Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide

Fares Saïdi; Oscar Javier Gamboa Marin; José Ignacio Veytia-Bucheli; Evgeny Vinogradov; Gokulakrishnan Ravicoularamin; Nicolas Y. Jolivet; Ahmad A. Kezzo; Eric Ramirez Esquivel; Adyasha Panda; Gaurav Sharma; Stephane Vincent; Charles Gauthier; Salim T. Islam

doi:10.1021/acsomega.2c03711

Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide

Fares Saïdi, Oscar Javier Gamboa Marin, José Ignacio Veytia-Bucheli, Evgeny Vinogradov, Gokulakrishnan Ravicoularamin, Nicolas Y. Jolivet, Ahmad A. Kezzo, Eric Ramirez Esquivel, Adyasha Panda, Gaurav Sharma, Stephane Vincent, Charles Gauthier, Salim T. Islam

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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 xanthus─a Gram-negative predatory social bacterium known to display complex outer membrane (OM) dynamics─via 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.

Original language	English
Pages (from-to)	34997-35013
Number of pages	17
Journal	ACS Omega
Volume	7
Issue number	39
DOIs	https://doi.org/10.1021/acsomega.2c03711
Publication status	Published - 4 Oct 2022

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10.1021/acsomega.2c03711

acsomega.2c03711Final published version, 6.34 MBLicence: CC BY-NC-ND

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Saïdi, F., Gamboa Marin, O. J., Veytia-Bucheli, J. I., Vinogradov, E., Ravicoularamin, G., Jolivet, N. Y., Kezzo, A. A., Ramirez Esquivel, E., Panda, A., Sharma, G., Vincent, S., Gauthier, C., & Islam, S. T. (2022). Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide. ACS Omega, 7(39), 34997-35013. https://doi.org/10.1021/acsomega.2c03711

@article{050c268fb7fe4fe2995809120fb350ab,

title = "Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide",

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 xanthus─a Gram-negative predatory social bacterium known to display complex outer membrane (OM) dynamics─via 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.",

author = "Fares Sa{\"i}di and {Gamboa Marin}, {Oscar Javier} and Veytia-Bucheli, {Jos{\'e} Ignacio} and Evgeny Vinogradov and Gokulakrishnan Ravicoularamin and Jolivet, {Nicolas Y.} and Kezzo, {Ahmad A.} and {Ramirez Esquivel}, Eric and Adyasha Panda and Gaurav Sharma and Stephane Vincent and Charles Gauthier and Islam, {Salim T.}",

note = "Funding Information: The authors thank Uwe Mamat for providing cells and expression constructs for KdsB-His, as well as Sam Dukan, Emilie Fugier, Audrey Dumont, and T{\^a}m Mignot for helping demonstrate the initial feasibility of M. xanthus 8-N -Kdo labeling. A Discovery operating grant (RGPIN-2016-06637) from the Natural Sciences and Engineering Research Council of Canada (NSERC) and a Discovery Award (2018-1400) from the Banting Research Foundation funded this work in the lab of S.T.I. F.S., N.Y.J., and A.A.K. were supported by funds from the former, while E.R.E. was supported by funds from the latter. F.S. (PhD), A.A.K. (MSc), and E.R.E. (MSc) were also supported by studentships from the Fondation Armand-Frappier, while F.S. and N.Y.J. were also supported by studentships from PROTEO (the Quebec Network for Research on Protein Function, Engineering, and Applications). O.J.G.M. was supported by PhD studentships from the Fondation Armand-Frappier and the Fonds de recherche du Qu{\'e}bec─Nature et technologies (FRQNT). Work in the lab of C.G. was supported through NSERC Discovery Awards (RGPIN-2016-04950 and RGPIN-2022-04515), and the R{\'e}seau qu{\'e}b{\'e}cois de recherche sur les m{\'e}dicaments (RQRM). The labs of C.G. and S.P.V. were jointly supported by a bilateral funding program between the Fonds de recherche du Qu{\'e}bec (FRQ) and the Fonds de la recherche scientifique (F.R.S-FNRS) (Convention PINT-BILAT-P R.P005.19, post-doctoral grant to J.I.B.V.). None of the above-mentioned funding sources had any input in the preparation of this article, or in the work described herein. 6 3 Publisher Copyright: {\textcopyright} 2022 The Authors. Published by American Chemical Society.",

year = "2022",

month = oct,

day = "4",

doi = "10.1021/acsomega.2c03711",

language = "English",

volume = "7",

pages = "34997--35013",

journal = "ACS Omega",

issn = "2470-1343",

publisher = "ACS",

number = "39",

}

Saïdi, F, Gamboa Marin, OJ, Veytia-Bucheli, JI, Vinogradov, E, Ravicoularamin, G, Jolivet, NY, Kezzo, AA, Ramirez Esquivel, E, Panda, A, Sharma, G, Vincent, S, Gauthier, C & Islam, ST 2022, 'Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide', ACS Omega, vol. 7, no. 39, pp. 34997-35013. https://doi.org/10.1021/acsomega.2c03711

Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide. / Saïdi, Fares; Gamboa Marin, Oscar Javier; Veytia-Bucheli, José Ignacio et al.
In: ACS Omega, Vol. 7, No. 39, 04.10.2022, p. 34997-35013.

Research output: Contribution to journal › Article › peer-review

TY - JOUR

T1 - Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide

AU - Saïdi, Fares

AU - Gamboa Marin, Oscar Javier

AU - Veytia-Bucheli, José Ignacio

AU - Vinogradov, Evgeny

AU - Ravicoularamin, Gokulakrishnan

AU - Jolivet, Nicolas Y.

AU - Kezzo, Ahmad A.

AU - Ramirez Esquivel, Eric

AU - Panda, Adyasha

AU - Sharma, Gaurav

AU - Vincent, Stephane

AU - Gauthier, Charles

AU - Islam, Salim T.

N1 - Funding Information: The authors thank Uwe Mamat for providing cells and expression constructs for KdsB-His, as well as Sam Dukan, Emilie Fugier, Audrey Dumont, and Tâm Mignot for helping demonstrate the initial feasibility of M. xanthus 8-N -Kdo labeling. A Discovery operating grant (RGPIN-2016-06637) from the Natural Sciences and Engineering Research Council of Canada (NSERC) and a Discovery Award (2018-1400) from the Banting Research Foundation funded this work in the lab of S.T.I. F.S., N.Y.J., and A.A.K. were supported by funds from the former, while E.R.E. was supported by funds from the latter. F.S. (PhD), A.A.K. (MSc), and E.R.E. (MSc) were also supported by studentships from the Fondation Armand-Frappier, while F.S. and N.Y.J. were also supported by studentships from PROTEO (the Quebec Network for Research on Protein Function, Engineering, and Applications). O.J.G.M. was supported by PhD studentships from the Fondation Armand-Frappier and the Fonds de recherche du Québec─Nature et technologies (FRQNT). Work in the lab of C.G. was supported through NSERC Discovery Awards (RGPIN-2016-04950 and RGPIN-2022-04515), and the Réseau québécois de recherche sur les médicaments (RQRM). The labs of C.G. and S.P.V. were jointly supported by a bilateral funding program between the Fonds de recherche du Québec (FRQ) and the Fonds de la recherche scientifique (F.R.S-FNRS) (Convention PINT-BILAT-P R.P005.19, post-doctoral grant to J.I.B.V.). None of the above-mentioned funding sources had any input in the preparation of this article, or in the work described herein. 6 3 Publisher Copyright: © 2022 The Authors. Published by American Chemical Society.

PY - 2022/10/4

Y1 - 2022/10/4

N2 - 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 xanthus─a Gram-negative predatory social bacterium known to display complex outer membrane (OM) dynamics─via 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.

AB - 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 xanthus─a Gram-negative predatory social bacterium known to display complex outer membrane (OM) dynamics─via 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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U2 - 10.1021/acsomega.2c03711

DO - 10.1021/acsomega.2c03711

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SN - 2470-1343

VL - 7

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JO - ACS Omega

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ER -

Evaluation of Azido 3-Deoxy- d - Manno-oct-2-ulosonic Acid (Kdo) Analogues for Click Chemistry-Mediated Metabolic Labeling of Myxococcus xanthus DZ2 Lipopolysaccharide

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