TY - JOUR
T1 - Enzymatic turnover of macromolecules generates long-lasting protein-water-coupled motions beyond reaction steady state
AU - Dielmann-Gessner, Jessica
AU - Grossman, Moran
AU - Nibali, Valeria Conti
AU - Born, Benjamin
AU - Solomonov, Inna
AU - Fields, Gregg B.
AU - Havenith, Martina
AU - Sagi, Irit
N1 - Weizmann Institute of Science National Postdoctoral Award Program; A.v.H. Humboldt Fellowship; Deutsche Forschungsgemeinschaft Cluster of Excellence RESOLV [EXC 1069]; Marie Curie program; Human Frontier Science Program [LT000336/2011]; National Institutes of Health [CA098799]; Ruhr University Bochum; Ressourcenverbund North Rhine Westphalia; Israel Science Foundation; Kimmelman Center at the Weizmann Institute; Ambach Family FundWe thank A. Frenkel (Yeshiva University), J. Bohon, M. Sullivan (Beamline X3B at the National Synchrotron Light Source), and Y. Udi (Weizmann Institute of Science) for help with X-ray absorption data collection; M. Heyden for assistance with molecular dynamics data analysis; D. Tworowski for assistance with docking; and D. Tokmina-Roszyk for the synthesis of the fluorogenic substrates. M.G. is an Awardee of the Weizmann Institute of Science National Postdoctoral Award Program for Advancing Women in Science and a recipient of an A.v.H. Humboldt Fellowship. M.G. and M.H. are supported by Deutsche Forschungsgemeinschaft Cluster of Excellence RESOLV Grant EXC 1069. V.C.N. thanks the Marie Curie program for financial support. B.B. acknowledges funding by the Human Frontier Science Program (LT000336/2011). G.B.F. and I. Sagi are supported by National Institutes of Health Grant CA098799. M.H. acknowledges financial support from the Ruhr University Bochum and the Ressourcenverbund North Rhine Westphalia for computer time. I. Sagi is supported by the Israel Science Foundation, the Kimmelman Center at the Weizmann Institute, and the Ambach Family Fund.
PY - 2014/12/16
Y1 - 2014/12/16
N2 - The main focus of enzymology is on the enzyme rates, substrate structures, and reactivity, whereas the role of solvent dynamics in mediating the biological reaction is often left aside owing to its complex molecular behavior. We used integrated X-ray- and terahertz-based time-resolved spectroscopic tools to study protein-water dynamics during proteolysis of collagen-like substrates by a matrix metalloproteinase. We show equilibration of structural kinetic transitions in the millisecond timescale during degradation of the two model substrates collagen and gelatin, which have different supersecondary structure and flexibility. Unexpectedly, the detected changes in collective enzyme-substrate-water-coupled motions persisted well beyond steady state for both substrates while displaying substrate-specific behaviors. Molecular dynamics simulations further showed that a hydration funnel (i.e., a gradient in retardation of hydrogen bond (HB) dynamics toward the active site) is substrate-dependent, exhibiting a steeper gradient for the more complex enzyme-collagen system. The long-lasting changes in protein-water dynamics reflect a collection of local energetic equilibrium states specifically formed during substrate conversion. Thus, the observed long-lasting water dynamics contribute to the net enzyme reactivity, impacting substrate binding, positional catalysis, and product release.
AB - The main focus of enzymology is on the enzyme rates, substrate structures, and reactivity, whereas the role of solvent dynamics in mediating the biological reaction is often left aside owing to its complex molecular behavior. We used integrated X-ray- and terahertz-based time-resolved spectroscopic tools to study protein-water dynamics during proteolysis of collagen-like substrates by a matrix metalloproteinase. We show equilibration of structural kinetic transitions in the millisecond timescale during degradation of the two model substrates collagen and gelatin, which have different supersecondary structure and flexibility. Unexpectedly, the detected changes in collective enzyme-substrate-water-coupled motions persisted well beyond steady state for both substrates while displaying substrate-specific behaviors. Molecular dynamics simulations further showed that a hydration funnel (i.e., a gradient in retardation of hydrogen bond (HB) dynamics toward the active site) is substrate-dependent, exhibiting a steeper gradient for the more complex enzyme-collagen system. The long-lasting changes in protein-water dynamics reflect a collection of local energetic equilibrium states specifically formed during substrate conversion. Thus, the observed long-lasting water dynamics contribute to the net enzyme reactivity, impacting substrate binding, positional catalysis, and product release.
UR - http://www.scopus.com/inward/record.url?scp=84919363043&partnerID=8YFLogxK
U2 - 10.1073/pnas.1410144111
DO - 10.1073/pnas.1410144111
M3 - مقالة
SN - 0027-8424
VL - 111
SP - 17857
EP - 17862
JO - Proceedings of the National Academy of Sciences of the United States of America
JF - Proceedings of the National Academy of Sciences of the United States of America
IS - 50
ER -