4.5 Article

The Effect of Linker Histone's Nucleosome Binding Affinity on Chromatin Unfolding Mechanisms

Journal

BIOPHYSICAL JOURNAL
Volume 101, Issue 7, Pages 1670-1680

Publisher

CELL PRESS
DOI: 10.1016/j.bpj.2011.07.044

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Funding

  1. National Science Foundation [MCB-0316771]
  2. National Institutes of Health [R01 GM55164]
  3. American Chemical Society [PRF39225-AC4]
  4. Philip Morris USA
  5. Philip Morris International
  6. Schlumberger Faculty

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Eukaryotic gene activation requires selective unfolding of the chromatin fiber to access the DNA for processes such as DNA transcription, replication, and repair. Mutation/modification experiments of linker histone (LH) H1 suggest the importance of dynamic mechanisms for LH binding/dissociation, but the effects on chromatin's unfolding pathway remain unclear. Here we investigate the stretching response of chromatin fibers by mesoscale modeling to complement single-molecule experiments, and present various unfolding mechanisms for fibers with different nucleosome repeat lengths (NRLs) with/without LH that are fixed to their cores or bind/unbind dynamically with different affinities. Fiber softening occurs for long compared to short NRL (due to facile stacking rearrangements), dynamic compared to static LH/core binding as well as slow rather than fast dynamic LH rebinding (due to DNA stem destabilization), and low compared to high LH concentration (due to DNA stem inhibition). Heterogeneous superbead constructs-nucleosome clusters interspersed with extended fiber regions emerge during unfolding of medium-NRL fibers and may be related to those observed experimentally. Our work suggests that fast and slow LH binding pools, present simultaneously in vivo, might act cooperatively to yield controlled fiber unfolding at low forces. Medium-NRL fibers with multiple dynamic LH pools offer both flexibility and selective DNA exposure, and may be evolutionarily suitable to regulate chromatin architecture and gene expression.

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