Bovine Serum Albumin Catalysed Hydrogen and Deuterium Evolution at Mercury Electrodes.

Chempluschem

Department of Biophysical Chemistry and Molecular Oncology, Institute of Biophysics of the Czech Academy of Sciences, v.v.i., Kralovopolska 135, 612 65, Brno, Czech Republic.

Published: July 2020

AI Article Synopsis

  • The hydrogen evolution reaction (HER) at mercury electrodes, influenced by proteins, allows for a sensitive, label-free analysis of protein structures.
  • The study showed that the stronger deuteron bond resulted in poorer deuteron transport by bovine serum albumin (BSA) at the hydrogen-deuterium interface, while also improving the structural stability of BSA.
  • A structural change was noted in denatured BSA, likely due to the destabilization of certain secondary structures, but no hydrogen/deuterium exchange was detected in the native form of BSA under the experimental conditions.

Article Abstract

The hydrogen evolution reaction (HER), catalysed by proteins at mercury electrodes and reflected in chronopotentiometric stripping peak H, provides a label-free and reagentless analytical technique that is sensitive to protein structure. Here we show how the kinetic isotope effect affected the HER catalysed by the protein bovine serum albumin (BSA). We found that the deuteron bond, which is stronger than that of a proton, contributed to less effective transport of deuterons mediated by BSA at the Hg|D O interface, and enhanced structural stability of the surface-attached native BSA in D O solution. A structural transition was also observed in the surface-attached urea-denatured BSA, and is probably due to the destabilisation of some secondary structural remnants retained by the 17 SS-bonds. Because the catalytically active groups involved in proton or deuteron transfer in native proteins are often exposed towards solutions and their protons exchange almost instantly, no signs of H/D exchange were observed in native BSA using peak H under the given conditions.

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Source
http://dx.doi.org/10.1002/cplu.202000348DOI Listing

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