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Cyclic Ion Mobility-Collision Activation Experiments Elucidate Protein Behavior in the Gas Phase

  • Charles Eldrid
  • , Aisha Ben-Younis
  • , Jakub Ujma
  • , Hannah Britt
  • , Tristan Cragnolini
  • , Symeon Kalfas
  • , Dale Cooper-Shepherd
  • , Nick Tomczyk
  • , Kevin Giles
  • , Mike Morris
  • , Rehana Akter
  • , Daniel Raleigh
  • , Konstantinos Thalassinos

Research output: Contribution to journalArticlepeer-review

39 Scopus citations

Abstract

Ion mobility coupled to mass spectrometry (IM-MS) is widely used to study protein dynamics and structure in the gas phase. Increasing the energy with which the protein ions are introduced to the IM cell can induce them to unfold, providing information on the comparative energetics of unfolding between different proteoforms. Recently, a high-resolution cyclic IM-mass spectrometer (cIM-MS) was introduced, allowing multiple, consecutive tandem IM experiments (IMn) to be carried out. We describe a tandem IM technique for defining detailed protein unfolding pathways and the dynamics of disordered proteins. The method involves multiple rounds of IM separation and collision activation (CA): IM-CA-IM and CA-IM-CA-IM. Here, we explore its application to studies of a model protein, cytochrome C, and dimeric human islet amyloid polypeptide (hIAPP), a cytotoxic and amyloidogenic peptide involved in type II diabetes. In agreement with prior work using single stage IM-MS, several unfolding events are observed for cytochrome C. IMn-MS experiments also show evidence of interconversion between compact and extended structures. IMn-MS data for hIAPP shows interconversion prior to dissociation, suggesting that the certain conformations have low energy barriers between them and transition between compact and extended forms.

Original languageEnglish
Pages (from-to)1545-1552
Number of pages8
JournalJournal of the American Society for Mass Spectrometry
Volume32
Issue number6
DOIs
StatePublished - Jun 2 2021

Keywords

  • ion-mobility mass spectrometry
  • protein unfolding

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