The circadian demethylation of a unique intronic deoxymethylCpG-rich island boosts the transcription of its cognate circadian clock output gene

Author:

Misra Nisha1,Damara Manohar1,Ye Tao1ORCID,Chambon Pierre123ORCID

Affiliation:

1. Institut de Génétique et de Biologie Moléculaire et Cellulaire, CNRS Unité Mixte de Recherche 7104, INSERM U1258, 67404 Illkirch, France

2. University of Strasbourg Institute for Advanced Study, 67404 Illkirch, France

3. Collège de France, Illkirch 67404, France

Abstract

We demonstrate that there is a tight functional relationship between two highly evolutionary conserved cell processes, i.e., the circadian clock (CC) and the circadian DNA demethylation–methylation of cognate deoxyCpG-rich islands. We have discovered that every circadian clock-controlled output gene (CCG), but not the core clock nor its immediate-output genes, contains a single cognate intronic deoxyCpG-rich island, the demethylation–methylation of which is controlled by the CC. During the transcriptional activation period, these intronic islands are demethylated and, upon dimerization of two YY1 protein binding sites located upstream to the transcriptional enhancer and downstream from the deoxyCpG-rich island, store activating components initially assembled on a cognate active enhancer (a RORE, a D-box or an E-box), in keeping with the generation of a transcriptionally active condensate that boosts the initiation of transcription of their cognate pre-mRNAs. We report how these single intronic deoxyCpG-rich islands are instrumental in such a circadian activation/repression transcriptional process.

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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