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[一种测定NAD依赖性氢化酶活性的生物发光方法]

[A bioluminescence method of determining the activity of NAD-dependent hydrogenase].

作者信息

Petushkov V N, Guseĭnov O A

出版信息

Prikl Biokhim Mikrobiol. 1992 Nov-Dec;28(6):907-11.

PMID:1494576
Abstract

An analytical multienzyme system composed of NAD-dependent hydrogenase of Alcaligenes eutrophus, and reductase and luciferase from luminous bacteria was studied. The rate of luminescence increase of this system was found to be proportional to hydrogenase activity. The apparent Michaelis constants for NAD and hydrogen were determined (5 and 40 microM, respectively). The pH optimum is 7.5-9.0. Over the NAD concentration range from 20 to 100 microM, the rate of luminescence increase changed by less than 10%. At higher concentrations of NAD a monotonous decreasing of the rate of luminescence increase was observed. The proposed multienzyme system can be used for measuring the hydrogenase activity and hydrogen concentration. The high sensitivity to hydrogen (0.1 nmol in sample) and to hydrogenase (0.5 mU) and specificity of the system enable its application in the development of a biosensor for rapid detection of hydrogen in a medium.

摘要

研究了一种由嗜碱假单胞菌的NAD依赖性氢化酶、发光细菌的还原酶和荧光素酶组成的分析多酶系统。发现该系统发光增加速率与氢化酶活性成正比。测定了NAD和氢气的表观米氏常数(分别为5和40 microM)。最适pH为7.5 - 9.0。在20至100 microM的NAD浓度范围内,发光增加速率变化小于10%。在较高NAD浓度下,观察到发光增加速率单调下降。所提出的多酶系统可用于测量氢化酶活性和氢气浓度。该系统对氢气(样品中0.1 nmol)和氢化酶(0.5 mU)具有高灵敏度以及特异性,使其能够应用于开发用于快速检测介质中氢气的生物传感器。

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