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应用原位生成苯乙醛的酶法测定对醛脱氢酶的表征

Characterization of Aldehyde Dehydrogenases Applying an Enzyme Assay with In Situ Formation of Phenylacetaldehydes.

作者信息

Zimmerling Juliane, Tischler Dirk, Großmann Carolin, Schlömann Michael, Oelschlägel Michel

机构信息

Interdisciplinary Ecological Center, Environmental Microbiology Group, TU Bergakademie Freiberg, Leipziger Str. 29, 09599, Freiberg, Germany.

出版信息

Appl Biochem Biotechnol. 2017 Jul;182(3):1095-1107. doi: 10.1007/s12010-016-2384-1. Epub 2017 Jan 6.

Abstract

Herein, different dehydrogenases (DH) were characterized by applying a novel two-step enzyme assay. We focused on the NAD(P)-dependent phenylacetaldehyde dehydrogenases because they produce industrially relevant phenylacetic acids, but they are not well studied due to limited substrate availability. The first assay step comprises a styrene oxide isomerase (440 U mg) which allows the production of pure phenylacetaldehydes (>70 mmol L) from commercially available styrene oxides. Thereafter, a DH of interest can be added to convert phenylacetaldehydes in a broad concentration range (0.05 to 1.25 mmol L). DH activity can be determined spectrophotometrically by following cofactor reduction or alternatively by RP-HPLC. This assay allowed the comparison of four aldehyde dehydrogenases and even of an alcohol dehydrogenase with respect to the production of phenylacetic acids (up to 8.4 U mg). FeaB derived from Escherichia coli K-12 was characterized in more detail, and for the first time, substituted phenylacetaldehydes had been converted. With this enzyme assay, characterization of dehydrogenases is possible although the substrates are not commercially available in sufficient quality but enzymatically producible. The advantages of this assay in comparison to the former one are discussed.

摘要

在此,通过应用一种新型的两步酶分析法对不同的脱氢酶(DH)进行了表征。我们关注的是依赖烟酰胺腺嘌呤二核苷酸(磷酸)的苯乙醛脱氢酶,因为它们能产生具有工业相关性的苯乙酸,但由于底物可用性有限,对其研究并不充分。分析的第一步包括一种环氧苯乙烯异构酶(440 U mg),它能从市售的环氧苯乙烯中生成纯的苯乙醛(>70 mmol L)。此后,可以加入感兴趣的脱氢酶,以在较宽的浓度范围(0.05至1.25 mmol L)内转化苯乙醛。脱氢酶活性可以通过监测辅因子还原反应利用分光光度法测定,或者通过反相高效液相色谱法测定。该分析方法能够比较四种醛脱氢酶,甚至一种醇脱氢酶在苯乙酸生成方面的情况(高达8.4 U mg)。对源自大肠杆菌K - 12的FeaB进行了更详细的表征,并且首次实现了对取代苯乙醛的转化。通过这种酶分析法,尽管底物无法以足够的质量从商业途径获取,但可通过酶促反应生成时,仍能够对脱氢酶进行表征。讨论了该分析方法相较于前一种方法的优势。

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