Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase

[Image: see text] Kinetic parameters are reported for the reactions of whole substrates (k(cat)/K(m), M(–1) s(–1)) (R)-glyceraldehyde 3-phosphate (GAP) and dihydroxyacetone phosphate (DHAP) and for the substrate pieces [(k(cat)/K(m))(E·HP(i))/K(d), M(–2) s(–1)] glycolaldehyde (GA) and phosphite dian...

Descripción completa

Detalles Bibliográficos
Autores principales: Richard, John P., Amyes, Tina L., Malabanan, M. Merced, Zhai, Xiang, Kim, Kalvin J., Reinhardt, Christopher J., Wierenga, Rik K., Drake, Eric J., Gulick, Andrew M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2016
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4934371/
https://www.ncbi.nlm.nih.gov/pubmed/27149328
http://dx.doi.org/10.1021/acs.biochem.6b00311
_version_ 1782441331881148416
author Richard, John P.
Amyes, Tina L.
Malabanan, M. Merced
Zhai, Xiang
Kim, Kalvin J.
Reinhardt, Christopher J.
Wierenga, Rik K.
Drake, Eric J.
Gulick, Andrew M.
author_facet Richard, John P.
Amyes, Tina L.
Malabanan, M. Merced
Zhai, Xiang
Kim, Kalvin J.
Reinhardt, Christopher J.
Wierenga, Rik K.
Drake, Eric J.
Gulick, Andrew M.
author_sort Richard, John P.
collection PubMed
description [Image: see text] Kinetic parameters are reported for the reactions of whole substrates (k(cat)/K(m), M(–1) s(–1)) (R)-glyceraldehyde 3-phosphate (GAP) and dihydroxyacetone phosphate (DHAP) and for the substrate pieces [(k(cat)/K(m))(E·HP(i))/K(d), M(–2) s(–1)] glycolaldehyde (GA) and phosphite dianion (HP(i)) catalyzed by the I172A/L232A mutant of triosephosphate isomerase from Trypanosoma brucei brucei (TbbTIM). A comparison with the corresponding parameters for wild-type, I172A, and L232A TbbTIM-catalyzed reactions shows that the effect of I172A and L232A mutations on ΔG(⧧) for the wild-type TbbTIM-catalyzed reactions of the substrate pieces is nearly the same as the effect of the same mutations on TbbTIM previously mutated at the second side chain. This provides strong evidence that mutation of the first hydrophobic side chain does not affect the functioning of the second side chain in catalysis of the reactions of the substrate pieces. By contrast, the effects of I172A and L232A mutations on ΔG(⧧) for wild-type TbbTIM-catalyzed reactions of the whole substrate are different from the effect of the same mutations on TbbTIM previously mutated at the second side chain. This is due to the change in the rate-determining step that determines the barrier to the isomerization reaction. X-ray crystal structures are reported for I172A, L232A, and I172A/L232A TIMs and for the complexes of these mutants to the intermediate analogue phosphoglycolate (PGA). The structures of the PGA complexes with wild-type and mutant enzymes are nearly superimposable, except that the space opened by replacement of the hydrophobic side chain is occupied by a water molecule that lies ∼3.5 Å from the basic side chain of Glu167. The new water at I172A mutant TbbTIM provides a simple rationalization for the increase in the activation barrier ΔG(⧧) observed for mutant enzyme-catalyzed reactions of the whole substrate and substrate pieces. By contrast, the new water at the L232A mutant does not predict the decrease in ΔG(⧧) observed for the mutant enzyme-catalyzed reactions of the substrate piece GA.
format Online
Article
Text
id pubmed-4934371
institution National Center for Biotechnology Information
language English
publishDate 2016
publisher American Chemical Society
record_format MEDLINE/PubMed
spelling pubmed-49343712017-05-05 Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase Richard, John P. Amyes, Tina L. Malabanan, M. Merced Zhai, Xiang Kim, Kalvin J. Reinhardt, Christopher J. Wierenga, Rik K. Drake, Eric J. Gulick, Andrew M. Biochemistry [Image: see text] Kinetic parameters are reported for the reactions of whole substrates (k(cat)/K(m), M(–1) s(–1)) (R)-glyceraldehyde 3-phosphate (GAP) and dihydroxyacetone phosphate (DHAP) and for the substrate pieces [(k(cat)/K(m))(E·HP(i))/K(d), M(–2) s(–1)] glycolaldehyde (GA) and phosphite dianion (HP(i)) catalyzed by the I172A/L232A mutant of triosephosphate isomerase from Trypanosoma brucei brucei (TbbTIM). A comparison with the corresponding parameters for wild-type, I172A, and L232A TbbTIM-catalyzed reactions shows that the effect of I172A and L232A mutations on ΔG(⧧) for the wild-type TbbTIM-catalyzed reactions of the substrate pieces is nearly the same as the effect of the same mutations on TbbTIM previously mutated at the second side chain. This provides strong evidence that mutation of the first hydrophobic side chain does not affect the functioning of the second side chain in catalysis of the reactions of the substrate pieces. By contrast, the effects of I172A and L232A mutations on ΔG(⧧) for wild-type TbbTIM-catalyzed reactions of the whole substrate are different from the effect of the same mutations on TbbTIM previously mutated at the second side chain. This is due to the change in the rate-determining step that determines the barrier to the isomerization reaction. X-ray crystal structures are reported for I172A, L232A, and I172A/L232A TIMs and for the complexes of these mutants to the intermediate analogue phosphoglycolate (PGA). The structures of the PGA complexes with wild-type and mutant enzymes are nearly superimposable, except that the space opened by replacement of the hydrophobic side chain is occupied by a water molecule that lies ∼3.5 Å from the basic side chain of Glu167. The new water at I172A mutant TbbTIM provides a simple rationalization for the increase in the activation barrier ΔG(⧧) observed for mutant enzyme-catalyzed reactions of the whole substrate and substrate pieces. By contrast, the new water at the L232A mutant does not predict the decrease in ΔG(⧧) observed for the mutant enzyme-catalyzed reactions of the substrate piece GA. American Chemical Society 2016-05-05 2016-05-31 /pmc/articles/PMC4934371/ /pubmed/27149328 http://dx.doi.org/10.1021/acs.biochem.6b00311 Text en Copyright © 2016 American Chemical Society This is an open access article published under an ACS AuthorChoice License (http://pubs.acs.org/page/policy/authorchoice_termsofuse.html) , which permits copying and redistribution of the article or any adaptations for non-commercial purposes.
spellingShingle Richard, John P.
Amyes, Tina L.
Malabanan, M. Merced
Zhai, Xiang
Kim, Kalvin J.
Reinhardt, Christopher J.
Wierenga, Rik K.
Drake, Eric J.
Gulick, Andrew M.
Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title_full Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title_fullStr Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title_full_unstemmed Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title_short Structure–Function Studies of Hydrophobic Residues That Clamp a Basic Glutamate Side Chain during Catalysis by Triosephosphate Isomerase
title_sort structure–function studies of hydrophobic residues that clamp a basic glutamate side chain during catalysis by triosephosphate isomerase
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4934371/
https://www.ncbi.nlm.nih.gov/pubmed/27149328
http://dx.doi.org/10.1021/acs.biochem.6b00311
work_keys_str_mv AT richardjohnp structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT amyestinal structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT malabananmmerced structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT zhaixiang structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT kimkalvinj structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT reinhardtchristopherj structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT wierengarikk structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT drakeericj structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase
AT gulickandrewm structurefunctionstudiesofhydrophobicresiduesthatclampabasicglutamatesidechainduringcatalysisbytriosephosphateisomerase

Ejemplares similares