Hydrogen-Deuterium Exchange Coupled to Top- and Middle-Down Mass Spectrometry Reveals Histone Tail Dynamics before and after Nucleosome Assembly

Kelly R. Karch, Mariel Coradin, Levani Zandarashvili, Zhong Yuan Kan, Morgan Gerace, S. Walter Englander, Ben E. Black, Benjamin A. Garcia

Research output: Contribution to journalArticlepeer-review

24 Scopus citations

Abstract

Until recently, a major limitation of hydrogen-deuterium exchange mass spectrometry (HDX-MS) was that resolution of deuterium localization was limited to the length of the peptide generated during proteolysis. However, electron transfer dissociation (ETD) has been shown to preserve deuterium label in the gas phase, enabling better resolution. To date, this technology remains mostly limited to small, already well-characterized proteins. Here, we optimize, expand, and adapt HDX-MS tandem MS (MS/MS) capabilities to accommodate histone and nucleosomal complexes on top-down HDX-MS/MS and middle-down HDX-MS/MS platforms and demonstrate that near site-specific resolution of deuterium localization can be obtained with high reproducibility. We are able to study histone tail dynamics in unprecedented detail, which have evaded analysis by traditional structural biology techniques for decades, revealing important insights into chromatin biology. Together, the results of these studies highlight the versatility, reliability, and reproducibility of ETD-based HDX-MS/MS methodology to interrogate large protein and protein/DNA complexes.

Original languageEnglish
Pages (from-to)1651-1663.e3
JournalStructure
Volume26
Issue number12
DOIs
StatePublished - Dec 4 2018

Keywords

  • electron transfer dissociation
  • histone tails
  • histones
  • hydrogen deuterium exchange
  • mass spectrometry
  • middle-down HDX
  • top-down HDX

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