Analysis of cellulose synthesis in a high-producing acetic acid bacterium Komagataeibacter hansenii

Martin Bimmer; Martin Reimer; Andreas Klingl; Christina Ludwig; Cordt Zollfrank; Wolfgang Liebl; Armin Ehrenreich

doi:10.1007/s00253-023-12461-z

Analysis of cellulose synthesis in a high-producing acetic acid bacterium Komagataeibacter hansenii

Appl Microbiol Biotechnol. 2023 May;107(9):2947-2967. doi: 10.1007/s00253-023-12461-z. Epub 2023 Mar 17.

Authors

Martin Bimmer¹, Martin Reimer², Andreas Klingl³, Christina Ludwig⁴, Cordt Zollfrank², Wolfgang Liebl¹, Armin Ehrenreich⁵

Affiliations

¹ School of Life Sciences, Technical University of Munich, Emil-Ramann-Straße 4, 85354, Freising, Germany.
² Technical University of Munich, Campus Straubing, Schulgasse 16, 94315, Straubing, Germany.
³ Plant Development, Ludwig-Maximilans-Universität München, Großhaderner Str.2, 82152, BiozentrumPlanegg-Martinsried, Germany.
⁴ Bavarian Center for Biomolecular Mass Spectrometry (BayBioMS), School of Life Sciences, Technical University of Munich, Gregor-Mendel-Straße 4, 85354, Freising, Germany.
⁵ School of Life Sciences, Technical University of Munich, Emil-Ramann-Straße 4, 85354, Freising, Germany. aehrenr@tum.de.

Abstract

Bacterial cellulose (BC) represents a renewable biomaterial with unique properties promising for biotechnology and biomedicine. Komagataeibacter hansenii ATCC 53,582 is a well-characterized high-yield producer of BC used in the industry. Its genome encodes three distinct cellulose synthases (CS), bcsAB1, bcsAB2, and bcsAB3, which together with genes for accessory proteins are organized in operons of different complexity. The genetic foundation of its high cellulose-producing phenotype was investigated by constructing chromosomal in-frame deletions of the CSs and of two predicted regulatory diguanylate cyclases (DGC), dgcA and dgcB. Proteomic characterization suggested that BcsAB1 was the decisive CS because of its high expression and its exclusive contribution to the formation of microcrystalline cellulose. BcsAB2 showed a lower expression level but contributes significantly to the tensile strength of BC and alters fiber diameter significantly as judged by scanning electron microscopy. Nevertheless, no distinct extracellular polymeric substance (EPS) from this operon was identified after static cultivation. Although transcription of bcsAB3 was observed, expression of the protein was below the detection limit of proteome analysis. Alike BcsAB2, deletion of BcsAB3 resulted in a visible reduction of the cellulose fiber diameter. The high abundance of BcsD and the accessory proteins CmcAx, CcpAx, and BglxA emphasizes their importance for the proper formation of the cellulosic network. Characterization of deletion mutants lacking the DGC genes dgcA and dgcB suggests a new regulatory mechanism of cellulose synthesis and cell motility in K. hansenii ATCC 53,582. Our findings form the basis for rational tailoring of the characteristics of BC. KEY POINTS: • BcsAB1 induces formation of microcrystalline cellulose fibers. • Modifications by BcsAB2 and BcsAB3 alter diameter of cellulose fibers. • Complex regulatory network of DGCs on cellulose pellicle formation and motility.

Keywords: Acetic acid bacteria; Bacterial cellulose; Cellulose fiber; Komagataeibacter hansenii; Markerless deletion; Proteomic analysis.

MeSH terms

Acetic Acid* / metabolism
Acetobacteraceae* / genetics
Acetobacteraceae* / metabolism
Cellulose / metabolism
Extracellular Polymeric Substance Matrix
Proteomics

Substances

Acetic Acid
Cellulose

Supplementary concepts

Komagataeibacter hansenii