Quantitative models for accelerated protein dissociation from nucleosomal DNA

Author:

Chen Cai12,Bundschuh Ralf132

Affiliation:

1. Biophysics Graduate Program, The Ohio State University, Columbus, OH, USA

2. Center for RNA Biology, The Ohio State University, Columbus, OH, USA

3. Departments of Physics and Chemistry & Biochemistry and Division of Hematology, The Ohio State University, Columbus, OH, USA

Abstract

Abstract Binding of transcription factors to their binding sites in promoter regions is the fundamental event in transcriptional gene regulation. When a transcription factor binding site is located within a nucleosome, the DNA has to partially unwrap from the nucleosome to allow transcription factor binding. This reduces the rate of transcription factor binding and is a known mechanism for regulation of gene expression via chromatin structure. Recently a second mechanism has been reported where transcription factor off-rates are dramatically increased when binding to target sites within the nucleosome. There are two possible explanations for such an increase in off-rate short of an active role of the nucleosome in pushing the transcription factor off the DNA: (i) for dimeric transcription factors the nucleosome can change the equilibrium between monomeric and dimeric binding or (ii) the nucleosome can change the equilibrium between specific and non-specific binding to the DNA. We explicitly model both scenarios and find that dimeric binding can explain a large increase in off-rate while the non-specific binding model cannot be reconciled with the large, experimentally observed increase. Our results suggest a general mechanism how nucleosomes increase transcription factor dissociation to promote exchange of transcription factors and regulate gene expression.

Publisher

Oxford University Press (OUP)

Subject

Genetics

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