Exploring the structural dynamics of proteins by pressure perturbation using macromolecular crystallography

Nathalie Colloc'h; Anne-Claire Dhaussy; Eric Girard

doi:10.1016/bs.mie.2023.06.007

Exploring the structural dynamics of proteins by pressure perturbation using macromolecular crystallography

Methods Enzymol. 2023:688:349-381. doi: 10.1016/bs.mie.2023.06.007. Epub 2023 Jul 26.

Authors

Nathalie Colloc'h¹, Anne-Claire Dhaussy², Eric Girard³

Affiliations

¹ Imagerie et stratégies thérapeutiques pour les cancers et tissus cérébraux (ISTCT), CNRS Université de Caen Normandie, Centre Cyceron, Caen, France.
² Normandie Université, CRISMAT UMR, Caen, France.
³ Univ. Grenoble Alpes, CEA, CNRS, IBS, Grenoble, France. Electronic address: eric.girard@ibs.fr.

PMID: 37748831
DOI: 10.1016/bs.mie.2023.06.007

Abstract

High pressure is a convenient thermodynamic parameter to probe the dynamics of proteins as it is intimately related to volume which is essential for protein function. To be biologically active, a protein fluctuates between different substates. Pressure perturbation can promote some hidden substates by modifying the population between them. High pressure macromolecular crystallography (HPMX) is a perfect tool to capture and to characterize such substates at a molecular level providing new insights on protein dynamics. The present chapter describes the use of the diamond anvil cell to perform HPMX experiments. It also provides tips on sample preparation and optimal data collection as well as on efficient analysis of the resulting high-pressure structures.

Keywords: HPMX; High pressure; Macromolecular crystallography; Protein dynamics; Protein substates.

MeSH terms

Crystallography
Macromolecular Substances
Specimen Handling*
Thermodynamics

Substances

Macromolecular Substances