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Loss of methylation in CpG sites in the NF-κB enhancer elements of inducible nitric oxide synthase is responsible for gene induction in human articular chondrocytes

De Andrés González, Mª Carmen; Imagawa, K.; Hashimoto, K.; González Martínez-Pedrayo, Antonio; Roach, H. I.; Goldring, M. B.; Oreffo, R. O. C.
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URI: http://hdl.handle.net/20.500.11940/3484
PMID: 23239081
DOI: 10.1002/art.37806
ISSN: 0004-3591
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Arthritis Rheum . 2013 Mar;65(3):732-42. (382.1Kb)
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Fecha de publicación
2013
Título de revista
ARTHRITIS AND RHEUMATISM
Tipo de contenido
Artigo
MeSH
Aged | Aged, 80 and over | Cartilage, Articular | Chondrocytes | CpG Islands | DNA Methylation | Enhancer Elements, Genetic | Female | Gene Expression Regulation, Enzymologic | Humans | Male | Middle Aged | NF-kappa B | Nitric Oxide Synthase Type II | Osteoarthritis, Hip | Primary Cell Culture | Promoter Regions, Genetic/physiology
Resumen
OBJECTIVE: To investigate whether the abnormal expression of inducible nitric oxide synthase (iNOS) by osteoarthritic (OA) human chondrocytes is associated with changes in the DNA methylation status in the promoter and/or enhancer elements of iNOS. METHODS: Expression of iNOS was quantified by quantitative reverse transcriptase-polymerase chain reaction. The DNA methylation status of the iNOS promoter and enhancer regions was determined by bisulfite sequencing or pyrosequencing. The effect of CpG methylation on iNOS promoter and enhancer activities was determined using a CpG-free luciferase vector and a CpG methyltransferase. Cotransfections with expression vectors encoding NF-kappaB subunits were carried out to analyze iNOS promoter and enhancer activities in response to changes in methylation status. RESULTS: The 1,000-bp iNOS promoter has only 7 CpG sites, 6 of which were highly methylated in both control and OA samples. The CpG site at -289 and the sites in the starting coding region were largely unmethylated in both groups. The NF-kappaB enhancer region at -5.8 kb was significantly demethylated in OA samples compared with control samples. This enhancer element was transactivated by cotransfection with the NF-kappaB subunit p65, alone or together with p50. Critically, methylation treatment of the iNOS enhancer element significantly decreased its activity in a reporter assay. CONCLUSION: These findings demonstrate the association between demethylation of specific NF-kappaB-responsive enhancer elements and the activation of iNOS transactivation in human OA chondrocytes, consistent with the differences in methylation status observed in vivo in normal and human OA cartilage and, importantly, show association with the OA process.

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