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Addressing structural heterogeneity in real-time tracking of protein dynamics triggered by caged compounds
Umeå University, Faculty of Science and Technology, Department of Chemistry.
Umeå University, Faculty of Science and Technology, Department of Chemistry.ORCID iD: 0000-0002-0706-7414
Umeå University, Faculty of Science and Technology, Department of Chemistry.ORCID iD: 0000-0001-7039-7312
Umeå University, Faculty of Science and Technology, Department of Chemistry.
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2025 (English)In: Journal of Molecular Biology, ISSN 0022-2836, E-ISSN 1089-8638, Vol. 437, no 24, article id 169476Article in journal (Refereed) Published
Abstract [en]

Protein molecules typically carry out their biological function by adopting multiple, transient conformations, which complicates their structural characterization. Synchrotron-based time-resolved X-ray solution scattering (TR-XSS) combined with triggering by caged compounds enables real-time monitoring of protein structural transitions in a wide range of protein targets. However, non-instantaneous release of photosensitive cages and undefined equilibrium states complicate data interpretation. In this work, we addressed these challenges with the Escherichia coli adenylate kinase (AdK) enzyme as a model system. To account for, and visualize, heterogeneity resulting from overlap between the ATP release kinetics and protein catalytic motions, we based the structural refinement on ensembles from a pool of putative target structures generated by molecular dynamics (MD) simulations. Under equilibrium conditions, protein conformations preferentially occupied intermediate states in which the ATP- and AMP-binding domains were never fully opened or closed. Upon ATP availability, ensembles successively shifted toward fully closed and open conformations accompanying partial unfolding, which is consistent with a cracking model for triggering the enzymatic reaction. The findings demonstrate that non-instantaneous substrate release can significantly impact protein transition kinetics but can be tackled with the use of ensemble-based structural refinement. Hence, this work establishes a framework for dissecting rapid protein conformational changes in solution induced by caged compounds.
Place, publisher, year, edition, pages
Elsevier, 2025. Vol. 437, no 24, article id 169476
Keywords [en]
adenylate kinase, ensemble optimization, genetic algorithm, protein dynamics, time-resolved X-ray solution scattering
National Category
Biochemistry Molecular Biology Physical Chemistry
Identifiers
URN: urn:nbn:se:umu:diva-245931DOI: 10.1016/j.jmb.2025.169476ISI: 001601268400001PubMedID: 41061951Scopus ID: 2-s2.0-105018718298OAI: oai:DiVA.org:umu-245931DiVA, id: diva2:2014919
Funder
Swedish Research Council, 2024-04385The Kempe Foundations, JCSMK 24-543Available from: 2025-11-19 Created: 2025-11-19 Last updated: 2026-03-30Bibliographically approved
In thesis
1. Characterizing ATP-dependent protein structural dynamics in solution
Open this publication in new window or tab >>Characterizing ATP-dependent protein structural dynamics in solution
2026 (English)Doctoral thesis, comprehensive summary (Other academic)
Alternative title[sv]
Karaktärisering av ATP-beroende strukturell proteindynamik i lösning
Abstract [en]

Proteins are dynamic molecules whose function depends on structural changes that occur over a broad range of timescales. Protein motions can be linked to important functionalities such as ligand binding, catalysis, transport and regulation. To understand such processes, it is necessary to go beyond determination of static structures and follow protein conformational changes in time. The work presented in this thesis focuses on ATP-dependent protein dynamics in solution using time-resolved X-ray solution scattering (TR-XSS), combined with molecular dynamics-based structural refinement and ensemble analysis. 

A detector readout-based TR-XSS setup was established using adenylate kinase (AdK) as a model system (Paper I). AdK is a soluble protein that carries out the interconversion of ATP, AMP and ADP, helping the cell balance adenine nucleotide levels. Using laser-induced release of caged-ATP, we collected time-resolved scattering data at a general-purpose synchrotron beamline, and the radiation damage, and data quality was evaluated. Although the temporal resolution was lower than what can be achieved at dedicated time-resolved beamlines, the setup enabled detection of structural changes on the millisecond timescale and provided a promising and accessible workflow for TR-XSS measurements.

Then we proceeded to investigate conformational heterogeneity and ATP-induced domain motions in AdK (Paper III). Ensemble based refinement was applied to time-resolved difference scattering data, showing that AdK exists as a heterogeneous conformational ensemble in solution. This ensemble shifts towards catalytically active conformations after ATP release. In later work (Paper IV), an application of an improved ATP releasing strategy, combined with TR-XSS and metadynamics-derived structure pools enabled us to resolve conformational changes in the microsecond range. These results showed that the substrate binding domains of AdK do not close simultaneously but follow a defined sequence of events and reach the closed state of the enzyme on a sub-millisecond timescale.

The final part of the work focused on a bacterial Ca2+ ATPase (LMCA1). We used TR-XSS combined with targeted molecular dynamics to investigate ATP-dependent structural changes in LMCA1 (Paper II). The results identified that phosphorylation is the rate-limiting step of the Ca2+ transport cycle.

Overall, this thesis demonstrates that TR-XSS, when combined with simulation-based structural refinement, is a powerful methodology for the study of structural dynamics in solution and makes a contribution to the characterization of ATP-driven protein function.
Place, publisher, year, edition, pages
Umeå: Umeå University, 2026. p. 76
National Category
Biophysics
Research subject
Physical Chemistry
Identifiers
urn:nbn:se:umu:diva-251554 (URN)978-91-8070-975-0 (ISBN)978-91-8070-976-7 (ISBN)
Public defence
2026-04-24, Aula Biologica, Linnaeus väg 7, 907 36 Umeå, Umeå, 09:00 (English)
Opponent
Supervisors
Available from: 2026-04-02 Created: 2026-03-30 Last updated: 2026-04-02Bibliographically approved

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Magkakis, KonstantinosOrädd, FredrikPett, ChristianLycksell, MarieAndersson, Magnus

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