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Original Article |
elizabet{at}cica.es
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Key Words: interleukin 1β • nitric oxide • FMR1 • CpG island methylation • gene repression
Methylation status of control regions in the genome plays a critical role in the regulation of gene expression 123. In susceptible genes containing 5' CpG islands, cytosine methylation favors a repressive chromatin structure that prevents the binding of transcriptional activators to the promoter 45. The molecular link between methyl groups on the DNA and the positioning of nucleosomes to form an inactive chromatin configuration has been recently elucidated 6. Well-known examples of methylation-dependent gene silencing are X-linked gene inactivation 7 and genomic imprinting 8, and changes in the pattern of DNA methylation occur during cell differentiation 910 and tumorigenesis 11121314. Hypermethylation of CpG islands can be associated with the silencing of some genes, such as fragile X mental retardation 1 (FMR1), causing inherited mental diseases 1516. Differential genomic DNA methylation also has the potential to influence the development of T cell cytokine production profiles 17. Here, we report that exposure to IL-1β (acting through inducible nitric oxide synthase [iNOS] induction) or direct application of NO donors induces in several cell types the suppression of the expression of FMR1 and other housekeeping genes containing a CpG island in their promoter. This effect is shown to be produced by DNA methylation resulting from activation of DNA methyltransferase (DNA MeTase). These observations demonstrate that IL-1β and NO, which are messenger molecules involved in a wide variety of pathophysiological processes, can have a direct effect on gene expression.
Cell Culture.
Reverse Transcription PCR.
Northern and Western Blots.
Southern Blot.
DNA MeTase Assay.
Other Enzymatic Assays.
Cell Proliferation Assay.
Materials and Methods
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Abstract
Materials and Methods
Results and Discussion
References
Materials.
IL-1β and IFN-
were purchased from Genzyme. S-nitroso-N-acetylpenicillamine (SNAP), N-methyl arginine (L-NMA and D-NMA), actinomycin D (ActD), trichostatin A (TSA), 5-aza-2'-deoxycytidine (AzadC), dithiothreitol (DTT), β-mercaptoethanol (β-ME), and protease inhibitors were obtained from Sigma Chemical Co. Sodium nitroprusside (SNP) was from Fluka. 2-amino-5,6-dihydro-6-methyl-4H-1,3-thiazine hydrochloride (AMT), S-ethylisothiourea hydrobromide (EIT), and L-N6-(1-iminoethyl)-lysine hydrochloride (L-NIL) were from Tocris Cookson, Ltd. 3-morpholinosydnonimine hydrochloride (SIN) was from ICN Iberica. Rediprime® DNA labeling system, [32P]dCTP, and cold and 3H-labeled S-adenosylmethionine were from Nycomed Amersham plc. Glutathione (GSH) and poly deoxyinosine-deoxycytosine (poly dI-dC) were from Boehringer Mannheim. Restriction enzymes were from Promega or New England Biolabs. All other reagents were of the best quality commercially available.
Insulin-producing rat RINm5F (RIN) cell, Jurkat T cell, and mouse leukemic monocyte-macrophage cell (RAW 264 cell) lines were grown in RPMI 1640 containing 10% heat-inactivated fetal bovine serum, 2 mM L-glutamine, 100 U/ml penicillin, 100 µg/ml streptomycin, and 2.5 µg/ml amphotericin B under 5% CO2 at 37°C. Human lymphocytes were obtained from peripheral blood of healthy donors as reported previously 18.
Total RNA was extracted from cell lines or fresh peripheral lymphocytes by the guanidine phenol method. RNA was reverse transcribed using random hexamers, and the cDNA was amplified using specific primers. PCR amplification of the CGG repeats at the FRAXA site and KH domains was carried as reported previously 1819. Amplification of hypoxanthine phosphoribosyltransferase gene (HPRT) in RIN cells was assessed using murine primers. Human specific primers were used for HPRT mRNA analysis in Jurkat T cells and fresh peripheral lymphocytes 7. Reverse transcription (RT)-PCR of ATP-ase or glyceraldehyde 3-phosphate dehydrogenase gene (GAPDH) was used as control. PCR products were visualized on agarose gel stained with ethidium bromide.
Northern blot of FMR1 gene was performed using 10 µg total RNA and 10 ng/ml of human FMR1 cDNA probe labeled with [
-32P]dCTP. Hybridization conditions were: 16 h at 42°C in 50% formamide, 6x saline-sodium phosphate-EDTA (SSPE), 5x Denhardt's solution, 0.5% SDS, 100 µg/ml herring sperm DNA. Wash conditions were: 2x SSPE, 0.1% SDS at room temperature and 0.1x SSPE, 0.1% SDS at 55°C. DNA MeTase expression was assayed with the same protocol using a specific 5-kb cDNA probe. Northern blot of iNOS and GAPDH was assayed by standard procedures. Western blot analysis of DNA MeTase was performed using 20–40 µg of nuclear protein extract resolved on 5% SDS-PAGE, transferred onto polyvinylidene difluoride membrane, and subjected to immunodetection using a 1:2,000 dilution of primary antibody and an enhanced chemiluminescence detection 13.
DNA samples were prepared from cultured cell lines by standard procedures. 10 µg of genomic DNA was digested overnight with the restriction enzymes EcoRI-EagI or HindIII-SacII, EagI and SacII being sensible to methylation. Restriction fragments were separated by electrophoresis on 0.8% agarose gel, Southern blotted, and hybridized with radiolabeled StB12.3 probe as described previously 20.
DNA MeTase activity was determined in nuclear protein extracts by the assay developed by Adams et al. 21 with minor modifications. Cells were lysed in buffer containing 20 mM Tris-HCl, pH 8, 137 mM NaCl, 5 mM MgCl2, 5 mM EDTA, 10% glycerol, 1 mM PMSF, 10 µg/ml aprotinin, 10 µg/ml leupeptin, and 100 µg/ml RNase. After centrifugation, nuclear extracts were prepared by resuspension of the crude nuclei in high salt buffer. 15–25 µg of proteins was incubated for 2 h at 37°C with 4 µg of poly (dI-dC) as template and 5.25 µM 3H-labeled S-adenosylmethionine (1 µCi; Amersham Pharmacia Biotech) as methyl donor. Reactions were stopped, proteins extracted, and DNA template was recovered by ethanol precipitation. RNA was removed by resuspension of the precipitates in NaOH; DNA was spotted on Whatman filters, dried, and then washed with trichloroacetic acid (5%) followed by ethanol, then ether. Filters were placed in the scintillation mixture, and DNA MeTase activity was determined by scintillation counting. Results were expressed as cpm per microgram of protein; all experiments were performed in duplicate. Background levels were determined in assays where poly (dI-dC) was omitted. Statistical analyses were performed using Student's t test.
Lactate dehydrogenase (LDH) and pyruvate kinase (PK) were measured by standard procedures in the 12,000 g supernatant of Jurkat T cell homogenate as described previously 22. Hexokinase (HK) was measured in the homogenate of Jurkat T cells as reported elsewhere 23. Statistical analyses were performed using Student's t test.
Cellular proliferation was determined by a colorimetric assay system using 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium (MTT) following the manufacturer's instructions (Cell Proliferation Kit I; Boehringer Mannheim).
Results and Discussion
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Abstract
Materials and Methods
Results and Discussion
References
Fragile X syndrome, the most common form of hereditary mental retardation 24, results from repression of the FMR1 gene due to the expansion of the CGG repeats in its first exon and methylation of the 5' CpG island. The latter alteration appears to be the primary cause of the disease, since hypermethylation of the CpG island in the active X chromosome is only observed in affected individuals, whereas there are cases with full expansion of the CGG repeats but with an unmethylated island that do not manifest the syndrome 2526. Furthermore, in vitro reactivation of the FMR1 gene by demethylating agents has been reported recently 27. We have observed a marked inhibitory effect of IL-1β on FMR1 gene expression in RIN cells assessed by RT-PCR of both KH domains and CGG repeats (Fig. 1, a–c). Inhibition of FMR1 expression was appreciable after 12 h of incubation with IL-1β, and complete suppression of the gene resulted with longer exposures (Fig. 1 a). Since IL-1β is known to be a powerful stimulus for induction of NOS in RIN and other cell types 2829, we investigated whether NO acted as a mediator of FMR1 repression. Fig. 1 b shows that SNP, an NO donor, mimics the action of IL-1β, and that the IL effect is fully prevented by the simultaneous addition of L-NMA, an inhibitor of NOS activity. This preventive effect was not observed when we used D-NMA (not shown). To further demonstrate that IL-1β exerts gene silencing via NO production, we used specific iNOS inhibitors such as AMT, EIT, and L-NIL and found that all of them also prevented the action of IL-1β (Fig. 1 c). To determine if FMR1 mRNA stability was altered by NO, ActD was used to inhibit RNA synthesis. As shown in Fig. 1 d, the time course of FMR1 mRNA degradation was not modified by the presence of SNP. Thus, production of NO by IL-1β or addition of NO precursors can produce FMR1 gene silencing. In preliminary experiments, we have observed that IFN-, which induces NO synthesis, as well as NO donors can also inhibit FMR1 expression in a monocyte-macrophage cell line (RAW 264 cells).
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The major mammalian DNA MeTase is a large protein with an NH2-terminal putative regulatory domain comprising two thirds of the protein with eight cysteine residues, and a COOH-terminal catalytic domain with the adenosylmethionine binding region and a proline-cysteine catalytic center 34. The signals and mechanisms involved in regulation of DNA MeTase activity are poorly understood. The NH2 terminus is unnecessary for catalysis, but its cleavage from the COOH terminus causes a large stimulation of the initial velocity of methylation of unmethylated DNA 34. The NH2 terminus contains a major phosphorylation site (serine 514) although its relevance in catalysis is uncertain, since treatment of the enzyme with phosphatases and kinases results in no significant effect on the catalytic rate 35. We assayed whether the effect of NO on DNA MeTase activity was due to activation of guanyl cyclase, by incubation of Jurkat T cells with 2 mM dibutyryl cGMP for 24 h. cGMP had no effect on either DNA MeTase activity or the expression of FMR1 gene (not shown). The Ras signaling pathway has been shown to increase DNA MeTase transcription 36, and recently it has been suggested that fos may transform cells through alterations in DNA methylation 33. Therefore, we tested if the expression of DNA MeTase could be altered by exposure of Jurkat T cells to an NO donor. Northern and Western blot analyses, shown in Fig. 4, a and b, respectively, indicate that NO does not affect the expression of the major human DNA MeTase. We have not studied the expression of the recently described DNA MeTase3A and DNA MeTase3B 37; however, it is very unlikely that they mediate the effects of NO described here, since these two enzymes are present mainly in embryonic tissues 37. Moreover, NO was able to activate DNA MeTase in a nuclear protein extract (see below), thus strongly suggesting that the regulation of the enzyme by NO is not dependent on transcription.
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NO is a broadly distributed signaling molecule involved in numerous physiological and pathophysiological processes 394041, but its action on the genome is poorly understood. Moreover, many actions of IL-1β are mediated by the induction of iNOS and the resulting NO production 4243. We show that by activating DNA MeTase, NO can induce methylation of 5' CpG islands and, hence, repress gene expression. Methylation/demethylation of DNA is known to be associated with X-linked gene inactivation, imprinting, and fragile X syndrome 7815. Changes in DNA methylation are also observed during development, the acquisition of T cell cytokine production profiles, and tumorigenesis 9101112131417, and several transcription factors actively promoting DNA demethylation have been reported 944. Our findings provide the first case of FMR1 gene silencing in situations other than fragile X syndrome, although the methylation status in the two conditions shows some differences. Methylation induced by NO was lost with time, and TSA reversed the inhibitory effect on gene expression induced by NO (see above). In contrast, it has been recently reported that TSA has no effect on transcription in cells from fragile X patients due to additional modifications in histone–DNA association 45. The marked repressive effect of IL-1β and NO on the expression of housekeeping genes, such as FMR1 and HPRT, with a CpG island in the promoter might be part of a general adaptive mechanism triggered in cells challenged by stressing situations.
It has been reported that nuclear factor 
B (NF-B) in B cells can induce specific demethylation of the Ig locus 46, and in some cells, including RIN cells, IL-1β receptor stimulation induces a cascade that activates NF-B 4748. In this work, we have shown that IL-1β clearly represses gene expression by a mechanism involving methylation. Our data indicate that the possible demethylating activity of NF-B in RIN cells does not counterbalance the increase in activity of the DNA MeTase. Similarly, in Jurkat T cells the incubation with PMA plus a calcium ionophore (A23187), which induce NF-B 49, does not prevent the inhibitory action of NO on gene expression (results not shown). However, it could be speculated that IL-1β transitorily represses housekeeping genes having CpG islands via NO production and methylation while inducing tissue/stage-specific gene expression by activating demethylation via NF-B. For instance, it has been reported that Ras induces an increase in demethylase activity in parallel to its induction of transcription of DNA MeTase 36.
Methylation of cytosine also gives an explanation for the high occurrence of genomic C–T transitions observed under exposure to NO 50. The abundance of 5-methylcytosine in methylated DNA favors the transition to thymine by simple deamination, which can occur spontaneously and is potentiated by NO 51. Finally, given the resemblance between certain viruses and housekeeping promoters 1, the reported antiviral action of NO 52 could be explained by methylation-dependent silencing of the viral genome. Interestingly, DNA MeTase is a housekeeping gene without 5' CpG island and, thus, its expression is insensitive to NO (see above). In contrast, it has a specific promoter containing activating protein (AP)-1, AP-2, and glucocorticoid response elements 53, suggesting a potentially high level of regulation by cellular signal transduction pathways.
In conclusion, we report here a novel action of IL-1β mediated by NO production. NO induces a posttranscriptional increase in the activity of DNA MeTase, resulting in CpG island methylation and suppression of gene expression. These results give new insights into the pathophysiological regulation of genes with CpG-rich promoters.
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Acknowledgments |
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This work is supported by grants from the Comisión Interministerial de Ciencia y Tecnología (SAF96-0205) and Servicio Andaluz de Salud.
Submitted: 25 June 1999
Revised: 17 September 1999
Accepted: 21 September 1999
B, nuclear factor B; NMA, N-methyl arginine; NO, nitric oxide; NOS, NO synthase; PK, pyruvate kinase; RIN, RINm5F; RT, reverse transcription; SIN, 3-morpholinosydnonimine hydrochloride; SNAP, S-nitroso-N-acetylpenicillamine; SNP, sodium nitroprusside; SSPE, saline-sodium phosphate-EDTA; TSA, trichostatin A.
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References |
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| TABLE OF CONTENTS |
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), and peroxynitrite (
) on the activity of DNA MeTase. (b) Time course of DNA MeTase activity in the presence of 50 µM SNAP (•), SNP (
), or expired SNAP (
). Values in plots a and b are expressed in percentage of control values by mean ± SEM of three or two independent experiments in duplicate. (c) Effect of reducing agents on DNA MeTase activity stimulated by 50 µM SNAP. The nuclear protein extract was incubated for 3 h without (control) or with 50 µM SNAP. Nuclear protein extracts were recovered, after washing, by centrifugation or by filtration in a Sephadex G-25 spin column. Samples were further incubated for 2 h with no addition (control and SNAP) or in the presence of 5 mM DTT (SNAP/DTT), 100 µM GSH (SNAP/GSH), or 100 µM β-ME (SNAP/β-ME). Values are expressed in percentage of control values by mean ± SEM of at least three independent experiments in duplicate. All the values of DNA MeTase activity in the presence of the reducing agents were significantly different (P < 0.001) from the value of enzymatic activity in the absence of the agents. The average DNA MeTase activity in basal conditions was 0.017 ± 0.005 (n = 15) pmol/h/µg protein. In each experiment, the basal DNA MeTase activity was set to 100%.
