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The Allosteric Regulation of Β-Ureidopropionase Depends on Fine-Tuned Stability of Active-Site Loops and Subunit Interfaces
Uppsala University, Disciplinary Domain of Science and Technology, Chemistry, Department of Chemistry - BMC, Biochemistry.ORCID iD: 0000-0002-5460-8375
Uppsala University, Disciplinary Domain of Science and Technology, Chemistry, Department of Chemistry - BMC. Uppsala University, Disciplinary Domain of Science and Technology, Biology, Department of Cell and Molecular Biology, Structural Biology.
Uppsala University, Disciplinary Domain of Science and Technology, Chemistry, Department of Chemistry - BMC. School of Science and Technology, Örebro University, 701 82 Örebro, Sweden.
Department of Medical Biochemistry and Biophysics, Karolinska Institute, Stockholm, Sweden.
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2023 (English)In: Biomolecules, E-ISSN 2218-273X, Vol. 13, no 12, article id 1763Article in journal (Refereed) Published
Abstract [en]

The activity of β-ureidopropionase, which catalyses the last step in the degradation of uracil, thymine, and analogous antimetabolites, is cooperatively regulated by the substrate and product of the reaction. This involves shifts in the equilibrium of the oligomeric states of the enzyme, but how these are achieved and result in changes in enzyme catalytic competence has yet to be determined. Here, the regulation of human β-ureidopropionase was further explored via site-directed mutagenesis, inhibition studies, and cryo-electron microscopy. The active-site residue E207, as well as H173 and H307 located at the dimer-dimer interface, are shown to play crucial roles in enzyme activation. Dimer association to larger assemblies requires closure of active-site loops, which positions the catalytically crucial E207 stably in the active site. H173 and H307 likely respond to ligand-induced changes in their environment with changes in their protonation states, which fine-tunes the active-site loop stability and the strength of dimer-dimer interfaces and explains the previously observed pH influence on the oligomer equilibrium. The correlation between substrate analogue structure and effect on enzyme assembly suggests that the ability to favourably interact with F205 may distinguish activators from inhibitors. The cryo-EM structure of human β-ureidopropionase assembly obtained at low pH provides first insights into the architecture of its activated state. and validates our current model of the allosteric regulation mechanism. Closed entrance loop conformations and dimer-dimer interfaces are highly conserved between human and fruit fly enzymes.
Place, publisher, year, edition, pages
MDPI, 2023. Vol. 13, no 12, article id 1763
Keywords [en]
5-fluorouracil metabolism, allosteric regulation, amidohydrolase, cryo-electron microscopy, pyrimidine degradation
National Category
Structural Biology Biochemistry Molecular Biology
Research subject
Biochemistry; Biology with specialization in Structural Biology
Identifiers
URN: urn:nbn:se:uu:diva-508072DOI: 10.3390/biom13121763ISI: 001130877800001PubMedID: 38136634OAI: oai:DiVA.org:uu-508072DiVA, id: diva2:1783189
Funder
Carl Tryggers foundation , CTS18:84
Note

Authors in the list of papers of Daniela Cederfelt's thesis: Daniela Cederfelt, Dilip Badjugar, Ayan Musse, Dirk Maurer, Berhard Lohkamp, Doreen Dobritzsh

Title in the list of papers of Daniela Cederfelt's thesis: The allosteric regulation of the anticancer drug-metabolizing β-ureidopropionase depends on fine-tuned active-site loop andsubunit interface stability

Available from: 2023-07-19 Created: 2023-07-19 Last updated: 2025-02-20Bibliographically approved
In thesis
1. Structural studies of drug targets and a drug metabolizing enzyme
Open this publication in new window or tab >>Structural studies of drug targets and a drug metabolizing enzyme
2023 (English)Doctoral thesis, comprehensive summary (Other academic)
Abstract [en]

The work presented in this thesis describes how structural information about a protein can be acquired, and how it can be used to answer scientific questions about proteins’ function, their dynamic behaviour and their interactions with other proteins or ligands.

The catalytic function of the pyrimidine-degrading, drug metabolizing enzyme β-ureidopropionase (βUP) is dependent on the shift between oligomeric states. Substitution of amino acids H173 and H307 in the dimer-dimer interface and E207Q in the active site revealed that these are crucial for βUP activation. Inhibition studies of substrate-and product analogues allowed for a hypothesis that the ability to interact with F205 might distinguish activators from inhibitors. The first structure of the activated higher oligomer state of human βUP was determined using cryogenic electron microscopy, and confirmed that the closed entrance loop conformations and dimer-dimer interfaces are conserved between HsβUP and DmβUP. 

Interactions between the epigenetic drug target SET and MYND domain containing protein 3 (SMYD3) and possible inhibitors were investigated. A crystal structure confirmed the covalent bond of a rationally designed, targeted inhibitor to C186 in the active site of SMYD3. A new allosteric binding site was discovered using a biosensor screen with a blocked active site. Crystal structures revealed the location of the new binding site, and the binding mode of the (S)-and (R) enantiomers of the allosteric inhibitor. Lastly, a fragment based drug discovery approach was taken, co-crystallizing and soaking SMYD3 with hits from a fragment screen. This resulted in four crystal structures with weak electron density of fragments at several locations in the enzyme. 

The dynamic acetylcholine binding protein (AChBP) is a homologue of a Cys-loop type ligand gated ion channel. Hits from various biosensor screens, of which some indicated conformational changes, were co-crystallized with AChBP. Seven crystal structures of AChBP in complex with hit compounds from the biophysical screens were determined. Small conformational changes in the Cys-loop were detected in several of the crystal structures, coinciding with the results from the biosensor screens.

In these studies, we explore new strategies for the investigation of the function and regulation of proteins relevant in drug discovery and optimization.
Place, publisher, year, edition, pages
Uppsala: Acta Universitatis Upsaliensis, 2023. p. 65
Series
Digital Comprehensive Summaries of Uppsala Dissertations from the Faculty of Science and Technology, ISSN 1651-6214 ; 2292
Keywords
Biochemistry, Biophysics, Protein structure, X-ray crystallography, Cryogenic electron microscopy, Enzymology, Drug discovery, Pyrimidine degradation
National Category
Biophysics Biochemistry Molecular Biology
Research subject
Biochemistry
Identifiers
urn:nbn:se:uu:diva-508764 (URN)978-91-513-1865-3 (ISBN)
Public defence
2023-09-26, B41, BMC, Husargatan 3, Uppsala, 09:00 (English)
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Available from: 2023-09-04 Created: 2023-08-08 Last updated: 2025-02-20

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Cederfelt, DanielaBadgujar, DilipDanielson, U. HelenaDobritzsch, Doreen

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