Literature DB >> 18492479

A colorimetric assay for steady-state analyses of iodo- and bromoperoxidase activities.

Elodie Verhaeghe1, David Buisson, Elisabeth Zekri, Catherine Leblanc, Philippe Potin, Yves Ambroise.   

Abstract

The standard assay for iodoperoxidase activity is based on the spectrophotometric detection of triiodide formed during the enzymatic reaction. However, chemical instability of I3- has limited the method to high iodide concentrations and acidic conditions. Here we describe a simple spectrophotometric assay for the determination of iodoperoxidase activities of vanadium haloperoxidases based on the halogenation of thymol blue. The relation between color and chemical entities produced by the vHPO/H(2)O(2)/I(-) catalytic system was characterized. The method was extended to bromine and, for the first time, allowed measurement of both iodo- and bromoperoxidase activities using the same assay. The kinetic parameters (K(m) and k(cat)) of bromide and iodide for vanadium bromoperoxidase from Ascophyllum nodosum were determined at pH 8.0 from steady-state kinetic analyses. The results are concordant with an ordered two-substrate mechanism. It is proposed that halide selectivity is guided by the chemical reactivity of peroxovanadium intermediate rather than substrate binding. This method is superior to the standard I3- assay, and we believe that it will find applications for the characterization of other vanadium as well as heme haloperoxidases.

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Year:  2008        PMID: 18492479     DOI: 10.1016/j.ab.2008.04.041

Source DB:  PubMed          Journal:  Anal Biochem        ISSN: 0003-2697            Impact factor:   3.365


  9 in total

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Authors:  Frithjof C Küpper; Lucy J Carpenter; Catherine Leblanc; Chiaki Toyama; Yuka Uchida; Benjamin H Maskrey; Joanne Robinson; Elodie F Verhaeghe; Gill Malin; George W Luther; Peter M H Kroneck; Bernard Kloareg; Wolfram Meyer-Klaucke; Yasuyuki Muramatsu; Ian L Megson; Philippe Potin; Martin C Feiters
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  9 in total

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