Beyond rational-biosensor-guided isolation of 100 independently evolved bacterial strain variants and comparative analysis of their genomes

Philipp T Baumann; Michael Dal Molin; Hannah Aring; Karin Krumbach; Moritz-Fabian Müller; Bas Vroling; Philana V van Summeren-Wesenhagen; Stephan Noack; Jan Marienhagen

doi:10.1186/s12915-023-01688-x

Beyond rational-biosensor-guided isolation of 100 independently evolved bacterial strain variants and comparative analysis of their genomes

BMC Biol. 2023 Sep 4;21(1):183. doi: 10.1186/s12915-023-01688-x.

Authors

Affiliations

¹ Institute of Bio- and Geosciences, Forschungszentrum Jülich, IBG-1: Biotechnology, 52425, Jülich, Germany.
² Department I of Internal Medicine, University of Cologne, 50937, Cologne, Germany.
³ Center for Molecular Medicine Cologne (CMMC), University of Cologne, 50931, Cologne, Germany.
⁴ Bioprodict GmbH, Nieuwe Marktstraat 54E, 6511AA, Nijmegen, The Netherlands.
⁵ SenseUp GmbH, C/O Campus Forschungszentrum, Wilhelm-Johnen-Strasse, 52428, Jülich, Germany.
⁶ Institute of Bio- and Geosciences, Forschungszentrum Jülich, IBG-1: Biotechnology, 52425, Jülich, Germany. j.marienhagen@fz-juelich.de.
⁷ Institute of Biotechnology, RWTH Aachen University, Worringer Weg 3, 52074, Aachen, Germany. j.marienhagen@fz-juelich.de.

Abstract

Background: In contrast to modern rational metabolic engineering, classical strain development strongly relies on random mutagenesis and screening for the desired production phenotype. Nowadays, with the availability of biosensor-based FACS screening strategies, these random approaches are coming back into fashion. In this study, we employ this technology in combination with comparative genome analyses to identify novel mutations contributing to product formation in the genome of a Corynebacterium glutamicum L-histidine producer. Since all known genetic targets contributing to L-histidine production have been already rationally engineered in this strain, identification of novel beneficial mutations can be regarded as challenging, as they might not be intuitively linkable to L-histidine biosynthesis.

Results: In order to identify 100 improved strain variants that had each arisen independently, we performed > 600 chemical mutagenesis experiments, > 200 biosensor-based FACS screenings, isolated > 50,000 variants with increased fluorescence, and characterized > 4500 variants with regard to biomass formation and L-histidine production. Based on comparative genome analyses of these 100 variants accumulating 10-80% more L-histidine, we discovered several beneficial mutations. Combination of selected genetic modifications allowed for the construction of a strain variant characterized by a doubled L-histidine titer (29 mM) and product yield (0.13 C-mol C-mol^-1) in comparison to the starting variant.

Conclusions: This study may serve as a blueprint for the identification of novel beneficial mutations in microbial producers in a more systematic manner. This way, also previously unexplored genes or genes with previously unknown contribution to the respective production phenotype can be identified. We believe that this technology has a great potential to push industrial production strains towards maximum performance.

Keywords: Biosensor; Comparative genome analysis; Corynebacterium glutamicum; Fluorescence-activated cell sorting; Genome sequencing; High-throughput screening; L-histidine; Metabolic engineering; Single-nucleotide polymorphism.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Bacteria*
Gene Editing
Histidine*
Mutagenesis
Mutation

Substances

Histidine