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Improved Methods for the Rapid Formation and Prevention of Advanced Glycation End Products (AGEs) In Vitro by Coupling to the Hypoxanthine/Xanthine Oxidase Assay System

机译:通过耦合至次黄嘌呤/黄嘌呤氧化酶测定系统快速形成和预防体外高级糖化终产物(AGEs)的改进方法

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Advanced glycation end products (AGEs) represent a set of molecules that contribute directly to the initiation and aggravation of diseases associated with ageing. AGEs are produced by the reaction between reducing sugars (or α-dicarbonyl compounds), proteins, and amino acid residues. Previous in vitro methods using non-enzymatic procedures described in the literature require an incubation period of 1–3 weeks to generate AGEs. In this study, the reaction time for the formation of AGEs (48 and 3 h) was significantly reduced by adaptation of methods previously described in the literature and coupling them to the free radical generation system termed hypoxanthine/xanthine oxidase assay. The incorporation of this assay into the experimental system accelerated the production of AGEs as a result of the formation of reactive oxygen species (ROS), as shown by increased fluorescence. The capacity of different classes of chemical compounds (aminoguanidine, chlorogenic acid, rutin, and methanol extracts of Hancornia speciosa Gomes) to inhibit protein glycation by acting as scavenging agents of α-dicarbonyl species was evaluated. Aminoguanidine and, especially, rutin identified in the leaf extracts of H. speciosa Gomes showed a high capacity to act as scavengers of reactive carbonyl species RCS-trapping, resulting in the inhibition of AGEs formation.
机译:晚期糖基化终末产物(AGEs)代表一组直接导致与衰老相关的疾病的发生和加剧的分子。 AGEs是由还原糖(或α-二羰基化合物),蛋白质和氨基酸残基之间的反应产生的。先前使用文献中描述的使用非酶促程序的体外方法需要1-3周的潜伏期才能产生AGEs。在这项研究中,通过改编先前文献中描述的方法并将其与称为次黄嘌呤/黄嘌呤氧化酶测定法的自由基生成系统偶联,可显着减少AGEs形成的反应时间(48和3 h)。如荧光增强所示,由于活性氧(ROS)的形成,该测定法并入实验系统加速了AGEs的产生。评估了不同种类的化合物(汉果角藻(Hancornia speciosa Gomes)的氨基胍,绿原酸,芦丁和甲醇提取物)通过充当α-二羰基物质的清除剂来抑制蛋白质糖基化的能力。幽门螺杆菌戈梅斯叶片提取物中鉴定出的氨基胍,尤其是芦丁,具有高活性,可以清除活性羰基物质RCS捕获,从而抑制AGEs的形成。

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