The enzymatic oxygen sensor cysteamine dioxygenase binds its protein substrates through their N-termini

Karishma Patel; Yannasittha Jiramongkol; Alexander Norman; Joshua W C Maxwell; Biswaranjan Mohanty; Richard J Payne; Kristina M Cook; Mark D White

doi:10.1016/j.jbc.2024.107653

The enzymatic oxygen sensor cysteamine dioxygenase binds its protein substrates through their N-termini

J Biol Chem. 2024 Sep;300(9):107653. doi: 10.1016/j.jbc.2024.107653. Epub 2024 Aug 8.

Authors

Karishma Patel¹, Yannasittha Jiramongkol², Alexander Norman³, Joshua W C Maxwell⁴, Biswaranjan Mohanty⁵, Richard J Payne⁴, Kristina M Cook⁶, Mark D White⁷

Affiliations

¹ School of Chemistry, The University of Sydney, Camperdown, NSW, Australia; School of Life and Environmental Sciences, The University of Sydney, Camperdown, NSW, Australia.
² School of Chemistry, The University of Sydney, Camperdown, NSW, Australia; Faculty of Science, Charles Perkins Centre, The University of Sydney, Camperdown, NSW, Australia.
³ School of Chemistry, The University of Sydney, Camperdown, NSW, Australia.
⁴ School of Chemistry, The University of Sydney, Camperdown, NSW, Australia; Australian Research Council Centre of Excellence for Innovations in Peptide and Protein Science, Sydney, NSW, Australia.
⁵ Sydney Analytical Core Research Facility, The University of Sydney, Camperdown, NSW, Australia.
⁶ Faculty of Medicine and Health, Charles Perkins Centre, The University of Sydney, Camperdown, NSW, Australia.
⁷ School of Chemistry, The University of Sydney, Camperdown, NSW, Australia. Electronic address: mark.white@sydney.edu.au.

Abstract

The non-heme iron-dependent dioxygenase 2-aminoethanethiol (aka cysteamine) dioxygenase (ADO) has recently been identified as an enzymatic oxygen sensor that coordinates cellular changes to hypoxia by regulating the stability of proteins bearing an N-terminal cysteine (Nt-cys) through the N-degron pathway. It catalyzes O₂-dependent Nt-cys sulfinylation, which promotes proteasomal degradation of the target. Only a few ADO substrates have been verified, including regulators of G-protein signaling (RGS) 4 and 5, and the proinflammatory cytokine interleukin-32, all of which exhibit cell and/or tissue specific expression patterns. ADO, in contrast, is ubiquitously expressed, suggesting it can regulate the stability of additional Nt-cys proteins in an O₂-dependent manner. However, the role of individual chemical groups, active site metal, amino acid composition, and globular structure on protein substrate association remains elusive. To help identify new targets and examine the underlying biochemistry of the system, we conducted a series of biophysical experiments to investigate the binding requirements of established ADO substrates RGS5 and interleukin-32. We demonstrate, using surface plasmon response and enzyme assays, that a free, unmodified Nt-thiol and Nt-amine are vital for substrate engagement through active site metal coordination, with residues next to Nt-cys moderately impacting association and catalytic efficiency. Additionally, we show, through ¹H-¹⁵N heteronuclear single quantum coherence nuclear magnetic resonance titrations, that the globular portion of RGS5 has limited impact on ADO association, with interactions restricted to the N-terminus. This work establishes key features involved in ADO substrate binding, which will help identify new protein targets and, subsequently, elucidate its role in hypoxic adaptation.

Keywords: ADO; N-degron pathway; enzyme kinetics; hypoxia; nuclear magnetic resonance; oxygen-sensing; posttranslational modification; protein degradation; surface plasmon resonance.

MeSH terms

Dioxygenases* / chemistry
Dioxygenases* / genetics
Dioxygenases* / metabolism
Humans
Oxygen* / chemistry
Oxygen* / metabolism
Protein Binding*
RGS Proteins / chemistry
RGS Proteins / genetics
RGS Proteins / metabolism
Substrate Specificity

Substances

cysteamine dioxygenase
Oxygen
Dioxygenases
RGS Proteins