Accelerated strain construction and characterization of C. glutamicum protein secretion by laboratory automation

Carolin Müller; Patrick J Bakkes; Patrick Lenz; Vera Waffenschmidt; Laura M Helleckes; Karl-Erich Jaeger; Wolfgang Wiechert; Andreas Knapp; Roland Freudl; Marco Oldiges

doi:10.1007/s00253-022-12017-7

Accelerated strain construction and characterization of C. glutamicum protein secretion by laboratory automation

Appl Microbiol Biotechnol. 2022 Jun;106(12):4481-4497. doi: 10.1007/s00253-022-12017-7. Epub 2022 Jun 27.

Authors

Carolin Müller^{1

2}, Patrick J Bakkes¹, Patrick Lenz³, Vera Waffenschmidt¹, Laura M Helleckes^{1

2}, Karl-Erich Jaeger^{1

3}, Wolfgang Wiechert^{1

4}, Andreas Knapp^{3

5}, Roland Freudl¹, Marco Oldiges^{6

7}

Affiliations

¹ Institute of Bio- and Geosciences IBG-1, Biotechnology, Forschungszentrum Jülich GmbH, 52425, Jülich, Germany.
² Institute of Biotechnology, RWTH Aachen University, 52062, Aachen, Germany.
³ Institute of Molecular Enzyme Technology, Heinrich Heine University Düsseldorf, Forschungszentrum Jülich, 52425, Jülich, Germany.
⁴ Computational Systems Biotechnology (AVT.CSB), RWTH Aachen University, 52062, Aachen, Germany.
⁵ Castrol Germany GmbH, 41179, Mönchengladbach, Germany.
⁶ Institute of Bio- and Geosciences IBG-1, Biotechnology, Forschungszentrum Jülich GmbH, 52425, Jülich, Germany. m.oldiges@fz-juelich.de.
⁷ Institute of Biotechnology, RWTH Aachen University, 52062, Aachen, Germany. m.oldiges@fz-juelich.de.

Abstract

Secretion of bacterial proteins into the culture medium simplifies downstream processing by avoiding cell disruption for target protein purification. However, a suitable signal peptide for efficient secretion needs to be identified, and currently, there are no tools available to predict optimal combinations of signal peptides and target proteins. The selection of such a combination is influenced by several factors, including protein biosynthesis efficiency and cultivation conditions, which both can have a significant impact on secretion performance. As a result, a large number of combinations must be tested. Therefore, we have developed automated workflows allowing for targeted strain construction and secretion screening using two platforms. Key advantages of this experimental setup include lowered hands-on time and increased throughput. In this study, the automated workflows were established for the heterologous production of Fusarium solani f. sp. pisi cutinase in Corynebacterium glutamicum. The target protein was monitored in culture supernatants via enzymatic activity and split GFP assay. Varying spacer lengths between the Shine-Dalgarno sequence and the start codon of Bacillus subtilis signal peptides were tested. Consistent with previous work on the secretory cutinase production in B. subtilis, a ribosome binding site with extended spacer length to up to 12 nt, which likely slows down translation initiation, does not necessarily lead to poorer cutinase secretion by C. glutamicum. The best performing signal peptides for cutinase secretion with a standard spacer length were identified in a signal peptide screening. Additional insights into the secretion process were gained by monitoring secretion stress using the C. glutamicum K9 biosensor strain. KEY POINTS: • Automated workflows for strain construction and screening of protein secretion • Comparison of spacer, signal peptide, and host combinations for cutinase secretion • Signal peptide screening for secretion by C. glutamicum using the split GFP assay.

Keywords: Laboratory automation; Ribosome binding site; Screening; Sec secretion; Signal peptide; Split GFP assay.

MeSH terms

Automation, Laboratory
Bacillus subtilis / genetics
Bacillus subtilis / metabolism
Corynebacterium glutamicum* / genetics
Corynebacterium glutamicum* / metabolism
Fusarium*
Protein Sorting Signals
Protein Transport

Substances

Protein Sorting Signals

Abstract

MeSH terms

Substances

Grants and funding