4.8 Article

A high-resolution map of transcriptional repression

Journal

ELIFE
Volume 6, Issue -, Pages -

Publisher

eLIFE SCIENCES PUBL LTD
DOI: 10.7554/eLife.22767

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Funding

  1. UK-China Scholarships for Excellence
  2. Wellcome [098021/Z/11/Z, 099276/Z/12/Z]
  3. Medical Research Council [MC-A652-5PY20]
  4. Wellcome Trust [098021/Z/11/Z, 099276/Z/12/Z] Funding Source: Wellcome Trust
  5. MRC [MC_UP_1102/5, MC_U120027516] Funding Source: UKRI
  6. Medical Research Council [MC_U120027516, MC_UP_1102/5, 1375534, 1583062, MC_PC_12009] Funding Source: researchfish

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Turning genes on and off is essential for development and homeostasis, yet little is known about the sequence and causal role of chromatin state changes during the repression of active genes. This is surprising, as defective gene silencing underlies developmental abnormalities and disease. Here we delineate the sequence and functional contribution of transcriptional repression mechanisms at high temporal resolution. Inducible entry of the NuRD-interacting transcriptional regulator Ikaros into mouse pre-B cell nuclei triggered immediate binding to target gene promoters. Rapid RNAP2 eviction, transcriptional shutdown, nucleosome invasion, and reduced transcriptional activator binding required chromatin remodeling by NuRD-associated Mi2beta/CHD4, but were independent of HDAC activity. Histone deacetylation occurred after transcriptional repression. Nevertheless, HDAC activity contributed to stable gene silencing. Hence, high resolution mapping of transcriptional repression reveals complex and interdependent mechanisms that underpin rapid transitions between transcriptional states, and elucidates the temporal order, functional role and mechanistic separation of NuRD-associated enzymatic activities.

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