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Efficient chemo-enzymatic gluten detoxification: reducing toxic epitopes for celiac patients improving functional properties

机译:高效的化学酵素面筋排毒:减少腹腔患者的毒性表位,改善功能特性

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摘要

Protein engineering of gluten, the exogenous effector in celiac disease, seeking its detoxification by selective chemical modification of toxic epitopes is a very attractive strategy and promising technology when compared to pharmacological treatment or genetic engineering of wheat. Here we present a simple and efficient chemo-enzymatic methodology that decreases celiac disease toxic epitopes of gluten proteins improving its technological value through microbial transglutaminase-mediated transamidation of glutamine with n-butylamine under reducing conditions. First, we found that using low concentrations of amine-nucleophile under non-reducing conditions, the decrease in toxic epitopes is mainly due to transglutaminase-mediated cross-linking. Second, using high amine nucleophile concentrations protein cross-linking is substantially reduced. Third, reducing conditions increase 7-fold the transamidation reaction further decreasing toxic epitopes amount. Fourth, using n-butylamine improves gluten hydrophobicity that strengthens the gluten network. These results open the possibility of tailoring gluten for producing hypoallergenic flours while still taking advantage of the unique viscoelastic properties of gluten.
机译:与小麦的药理处理或基因工程相比,面筋的蛋白质工程(腹腔疾病的外源性效应物)通过对有毒抗原表位进行选择性化学修饰来寻求排毒是一项非常诱人的策略和有希望的技术。在这里,我们提出了一种简单有效的化学酶学方法,该方法可降低谷蛋白的乳糜泻毒性表位,并通过微生物转谷氨酰胺酶介导的谷氨酰胺与正丁胺在还原条件下的酰胺化而提高其技术价值。首先,我们发现在非还原条件下使用低浓度的胺亲核试剂,毒性表位的降低主要是由于转谷氨酰胺酶介导的交联。第二,使用高浓度的胺亲核试剂,可大大减少蛋白质的交联。第三,还原条件使氨基转移反应增加了7倍,从而进一步降低了毒性表位的数量。第四,使用正丁胺可改善面筋疏水性,从而增强面筋网络。这些结果打开了制备面筋以生产低变应原面粉的可能性,同时仍然利用了面筋独特的粘弹性质。

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