TY - JOUR
T1 - Enzymes as viscoelastic catalytic machines
AU - Weinreb, Eyal
AU - McBride, John M.
AU - Siek, Marta
AU - Rougemont, Jacques
AU - Renault, Renaud
AU - Peleg, Yoav
AU - Unger, Tamar
AU - Albeck, Shira
AU - Fridmann-Sirkis, Yael
AU - Lushchekina, Sofya
AU - Sussman, Joel L.
AU - Grzybowski, Bartosz A.
AU - Zocchi, Giovanni
AU - Eckmann, Jean Pierre
AU - Moses, Elisha
AU - Tlusty, Tsvi
N1 - Publisher Copyright: © The Author(s), under exclusive licence to Springer Nature Limited 2025.
PY - 2025/3/28
Y1 - 2025/3/28
N2 - The catalytic cycle involves internal motions and conformational changes that allow enzymes to specifically bind to substrates, reach the transition state and release the product. Such mechanical interactions and motions are often long ranged so that mutations of residues far from the active site can modulate the enzymatic cycle. In particular, regions that undergo high strain during the cycle give mechanical flexibility to the protein, which is crucial for protein motion. Here we directly probe the connection between strain, flexibility and functionality, and we quantify how distant high-strain residues modulate the catalytic function via long-ranged force transduction. We measure the rheological and catalytic properties of wild-type guanylate kinase and of its mutants with a single amino acid replacement in low-/high-strain regions and in binding/non-binding regions. The rheological response of the protein to an applied oscillating force fits a continuum model of a viscoelastic material whose mechanical properties are significantly affected by mutations in high-strain regions, as opposed to mutations in control regions. Furthermore, catalytic activity assays show that mutations in high-strain or binding regions tend to reduce activity, whereas mutations in low-strain, non-binding regions are neutral. These findings suggest that enzymes act as viscoelastic catalytic machines with sequence-encoded mechanical specifications.
AB - The catalytic cycle involves internal motions and conformational changes that allow enzymes to specifically bind to substrates, reach the transition state and release the product. Such mechanical interactions and motions are often long ranged so that mutations of residues far from the active site can modulate the enzymatic cycle. In particular, regions that undergo high strain during the cycle give mechanical flexibility to the protein, which is crucial for protein motion. Here we directly probe the connection between strain, flexibility and functionality, and we quantify how distant high-strain residues modulate the catalytic function via long-ranged force transduction. We measure the rheological and catalytic properties of wild-type guanylate kinase and of its mutants with a single amino acid replacement in low-/high-strain regions and in binding/non-binding regions. The rheological response of the protein to an applied oscillating force fits a continuum model of a viscoelastic material whose mechanical properties are significantly affected by mutations in high-strain regions, as opposed to mutations in control regions. Furthermore, catalytic activity assays show that mutations in high-strain or binding regions tend to reduce activity, whereas mutations in low-strain, non-binding regions are neutral. These findings suggest that enzymes act as viscoelastic catalytic machines with sequence-encoded mechanical specifications.
UR - http://www.scopus.com/inward/record.url?scp=105001474916&partnerID=8YFLogxK
U2 - 10.1038/s41567-025-02825-9
DO - 10.1038/s41567-025-02825-9
M3 - مقالة
SN - 1745-2473
JO - Nature Physics
JF - Nature Physics
M1 - msac217
ER -