 2018/09868-7); Conselho Nacional de Pesquisa e Desenvolvimento (CNPq - JSJ # 1649692015-2). We would like to thank Ms. Julieta Scialfa Falcão for excellent technical assistance.
AUTHORSHIP
José Sinésio-Jr – melatonin supplementation, data acquisition/analysis; Paula Bargi-Souza – data acquisition/analysis/interpretation, drafting of the manuscript, critical revision of the manuscript; Raphael Afonso Matos, Eduardo de Almeida Leite, Daniella do Carmo Buonfiglio, Jéssica Andrade-Silva and Lívia Clemente Motta-Teixeira – melatonin supplementation; Rui Curi, Martin Elliot Young and José Cipolla-Neto – critical revision of the manuscript; Rodrigo Antonio Peliciari-Garcia – data acquisition/analysis/interpretation, drafting of the manuscript, critical revision of the manuscript and approval of the article.
CONFLICT INTEREST
The authors declare no conflict of interest.
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