CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli

CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli

Protein engineering plays an increasingly important role in developing new and optimizing existing metabolic pathways for biosynthesis. Conventional screening approach of libraries of gene and enzyme variants is often done using a host strain under conditions not relevant to the cultivation or intra...

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Main Authors: Minliang Chen, Lin Chen, An-Ping Zeng
Format: Article
Language:English
Published: Elsevier 2019-12-01
Series:Metabolic Engineering Communications
Online Access:http://www.sciencedirect.com/science/article/pii/S2214030119300045
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spelling doaj-d5b8a1c563d8496f9dc5faa24934b13b2020-11-25T02:20:16ZengElsevierMetabolic Engineering Communications2214-03012019-12-019CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coliMinliang Chen0Lin Chen1An-Ping Zeng2Institute of Bioprocess and Biosystems Engineering, Hamburg University of Technology, D-21073, Hamburg, GermanyInstitute of Bioprocess and Biosystems Engineering, Hamburg University of Technology, D-21073, Hamburg, GermanyInstitute of Bioprocess and Biosystems Engineering, Hamburg University of Technology, D-21073, Hamburg, Germany; Beijing Advanced Innovation Center for Soft Matter Science and Engineering, Beijing University of Chemical Technology, North Third Ring Road 15, 100029, Beijing, China; Corresponding author. Institute of Bioprocess and Biosystems Engineering, Hamburg University of Technology, Denickestr. 15, D-21073, Hamburg, Germany.Protein engineering plays an increasingly important role in developing new and optimizing existing metabolic pathways for biosynthesis. Conventional screening approach of libraries of gene and enzyme variants is often done using a host strain under conditions not relevant to the cultivation or intracellular conditions of the later production strain. This does not necessarily result in the identification of the best enzyme variant for in vivo use in the production strain. In this work, we propose a method which integrates CRISPR/Cas9-facilitated engineering of the target gene(s) with growth-coupled and sensor-guided in vivo screening (CGSS) for protein engineering and pathway optimization. The efficiency of the method is demonstrated for engineering 3-deoxy-D-arabino-heptulosonate-7-phosphate (DAHP) synthase AroG, a key enzyme in the chorismate pathway for the synthesis of aromatic amino acids (AAAs), to obtain variants of AroG (AroGfbr) with increased resistance to feedback inhibition of Phe. Starting from a tryptophan (Trp)-producing E. coli strain (harboring a reported Phe-resistant AroG variant AroGS180F), the removal of all the endogenous DAHP synthases makes the growth of this strain dependent on the activity of an introduced AroG variant. The different catalytic efficiencies of AroG variants lead to different intracellular concentration of Trp which is sensed by a Trp biosensor (TnaC-eGFP). Using the growth rate and the signal strength of the biosensor as criteria, we successfully identified several novel Phe-resistant AroG variants (including the best one AroGD6G−D7A) which exhibited higher specific enzyme activity than that of the reference variant AroGS180F at the presence of 40 mM Phe. The replacement of AroGS180F with the newly identified AroGD6G−D7A in the Trp-producing strain significantly improved the Trp production by 38.5% (24.03 ± 1.02 g/L at 36 h) in a simple fed-batch fermentation. Keywords: CRISPR/Cas9, Protein engineering, Trp biosensor, DAHP synthase, Feedback inhibitionhttp://www.sciencedirect.com/science/article/pii/S2214030119300045
collection DOAJ
language English
format Article
sources DOAJ
author Minliang Chen
Lin Chen
An-Ping Zeng
spellingShingle Minliang Chen
Lin Chen
An-Ping Zeng
CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
Metabolic Engineering Communications
author_facet Minliang Chen
Lin Chen
An-Ping Zeng
author_sort Minliang Chen
title CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
title_short CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
title_full CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
title_fullStr CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
title_full_unstemmed CRISPR/Cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in E. coli
title_sort crispr/cas9-facilitated engineering with growth-coupled and sensor-guided in vivo screening of enzyme variants for a more efficient chorismate pathway in e. coli
publisher Elsevier
series Metabolic Engineering Communications
issn 2214-0301
publishDate 2019-12-01
description Protein engineering plays an increasingly important role in developing new and optimizing existing metabolic pathways for biosynthesis. Conventional screening approach of libraries of gene and enzyme variants is often done using a host strain under conditions not relevant to the cultivation or intracellular conditions of the later production strain. This does not necessarily result in the identification of the best enzyme variant for in vivo use in the production strain. In this work, we propose a method which integrates CRISPR/Cas9-facilitated engineering of the target gene(s) with growth-coupled and sensor-guided in vivo screening (CGSS) for protein engineering and pathway optimization. The efficiency of the method is demonstrated for engineering 3-deoxy-D-arabino-heptulosonate-7-phosphate (DAHP) synthase AroG, a key enzyme in the chorismate pathway for the synthesis of aromatic amino acids (AAAs), to obtain variants of AroG (AroGfbr) with increased resistance to feedback inhibition of Phe. Starting from a tryptophan (Trp)-producing E. coli strain (harboring a reported Phe-resistant AroG variant AroGS180F), the removal of all the endogenous DAHP synthases makes the growth of this strain dependent on the activity of an introduced AroG variant. The different catalytic efficiencies of AroG variants lead to different intracellular concentration of Trp which is sensed by a Trp biosensor (TnaC-eGFP). Using the growth rate and the signal strength of the biosensor as criteria, we successfully identified several novel Phe-resistant AroG variants (including the best one AroGD6G−D7A) which exhibited higher specific enzyme activity than that of the reference variant AroGS180F at the presence of 40 mM Phe. The replacement of AroGS180F with the newly identified AroGD6G−D7A in the Trp-producing strain significantly improved the Trp production by 38.5% (24.03 ± 1.02 g/L at 36 h) in a simple fed-batch fermentation. Keywords: CRISPR/Cas9, Protein engineering, Trp biosensor, DAHP synthase, Feedback inhibition
url http://www.sciencedirect.com/science/article/pii/S2214030119300045
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AT linchen crisprcas9facilitatedengineeringwithgrowthcoupledandsensorguidedinvivoscreeningofenzymevariantsforamoreefficientchorismatepathwayinecoli
AT anpingzeng crisprcas9facilitatedengineeringwithgrowthcoupledandsensorguidedinvivoscreeningofenzymevariantsforamoreefficientchorismatepathwayinecoli
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