A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis

Enzyme I (EI) of the bacterial phosphotransferase system (PTS) is a master regulator of bacterial metabolism and a promising target for development of a new class of broad-spectrum antibiotics. The catalytic activity of EI is mediated by several intradomain, interdomain, and intersubunit conformatio...

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Autores principales: Purslow, Jeffrey A., Thimmesch, Jolene N., Sivo, Valeria, Nguyen, Trang T., Khatiwada, Balabhadra, Dotas, Rochelle R., Venditti, Vincenzo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2021
Materias:
Molecular Biosciences
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8295985/
https://www.ncbi.nlm.nih.gov/pubmed/34307459
http://dx.doi.org/10.3389/fmolb.2021.699203
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author Purslow, Jeffrey A.
Thimmesch, Jolene N.
Sivo, Valeria
Nguyen, Trang T.
Khatiwada, Balabhadra
Dotas, Rochelle R.
Venditti, Vincenzo
author_facet Purslow, Jeffrey A.
Thimmesch, Jolene N.
Sivo, Valeria
Nguyen, Trang T.
Khatiwada, Balabhadra
Dotas, Rochelle R.
Venditti, Vincenzo
author_sort Purslow, Jeffrey A.
collection PubMed
description Enzyme I (EI) of the bacterial phosphotransferase system (PTS) is a master regulator of bacterial metabolism and a promising target for development of a new class of broad-spectrum antibiotics. The catalytic activity of EI is mediated by several intradomain, interdomain, and intersubunit conformational equilibria. Therefore, in addition to its relevance as a drug target, EI is also a good model for investigating the dynamics/function relationship in multidomain, oligomeric proteins. Here, we use solution NMR and protein design to investigate how the conformational dynamics occurring within the N-terminal domain (EIN) affect the activity of EI. We show that the rotameric g (+)-to-g (−) transition of the active site residue His(189) χ2 angle is decoupled from the state A-to-state B transition that describes a ∼90° rigid-body rearrangement of the EIN subdomains upon transition of the full-length enzyme to its catalytically competent closed form. In addition, we engineered EIN constructs with modulated conformational dynamics by hybridizing EIN from mesophilic and thermophilic species, and used these chimeras to assess the effect of increased or decreased active site flexibility on the enzymatic activity of EI. Our results indicate that the rate of the autophosphorylation reaction catalyzed by EI is independent from the kinetics of the g (+)-to-g (−) rotameric transition that exposes the phosphorylation site on EIN to the incoming phosphoryl group. In addition, our work provides an example of how engineering of hybrid mesophilic/thermophilic chimeras can assist investigations of the dynamics/function relationship in proteins, therefore opening new possibilities in biophysics.
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spelling pubmed-82959852021-07-23 A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis Purslow, Jeffrey A. Thimmesch, Jolene N. Sivo, Valeria Nguyen, Trang T. Khatiwada, Balabhadra Dotas, Rochelle R. Venditti, Vincenzo Front Mol Biosci Molecular Biosciences Enzyme I (EI) of the bacterial phosphotransferase system (PTS) is a master regulator of bacterial metabolism and a promising target for development of a new class of broad-spectrum antibiotics. The catalytic activity of EI is mediated by several intradomain, interdomain, and intersubunit conformational equilibria. Therefore, in addition to its relevance as a drug target, EI is also a good model for investigating the dynamics/function relationship in multidomain, oligomeric proteins. Here, we use solution NMR and protein design to investigate how the conformational dynamics occurring within the N-terminal domain (EIN) affect the activity of EI. We show that the rotameric g (+)-to-g (−) transition of the active site residue His(189) χ2 angle is decoupled from the state A-to-state B transition that describes a ∼90° rigid-body rearrangement of the EIN subdomains upon transition of the full-length enzyme to its catalytically competent closed form. In addition, we engineered EIN constructs with modulated conformational dynamics by hybridizing EIN from mesophilic and thermophilic species, and used these chimeras to assess the effect of increased or decreased active site flexibility on the enzymatic activity of EI. Our results indicate that the rate of the autophosphorylation reaction catalyzed by EI is independent from the kinetics of the g (+)-to-g (−) rotameric transition that exposes the phosphorylation site on EIN to the incoming phosphoryl group. In addition, our work provides an example of how engineering of hybrid mesophilic/thermophilic chimeras can assist investigations of the dynamics/function relationship in proteins, therefore opening new possibilities in biophysics. Frontiers Media S.A. 2021-07-08 /pmc/articles/PMC8295985/ /pubmed/34307459 http://dx.doi.org/10.3389/fmolb.2021.699203 Text en Copyright © 2021 Purslow, Thimmesch, Sivo, Nguyen, Khatiwada, Dotas and Venditti. https://creativecommons.org/licenses/by/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Molecular Biosciences
Purslow, Jeffrey A.
Thimmesch, Jolene N.
Sivo, Valeria
Nguyen, Trang T.
Khatiwada, Balabhadra
Dotas, Rochelle R.
Venditti, Vincenzo
A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title_full A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title_fullStr A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title_full_unstemmed A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title_short A Single Point Mutation Controls the Rate of Interconversion Between the g (+) and g (−) Rotamers of the Histidine 189 χ2 Angle That Activates Bacterial Enzyme I for Catalysis
title_sort single point mutation controls the rate of interconversion between the g (+) and g (−) rotamers of the histidine 189 χ2 angle that activates bacterial enzyme i for catalysis
topic Molecular Biosciences
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8295985/
https://www.ncbi.nlm.nih.gov/pubmed/34307459
http://dx.doi.org/10.3389/fmolb.2021.699203
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