Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution

BACKGROUND: Epoxide hydrolase can regioselectively catalyze the oxirane ring-opening hydrolysis of rac-epoxides producing the corresponding chiral diols. In our laboratory, a gene named pveh1 encoding an EH from Phaseolus vulgaris was cloned. Although the directed modification of PvEH1 was carried o...

Descripción completa

Detalles Bibliográficos
Autores principales: Zong, Xun-Cheng, Li, Chuang, Xu, Yao-Hui, Hu, Die, Hu, Bo-Chun, Zang, Jia, Wu, Min-Chen
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2019
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6859628/
https://www.ncbi.nlm.nih.gov/pubmed/31739786
http://dx.doi.org/10.1186/s12934-019-1252-4
_version_ 1783471155779207168
author Zong, Xun-Cheng
Li, Chuang
Xu, Yao-Hui
Hu, Die
Hu, Bo-Chun
Zang, Jia
Wu, Min-Chen
author_facet Zong, Xun-Cheng
Li, Chuang
Xu, Yao-Hui
Hu, Die
Hu, Bo-Chun
Zang, Jia
Wu, Min-Chen
author_sort Zong, Xun-Cheng
collection PubMed
description BACKGROUND: Epoxide hydrolase can regioselectively catalyze the oxirane ring-opening hydrolysis of rac-epoxides producing the corresponding chiral diols. In our laboratory, a gene named pveh1 encoding an EH from Phaseolus vulgaris was cloned. Although the directed modification of PvEH1 was carried out, the mutant PvEH1(Y3) showed a limited degree of enantioconvergence towards racemic (rac-) m-chlorostyrene oxide (mCSO). RESULTS: PvEH1 and PvEH1(Y3) were combinatively subjected to laboratory evolution to further enhance the enantioconvergence of PvEH1(Y3) towards rac-mCSO. Firstly, the substrate-binding pocket of PvEH1 was identified using a CAVER 3.0 software, and divided into three zones. After all residues in zones 1 and 3 were subjected to leucine scanning, two E. coli transformants, E. coli/pveh1(Y149L) and /pveh1(P184L), were selected, by which rac-mCSO was transformed into (R)-m-chlorophenyl-1,2-ethanediol (mCPED) having 55.1% and 27.2% ee(p). Secondly, two saturation mutagenesis libraries, E. coli/pveh1(Y149X) and /pveh1(P184X) (X: any one of 20 residues) were created at sites Y149 and P184 of PvEH1. Among all transformants, both E. coli/pveh1(Y149L) (65.8% α(S) and 55.1% ee(p)) and /pveh1(P184W) (66.6% α(S) and 59.8% ee(p)) possessed the highest enantioconvergences. Finally, the combinatorial mutagenesis was conducted by replacements of both Y149L and P184W in PvEH1(Y3), constructing E. coli/pveh1(Y3Z2), whose α(S) reached 97.5%, higher than that (75.3%) of E. coli/pveh1(Y3). In addition, the enantioconvergent hydrolysis of 20 mM rac-mCSO was performed by E. coli/pveh1(Y3Z2), giving (R)-mCPED with 95.2% ee(p) and 97.2% yield. CONCLUSIONS: In summary, the enantioconvergence of PvEH1(Y3Z2) was successfully improved by laboratory evolution, which was based on the study of substrate-binding pocket by leucine scanning. Our present work introduced an effective strategy for the directed modification of enantioconvergence of PvEH1.
format Online
Article
Text
id pubmed-6859628
institution National Center for Biotechnology Information
language English
publishDate 2019
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-68596282019-12-12 Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution Zong, Xun-Cheng Li, Chuang Xu, Yao-Hui Hu, Die Hu, Bo-Chun Zang, Jia Wu, Min-Chen Microb Cell Fact Research BACKGROUND: Epoxide hydrolase can regioselectively catalyze the oxirane ring-opening hydrolysis of rac-epoxides producing the corresponding chiral diols. In our laboratory, a gene named pveh1 encoding an EH from Phaseolus vulgaris was cloned. Although the directed modification of PvEH1 was carried out, the mutant PvEH1(Y3) showed a limited degree of enantioconvergence towards racemic (rac-) m-chlorostyrene oxide (mCSO). RESULTS: PvEH1 and PvEH1(Y3) were combinatively subjected to laboratory evolution to further enhance the enantioconvergence of PvEH1(Y3) towards rac-mCSO. Firstly, the substrate-binding pocket of PvEH1 was identified using a CAVER 3.0 software, and divided into three zones. After all residues in zones 1 and 3 were subjected to leucine scanning, two E. coli transformants, E. coli/pveh1(Y149L) and /pveh1(P184L), were selected, by which rac-mCSO was transformed into (R)-m-chlorophenyl-1,2-ethanediol (mCPED) having 55.1% and 27.2% ee(p). Secondly, two saturation mutagenesis libraries, E. coli/pveh1(Y149X) and /pveh1(P184X) (X: any one of 20 residues) were created at sites Y149 and P184 of PvEH1. Among all transformants, both E. coli/pveh1(Y149L) (65.8% α(S) and 55.1% ee(p)) and /pveh1(P184W) (66.6% α(S) and 59.8% ee(p)) possessed the highest enantioconvergences. Finally, the combinatorial mutagenesis was conducted by replacements of both Y149L and P184W in PvEH1(Y3), constructing E. coli/pveh1(Y3Z2), whose α(S) reached 97.5%, higher than that (75.3%) of E. coli/pveh1(Y3). In addition, the enantioconvergent hydrolysis of 20 mM rac-mCSO was performed by E. coli/pveh1(Y3Z2), giving (R)-mCPED with 95.2% ee(p) and 97.2% yield. CONCLUSIONS: In summary, the enantioconvergence of PvEH1(Y3Z2) was successfully improved by laboratory evolution, which was based on the study of substrate-binding pocket by leucine scanning. Our present work introduced an effective strategy for the directed modification of enantioconvergence of PvEH1. BioMed Central 2019-11-18 /pmc/articles/PMC6859628/ /pubmed/31739786 http://dx.doi.org/10.1186/s12934-019-1252-4 Text en © The Author(s) 2019 Open AccessThis article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.
spellingShingle Research
Zong, Xun-Cheng
Li, Chuang
Xu, Yao-Hui
Hu, Die
Hu, Bo-Chun
Zang, Jia
Wu, Min-Chen
Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title_full Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title_fullStr Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title_full_unstemmed Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title_short Substantially improving the enantioconvergence of PvEH1, a Phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
title_sort substantially improving the enantioconvergence of pveh1, a phaseolus vulgaris epoxide hydrolase, towards m-chlorostyrene oxide by laboratory evolution
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6859628/
https://www.ncbi.nlm.nih.gov/pubmed/31739786
http://dx.doi.org/10.1186/s12934-019-1252-4
work_keys_str_mv AT zongxuncheng substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT lichuang substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT xuyaohui substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT hudie substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT hubochun substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT zangjia substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution
AT wuminchen substantiallyimprovingtheenantioconvergenceofpveh1aphaseolusvulgarisepoxidehydrolasetowardsmchlorostyreneoxidebylaboratoryevolution

Ejemplares similares