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An automated workflow for enhancing microbial bioprocess optimization on a novel microbioreactor platform

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TLDR
The optimization of heterologous protein expression in microbial systems currently requires extensive testing of biological and bioprocess engineering parameters, which can be efficiently boosted by using a microtiter plate cultivation setup embedded into a liquid-handling system, providing more throughput by parallelization and automation.
Abstract
Background: High-throughput methods are widely-used for strain screening effectively resulting in binary information regarding high or low productivity. Nevertheless achieving quantitative and scalable parameters for fast bioprocess development is much more challenging, especially for heterologous protein production. Here, the nature of the foreign protein makes it impossible to predict the, e.g. best expression construct, secretion signal peptide, inductor concentration, induction time, temperature and substrate feed rate in fed-batch operation to name only a few. Therefore, a high number of systematic experiments are necessary to elucidate the best conditions for heterologous expression of each new protein of interest. Results: To increase the throughput in bioprocess development, we used a microtiter plate based cultivation system (Biolector) which was fully integrated into a liquid-handling platform enclosed in laminar airflow housing. This automated cultivation platform was used for optimization of the secretory production of a cutinase from Fusarium solani pisi with Corynebacterium glutamicum. The online monitoring of biomass, dissolved oxygen and pH in each of the microtiter plate wells enables to trigger sampling or dosing events with the pipetting robot used for a reliable selection of best performing cutinase producers. In addition to this, further automated methods like media optimization and induction profiling were developed and validated. All biological and bioprocess parameters were exclusively optimized at microtiter plate scale and showed perfect scalable results to 1 L and 20 L stirred tank bioreactor scale. Conclusions: The optimization of heterologous protein expression in microbial systems currently requires extensive testing of biological and bioprocess engineering parameters. This can be efficiently boosted by using a microtiter plate cultivation setup embedded into a liquid-handling system, providing more throughput by parallelization and automation. Due to improved statistics by replicate cultivations, automated downstream analysis, and scalable process information, this setup has superior performance compared to standard microtiter plate cultivation.

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Journal ArticleDOI

High-throughput recombinant protein expression in Escherichia coli: current status and future perspectives.

TL;DR: This review describes several state-of-the-art approaches suitable for the cloning, expression and purification, conducted in parallel, of numerous molecules, and discusses recent progress related to soluble protein expression, mRNA folding, fusion tags, post-translational modification and production of membrane proteins.
Journal ArticleDOI

Signal peptides for recombinant protein secretion in bacterial expression systems

TL;DR: As outlined in this review, the most promising way to find the optimal signal peptide for a desired protein is to screen the largest possible diversity of signal peptides, either generated by signal peptIDE variation using large sign peptide libraries or, alternatively, by optimization of a given signal peptile using site-directed or random mutagenesis strategies.
Journal ArticleDOI

Construction of a Prophage-Free Variant of Corynebacterium glutamicum ATCC 13032 for Use as a Platform Strain for Basic Research and Industrial Biotechnology

TL;DR: The deletion of the prophages without any negative effect results in a novel platform strain for metabolic engineering and represents a useful step toward the construction of a C. glutamicum chassis genome of strain ATCC 13032 for biotechnological applications and synthetic biology.
Journal ArticleDOI

Zymomonas mobilis as a model system for production of biofuels and biochemicals

TL;DR: This review of work to develop Z. mobilis as a model system for biofuel production from the perspectives of substrate utilization, development for industrial robustness, potential product spectrum, strain evaluation and fermentation strategies, and perspectives related to classical genetic tools and emerging technologies.
Journal ArticleDOI

Advanced technologies for improved expression of recombinant proteins in bacteria: perspectives and applications

TL;DR: An impression of expression technologies developed in recent times for enhanced production of heterologous proteins in E. coli are provided, which are of foremost importance for diverse applications in microbiology and biopharmaceutical production.
References
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Journal ArticleDOI

Recombinant protein expression in Escherichia coli.

TL;DR: Recent progress in the fundamental understanding of transcription, translation, and protein folding in E. coli, together with serendipitous discoveries and the availability of improved genetic tools are making this bacterium more valuable than ever for the expression of complex eukaryotic proteins.
Journal ArticleDOI

Strategies for achieving high-level expression of genes in Escherichia coli.

TL;DR: Progress in the understanding of several biological processes promises to broaden the usefulness of Escherichia coli as a tool for gene expression and the remarkable increase in the availability of fusion partners offers a wide range of tools for improved protein folding, solubility, protection from proteases, yield, and secretion into the culture medium.
Journal ArticleDOI

Glycogen, hyaluronate, and some other polysaccharides greatly enhance the formation of exolipase by Serratia marcescens.

TL;DR: Exopolysaccharide, isolated from growth medium of Serratia marcescens SM-6, enhanced the exolipase formation as efficiently as hyaluronate, and was discussed mainly in terms of the "detachment hypothesis."
BookDOI

Handbook of Corynebacterium glutamicum

TL;DR: Part I: History A Short History of the Birth of the Amino Acid Industry in Japan, S. Kinoshita and Part II: Taxonomy Corynebacterium Taxonomy, W.D. Liebl.
Journal ArticleDOI

Isoleucine synthesis in Corynebacterium glutamicum: molecular analysis of the ilvB-ilvN-ilvC operon.

TL;DR: The amounts of the ilvBNC and ilvNC transcripts increased in response to the addition of alpha-ketobutyrate to the growth medium, correlated to an increase in specific AHAS activity, whereas IR activity was not increased because of the relatively large amount of theIlvC transcript present under all conditions assayed.
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