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Evolution of an acylase active on cephalosporin C

机译:对头孢菌素C有活性的酰基转移酶的进化

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摘要

Semisynthetic cephalosporins are synthesized from 7-amino cephalosporanic acid, which is produced by chemical deacylation or by a two-step enzymatic process of the natural antibiotic cephalosporin C. The known acylases take glutaryl-7-amino cephalosporanic acid as a primary substrate, and their specificity and activity are too low for cephalosporin C. Starting from a known glutaryl-7-amino cephalosporanic acid acylase as the protein scaffold, an acylase gene optimized for expression in Escherichia coli and for molecular biology manipulations was designed. Subsequently we used error-prone PCR mutagenesis, a molecular modeling approach combined with site-saturation mutagenesis, and site-directed mutagenesis to produce enzymes with a cephalosporin C/glutaryl-7-amino cephalosporanic acid catalytic efficiency that was increased up to 100-fold, and with a significant and higher maximal activity on cephalosporin C as compared to glutaryl-7-amino cephalosporanic acid (e.g., 3.8 vs. 2.7 U/mg protein, respectively, for the A215Y-H296S-H309S mutant). Our data in a bioreactor indicate an ~90% conversion of cephalosporin C to 7-amino-cephalosporanic acid in a single deacylation step. The evolved acylase variants we produced are enzymes with a new substrate specificity, not found in nature, and represent a hallmark for industrial production of 7-amino cephalosporanic acid.
机译:半合成的头孢菌素是由7-氨基头孢菌素酸合成的,它是通过化学脱酰作用或通过天然抗生素头孢菌素C的两步酶促过程制得的。已知的酰基转移酶以戊二酰-7-氨基头孢菌素酸为主要底物,对头孢菌素C的特异性和活性太低。从已知的戊二酰7-氨基头孢菌酸酰基转移酶作为蛋白质支架,设计了一种在大肠杆菌中表达和分子生物学操作优化的酰基转移酶基因。随后,我们使用易于出错的PCR诱变,分子建模方法与位点饱和诱变相结合,并进行定点诱变,以产生具有头孢菌素C /戊二酰-7-氨基头孢烷酸催化效率提高到100倍的酶与戊二酰基-7-氨基头孢菌酸相比,对头孢菌素C具有显着更高的最大活性(例如,A215Y-H296S-H309S突变体分别为3.8 vs. 2.7 U / mg蛋白)。我们在生物反应器中的数据表明,在单个脱酰步骤中,约90%的头孢菌素C转化为7-氨基-头孢菌酸。我们生产的进化的酰基转移酶是具有自然界中未发现的具有新底物特异性的酶,代表了工业生产7-氨基头孢烷酸的标志。

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