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Feeding pregnant rats a protein-restricted diet persistently alters the methylation of specific cytosines in the hepatic PPARα promoter of the offspring

Published online by Cambridge University Press:  01 August 2008

Karen A. Lillycrop
Affiliation:
Development and Cell Biology, Biomedical Sciences Building, University of Southampton, Bassett Crescent East, SouthamptonSO16 7PX, UK
Emma S. Phillips
Affiliation:
Development and Cell Biology, Biomedical Sciences Building, University of Southampton, Bassett Crescent East, SouthamptonSO16 7PX, UK
Christopher Torrens
Affiliation:
Institute of Developmental Sciences Building, Centre for DOHaD, Southampton General Hospital, Tremona Road, SouthamptonSO16 6YD, UK
Mark A. Hanson
Affiliation:
Institute of Developmental Sciences Building, Centre for DOHaD, Southampton General Hospital, Tremona Road, SouthamptonSO16 6YD, UK
Alan A. Jackson
Affiliation:
Institute of Human Nutrition, Southampton General Hospital, Tremona Road, SouthamptonSO16 6YD, UK
Graham C. Burdge*
Affiliation:
Institute of Human Nutrition, Institute of Developmental Sciences Building, Southampton General Hospital, Tremona Road, SouthamptonSO16 6YD, UK
*
*Corresponding author: Dr G. C. Burdge, fax +44 23 8079 5255, email [email protected]
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Abstract

Induction of an altered phenotype by prenatal under-nutrition involves changes in the epigenetic regulation of specific genes. We investigated the effect of feeding pregnant rats a protein-restricted (PR) diet with different amounts of folic acid on the methylation of individual CpG dinucleotides in the hepatic PPARα promoter in juvenile offspring, and the effect of the maternal PR diet on CpG methylation in adult offspring. Pregnant rats (five per group) were fed 180 g/kg casein (control) or 90 g/kg casein with 1 mg/kg folic acid (PR), or 90 g/kg casein and 5 mg/kg folic acid (PRF). Offspring were killed on postnatal day 34 (five males and females per group) and day 80 (five males per group). Methylation of sixteen CpG dinucleotides in the PPARα promoter was measured by pyrosequencing. Mean PPARα promoter methylation in the PR offspring (4·5 %) was 26 % lower than controls (6·1 %) due to specific reduction at CpG dinucleotides 2 (40 %), 3 (43 %), 4 (33 %) and 16 (48 %) (P < 0·05). There was no significant difference in methylation at these CpG between control and PRF offspring. Methylation of CpG 5 and 8 was higher (47 and 63 %, respectively, P < 0·05) in the PRF offspring than control or PR offspring. The methylation pattern in day 80 PR offspring was comparable to day 34 PR offspring. These data show for the first time that prenatal nutrition induces differential changes to the methylation of individual CpG dinucleotides in juvenile rats which persist in adults.

Type
Short Communication
Copyright
Copyright © The Authors 2008

There is an increasing awareness that aspects of the prenatal environment, including nutrition, provide cues which act through developmental plasticity to alter the phenotype of the offspring(Reference Bateson, Barker, Clutton-Brock, Deb, D'Udine, Foley, Gluckman, Godfrey, Kirkwood, Lahr, McNamara, Metcalfe, Monaghan, Spencer and Sultan1). In man, such developmental cues contribute to the early origins of risk of chronic diseases(Reference Godfrey and Barker2). In rats, variations in the phenotype of the offspring are induced by feeding pregnant dams a diet with a moderate reduction in protein(Reference Langley and Jackson3). Induced changes to the phenotype which persist throughout the life-span involve stable alterations to the expression of the genome(Reference Burdge, Hanson, Slater-Jefferies and Lillycrop4). Epigenetic regulation of genes, specifically methylation of clusters of CpG dinucleotides (islands) and covalent modifications of histones in promoter regions, are established during early life and confer stable silencing of transcription which is critical for cell differentiation(Reference Bird5). We have shown that feeding pregnant rats a protein-restricted (PR) diet during pregnancy increased glucocorticoid receptor (GR) and PPARα expression in the liver of the offspring by inducing hypomethylation of their respective promoters, possibly by decreasing DNA methyltransferase-1 expression, and increasing levels of transcription-permissive histone modifications(Reference Burdge, Phillips, Dunn, Jackson and Lillycrop6Reference Lillycrop, Slater-Jefferies, Hanson, Godfrey, Jackson and Burdge8). Hypomethylation and the resulting increase in GR and PPARα expression was prevented by increasing the folic acid content of the PR diet(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7). In human umbilical cord, DNA methyltransferase-1, but not DNA methyltransferase-3a, expression was positively associated with methylation of the GR promoter(Reference Lillycrop, Slater-Jefferies, Hanson, Godfrey, Jackson and Burdge8). Overall, these findings suggest an epigenetic mechanism by which prenatal nutrition may induce an altered phenotype in the offspring.

The promoter regions of many genes contain several CpG dinucleotides at which induced changes in methylation, and hence epigenetic regulation, might occur. For example, increased pup licking and grooming by lactating rats decreased stress response in the adult offspring by increasing GR expression in the hippocampus through differential hypomethylation of individual CpG dinucleotides in the GR promoter, leading to the altered binding of transcription factors(Reference Liu, Diorio, Tannenbaum, Caldji, Francis, Freedman, Sharma, Pearson, Plotsky and Meaney9Reference Weaver, Cervoni, Champagne, D'Alessio, Sharma, Seckl, Dymov, Szyf and Meaney11). One example is the binding of NF1A which was regulated by the methylation of a single cytosine(Reference Liu, Diorio, Tannenbaum, Caldji, Francis, Freedman, Sharma, Pearson, Plotsky and Meaney9Reference Weaver, Cervoni, Champagne, D'Alessio, Sharma, Seckl, Dymov, Szyf and Meaney11). However, it is not known whether maternal under-nutrition during pregnancy alters the methylation of specific CpG dinucleotides within a gene promoter or if all CpG are affected to the same extent. Furthermore, it is not known whether such patterns of methylation, once induced, are permanent. We have investigated the effect of feeding pregnant rats a PR diet on the methylation of individual CpG dinucleotides in the PPARα promoter in the liver, in both juvenile and adult offspring. We also investigated the effect of increasing the folic acid content of the PR diet on CpG methylation of the PPARα promoter in juvenile offspring.

Materials and methods

Animal procedures

In order to validate assessment of promoter methylation by methylation-sensitive RT–PCR which we have used previously(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7, Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12), the livers studied here were from the same rats. The sample size at both ages was sufficient to detect significant differences in promoter methylation between dietary groups(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7, Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12). All animal procedures were conducted in accordance with the UK Home Office Animals (Scientific Procedures) Act (1986). Briefly, Virgin Wistar rats (five per dietary group) were fed from conception to delivery with isoenergetic diets containing either 180 g/kg casein and 1 mg/kg folic acid (control), 90 g/kg casein and 1 mg/kg folic acid (PR) or 90 g/kg casein and 5 mg/kg folic acid (PRF). The composition of the diets has been described previously(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7). Dams were fed a standard semi-purified diet (AIN 76A; SDS Ltd) from delivery(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7). Litters were reduced to eight at birth, equal numbers of males and females, and offspring were weaned on to AIN 76A at day 28 and were killed at day 34 ( juvenile; one liver from each litter was selected for analysis, male to female 3:2) or day 80 (adult; males only, one liver from each litter was selected for analysis, five per group) days. Livers were excised immediately, frozen in liquid nitrogen and stored at − 80°C.

Analysis of the methylation status of individual CpG dinucleotides in the hepatic PPARα promoter and PPARα mRNA expression

Genomic DNA was prepared as described(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7) and bisulphite conversion was carried out using the EZ DNA methylation kit (ZymoResearch). The pyrosequencing reaction was carried out by Biotage. Modified DNA was amplified using hot start Taq DNA polymerase (Qiagen) with the following primers: forward GGGGTGTGTTTAGTTTTGAAT, reverse TCACCCCTATCCTAAAACC. PCR products were immobilised on streptavidin–sepharose beads (Amersham), washed, denatured and released into annealing buffer containing the sequencing primer GGGATTTAGTAGGGGA (Biotage). Pyroseqeuncing was carried out using the SQA kit on a PSQ 96MA machine (Biotage) and the percentage methylation was calculated using the beta version of the Pyro Q CpG software from Biotage. Assay precision was between 0·8 and 1·8 % standard deviation and detection limits were 2–5 % methylation. The location of the CpG island in the PPARα promoter is shown in Fig. 1 (a) and the sequence in Fig. 1 (b). Putative transcription factor binding sites were deduced using Genomatix Matinspector (Genomatix Software GmbH).

Fig. 1 (a), Structure of the PPARα gene (www.ensembl.org, gene identity number ENSRNOG00000021463). The location of the CpG island was identified using Methprimer (www.urogene.org/methprimer). (b), Nucleotide sequence of the CpG island showing individual CpG dinucleotides and putative transcription factor binding sites. (c, d), Methylation of individual CpG dinucleotides in the PPARα promoter in the liver of the offspring of rats fed either a control (■), protein-restricted (□) or protein-restricted with increased folic acid content ( ) diet during pregnancy. Values are means with standard deviations depicted by vertical bars. (c), Day 34 male and female offspring (five per group). Mean values were significantly different from those of the control group (one-way ANOVA with Dunnett's post hoc test): *P < 0·05. (d), Day 80 male offspring (five per group). Mean values were significantly different from those of the control group (Student's unpaired t test): *P < 0·05. AHR, aryl hydrocarbon receptor; CPBP, core promoter-binding protein; CREB, cAMP responsive element binding protein; EGRG, Wilms tumour factor; HESF, hey-like transcriptional repressor; MAZ, Myc-associated zinc finger protein; NRF1, nuclear respiratory factor 1; SP1, specificity protein 1; USF, upstream stimulatory factor; WHNF, winged helix protein; ZF5F, zinc finger domain transcription factor.

In order to assess the extent to which the methylation status of individual CpG is associated with PPARα mRNA expression we carried out correlation analysis using data published previously where details of the analytical methods are described(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7, Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12).

Statistical analysis

Values are means and standard deviations of the methylation for individual CpG dinucleotides expressed relative to the control offspring. For the three groups of offspring studied at 34 d, values within each CpG were compared by one-way ANOVA with Dunnett's post hoc analysis. For the two groups of male offspring studied at 80 d, statistical comparisons were by Student's unpaired t test. Calculation of Pearson's correlation coefficient was used to determine the relationship between methylation status of individual CpG in the PPARα promoter and mRNA expression. Results were combined irrespective of age or maternal diet in order to provide sufficient data-points for correlation analysis.

Results

The results of analysis of the methylation status of the PPARα promoter at day 34 are summarised in Fig. 1 (c). One-way ANOVA showed that there were significant differences in methylation between maternal dietary groups at CpG 2, 3, 4, 5, 8 and 16 (P < 0·05) and a non-significant trend (P < 0·1) at CpG 7, 10 and 11. Mean methylation of the PPARα promoter in offspring of the dams fed a PR diet during pregnancy (4·5 %) was significantly lower (26 %, P < 0·05) than controls (6·1 %) due to selective reduction in methylation (P < 0·05) at CpG 2 (40 %), 3 (43 %), 4 (33 %) and 16 (48 %). There was no significant difference in the methylation of these CpG dinucleotides between control and PRF offspring. There was a non-significant trend (P < 0·1) towards lower methylation at CpG 7, 10 and 11 in the offspring of the PR v. control dams, but not in the offspring of dams fed the PRF diet. Although there was no significant difference in methylation at CpG 5 and 8 between offspring of control and PR dams, methylation was significantly higher (P < 0·05) in the offspring of the dams fed the PRF diet compared to controls (47 and 63 %, respectively).

There was no significant difference in the mean level or CpG-specific methylation in the PPARα promoter between offspring of control dams at days 34 and 80 (Fig. 1 (c), (d)). Mean promoter methylation was 28 % (P < 0·05) lower in the day 80 PR offspring (5·1 %) compared to controls (7·1 %). The methylation status of specific CpG dinucleotides in the hepatic PPARα promoter was significantly lower in the offspring of PR dams (CpG 2, 72 %; 3, 16 %; 4, 23 %; 7, 42 %; 9, 39 %; 16, 51 %; P < 0·05) compared to the offspring of the control dams (Fig. 1 (d)). Mean difference between offspring of control and PR dams in methylation across all CpG measured was 39 %.

We have published previously the level of PPARα mRNA expression in these samples(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7). There was a significant negative relationship between the methylation status of CpG 3 and 16 (both P < 0·05) such that variation in the level of methylation at CpG 3 predicted 43 % and at CpG 16 predicted 39 % of the difference between individuals in PPARα mRNA expression.

Discussion

The results of the present study show for the first time that feeding a PR diet to pregnant rats induces hypomethylation of specific CpG dinucleotides in the hepatic PPARα promoter in juvenile offspring. This pattern of cytosine hypomethylation was also found in adult male offspring. In day 34 offspring, the PRF diet prevented hypomethylation of these CpG dinucleotides, but induced hypermethylation of two other CpG.

The present findings agree with our previous data which showed using methylation-specific RT–PCR that feeding a PR diet to pregnant rats induced an overall 26 % reduction in methylation of the PPARα promoter in the liver of the juvenile and adult offspring(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7, Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12). The level of methylation within the PPARα promoter region was low (4–10 %) compared to that reported by Weaver et al. (Reference Weaver, Cervoni, Champagne, D'Alessio, Sharma, Seckl, Dymov, Szyf and Meaney11) for GR in the hippocampus (14–58 %). However, we did find significant differences in the level of methylation of individual CpG between the control and PR offspring. Moreover, absolute levels of methylation of specific CpG dinucleotides in the PPARα promoter had a significant negative relationship with mRNA expression. This suggests the magnitude of variation in CpG methylation was sufficient to alter transcription(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7) and is consistent with the suggestion that variations in relatively low levels of methylation, compared to imprinted genes, allow fine control of transcription by changing the balance in transcription factor regulation(Reference Mühlisch, Bajanowski, Rickert, Roggendorf, Würthwein, Jürgens and Frühwald13). Such subtle changes in epigenetic regulation are more consistent with the graded changes in phenotype induced by the early life environment than the gross phenotypic changes caused by large changes in the methylation of imprinted genes.

The CpG dinucleotides in the PPARα promoter coincided with the putative binding sites of a number of transcription factors which have an important regulatory role in a wide range of cellular processes (Fig. 1 (b)). It is possible that the differences in methylation of specific CpG dinucleotides observed may change the regulation of transcription in response to individual transcription factors and consequently the capacity of the tissue to respond to a metabolic challenge. Interestingly, the two CpG which showed an association between methylation and mRNA expression are located within putative binding sites for the transcription factors specificity protein 1 and winged helix protein, respectively. However, the transcription factor binding sites in Fig. 1 (b) are illustrative and the precise effect of differences in CpG methylation between offspring from different maternal dietary groups on transcription factor binding awaits experimental investigation.

The present findings agree in both direction and overall magnitude of effect with our previous data which showed, using methylation-specific RT–PCR, that feeding a PR diet to pregnant rats induced overall hypomethylation of the PPARα promoter in the liver of the juvenile and adult offspring(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7, Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12). The present data also show that prenatal under-nutrition induced hypomethylation of specific CpG dinucleotides, rather than altering the methylation of all CpG in the PPARα promoter. This is in agreement with the effects of maternal nursing behaviour on the epigenetic regulation of GR(Reference Weaver, Cervoni, Champagne, D'Alessio, Sharma, Seckl, Dymov, Szyf and Meaney11). Together these studies suggest that very different aspects of the early life environment induce highly specific changes to the epigenotype of the offspring.

Feeding the PRF diet to pregnant rats prevented hypomethylation of CpG which showed reduced methylation in the PR offspring, which is consistent with our previous findings(Reference Lillycrop, Phillips, Jackson, Hanson and Burdge7). However, CpG 5 and 8 were hypermethylated in the PRF offspring which suggests that there may be subtle effects of increased maternal folic acid intake which were not detected by overall assessment of promoter methylation, but which may still alter gene function.

DNA methyltransferase-1 expression and binding of specific transcription factors is reduced in the liver of the offspring of dams fed a PR diet during pregnancy, while this is prevented by increasing the folic acid content of the PR diet(Reference Lillycrop, Slater-Jefferies, Hanson, Godfrey, Jackson and Burdge8). Since DNA methyltransferase-1 is targeted to specific genes(Reference Robertson, Ait-Si-Ali, Yokochi, Wade, Jones and Wolffe14) and CpG dinucleotides(Reference Valinluck and Sowers15), altered DNA methyltransferase-1 expression may provide a mechanism for induction of hypomethylation of specific genes and individual CpG, although how such targeting may occur is not known.

One key principle of the developmental origins of disease hypothesis is that phenotypic characteristics induced in early life persist into adulthood(Reference Godfrey and Barker2). We have shown that overall changes in the methylation of the GR and PPARα promoters persist in adult offspring(Reference Burdge, Slater-Jefferies, Torrens, Phillips, Hanson and Lillycrop12). The findings of the present study show that the pattern of methylation of specific CpG dinucleotides in the hepatic PPARα promoter in adult offspring of PR dams compared to controls were essentially the same as in juvenile offspring. This suggests that the pattern of methylation of individual CpG induced in early life persists into adulthood.

Together these results show that nutrient constraint before birth induces persistent CpG-specific changes to the epigenetic regulation of the PPARα promoter and that these changes are associated with altered mRNA expression. If this were to occur in man, the precise pattern of CpG methylation may provide one mechanism for graded differences in phenotype induced by the developmental environment which result in differential risk of disease.

Acknowledgements

G. C. B., K. A. L. and M. A. H. designed the study. E. S. P., K. A. L. and C. T. carried out the experimental work. G. C. B., K. A. L. and M. A. H. wrote the paper with contributions from the other authors. G. C. B. and M. A. H. receive salary support from the British Heart Foundation who also funded part of the study. The remainder of the financial support was from departmental funds. There are no conflicts of interest.

References

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Figure 0

Fig. 1 (a), Structure of the PPARα gene (www.ensembl.org, gene identity number ENSRNOG00000021463). The location of the CpG island was identified using Methprimer (www.urogene.org/methprimer). (b), Nucleotide sequence of the CpG island showing individual CpG dinucleotides and putative transcription factor binding sites. (c, d), Methylation of individual CpG dinucleotides in the PPARα promoter in the liver of the offspring of rats fed either a control (■), protein-restricted (□) or protein-restricted with increased folic acid content () diet during pregnancy. Values are means with standard deviations depicted by vertical bars. (c), Day 34 male and female offspring (five per group). Mean values were significantly different from those of the control group (one-way ANOVA with Dunnett's post hoc test): *P < 0·05. (d), Day 80 male offspring (five per group). Mean values were significantly different from those of the control group (Student's unpaired t test): *P < 0·05. AHR, aryl hydrocarbon receptor; CPBP, core promoter-binding protein; CREB, cAMP responsive element binding protein; EGRG, Wilms tumour factor; HESF, hey-like transcriptional repressor; MAZ, Myc-associated zinc finger protein; NRF1, nuclear respiratory factor 1; SP1, specificity protein 1; USF, upstream stimulatory factor; WHNF, winged helix protein; ZF5F, zinc finger domain transcription factor.