The alphaPROX assay: fluorescence screening of the inhibitory effects of hydrophilic antioxidants on protein oxidation

TY - JOUR

T1 - The alphaPROX assay

T2 - fluorescence screening of the inhibitory effects of hydrophilic antioxidants on protein oxidation

AU - Fruhwirth, Gilbert O

AU - Wagner, Franz S

AU - Hermetter, Albin

PY - 2006/2

Y1 - 2006/2

N2 - We report on a new and convenient high-throughput fluorescence technique for determining antioxidant capacities of hydrophilic food samples. The new method is called alphaPROX (anti protein oxidation) and is based on an equimolar complex of diphenylhexatriene propionic acid (DPHPA) and bovine serum albumin (BSA) in aqueous buffer at pH 7.4. DPHPA is a reporter fluorophore that becomes nonfluorescent upon free radical-induced oxidation. In a typical assay, the DPHPA/BSA complex is challenged with peroxyl radicals and shows almost the same susceptibility to oxidation as unlabeled BSA. The progress of protein oxidation and its inhibition by antioxidants at physiological pH is determined from the time-dependent decrease in DPHPA fluorescence intensity. The alphaPROX method was compared to other techniques frequently used to measure antioxidant capacities. In this article, representative results are provided for the inhibitory effects of pure food components, fruit juices, wines, and various polar plant extracts on protein oxidation.

AB - We report on a new and convenient high-throughput fluorescence technique for determining antioxidant capacities of hydrophilic food samples. The new method is called alphaPROX (anti protein oxidation) and is based on an equimolar complex of diphenylhexatriene propionic acid (DPHPA) and bovine serum albumin (BSA) in aqueous buffer at pH 7.4. DPHPA is a reporter fluorophore that becomes nonfluorescent upon free radical-induced oxidation. In a typical assay, the DPHPA/BSA complex is challenged with peroxyl radicals and shows almost the same susceptibility to oxidation as unlabeled BSA. The progress of protein oxidation and its inhibition by antioxidants at physiological pH is determined from the time-dependent decrease in DPHPA fluorescence intensity. The alphaPROX method was compared to other techniques frequently used to measure antioxidant capacities. In this article, representative results are provided for the inhibitory effects of pure food components, fruit juices, wines, and various polar plant extracts on protein oxidation.

KW - Antioxidants

KW - Beverages

KW - Diphenylhexatriene

KW - Fluorescence

KW - Food Analysis

KW - Fruit

KW - Hydrogen-Ion Concentration

KW - Hydrophobic and Hydrophilic Interactions

KW - Molecular Structure

KW - Oxidation-Reduction

KW - Plant Extracts

KW - Seeds

KW - Serum Albumin, Bovine

KW - Time Factors

KW - Wine

U2 - 10.1007/s00216-005-0179-2

DO - 10.1007/s00216-005-0179-2

M3 - Article

C2 - 16440197

SN - 1618-2642

VL - 384

SP - 703

EP - 712

JO - ANALYTICAL AND BIOANALYTICAL CHEMISTRY

JF - ANALYTICAL AND BIOANALYTICAL CHEMISTRY

IS - 3

ER -