DypB peroxidase for aflatoxin removal: New insights into the toxin degradation process

黄曲霉毒素 化学 降级(电信) 真菌毒素 过氧化物酶 毒素 致癌物 生物化学 组合化学 食品科学 电信 计算机科学
作者
Vincenzo Mangini,Elena Rosini,Rocco Caliandro,Giuseppe Felice Mangiatordi,Pietro Delre,Anna Giovanna Sciancalepore,Loredano Pollegioni,Miriam Haidukowski,Marco Mazzorana,Mark W. Sumarah,Justin B. Renaud,Ralf Flaig,Giuseppina Mulè,Benny Danilo Belviso,Martina Loi
出处
期刊:Chemosphere [Elsevier]
卷期号:349: 140826-140826 被引量:6
标识
DOI:10.1016/j.chemosphere.2023.140826
摘要

Aflatoxin B1 (AFB1) is one of the most potent carcinogens and a widespread food and feed contaminant. As for other toxins, many efforts are devoted to find efficient and environmentally-friendly methods to degrade AFB1, such as enzymatic treatments, thus improving the safety of food and feed products. In this regard, the dye decolorizing peroxidase of type B (DypB) can efficiently degrade AFB1. The molecular mechanism, which is required to drive protein optimization in view of the usage of DypB as a mycotoxin reduction agent in large scale application, is unknown. Here, we focused on the role of four DypB residues in the degradation of AFB1 by alanine-scanning (residues 156, 215, 239 and 246), which were identified from biochemical assays to be kinetically relevant for the degradation. As a result of DypB degradation, AFB1 is converted into four products. Interestingly, the relative abundancy of these products depends on the replaced residues. Molecular dynamics simulations were used to investigate the role of these residues in the binding step between protein and manganese, a metal ion which is expected to be involved in the degradation process. We found that the size of the haem pocket as well as conformational changes in the protein structure could play a role in determining the kinetics of AFB1 removal and, consequently, guide the process towards specific degradation products.

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