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Azoreductase activity of dye-decolorizing bacteria isolated from the human gut microbiota

机译:从人体肠道菌群中分离出的染料脱色细菌的氮还原酶活性

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摘要

The gut microbiota enriches the human gene pool and contributes to xenobiotic metabolism. Microbial azoreductases modulate the reduction of azo-bonds, activating produgs and azo polymer-coated dosage forms, or degrading food additives. Here, we aimed to screen the healthy human gut microbiota for food colorant-reducing activity and to characterize factors modulating it. Four representative isolates from screened fecal samples were identified as E. coli (AZO-Ec), E. faecalis (AZO-Ef), E. avium (AZO-Ev) and B. cereus (AZO-Bc). Both AZO-Ef and AZO-Ev decolorized amaranth aerobically and microaerophilically while AZO-Ec and AZO-Bc had higher aerobic reduction rates. The isolates varied in their activities against different dyes, and the azo-reduction activity mostly followed zero-order reaction kinetics, with a few exceptions. Additionally, the isolates had different pH dependence, e.g., AZO-Ec was not affected by pH variation while AZO-Bc exhibited variable degradation kinetics at different pH levels. Cell-free extracts showed NADH-dependent enzymatic activities 14–19 times higher than extracellular fractions. FMN did not affect the reducing activity of AZO-Ef cell-free extract, whereas AZO-Ec, AZO-Ev and AZO-Bc had significantly higher reduction rates in its presence (P values = 0.02, 0.0001 and 0.02, respectively). Using Degenerate primers allowed the amplification of azoreductase genes, whose sequences were 98–99% similar to genes encoding FMN-dependent-NADH azoreductases.
机译:肠道菌群丰富了人类基因库,并促进了异种生物的代谢。微生物偶氮还原酶可调节偶氮键的还原,激活前药和偶氮聚合物包衣的剂型或降解食品添加剂。在这里,我们旨在筛选健康的人类肠道菌群,以减少食物色素的活性,并表征调节其的因素。筛选出的粪便样本中有四个代表性的分离株被鉴定为大肠杆菌(AZO-Ec),粪肠球菌(AZO-Ef),禽肠杆菌(AZO-Ev)和蜡状芽孢杆菌(AZO-Bc)。 AZO-Ef和AZO-Ev均需氧和微需氧地使a菜脱色,而AZO-Ec和AZO-Bc的需氧减少率更高。分离物对不同染料的活性各不相同,偶氮还原活性大多遵循零级反应动力学,只有少数例外。另外,分离物具有不同的pH依赖性,例如,AZO-Ec不受pH变化的影响,而AZO-Bc在不同pH水平下表现出可变的降解动力学。无细胞提取物显示出NADH依赖性酶活性比细胞外组分高14-19倍。 FMN不会影响AZO-Ef无细胞提取物的还原活性,而AZO-Ec,AZO-Ev和AZO-Bc在其存在下的还原率明显更高(分别为P值= 0.02、0.0001和0.02)。使用简并引物可以扩增偶氮还原酶基因,其序列与编码FMN依赖性NADH偶氮还原酶的基因相似,为98–99%。

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