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Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis

The development of efficient, low-cost, and robust expression systems is important for the mass production of proteins and natural products in large amounts using cell factories. Glycerol is an ideal carbon source for large-scale fermentation due to its low cost and favorable maintenance of the ferm...

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Autores principales: Han, Laichuang, Chen, Qiaoqing, Luo, Jie, Cui, Wenjing, Zhou, Zhemin
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Microbiology 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9604022/
https://www.ncbi.nlm.nih.gov/pubmed/36036634
http://dx.doi.org/10.1128/spectrum.01322-22
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author Han, Laichuang
Chen, Qiaoqing
Luo, Jie
Cui, Wenjing
Zhou, Zhemin
author_facet Han, Laichuang
Chen, Qiaoqing
Luo, Jie
Cui, Wenjing
Zhou, Zhemin
author_sort Han, Laichuang
collection PubMed
description The development of efficient, low-cost, and robust expression systems is important for the mass production of proteins and natural products in large amounts using cell factories. Glycerol is an ideal carbon source for large-scale fermentation due to its low cost and favorable maintenance of the fermentation process. Here, we used the antiterminator protein GlpP and its target promoter P(glpD) to construct a highly efficient glycerol-inducible expression system (GIES) in Bacillus subtilis. This system was able to express heterologous genes in an autoinducible manner based on the sequential utilization of glucose and glycerol under the regulation of carbon catabolite repression. In such a system, the concentration of glycerol regulated the strength of gene expression, and the concentration of glucose affected both the timing of induction and the strength of gene expression. By enhancing GlpP, the GIES was further strengthened for high-level intracellular expression of aspartase and secretory expression of nattokinase. High yields of nattokinase in a 5-L fermenter through batch and fed-batch fermentation demonstrated the potential to apply the GIES for large-scale enzyme production. Through the evolution of the −10 box of P(glpD), mutants with gradient activities were obtained. In addition, hybrid glycerol-inducible promoters were successfully constructed by combining the constitutive promoters and the 5′ untranslated region of P(glpD). Collectively, this study developed a GIES to obtain high-value products from inexpensive glycerol. More importantly, the great potential of the pair of inherent terminator and antiterminator protein as a portable biological tool for various purposes in synthetic biology is proposed. IMPORTANCE In this study, a GIES was constructed in B. subtilis by employing the antiterminator protein GlpP and the GlpP-regulated promoter P(glpD). Based on the sequential utilization of glucose and glycerol by B. subtilis, the GIES was able to express genes in an autoinducible manner. The amounts and ratio of glucose and glycerol can regulate the gene induction timing and expression strength. The GIES was further applied for high yields of nattokinase, and its robustness in production scale-up was confirmed in a 5-L fermenter. The high-level expression of heterologous proteins demonstrated the huge application potential of the GIES. Furthermore, mutants of P(glpD) with gradient activities and hybrid glycerol-inducible promoters were obtained through the evolution of the −10 box of P(glpD) and the combination of the constitutive promoters and the 5′ untranslated region of P(glpD), respectively. These results demonstrated the use of the antiterminator protein as a regulator for various purposes in synthetic biology.
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spelling pubmed-96040222022-10-27 Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis Han, Laichuang Chen, Qiaoqing Luo, Jie Cui, Wenjing Zhou, Zhemin Microbiol Spectr Research Article The development of efficient, low-cost, and robust expression systems is important for the mass production of proteins and natural products in large amounts using cell factories. Glycerol is an ideal carbon source for large-scale fermentation due to its low cost and favorable maintenance of the fermentation process. Here, we used the antiterminator protein GlpP and its target promoter P(glpD) to construct a highly efficient glycerol-inducible expression system (GIES) in Bacillus subtilis. This system was able to express heterologous genes in an autoinducible manner based on the sequential utilization of glucose and glycerol under the regulation of carbon catabolite repression. In such a system, the concentration of glycerol regulated the strength of gene expression, and the concentration of glucose affected both the timing of induction and the strength of gene expression. By enhancing GlpP, the GIES was further strengthened for high-level intracellular expression of aspartase and secretory expression of nattokinase. High yields of nattokinase in a 5-L fermenter through batch and fed-batch fermentation demonstrated the potential to apply the GIES for large-scale enzyme production. Through the evolution of the −10 box of P(glpD), mutants with gradient activities were obtained. In addition, hybrid glycerol-inducible promoters were successfully constructed by combining the constitutive promoters and the 5′ untranslated region of P(glpD). Collectively, this study developed a GIES to obtain high-value products from inexpensive glycerol. More importantly, the great potential of the pair of inherent terminator and antiterminator protein as a portable biological tool for various purposes in synthetic biology is proposed. IMPORTANCE In this study, a GIES was constructed in B. subtilis by employing the antiterminator protein GlpP and the GlpP-regulated promoter P(glpD). Based on the sequential utilization of glucose and glycerol by B. subtilis, the GIES was able to express genes in an autoinducible manner. The amounts and ratio of glucose and glycerol can regulate the gene induction timing and expression strength. The GIES was further applied for high yields of nattokinase, and its robustness in production scale-up was confirmed in a 5-L fermenter. The high-level expression of heterologous proteins demonstrated the huge application potential of the GIES. Furthermore, mutants of P(glpD) with gradient activities and hybrid glycerol-inducible promoters were obtained through the evolution of the −10 box of P(glpD) and the combination of the constitutive promoters and the 5′ untranslated region of P(glpD), respectively. These results demonstrated the use of the antiterminator protein as a regulator for various purposes in synthetic biology. American Society for Microbiology 2022-08-29 /pmc/articles/PMC9604022/ /pubmed/36036634 http://dx.doi.org/10.1128/spectrum.01322-22 Text en Copyright © 2022 Han et al. https://creativecommons.org/licenses/by/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Research Article
Han, Laichuang
Chen, Qiaoqing
Luo, Jie
Cui, Wenjing
Zhou, Zhemin
Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title_full Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title_fullStr Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title_full_unstemmed Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title_short Development of a Glycerol-Inducible Expression System for High-Yield Heterologous Protein Production in Bacillus subtilis
title_sort development of a glycerol-inducible expression system for high-yield heterologous protein production in bacillus subtilis
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9604022/
https://www.ncbi.nlm.nih.gov/pubmed/36036634
http://dx.doi.org/10.1128/spectrum.01322-22
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