Evaluation of Azido
3‑Deoxy‑d-<i>manno</i>-oct-2-ulosonic
Acid (Kdo) Analogues for Click
Chemistry-Mediated Metabolic Labeling of Myxococcus
xanthus DZ2 Lipopolysaccharide

Adyasha Panda (13849641); Ahmad A. Kezzo (13849635); Charles Gauthier (1451917); Eric Ramirez Esquivel (13849638); Evgeny Vinogradov (159941); Fares Saïdi (13849623); Gaurav Sharma (749390); Gokulakrishnan Ravicoularamin (8953256); José Ignacio Veytia-Bucheli (13849629); Nicolas Y. Jolivet (13849632); Oscar Javier Gamboa Marin (13849626); Salim T. Islam (8953238); Stéphane
P. Vincent (13849644)

Evaluation of Azido 3‑Deoxy‑d-<i>manno</i>-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide

Authors: Adyasha Panda (13849641)
Ahmad A. Kezzo (13849635)
Charles Gauthier (1451917)
Eric Ramirez Esquivel (13849638)
Evgeny Vinogradov (159941)
Fares Saïdi (13849623)
Gaurav Sharma (749390)
Gokulakrishnan Ravicoularamin (8953256)
José Ignacio Veytia-Bucheli (13849629)
Nicolas Y. Jolivet (13849632)
Oscar Javier Gamboa Marin (13849626)
Salim T. Islam (8953238)
Stéphane P. Vincent (13849644)
Publication date: 23 September 2022
Publisher: 'American Chemical Society (ACS)'
Doi

Abstract

Metabolic labeling paired with click chemistry is a powerful approach for selectively imaging the surfaces of diverse bacteria. Herein, we explored the feasibility of labeling the lipopolysaccharide (LPS) of Myxococcus xanthusa Gram-negative predatory social bacterium known to display complex outer membrane (OM) dynamicsvia growth in the presence of distinct azido (-N3) analogues of 3-deoxy-d-manno-oct-2-ulosonic acid (Kdo). Determination of the LPS carbohydrate structure from strain DZ2 revealed the presence of one Kdo sugar in the core oligosaccharide, modified with phosphoethanolamine. The production of 8-azido-8-deoxy-Kdo (8-N3-Kdo) was then greatly improved over previous reports via optimization of the synthesis of its 5-azido-5-deoxy-d-arabinose precursor to yield gram amounts. The novel analogue 7-azido-7-deoxy-Kdo (7-N3-Kdo) was also synthesized, with both analogues capable of undergoing in vitro strain-promoted azide–alkyne cycloaddition (SPAAC) “click” chemistry reactions. Slower and faster growth of M. xanthus was displayed in the presence of 8-N3-Kdo and 7-N3-Kdo (respectively) compared to untreated cells, with differences also seen for single-cell gliding motility and type IV pilus-dependent swarm community expansion. While the surfaces of 8-N3-Kdo-grown cells were fluorescently labeled following treatment with dibenzocyclooctyne-linked fluorophores, the surfaces of 7-N3-Kdo-grown cells could not undergo fluorescent tagging. Activity analysis of the KdsB enzyme required to activate Kdo prior to its integration into nascent LPS molecules revealed that while 8-N3-Kdo is indeed a substrate of the enzyme, 7-N3-Kdo is not. Though a lack of M. xanthus cell aggregation was shown to expedite growth in liquid culture, 7-N3-Kdo-grown cells did not manifest differences in intrinsic clumping relative to untreated cells, suggesting that 7-N3-Kdo may instead be catabolized by the cells. Ultimately, these data provide important insights into the synthesis and cellular processing of valuable metabolic labels and establish a basis for the elucidation of fundamental principles of OM dynamism in live bacterial cells

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