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Detecting proteins complex formation using steady-state diffusion in a nanochannel

Durand, Nicolas ; Saveriades, Elli ; Renaud, Philippe

In: Analytical and Bioanalytical Chemistry, 2009, vol. 394, no. 2, p. 421-425

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    Titre
    • Detecting proteins complex formation using steady-state diffusion in a nanochannel
    Auteur
    • Durand, Nicolas. Microsystems Laboratory, STI-LMIS, EPFL, 1015, Lausanne, Switzerland
    • Saveriades, Elli. Microsystems Laboratory, STI-LMIS, EPFL, 1015, Lausanne, Switzerland
    • Renaud, Philippe. Microsystems Laboratory, STI-LMIS, EPFL, 1015, Lausanne, Switzerland
    Type de document
    • Postprint
    Langue
    • Anglais
    Publié dans
    • Analytical and Bioanalytical Chemistry, 2009, vol. 394, no. 2, p. 421-425. Springer-Verlag
    Autre version électronique
    Identifiant OAI-PMH
    • oai:doc.rero.ch:318002
    Summary
    In this work, we present theoretical and experimental studies of nanofluidic channels as a potential biosensor for measuring rapid protein complex formation. Using the specific properties offered by nanofluidics, such as the decrease of effective diffusion of biomolecules in confined spaces, we are able to monitor the binding affinity of two proteins. We propose a theoretical model describing the concentration profile of proteins in a nanoslit and show that a complex composed by two bound biomolecules induces a wider diffusion profile than a single protein when driven through a nanochannel. To validate this model experimentally, we measured the increase of the fluorescent diffusion profile when specific biotinylated dextran was added to fluorescent streptavidin. We report here a direct and relatively simple technique to measure the affinity between proteins. Figure We present theoretical and experimental studies of nanofluidic channels as potential biosensors for rapidly measuring protein complex formation. Our system is based on steady-state diffusion effects which are observed inside a nanoslit