Oxime blot: A novel method for reliable and sensitive detection of carbonylated proteins in diverse biological systems

蛋白质羰基化 衍生化 化学 免疫沉淀 组合化学 色谱法 污渍 生物化学 氧化应激 高效液相色谱法 氧化损伤 基因
作者
Romain Ladouce,Guillaume Combes,Katarina Trajković,Irena Drmić Hofman,Mladen Merćep
出处
期刊:Redox biology [Elsevier BV]
卷期号:63: 102743-102743 被引量:1
标识
DOI:10.1016/j.redox.2023.102743
摘要

Oxidative stress and oxidative protein damage occur in various biological processes and diseases. The carbonyl group on amino acid side chains is the most widely used protein oxidation biomarker. Carbonyl groups are commonly detected indirectly through their reaction with 2,4-dinitrophenylhydrazine (DNPH) and subsequent labeling with an anti-DNP antibody. However, the DNPH immunoblotting method lacks protocol standardization, exhibits technical bias, and has low reliability. To overcome these shortcomings, we have developed a new blotting method in which the carbonyl group reacts with the biotin-aminooxy probe to form a chemically stable oxime bond. The reaction speed and the extent of the carbonyl group derivatization are increased by adding a p-phenylenediamine (pPDA) catalyst under neutral pH conditions. These improvements are crucial since they ensure that the carbonyl derivatization reaction reaches a plateau within hours and increases the sensitivity and robustness of protein carbonyl detection. Furthermore, derivatization under pH-neutral conditions facilitates a good SDS-PAGE protein migration pattern, avoids protein loss by acidic precipitation, and is directly compatible with protein immunoprecipitation. This work describes the new Oxime blot method and demonstrates its use in detecting protein carbonylation in complex matrices from diverse biological samples.

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