Literature DB >> 21768347

Histone fold modifications control nucleosome unwrapping and disassembly.

Marek Simon1, Justin A North, John C Shimko, Robert A Forties, Michelle B Ferdinand, Mridula Manohar, Meng Zhang, Richard Fishel, Jennifer J Ottesen, Michael G Poirier.   

Abstract

Nucleosomes are stable DNA-histone protein complexes that must be unwrapped and disassembled for genome expression, replication, and repair. Histone posttranslational modifications (PTMs) are major regulatory factors of these nucleosome structural changes, but the molecular mechanisms associated with PTM function remains poorly understood. Here we demonstrate that histone PTMs within distinct structured regions of the nucleosome directly regulate the inherent dynamic properties of the nucleosome. Precise PTMs were introduced into nucleosomes by chemical ligation. Single molecule magnetic tweezers measurements determined that only PTMs near the nucleosome dyad increase the rate of histone release in unwrapped nucleosomes. In contrast, FRET and restriction enzyme analysis reveal that only PTMs throughout the DNA entry-exit region increase unwrapping and enhance transcription factor binding to nucleosomal DNA. These results demonstrate that PTMs in separate structural regions of the nucleosome control distinct dynamic events, where the dyad regulates disassembly while the DNA entry-exit region regulates unwrapping. These studies are consistent with the conclusion that histone PTMs may independently influence nucleosome dynamics and associated chromatin functions.

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Year:  2011        PMID: 21768347      PMCID: PMC3150920          DOI: 10.1073/pnas.1106264108

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  52 in total

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3.  Acetylation of histone H3 at the nucleosome dyad alters DNA-histone binding.

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  104 in total

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2.  PHF1 Tudor and N-terminal domains synergistically target partially unwrapped nucleosomes to increase DNA accessibility.

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3.  Traceless semisynthesis of a set of histone 3 species bearing specific lysine methylation marks.

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5.  Scratching the (lateral) surface of chromatin regulation by histone modifications.

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6.  Preparing semisynthetic and fully synthetic histones h3 and h4 to modify the nucleosome core.

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8.  Bridging chromatin structure and function over a range of experimental spatial and temporal scales by molecular modeling.

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Review 9.  Micro- and nanoscale devices for the investigation of epigenetics and chromatin dynamics.

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Review 10.  Histone variants: the tricksters of the chromatin world.

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