Modular bioengineering of whole-cell catalysis for sialo-oligosaccharide production: coordinated co-expression of CMP-sialic acid synthetase and sialyltransferase

Sabine Schelch; Manuel Eibinger; Jasmin Zuson; Jürgen Kuballa; Bernd Nidetzky

doi:10.1186/s12934-023-02249-1

Modular bioengineering of whole-cell catalysis for sialo-oligosaccharide production: coordinated co-expression of CMP-sialic acid synthetase and sialyltransferase

Microb Cell Fact. 2023 Nov 27;22(1):241. doi: 10.1186/s12934-023-02249-1.

Authors

Sabine Schelch^{1

2}, Manuel Eibinger², Jasmin Zuson^{1

2}, Jürgen Kuballa³, Bernd Nidetzky^{4

5}

Affiliations

¹ Austrian Centre of Industrial Biotechnology, Krenngasse 37, 8010, Graz, Austria.
² Institute of Biotechnology and Biochemical Engineering, Graz University of Technology, NAWI Graz, Petersgasse 12, 8010, Graz, Austria.
³ GALAB Laboratories GmbH, Am Schleusengraben 7, 21029, Hamburg, Germany.
⁴ Austrian Centre of Industrial Biotechnology, Krenngasse 37, 8010, Graz, Austria. bernd.nidetzky@tugraz.at.
⁵ Institute of Biotechnology and Biochemical Engineering, Graz University of Technology, NAWI Graz, Petersgasse 12, 8010, Graz, Austria. bernd.nidetzky@tugraz.at.

Abstract

Background: In whole-cell bio-catalysis, the biosystems engineering paradigm shifts from the global reconfiguration of cellular metabolism as in fermentation to a more focused, and more easily modularized, optimization of comparably short cascade reactions. Human milk oligosaccharides (HMO) constitute an important field for the synthetic application of cascade bio-catalysis in resting or non-living cells. Here, we analyzed the central catalytic module for synthesis of HMO-type sialo-oligosaccharides, comprised of CMP-sialic acid synthetase (CSS) and sialyltransferase (SiaT), with the specific aim of coordinated enzyme co-expression in E. coli for reaction flux optimization in whole cell conversions producing 3'-sialyllactose (3SL).

Results: Difference in enzyme specific activity (CSS from Neisseria meningitidis: 36 U/mg; α2,3-SiaT from Pasteurella dagmatis: 5.7 U/mg) was compensated by differential protein co-expression from tailored plasmid constructs, giving balance between the individual activities at a high level of both (α2,3-SiaT: 9.4 × 10² U/g cell dry mass; CSS: 3.4 × 10² U/g cell dry mass). Finally, plasmid selection was guided by kinetic modeling of the coupled CSS-SiaT reactions in combination with comprehensive analytical tracking of the multistep conversion (lactose, N-acetyl neuraminic acid (Neu5Ac), cytidine 5'-triphosphate; each up to 100 mM). The half-life of SiaT in permeabilized cells (≤ 4 h) determined the efficiency of 3SL production at 37 °C. Reaction at 25 °C gave 3SL (40 ± 4 g/L) in ∼ 70% yield within 3 h, reaching a cell dry mass-specific productivity of ∼ 3 g/(g h) and avoiding intermediary CMP-Neu5Ac accumulation.

Conclusions: Collectively, balanced co-expression of CSS and SiaT yields an efficient (high-flux) sialylation module to support flexible development of E. coli whole-cell catalysts for sialo-oligosaccharide production.

Keywords: 3ʹ-Sialyllactose; Co-expression; Multienzyme cascade reaction; Sialo-oligosaccharides; Whole-cell bio-catalysis; α2,3‐Sialyltransferase.

MeSH terms

Bioengineering
Catalysis
Escherichia coli* / metabolism
Humans
N-Acylneuraminate Cytidylyltransferase* / genetics
N-Acylneuraminate Cytidylyltransferase* / metabolism
Oligosaccharides / metabolism
Sialyltransferases / genetics
Sialyltransferases / metabolism

Substances

N-Acylneuraminate Cytidylyltransferase
Oligosaccharides
Sialyltransferases

Grants and funding

COMET K2 acib: next generation bioproduction/Österreichische Forschungsförderungsgesellschaft