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通过用来自大肠杆菌MC1061的抗冻融硝酸盐还原酶还原硝酸盐间接测定一氧化氮的产生。

Indirect determination of nitric oxide production by reduction of nitrate with a freeze-thawing-resistant nitrate reductase from Escherichia coli MC1061.

作者信息

Arias-Negrete Sergio, Jiménez-Romero Luis A, Solís-Martínez Martha O, Ramírez-Emiliano Joel, Avila Eva E, Cuéllar-Mata Patricia

机构信息

Instituto de Investigación en Biología Experimental, Universidad de Guanajuato, 36000 Guanajuato, Gto., Mexico.

出版信息

Anal Biochem. 2004 May 1;328(1):14-21. doi: 10.1016/j.ab.2004.01.026.

DOI:10.1016/j.ab.2004.01.026
PMID:15081902
Abstract

Preparation of a nitrate reductase lysate of Escherichia coli MC1061 to measure nitrate and nitrite in biologic fluids is described. To obtain the crude bacterial lysate containing nitrate reductase activity, E. coli MC1061 was subjected to 16-20 freeze-thawing cycles, from -70 to 60 degrees C, until nitrite reductase activity was < or = 25%. Nitrate reductase activity was detected mainly in the crude preparation. To validate the nitrate reduction procedure, standard nitrate solutions (1.6-100 microM) were incubated with the nitrate reductase preparation for 3 h at 37 degrees C, and nitrite was estimated by the Griess reaction in a microassay. Nitrate solutions were reduced to nitrite in a range of 60-70%. Importantly, no cofactors were necessary to perform nitrate reduction. The biological samples were first reduced with the nitrate reductase preparation. After centrifugation, samples were deproteinized with either methanol/ether or zinc sulfate and nitrite was quantified. The utility of the nitrate reductase preparation was assessed by nitrate+nitrite determination in serum of animals infected with the protozoan Entamoeba histolytica or the bacteria E. coli and in the supernatant of cultured lipopolysaccharide-stimulated RAW 264.7 mouse macrophages. Our results indicate that the nitrate reductase-containing lysate provides a convenient tool for the reduction of nitrate to determine nitrate+nitrite in biological fluids by spectrophotometric methods.

摘要

本文描述了制备大肠杆菌MC1061的硝酸还原酶裂解物以测定生物体液中硝酸盐和亚硝酸盐的方法。为获得含有硝酸还原酶活性的粗细菌裂解物,将大肠杆菌MC1061在-70至60摄氏度下进行16 - 20次冻融循环,直至亚硝酸还原酶活性≤25%。硝酸还原酶活性主要在粗制品中检测到。为验证硝酸还原程序,将标准硝酸盐溶液(1.6 - 100 microM)与硝酸还原酶制品在37摄氏度下孵育3小时,并用微量测定法中的格里斯反应估计亚硝酸盐。硝酸盐溶液在60 - 70%的范围内被还原为亚硝酸盐。重要的是,进行硝酸盐还原不需要辅因子。生物样品首先用硝酸还原酶制品进行还原。离心后,样品用甲醇/乙醚或硫酸锌脱蛋白,并对亚硝酸盐进行定量。通过测定感染原生动物溶组织内阿米巴或细菌大肠杆菌的动物血清以及培养的脂多糖刺激的RAW 264.7小鼠巨噬细胞上清液中的硝酸盐+亚硝酸盐,评估了硝酸还原酶制品的实用性。我们的结果表明,含硝酸还原酶的裂解物为通过分光光度法将硝酸盐还原以测定生物体液中的硝酸盐+亚硝酸盐提供了一种便捷工具。

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Indirect determination of nitric oxide production by reduction of nitrate with a freeze-thawing-resistant nitrate reductase from Escherichia coli MC1061.通过用来自大肠杆菌MC1061的抗冻融硝酸盐还原酶还原硝酸盐间接测定一氧化氮的产生。
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