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Rapid and Sensitive Detection of Aspergillus niger Using a Single-Mediator System Combined with Redox Cycling

机译:使用单介子系统结合氧化还原循环的快速敏感地检测曲霉尼日尔

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摘要

Rapid and sensitive mold detection is becoming increasingly important, especially in indoor environments. Common mold detection methods based on double mediated electron transfer between an electrode and molds are not highly sensitive and reproducible, although they are rapid and simple. Here, we report a sensitive and reproducible detection method specific to Aspergillus niger (A. niger), based on a single-mediator system combined with electrochemical-chemical (EC) redox cycling. Intracellular NAD(P)H-oxidizing enzymes in molds can convert electro-inactive hydroxy-nitro(so)arenes into electro-active hydroxy-aminoarenes. Since the membrane and wall of A. niger is well permeable to both a substrate (4-nitro-1-naphthol) and a reduced product (4-amino-1-naphthol) in tris buffer (pH 7.5) solution, the electrochemical signal is increased in the presence of A. niger due to two reactions: (i) enzymatic reduction of the substrate to the reduced product and (ii) electrochemical oxidation of the reduced product to an oxidized product. When a reducing agent (NADH) is present in the solution, the oxidized product is reduced back to the reduced product and then electrochemically reoxidized. This EC redox cycling significantly amplifies the electrochemical signal. Moreover, the background level is low and highly reproducible because the substrate and the reducing agent are electro-inactive at an applied potential of 0.20 V. The calculated detection limit for A. niger in a common double mediator system consisting of Fe(CN)(6)(3-) and menadione is similar to 2 X 10(4) colony-forming unit (CFU)/mL, but the detection limit in the single-mediator system combined with EC redox cycling is similar to 2 X 10(3) CFU/mL, indicating that the newly developed single-mediator system is more sensitive. Importantly, the detection method requires only an incubation period of 10 min and does not require a washing step, an electrode modification step, or a specific probe.
机译:快速和敏感的模具检测变得越来越重要,尤其是在室内环境中。虽然它们迅速简单,但基于电极和模具之间的双介导电子传递的常见模具检测方法不高度敏感和可重复。这里,我们报告了一种敏感性和可重复的检测方法,其特异于曲霉(A.Niger),基于单介体系统与电化学 - 化学(EC)氧化还原循环结合。模具中的细胞内NAD(P)H氧化酶可以将电活性羟基 - 硝基(SO)转化为电活性羟基氨基氨基。由于A的膜和壁的膜和奈埃壁对Tris缓冲液(pH7.5)溶液中的基材(4-硝基-1-萘糖醇)和还原产物(4-氨基-1-萘酚)渗透,因此电化学信号由于两种反应存在,在A.尼日尔的存在下增加当在溶液中存在还原剂(NADH)时,将氧化产物减少回还原产物,然后电化学再氧化。该EC氧化还原循环显着放大电化学信号。此外,背景水平低且高度可再现,因为基材和还原剂在0.20V的施加电位下是电失效的。在由Fe(CN)组成的普通双介体系统中的A.尼日尔的计算检测限。 6)(3-)和男女淋巴胺类似于2×10(4)个菌落 - 形成单位(CFU)/ mL,但单晶蛋白系统中的检测限与EC氧化还原循环相似,类似于2×10(3 )CFU / ml,表明新开发的单介子系统更敏感。重要的是,检测方法仅需要10分钟的孵育周期,并且不需要洗涤步骤,电极改性步骤或特定探针。

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