Intragenic DNA methylation alters chromatin structure and elongation efficiency in mammalian cells

Transcriptional silencing in mammals is often associated with promoter methylation. However, a considerable number of genomic methylated CpGs exist in transposable elements, which are frequently found in intronic regions. To determine whether intragenic methylation influences transcription efficienc...

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Veröffentlicht in:Nature structural & molecular biology 2004-11, Vol.11 (11), p.1068-1075
Hauptverfasser: Lorincz, Matthew C, Dickerson, David R, Schmitt, Mike, Groudine, Mark
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Sprache:eng
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Zusammenfassung:Transcriptional silencing in mammals is often associated with promoter methylation. However, a considerable number of genomic methylated CpGs exist in transposable elements, which are frequently found in intronic regions. To determine whether intragenic methylation influences transcription efficiency, we used the Cre/ loxP -based system, RMCE, to introduce a transgene, methylated exclusively in a region downstream of the promoter, into a specific genomic site. This methylation pattern was maintained in vivo , and yielded a clear decrease in transgene expression relative to an unmethylated control. Notably, RNA polymerase II (Pol II) was depleted exclusively in the methylated region, as was histone H3 di- and trimethylated on Lys4 and acetylated on Lys9 and Lys14. As the methylated region adopts a closed chromatin structure in vivo , we propose that dense intragenic DNA methylation in mammalian cells initiates formation of a chromatin structure that reduces the efficiency of Pol II elongation.
ISSN:1545-9993
1545-9985
DOI:10.1038/nsmb840