Mechanistic details of the actinobacterial lyase-catalyzed degradation reaction of 2-hydroxyisobutyryl-CoA

Michael Zahn; Gerhard König; Huy Viet Cuong Pham; Barbara Seroka; Ryszard Lazny; Guangli Yang; Ouathek Ouerfelli; Zenon Lotowski; Thore Rohwerder

doi:10.1016/j.jbc.2021.101522

Mechanistic details of the actinobacterial lyase-catalyzed degradation reaction of 2-hydroxyisobutyryl-CoA

J Biol Chem. 2022 Jan;298(1):101522. doi: 10.1016/j.jbc.2021.101522. Epub 2021 Dec 22.

Authors

Michael Zahn¹, Gerhard König², Huy Viet Cuong Pham³, Barbara Seroka⁴, Ryszard Lazny⁴, Guangli Yang⁵, Ouathek Ouerfelli⁵, Zenon Lotowski⁴, Thore Rohwerder⁶

Affiliations

¹ Centre for Enzyme Innovation, School of Biological Sciences, Institute of Biological and Biomedical Sciences, University of Portsmouth, Portsmouth, United Kingdom. Electronic address: michael.zahn@port.ac.uk.
² Centre for Enzyme Innovation, School of Biological Sciences, Institute of Biological and Biomedical Sciences, University of Portsmouth, Portsmouth, United Kingdom.
³ Department of Environmental Microbiology, Helmholtz Centre for Environmental Research - UFZ, Leipzig, Germany.
⁴ Faculty of Chemistry, University of Bialystok, Bialystok, Poland.
⁵ Organic Synthesis Core Facility, Memorial Sloan Kettering Cancer Center (MSKCC), New York, New York, USA.
⁶ Department of Environmental Microbiology, Helmholtz Centre for Environmental Research - UFZ, Leipzig, Germany. Electronic address: thore.rohwerder@ufz.de.

Abstract

Actinobacterial 2-hydroxyacyl-CoA lyase reversibly catalyzes the thiamine diphosphate-dependent cleavage of 2-hydroxyisobutyryl-CoA to formyl-CoA and acetone. This enzyme has great potential for use in synthetic one-carbon assimilation pathways for sustainable production of chemicals, but lacks details of substrate binding and reaction mechanism for biochemical reengineering. We determined crystal structures of the tetrameric enzyme in the closed conformation with bound substrate, covalent postcleavage intermediate, and products, shedding light on active site architecture and substrate interactions. Together with molecular dynamics simulations of the covalent precleavage complex, the complete catalytic cycle is structurally portrayed, revealing a proton transfer from the substrate acyl Cβ hydroxyl to residue E493 that returns it subsequently to the postcleavage Cα-carbanion intermediate. Kinetic parameters obtained for mutants E493A, E493Q, and E493K confirm the catalytic role of E493 in the WT enzyme. However, the 10- and 50-fold reduction in lyase activity in the E493A and E493Q mutants, respectively, compared with WT suggests that water molecules may contribute to proton transfer. The putative catalytic glutamate is located on a short α-helix close to the active site. This structural feature appears to be conserved in related lyases, such as human 2-hydroxyacyl-CoA lyase 2. Interestingly, a unique feature of the actinobacterial 2-hydroxyacyl-CoA lyase is a large C-terminal lid domain that, together with active site residues L127 and I492, restricts substrate size to ≤C5 2-hydroxyacyl residues. These details about the catalytic mechanism and determinants of substrate specificity pave the ground for designing tailored catalysts for acyloin condensations for one-carbon and short-chain substrates in biotechnological applications.

Keywords: 2-hydroxyacyl-CoA synthase; Actinomycetospora; carbonyl compounds; formate assimilation; glycolyl-CoA; mono-carbon extension; oxalyl-CoA decarboxylase; x-ray diffraction.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Acyl Coenzyme A* / chemistry
Acyl Coenzyme A* / metabolism
Carbon
Catalysis
Catalytic Domain
Crystallography, X-Ray
Humans
Lyases* / chemistry
Lyases* / metabolism
Protons
Structure-Activity Relationship
Substrate Specificity

Substances

Acyl Coenzyme A
Protons
Carbon
Lyases

Abstract

Publication types

MeSH terms

Substances

Grants and funding