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高通量筛选定向进化的氨基香豆素酰胺合成酶。

A high-throughput screen for directed evolution of aminocoumarin amide synthetases.

机构信息

Department of Chemistry, North Carolina State University, Raleigh, NC 27695, USA.

出版信息

Anal Biochem. 2011 Dec 1;419(1):61-6. doi: 10.1016/j.ab.2011.07.037. Epub 2011 Aug 6.

Abstract

The biosynthesis of aminocoumarin antibiotics involves the action of amide synthetases which construct amide bonds between aminocoumarins and various acyl moieties. Libraries of aminocoumarin analogues have been generated by in vivo fermentation, via feeding known amide synthetase substrates into producing microbial strains. Critically, such feeding studies rely on the inherent or engineered substrate promiscuity of each amide synthetase. We have initiated a program of directed evolution in order to create mutant amide synthetases for the synthesis of new nonnatural amino coumarin analogues. We used the clorobiocin enzyme CloL as a model amide synthetase to design and validate a fluorimetric high-throughput screen, which can be used to report the activity of mutant amide synthetases toward a broad range of coumarin and acyl donor substrates. Our assay monitors the decrease in fluorescence of aminocoumarins on acylation. The utility of the assay was illustrated by screening a library of amide synthetase mutants created by error-prone PCR. The substrate specificity of an amide synthetase was also rapidly probed using this assay, affording several newly identified substrates. It is anticipated that this high-throughput screen will accelerate the creation of amide synthetase mutants with new specificities by directed evolution.

摘要

氨基香豆素抗生素的生物合成涉及酰胺合成酶的作用,酰胺合成酶在氨基香豆素和各种酰基部分之间构建酰胺键。通过向产生微生物菌株中添加已知的酰胺合成酶底物,已经通过体内发酵生成了氨基香豆素类似物文库。至关重要的是,这种喂养研究依赖于每种酰胺合成酶固有的或工程化的底物广谱性。我们已经启动了一个定向进化计划,以创建用于合成新的非天然氨基酸香豆素类似物的突变型酰胺合成酶。我们使用氯罗菌素酶 CloL 作为模型酰胺合成酶来设计和验证一种荧光高通量筛选方法,该方法可用于报告突变型酰胺合成酶对广泛的香豆素和酰基供体底物的活性。我们的测定通过监测酰化过程中氨基香豆素的荧光减弱来监测。易错 PCR 产生的酰胺合成酶突变文库的筛选说明了该测定的实用性。该测定还快速探测了酰胺合成酶的底物特异性,提供了几种新鉴定的底物。预计这种高通量筛选将通过定向进化加速具有新特异性的酰胺合成酶突变体的创建。

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