Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates

BACKGROUND: Structural comparison between bacterial CueO and fungal laccases has suggested that a charged residue Glu (E106) in CueO replaces the corresponding residue Phe in fungal laccases at the gate of the tunnel connecting type II copper to the protein surface and an extra α-helix (L351-G378) n...

Descripción completa

Detalles Bibliográficos
Autores principales: Li, Yadong, Gong, Zijun, Li, Xin, Li, Yang, Wang, Xing-Guo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2011
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3123277/
https://www.ncbi.nlm.nih.gov/pubmed/21624144
http://dx.doi.org/10.1186/1471-2091-12-30
_version_ 1782206959545483264
author Li, Yadong
Gong, Zijun
Li, Xin
Li, Yang
Wang, Xing-Guo
author_facet Li, Yadong
Gong, Zijun
Li, Xin
Li, Yang
Wang, Xing-Guo
author_sort Li, Yadong
collection PubMed
description BACKGROUND: Structural comparison between bacterial CueO and fungal laccases has suggested that a charged residue Glu (E106) in CueO replaces the corresponding residue Phe in fungal laccases at the gate of the tunnel connecting type II copper to the protein surface and an extra α-helix (L351-G378) near the type I copper site covers the substrate binding pocket and might compromise the electron transfer from substrate to type I copper. To test this hypothesis, several mutants were made in Klebsiella sp. 601 multicopper oxidase, which is highly homologous to E. coli CueO with a similarity of 90% and an identity of 78%. RESULTS: The E106F mutant gave smaller K(m )(2.4-7fold) and k(cat )(1-4.4 fold) values for all three substrates DMP, ABTS and SGZ as compared with those for the wild-type enzyme. Its slightly larger k(cat)/K(m )values for three substrates mainly come from the decreased K(m). Deleting α-helix (L351-G378) resulted in the formation of inactive inclusion body when the mutant (Δ)α351-378 was expressed in E. coli. Another mutant α351-380M was then made via substitution of seven amino acid residues in the α-helix (L351-G378) region. The α351-380M mutant was active, and displayed a far-UV CD spectrum markedly different from that for wild-type enzyme. Kinetic studies showed the α351-380M mutant gave very low K(m )values for DMP, ABTS and SGZ, 4.5-, 1.9- and 7-fold less than those for the wild type. In addition, k(cat)/K(m )values were increased, 9.4-fold for DMP, similar for ABTS and 3-fold for SGZ. CONCLUSION: The Glu residue at position 106 appears not to be the only factor affecting the copper binding, and it may also play a role in maintaining enzyme conformation. The α-helix (L351-G378) may not only block access to the type I copper site but also play a role in substrate specificities of bacterial MCOs. The α351-380M mutant catalyzing oxidation of the phenolic substrate DMP effectively would be very useful in green chemistry.
format Online
Article
Text
id pubmed-3123277
institution National Center for Biotechnology Information
language English
publishDate 2011
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-31232772011-06-25 Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates Li, Yadong Gong, Zijun Li, Xin Li, Yang Wang, Xing-Guo BMC Biochem Research Article BACKGROUND: Structural comparison between bacterial CueO and fungal laccases has suggested that a charged residue Glu (E106) in CueO replaces the corresponding residue Phe in fungal laccases at the gate of the tunnel connecting type II copper to the protein surface and an extra α-helix (L351-G378) near the type I copper site covers the substrate binding pocket and might compromise the electron transfer from substrate to type I copper. To test this hypothesis, several mutants were made in Klebsiella sp. 601 multicopper oxidase, which is highly homologous to E. coli CueO with a similarity of 90% and an identity of 78%. RESULTS: The E106F mutant gave smaller K(m )(2.4-7fold) and k(cat )(1-4.4 fold) values for all three substrates DMP, ABTS and SGZ as compared with those for the wild-type enzyme. Its slightly larger k(cat)/K(m )values for three substrates mainly come from the decreased K(m). Deleting α-helix (L351-G378) resulted in the formation of inactive inclusion body when the mutant (Δ)α351-378 was expressed in E. coli. Another mutant α351-380M was then made via substitution of seven amino acid residues in the α-helix (L351-G378) region. The α351-380M mutant was active, and displayed a far-UV CD spectrum markedly different from that for wild-type enzyme. Kinetic studies showed the α351-380M mutant gave very low K(m )values for DMP, ABTS and SGZ, 4.5-, 1.9- and 7-fold less than those for the wild type. In addition, k(cat)/K(m )values were increased, 9.4-fold for DMP, similar for ABTS and 3-fold for SGZ. CONCLUSION: The Glu residue at position 106 appears not to be the only factor affecting the copper binding, and it may also play a role in maintaining enzyme conformation. The α-helix (L351-G378) may not only block access to the type I copper site but also play a role in substrate specificities of bacterial MCOs. The α351-380M mutant catalyzing oxidation of the phenolic substrate DMP effectively would be very useful in green chemistry. BioMed Central 2011-05-31 /pmc/articles/PMC3123277/ /pubmed/21624144 http://dx.doi.org/10.1186/1471-2091-12-30 Text en Copyright ©2011 Li et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Li, Yadong
Gong, Zijun
Li, Xin
Li, Yang
Wang, Xing-Guo
Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title_full Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title_fullStr Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title_full_unstemmed Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title_short Engineering Klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
title_sort engineering klebsiella sp. 601 multicopper oxidase enhances the catalytic efficiency towards phenolic substrates
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3123277/
https://www.ncbi.nlm.nih.gov/pubmed/21624144
http://dx.doi.org/10.1186/1471-2091-12-30
work_keys_str_mv AT liyadong engineeringklebsiellasp601multicopperoxidaseenhancesthecatalyticefficiencytowardsphenolicsubstrates
AT gongzijun engineeringklebsiellasp601multicopperoxidaseenhancesthecatalyticefficiencytowardsphenolicsubstrates
AT lixin engineeringklebsiellasp601multicopperoxidaseenhancesthecatalyticefficiencytowardsphenolicsubstrates
AT liyang engineeringklebsiellasp601multicopperoxidaseenhancesthecatalyticefficiencytowardsphenolicsubstrates
AT wangxingguo engineeringklebsiellasp601multicopperoxidaseenhancesthecatalyticefficiencytowardsphenolicsubstrates

Ejemplares similares