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Fluorescence "Turn-on" Lectin Sensors Fabricated by Ligand-Assisted Labeling Probes for Detecting Protein-Glycoprotein Interactions
Journal article   Peer reviewed

Fluorescence "Turn-on" Lectin Sensors Fabricated by Ligand-Assisted Labeling Probes for Detecting Protein-Glycoprotein Interactions

Pei-Jhen Li, Mohammad Tarigue Anwar, Chen-Yo Fan, Duane Juang, Hsin-Yi Lin, Tsung-Che Chang, Sachin Kisan Kawade, Hsiang-Jung Chen, Yu-Ju Chen and Kui-Thong Tan
Biomacromolecules, Vol.21(2), pp.815-824
02/10/2020
Handle:
https://hdl.handle.net/10192/79139
PMID: 31891486

Abstract

Biosensing Techniques - methods Fluorescent Dyes - chemistry Fluorescent Dyes - metabolism Glycoproteins - chemistry Glycoproteins - metabolism HeLa Cells Humans Lectins - chemistry Lectins - metabolism Micrococcaceae - metabolism Protein Interaction Domains and Motifs - physiology Protein Structure, Secondary Protein Structure, Tertiary Ligands
Elucidation of protein-protein interactions (PPIs) is often very challenging and yields complex and unclear results. Lectin-glycoprotein interactions are especially difficult to study due to the noncovalent nature of the interactions and inherently low binding affinities of proteins to glycan ligands on glycoproteins. Here, we report a "ligand-directed labeling probe (LLP)"-based approach to fabricate protein probes for elucidating protein-glycoprotein interactions. LLP was designed with dual photoactivatable groups for the introduction of an alkyne handle proximal to the carbohydrate-binding pocket of lectins, agglutinin 120 (RCA ) and recombinant human Siglec-2-Fc. In proof-of-principle studies, alkynylated lectins were conjugated with a photoreactive diazirine cross-linker and an environment-sensitive fluorophore, respectively, by the bioorthogonal click reaction. The modified RCA or Siglec-2-Fc was used for detecting the interaction with the target glycoprotein in the solution or endogenously expressed glycoproteins on live HeLa cells. We anticipate that the fabrication of these protein probes will accelerate the discovery of novel PPIs.

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