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Reversible detection of proteases and their inhibitors by a pulsed chronopotentiometric polyion-sensitive electrode
Authors:Xu Yida  Shvarev Alexey  Makarychev-Mikhailov Sergey  Bakker Eric
Affiliation:a Department of Chemistry, Purdue University, IN 47907, USA
b Department of Chemistry, Oregon State University, OR 97331, USA
c Nanochemistry Research Institute, Department of Applied Chemistry, Curtin University of Technology, Perth, WA 6485, Australia
Abstract:Polymer membrane electrodes operated by pulsed chronopotentiometry have recently been introduced to replace traditional ion-selective electrodes for a number of applications. While ion-selective electrodes for the polycation protamine have been reported, for instance, a pulsed chronopotentiometric readout mode (called here pulstrode) provides improved stability and reproducibility while exhibiting sufficient selectivity for the direct detection of protamine in undiluted whole blood samples. Here, such protamine-sensitive pulstrodes are applied for the real-time detection of the activity of the protease trypsin and its soybean inhibitor. This is possible because small fragments produced by the trypsin digestion are not detectable by the protamine-sensing membrane. The real-time response to the proteolytic reaction is shown to exhibit good reproducibility and reversibility, and the initial reaction rate is dependent on the concentration of the protease and its inhibitor.
Keywords:Protamine   Trypsin   Membrane electrode   Pulsed chronopotentiometry   Enzyme detection
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