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A generic approach based on long-lifetime fluorophores for the assessment of protein binding to polymer nanoparticles by fluorescence anisotropy.

Marwa A AhmedDóra HesszBenjámin GyarmatiMirkó PáncsicsNorbert KovácsRóbert E GyurcsányiMiklós KubinyiViola Horváth
Published in: Nanoscale (2024)
Quantitation of protein-nanoparticle interactions is essential for the investigation of the protein corona around NPs in vivo and when using synthetic polymer nanoparticles as affinity reagents for selective protein recognition in vitro . Here, a method based on steady-state fluorescence anisotropy measurement is presented as a novel, separation-free tool for the assessment of protein-nanoparticle interactions. For this purpose, a long-lifetime luminescent Ru-complex is used for protein labelling, which exhibits low anisotropy when conjugated to the protein but displays high anisotropy when the proteins are bound to the much larger polymer nanoparticles. As a proof of concept, the interaction of lysozyme with poly( N -isopropylacrylamide- co-N-tert -butylacrylamide- co -acrylic acid) nanoparticles is studied, and fluorescence anisotropy measurements are used to establish the binding kinetics, binding isotherm and a competitive binding assay.
Keyphrases
  • binding protein
  • protein protein
  • amino acid
  • mass spectrometry
  • small molecule
  • transcription factor
  • tandem mass spectrometry
  • high performance liquid chromatography
  • iron oxide