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微生物培养物中儿茶酚型铁载体的比色测定

Colorimetric determination of catechol siderophores in microbial cultures.

作者信息

Rioux C, Jordan D C, Rattray J B

出版信息

Anal Biochem. 1983 Aug;133(1):163-9. doi: 10.1016/0003-2697(83)90238-5.

DOI:10.1016/0003-2697(83)90238-5
PMID:6227261
Abstract

A highly sensitive spectrophotometric method for the selective detection of catechol compounds such as catechol siderophores (e.g., enterobactin) is described. The basis of the method involves the ability of the vicinal aromatic hydroxyl groups under acidic conditions to bring about a reduction of Fe3+ (from ferric ammonium citrate) to Fe2+. Detection of Fe2+ in the presence of Fe3+ is made with 1,10-phenanthroline under previously established conditions. The assay mixture is heated at 60 degrees C for 1 h to accelerate the development of color which is subsequently measured at 510 nm. The Beer-Lambert law is obeyed over the range of 0.16 to 60 microM 2,3-dihydroxybenzoic acid. Compared to the Arnow nitration method, the assay is more responsive, is approximately seven times more sensitive, and is effective with catechols substituted at positions 3 and 4. The method gives positive results with catechols such as DL-DOPA, L-dopamine, (+/-)-epinephrine, and DL-norepinephrine. Very rapid color development is obtained with ascorbic acid and p-diols, while m-diols are poorly detected. Low degrees of reactivity are shown by hydroxylamino and hydroxamate compounds. Phenolic, sulfydryl, indolyl, and quinonyl derivatives do not interfere with the reaction. The method has been adapted to determine catechol compounds in the culture medium of bacterial cells grown at different iron concentrations.

摘要

描述了一种用于选择性检测儿茶酚化合物(如儿茶酚型铁载体,例如肠杆菌素)的高灵敏度分光光度法。该方法的基础是邻位芳香族羟基在酸性条件下能够将Fe3 +(来自柠檬酸铁铵)还原为Fe2 +。在先前确定的条件下,用1,10 - 菲啰啉检测Fe3 +存在下的Fe2 +。将测定混合物在60℃加热1小时以加速显色,随后在510nm处测量吸光度。在0.16至60μM的2,3 - 二羟基苯甲酸范围内符合比尔 - 朗伯定律。与阿诺硝化法相比,该测定法响应性更强,灵敏度约高七倍,并且对3位和4位取代的儿茶酚有效。该方法对DL - 多巴、L - 多巴胺、(±) - 肾上腺素和DL - 去甲肾上腺素等儿茶酚给出阳性结果。抗坏血酸和对二醇能很快显色,而间二醇则难以检测。羟氨基和异羟肟酸化合物的反应活性较低。酚类、巯基、吲哚基和醌基衍生物不干扰该反应。该方法已适用于测定在不同铁浓度下生长的细菌细胞培养基中的儿茶酚化合物。

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