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用于腈水解酶产生菌的新型灵敏高通量筛选策略。

Novel sensitive high-throughput screening strategy for nitrilase-producing strains.

作者信息

Zhu Qing, Fan Ao, Wang Yuanshan, Zhu Xiaoqin, Wang Zhao, Wu Minghuo, Zheng Yuguo

机构信息

Institute of Bioengineering, Zhejiang University of Technology (Chaohui Campus), Hangzhou 310014, China.

出版信息

Appl Environ Microbiol. 2007 Oct;73(19):6053-7. doi: 10.1128/AEM.01089-07. Epub 2007 Aug 3.

Abstract

Nitrilases have found wide use in the pharmaceutical industry for the production of fine chemicals, and it is important to have a method by which to screen libraries of isolated or engineered nitrilase variants (including bacteria and fungi). The conventional methods, such as high-performance liquid chromatography, liquid chromatography-mass spectrometry, capillary electrophoresis, or gas chromatography, are tedious and time-consuming. Therefore, a direct and sensitive readout of the nitrilase's activity has to be considered. In this paper, we report a novel time-resolved luminescent probe: o-hydroxybenzonitrile derivatives could be applied to detect the activity of the nitrilases. By the action of nitrilases, o-hydroxybenzonitrile derivatives can be transformed to the corresponding salicylic acid derivatives, which, upon binding Tb(3+), serve as a photon antenna and sensitize Tb(3+) luminescence. Because of the time-resolved property of the luminescence, the background from the other proteins (especially in the fermentation system) in the assay could be reduced and, therefore, the sensitivity was increased. Moreover, because the detection was performed on a 96- or 384-well plate, the activity of the nitrilases from microorganisms could be determined quickly. Based on this strategy, the best fermentation conditions for nitrilase-producing strains were obtained.

摘要

腈水解酶在制药工业中已被广泛用于精细化学品的生产,因此拥有一种筛选分离或工程化腈水解酶变体文库(包括细菌和真菌)的方法很重要。传统方法,如高效液相色谱法、液相色谱 - 质谱法、毛细管电泳法或气相色谱法,既繁琐又耗时。因此,必须考虑一种直接且灵敏的腈水解酶活性读出方法。在本文中,我们报道了一种新型的时间分辨发光探针:邻羟基苯甲腈衍生物可用于检测腈水解酶的活性。通过腈水解酶的作用,邻羟基苯甲腈衍生物可转化为相应的水杨酸衍生物,后者在与Tb(3+)结合后,作为光子天线并敏化Tb(3+)发光。由于发光的时间分辨特性,可降低测定中其他蛋白质(尤其是在发酵系统中)产生的背景,从而提高灵敏度。此外,由于检测是在96孔或384孔板上进行的,因此可以快速测定微生物腈水解酶的活性。基于此策略,获得了产腈水解酶菌株的最佳发酵条件。

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