2021
DOI: 10.1039/d0sc05360k
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Introducing affinity and selectivity into galectin-targeting nanoparticles with fluorinated glycan ligands

Abstract: A chemo-enzymatic site-specific fluorination strategy is employed to obtain glyco-nanoparticles with tuneable selectivity towards galectins.

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Cited by 28 publications
(37 citation statements)
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“…Selected structures of deoxyfluorinated lacto-N-biose analogues conjugated to PHEA coated gold nanoparticles and the binding affinities of the resulting multivalent systems to Gal-3 and Gal-7 expressed as K d . [16] PHEA = poly(hydroxyethyl acrylamide). ND = observed affinity was too low to be determined.…”
Section: Resultsmentioning
confidence: 99%
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“…Selected structures of deoxyfluorinated lacto-N-biose analogues conjugated to PHEA coated gold nanoparticles and the binding affinities of the resulting multivalent systems to Gal-3 and Gal-7 expressed as K d . [16] PHEA = poly(hydroxyethyl acrylamide). ND = observed affinity was too low to be determined.…”
Section: Resultsmentioning
confidence: 99%
“…Gal-3 has also been recently probed with nanoparticles carrying deoxyfluorinated lacto-N-biose and the 6'-position has been confirmed as critical because deoxyfluorination at C6' abolished binding. [16] The introduction of a highly polar CÀ F bond can strengthen noncovalent ligand-protein interaction for example via electrostatic and dipolar interactions with cationic residues (e. g. the guanidinium group) and protein backbone or side-chain amide groups. [60] While this strategy to improve affinity of protein ligands was generally exceptionally fruitful, including galectin ligands fluorinated at aryl substituents [13,61] or polyfluorinated carbohydrates, [62] mono-deoxyfluorinated oligosaccharides typically display similar, attenuated or abrogated affinity to lectins in comparison with the natural ligands.…”
Section: Discussionmentioning
confidence: 99%
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