Glycosyl transferase GT2 genes mediate the biosynthesis of an unusual (1,3;1,4)‐β‐glucan exopolysaccharide in the bacterium Sarcina ventriculi

Author:

Lampugnani Edwin R.12ORCID,Ford Kris13,Ho Yin Ying1ORCID,van de Meene Allison14ORCID,Lahnstein Jelle5ORCID,Tan Hwei‐Ting5ORCID,Burton Rachel A.5ORCID,Fincher Geoffrey B.5ORCID,Shafee Thomas3ORCID,Bacic Antony13ORCID,Zimmer Jochen67ORCID,Xing Xiaohui8ORCID,Bulone Vincent58ORCID,Doblin Monika S.13ORCID,Roberts Eric M.9ORCID

Affiliation:

1. School of BioSciences University of Melbourne Parkville Victoria Australia

2. Menzies Institute for Medical Research, College of Health and Medicine University of Tasmania Hobart Tasmania Australia

3. La Trobe Institute for Sustainable Agriculture and Food La Trobe University Bundoora Victoria Australia

4. Ian Holmes Imaging Centre, Bio21 The University of Melbourne Parkville Victoria Australia

5. School of Agriculture, Food and Wine University of Adelaide Glen Osmond South Australia Australia

6. Howard Hughes Medical Institute University of Virginia School of Medicine Charlottesville Virginia USA

7. Department of Molecular Physiology and Biological Physics University of Virginia School of Medicine Charlottesville Virginia USA

8. Division of Glycoscience, Department of Chemistry, School of Engineering Sciences in Chemistry, Biotechnology and Health, Royal Institute of Technology (KTH) AlbaNova University Centre Stockholm Sweden

9. Department of Biology Rhode Island College Providence Rhode Island USA

Abstract

AbstractLinear, unbranched (1,3;1,4)‐β‐glucans (mixed‐linkage glucans or MLGs) are commonly found in the cell walls of grasses, but have also been detected in basal land plants, algae, fungi and bacteria. Here we show that two family GT2 glycosyltransferases from the Gram‐positive bacterium Sarcina ventriculi are capable of synthesizing MLGs. Immunotransmission electron microscopy demonstrates that MLG is secreted as an exopolysaccharide, where it may play a role in organizing individual cells into packets that are characteristic of Sarcina species. Heterologous expression of these two genes shows that they are capable of producing MLGs in planta, including an MLG that is chemically identical to the MLG secreted from S. ventriculi cells but which has regularly spaced (1,3)‐β‐linkages in a structure not reported previously for MLGs. The tandemly arranged, paralogous pair of genes are designated SvBmlgs1 and SvBmlgs2. The data indicate that MLG synthases have evolved different enzymic mechanisms for the incorporation of (1,3)‐β‐ and (1,4)‐β‐glucosyl residues into a single polysaccharide chain. Amino acid variants associated with the evolutionary switch from (1,4)‐β‐glucan (cellulose) to MLG synthesis have been identified in the active site regions of the enzymes. The presence of MLG synthesis in bacteria could prove valuable for large‐scale production of MLG for medical, food and beverage applications.

Funder

Australia and Pacific Science Foundation

Botany Foundation, Faculty of Science, University of Melbourne

U.S. Department of Energy

Australian Research Council

Publisher

Wiley

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