Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis

Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis

Abstract Background FK506, a macrolide mainly with immunosuppressive activity, can be produced by various Streptomyces strains. However, one of the major challenges in the fermentation of FK506 is its insufficient production, resulting in high fermentation costs and environmental burdens. Herein, we...

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Main Authors: Qing-Bin Wu, Xiao-Ying Zhang, Xin-Ai Chen, Yong-Quan Li
Format: Article
Language:English
Published: BMC 2021-08-01
Series:Microbial Cell Factories
Subjects:
Streptomyces tsukubaensis
FK506
Hyper-production
Metabolic engineering
Biosynthetic gene cluster refactoring
Regulatory circuits
Online Access:https://doi.org/10.1186/s12934-021-01660-w
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spelling doaj-4f73078de95a4f01a5ec0b8fcee0c8702021-08-29T11:43:35ZengBMCMicrobial Cell Factories1475-28592021-08-0120111110.1186/s12934-021-01660-wImprovement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensisQing-Bin Wu0Xiao-Ying Zhang1Xin-Ai Chen2Yong-Quan Li3First Affiliated Hospital and Institute of Pharmaceutical Biotechnology, Zhejiang University School of MedicineFirst Affiliated Hospital and Institute of Pharmaceutical Biotechnology, Zhejiang University School of MedicineFirst Affiliated Hospital and Institute of Pharmaceutical Biotechnology, Zhejiang University School of MedicineFirst Affiliated Hospital and Institute of Pharmaceutical Biotechnology, Zhejiang University School of MedicineAbstract Background FK506, a macrolide mainly with immunosuppressive activity, can be produced by various Streptomyces strains. However, one of the major challenges in the fermentation of FK506 is its insufficient production, resulting in high fermentation costs and environmental burdens. Herein, we tried to improve its production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis. Results First, basing on the genome sequencing and analysis, putative competitive pathways were deleted. A better parental strain L19-2 with increased FK506 production from 140.3 to 170.3 mg/L and a cleaner metabolic background was constructed. Subsequently, the FK506 biosynthetic gene cluster was refactored by in-situ promoter-substitution strategy basing on the regulatory circuits. This strategy enhanced transcription levels of the entire FK506 biosynthetic gene cluster in a fine-tuning manner and dramatically increased the FK506 production to 410.3 mg/mL, 1.41-fold higher than the parental strain L19-2 (170.3 mg/L). Finally, the FK506 production was further increased from 410.3 to 603 mg/L in shake-flask culture by adding L-isoleucine at a final concentration of 6 g/L. Moreover, the potential of FK506 production capacity was also evaluated in a 15-L fermenter, resulting in the FK506 production of 830.3 mg/L. Conclusion From the aspects of competitive pathways, refactoring of the FK506 biosynthetic gene cluster and nutrients-addition, a strategy for hyper-production and potentially industrial application of FK506 was developed and a hyper-production strain L19-9 was constructed. The strategy presented here can be generally applicable to other Streptomyces for improvement of FK506 production and streamline hyper-production of other valuable secondary metabolites.https://doi.org/10.1186/s12934-021-01660-wStreptomyces tsukubaensisFK506Hyper-productionMetabolic engineeringBiosynthetic gene cluster refactoringRegulatory circuits
collection DOAJ
language English
format Article
sources DOAJ
author Qing-Bin Wu
Xiao-Ying Zhang
Xin-Ai Chen
Yong-Quan Li
spellingShingle Qing-Bin Wu
Xiao-Ying Zhang
Xin-Ai Chen
Yong-Quan Li
Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
Microbial Cell Factories
Streptomyces tsukubaensis
FK506
Hyper-production
Metabolic engineering
Biosynthetic gene cluster refactoring
Regulatory circuits
author_facet Qing-Bin Wu
Xiao-Ying Zhang
Xin-Ai Chen
Yong-Quan Li
author_sort Qing-Bin Wu
title Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
title_short Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
title_full Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
title_fullStr Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
title_full_unstemmed Improvement of FK506 production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis
title_sort improvement of fk506 production via metabolic engineering-guided combinational strategies in streptomyces tsukubaensis
publisher BMC
series Microbial Cell Factories
issn 1475-2859
publishDate 2021-08-01
description Abstract Background FK506, a macrolide mainly with immunosuppressive activity, can be produced by various Streptomyces strains. However, one of the major challenges in the fermentation of FK506 is its insufficient production, resulting in high fermentation costs and environmental burdens. Herein, we tried to improve its production via metabolic engineering-guided combinational strategies in Streptomyces tsukubaensis. Results First, basing on the genome sequencing and analysis, putative competitive pathways were deleted. A better parental strain L19-2 with increased FK506 production from 140.3 to 170.3 mg/L and a cleaner metabolic background was constructed. Subsequently, the FK506 biosynthetic gene cluster was refactored by in-situ promoter-substitution strategy basing on the regulatory circuits. This strategy enhanced transcription levels of the entire FK506 biosynthetic gene cluster in a fine-tuning manner and dramatically increased the FK506 production to 410.3 mg/mL, 1.41-fold higher than the parental strain L19-2 (170.3 mg/L). Finally, the FK506 production was further increased from 410.3 to 603 mg/L in shake-flask culture by adding L-isoleucine at a final concentration of 6 g/L. Moreover, the potential of FK506 production capacity was also evaluated in a 15-L fermenter, resulting in the FK506 production of 830.3 mg/L. Conclusion From the aspects of competitive pathways, refactoring of the FK506 biosynthetic gene cluster and nutrients-addition, a strategy for hyper-production and potentially industrial application of FK506 was developed and a hyper-production strain L19-9 was constructed. The strategy presented here can be generally applicable to other Streptomyces for improvement of FK506 production and streamline hyper-production of other valuable secondary metabolites.
topic Streptomyces tsukubaensis
FK506
Hyper-production
Metabolic engineering
Biosynthetic gene cluster refactoring
Regulatory circuits
url https://doi.org/10.1186/s12934-021-01660-w
work_keys_str_mv AT qingbinwu improvementoffk506productionviametabolicengineeringguidedcombinationalstrategiesinstreptomycestsukubaensis
AT xiaoyingzhang improvementoffk506productionviametabolicengineeringguidedcombinationalstrategiesinstreptomycestsukubaensis
AT xinaichen improvementoffk506productionviametabolicengineeringguidedcombinationalstrategiesinstreptomycestsukubaensis
AT yongquanli improvementoffk506productionviametabolicengineeringguidedcombinationalstrategiesinstreptomycestsukubaensis
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