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荧光假单胞菌的芳基乙腈酶和木薯的(S)-氧腈酶在毕赤酵母中的共表达用于(S)-扁桃酸的合成。

Simultaneous expression of an arylacetonitrilase from Pseudomonas fluorescens and a (S)-oxynitrilase from Manihot esculenta in Pichia pastoris for the synthesis of (S)-mandelic acid.

作者信息

Rustler Sven, Motejadded Hassan, Altenbuchner Josef, Stolz Andreas

机构信息

Institut für Mikrobiologie, Universität Stuttgart, Allmandring 31, Stuttgart, Germany.

出版信息

Appl Microbiol Biotechnol. 2008 Aug;80(1):87-97. doi: 10.1007/s00253-008-1531-1. Epub 2008 Jun 4.

DOI:10.1007/s00253-008-1531-1
PMID:18523765
Abstract

The arylacetonitrilase of Pseudomonas fluorescens EBC191 catalyzes the conversion of (S)-mandelonitrile to (S)-mandelic acid and (S)-mandeloamide. This biotransformation is optimally performed under acidic pH values because (S)-mandelonitrile rapidly decomposes under neutral conditions. Therefore, the gene encoding the arylacetonitrilase of P. fluorescens EBC191 was integrated and expressed under the control of the AOX1 promoter in the methylotrophic yeast Pichia pastoris which was supposed to act as an acidotolerant expression system. These recombinant strains hydrolyzed (R,S)-mandelonitrile at pH values >or=3 to mandelic acid and mandeloamide and were more acidotolerant than previously constructed Escherichia coli whole cell catalysts synthesizing the same nitrilase activity. Subsequently, recombinant P. pastoris strains were constructed which simultaneously expressed the (S)-oxynitrilase of Manihot esculenta and the arylacetonitrilase of P. fluorescens EBC191 each under the control of individual AOX1 promoters in order to obtain a whole cell catalyst for the synthesis of (S)-mandelic acid from benzaldehyde and cyanide. Resting cells of the recombinant strains converted under acidic conditions benzaldehyde and cyanide initially to mandelonitrile which was immediately converted to mandelic acid and mandeloamide. The chiral analysis of the products formed revealed a high enantiomeric excess for the (S)-enantiomers.

摘要

荧光假单胞菌EBC191的芳基乙腈酶催化(S)-扁桃腈转化为(S)-扁桃酸和(S)-扁桃酰胺。这种生物转化在酸性pH值条件下能最佳地进行,因为(S)-扁桃腈在中性条件下会迅速分解。因此,编码荧光假单胞菌EBC191芳基乙腈酶的基因在甲基营养型酵母毕赤酵母中,在AOX1启动子的控制下进行整合和表达,毕赤酵母被认为是一种耐酸表达系统。这些重组菌株在pH值≥3的条件下将(R,S)-扁桃腈水解为扁桃酸和扁桃酰胺,并且比先前构建的合成相同腈酶活性的大肠杆菌全细胞催化剂更耐酸。随后,构建了重组毕赤酵母菌株,其在各自独立的AOX1启动子控制下同时表达木薯的(S)-醇腈酶和荧光假单胞菌EBC191的芳基乙腈酶,以便获得一种用于从苯甲醛和氰化物合成(S)-扁桃酸的全细胞催化剂。重组菌株的静息细胞在酸性条件下首先将苯甲醛和氰化物转化为扁桃腈,然后扁桃腈立即被转化为扁桃酸和扁桃酰胺。对所形成产物的手性分析表明,(S)-对映体具有很高的对映体过量。

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