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High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase

Cadaverine is a C5 diamine monomer used for the production of bio-based polyamide 510. Cadaverine is produced by the decarboxylation of l-lysine using a lysine decarboxylase (LDC). In this study, we developed recombinant Escherichia coli strains for the expression of LDC from Hafnia alvei. The resul...

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Autores principales: Kim, Hee Taek, Baritugo, Kei-Anne, Oh, Young Hoon, Kang, Kyoung-Hee, Jung, Ye Jean, Jang, Seyoung, Song, Bong Keun, Kim, Il-Kwon, Lee, Myung Ock, Hwang, Yong Taek, Park, Kyungmoon, Park, Si Jae, Joo, Jeong Chan
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6680443/
https://www.ncbi.nlm.nih.gov/pubmed/31337154
http://dx.doi.org/10.3390/polym11071184
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author Kim, Hee Taek
Baritugo, Kei-Anne
Oh, Young Hoon
Kang, Kyoung-Hee
Jung, Ye Jean
Jang, Seyoung
Song, Bong Keun
Kim, Il-Kwon
Lee, Myung Ock
Hwang, Yong Taek
Park, Kyungmoon
Park, Si Jae
Joo, Jeong Chan
author_facet Kim, Hee Taek
Baritugo, Kei-Anne
Oh, Young Hoon
Kang, Kyoung-Hee
Jung, Ye Jean
Jang, Seyoung
Song, Bong Keun
Kim, Il-Kwon
Lee, Myung Ock
Hwang, Yong Taek
Park, Kyungmoon
Park, Si Jae
Joo, Jeong Chan
author_sort Kim, Hee Taek
collection PubMed
description Cadaverine is a C5 diamine monomer used for the production of bio-based polyamide 510. Cadaverine is produced by the decarboxylation of l-lysine using a lysine decarboxylase (LDC). In this study, we developed recombinant Escherichia coli strains for the expression of LDC from Hafnia alvei. The resulting recombinant XBHaLDC strain was used as a whole cell biocatalyst for the high-level bioconversion of l-lysine into cadaverine without the supplementation of isopropyl β-d-1-thiogalactopyranoside (IPTG) for the induction of protein expression and pyridoxal phosphate (PLP), a key cofactor for an LDC reaction. The comparison of results from enzyme characterization of E. coli and H. alvei LDC revealed that H. alvei LDC exhibited greater bioconversion ability than E. coli LDC due to higher levels of protein expression in all cellular fractions and a higher specific activity at 37 °C (1825 U/mg protein > 1003 U/mg protein). The recombinant XBHaLDC and XBEcLDC strains were constructed for the high-level production of cadaverine. Recombinant XBHaLDC produced a 1.3-fold higher titer of cadaverine (6.1 g/L) than the XBEcLDC strain (4.8 g/L) from 10 g/L of l-lysine. Furthermore, XBHaLDC, concentrated to an optical density (OD(600)) of 50, efficiently produced 136 g/L of cadaverine from 200 g/L of l-lysine (97% molar yield) via an IPTG- and PLP-free whole cell bioconversion reaction. Cadaverine synthesized via a whole cell biocatalyst reaction using XBHaLDC was purified to polymer grade, and purified cadaverine was successfully used for the synthesis of polyamide 510. In conclusion, an IPTG- and PLP-free whole cell bioconversion process of l-lysine into cadaverine, using recombinant XBHaLDC, was successfully utilized for the production of bio-based polyamide 510, which has physical and thermal properties similar to polyamide 510 synthesized from chemical-grade cadaverine.
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spelling pubmed-66804432019-08-09 High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase Kim, Hee Taek Baritugo, Kei-Anne Oh, Young Hoon Kang, Kyoung-Hee Jung, Ye Jean Jang, Seyoung Song, Bong Keun Kim, Il-Kwon Lee, Myung Ock Hwang, Yong Taek Park, Kyungmoon Park, Si Jae Joo, Jeong Chan Polymers (Basel) Article Cadaverine is a C5 diamine monomer used for the production of bio-based polyamide 510. Cadaverine is produced by the decarboxylation of l-lysine using a lysine decarboxylase (LDC). In this study, we developed recombinant Escherichia coli strains for the expression of LDC from Hafnia alvei. The resulting recombinant XBHaLDC strain was used as a whole cell biocatalyst for the high-level bioconversion of l-lysine into cadaverine without the supplementation of isopropyl β-d-1-thiogalactopyranoside (IPTG) for the induction of protein expression and pyridoxal phosphate (PLP), a key cofactor for an LDC reaction. The comparison of results from enzyme characterization of E. coli and H. alvei LDC revealed that H. alvei LDC exhibited greater bioconversion ability than E. coli LDC due to higher levels of protein expression in all cellular fractions and a higher specific activity at 37 °C (1825 U/mg protein > 1003 U/mg protein). The recombinant XBHaLDC and XBEcLDC strains were constructed for the high-level production of cadaverine. Recombinant XBHaLDC produced a 1.3-fold higher titer of cadaverine (6.1 g/L) than the XBEcLDC strain (4.8 g/L) from 10 g/L of l-lysine. Furthermore, XBHaLDC, concentrated to an optical density (OD(600)) of 50, efficiently produced 136 g/L of cadaverine from 200 g/L of l-lysine (97% molar yield) via an IPTG- and PLP-free whole cell bioconversion reaction. Cadaverine synthesized via a whole cell biocatalyst reaction using XBHaLDC was purified to polymer grade, and purified cadaverine was successfully used for the synthesis of polyamide 510. In conclusion, an IPTG- and PLP-free whole cell bioconversion process of l-lysine into cadaverine, using recombinant XBHaLDC, was successfully utilized for the production of bio-based polyamide 510, which has physical and thermal properties similar to polyamide 510 synthesized from chemical-grade cadaverine. MDPI 2019-07-14 /pmc/articles/PMC6680443/ /pubmed/31337154 http://dx.doi.org/10.3390/polym11071184 Text en © 2019 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Kim, Hee Taek
Baritugo, Kei-Anne
Oh, Young Hoon
Kang, Kyoung-Hee
Jung, Ye Jean
Jang, Seyoung
Song, Bong Keun
Kim, Il-Kwon
Lee, Myung Ock
Hwang, Yong Taek
Park, Kyungmoon
Park, Si Jae
Joo, Jeong Chan
High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title_full High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title_fullStr High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title_full_unstemmed High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title_short High-Level Conversion of l-lysine into Cadaverine by Escherichia coli Whole Cell Biocatalyst Expressing Hafnia alvei l-lysine Decarboxylase
title_sort high-level conversion of l-lysine into cadaverine by escherichia coli whole cell biocatalyst expressing hafnia alvei l-lysine decarboxylase
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6680443/
https://www.ncbi.nlm.nih.gov/pubmed/31337154
http://dx.doi.org/10.3390/polym11071184
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