Measuring dynamic changes in histone modifications and nucleosome density during activated transcription in budding yeast.

Chhabi K Govind, Daniel Ginsburg, Alan G Hinnebusch
Author Information
  1. Chhabi K Govind: Department of Biological Sciences, Oakland University, Rochester, MI, USA. govind@oakland.edu

Abstract

Chromatin immunoprecipitation is widely utilized to determine the in vivo binding of factors that regulate transcription. This procedure entails formaldehyde-mediated cross-linking of proteins and isolation of soluble chromatin followed by shearing. The fragmented chromatin is subjected to immunoprecipitation using antibodies against the protein of interest and the associated DNA is identified using quantitative PCR. Since histones are posttranslationally modified during transcription, this technique can be effectively used to determine the changes in histone modifications that occur during transcription. In this paper, we describe a detailed methodology to determine changes in histone modifications in budding yeast that takes into account reductions in nucleosome.

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Grants

  1. R01 GM095514/NIGMS NIH HHS

MeSH Term

Chemical Precipitation
Chromatin Immunoprecipitation
Cross-Linking Reagents
DNA, Fungal
Histones
Molecular Biology
Nucleosomes
Polymerase Chain Reaction
Protein Processing, Post-Translational
Saccharomycetales
Solubility
Transcription, Genetic

Chemicals

Cross-Linking Reagents
DNA, Fungal
Histones
Nucleosomes

Word Cloud

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