par Fuks, François 
;Hurd, Paul J.;Wolf, Daniel;Nan, Xinsheng;Bird, Adrian P;Kouzarides, Tony
Référence The Journal of biological chemistry, 278, 6, page (4035-4040)
Publication Publié, 2003-02
;Hurd, Paul J.;Wolf, Daniel;Nan, Xinsheng;Bird, Adrian P;Kouzarides, TonyRéférence The Journal of biological chemistry, 278, 6, page (4035-4040)
Publication Publié, 2003-02
Article révisé par les pairs
| Résumé : | DNA methylation plays an important role in mammalian development and correlates with chromatin-associated gene silencing. The recruitment of MeCP2 to methylated CpG dinucleotides represents a major mechanism by which DNA methylation can repress transcription. MeCP2 silences gene expression partly by recruiting histone deacetylase (HDAC) activity, resulting in chromatin remodeling. Here, we show that MeCP2 associates with histone methyltransferase activity in vivo and that this activity is directed against Lys(9) of histone H3. Two characterized repression domains of MeCP2 are involved in tethering the histone methyltransferase to MeCP2. We asked if MeCP2 can deliver Lys(9) H3 methylation to the H19 gene, whose activity it represses. We show that the presence of MeCP2 on nucleosomes within the repressor region of the H19 gene (the differentially methylated domain) coincides with an increase in H3 Lys(9) methylation. Our data provide evidence that MeCP2 reinforces a repressive chromatin state by acting as a bridge between two global epigenetic modifications, DNA methylation and histone methylation. |
