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一种源自渗滤液宏基因组文库的新型VIII族羧酸酯酶对头孢硝噻吩表现出混杂的β-内酰胺酶活性。

A novel family VIII carboxylesterase derived from a leachate metagenome library exhibits promiscuous beta-lactamase activity on nitrocefin.

作者信息

Rashamuse Konanani, Magomani Victoria, Ronneburg Tina, Brady Dean

机构信息

Enzyme Technologies, CSIR Biosciences, Private Bag X2, Modderfontein, Johannesburg 1645, South Africa.

出版信息

Appl Microbiol Biotechnol. 2009 Jun;83(3):491-500. doi: 10.1007/s00253-009-1895-x. Epub 2009 Feb 4.

DOI:10.1007/s00253-009-1895-x
PMID:19190902
Abstract

The realization that majority of microbes are not amenable to cultivation as isolates under laboratory conditions has led to the culture-independent metagenomic approach as a novel technique for novel biocatalyst discovery. A leachate fosmid shotgun metagenome library was constructed and subsequently screened for esterolytic activities on a tributyrin agar medium. Nucleotide sequencing and translational analysis of an esterase-positive fosmid clone led to the identification of a 1,281 bp esterase gene (estC) encoding a protein (EstC) of 427 aa with translated molecular weight of 46.3 kDa. The EstC primary structure contained a signal leader peptide (29 aa), which could be cleaved to form a mature protein of 398 aa with molecular weight 43.3 kDa. Homology searches revealed that EstC belonged to the family VIII esterases, which exploit a serine residue within the S-x-x-K motif as a catalytic nucleophile. Substrate specificity studies showed that EstC prefers short to medium acyl chain length of p-nitrophenyl esters, a characteristic typical of "true" carboxylesterases. Moreover, EstC represents the first member of the family VIII esterases with a leader peptide and a detectable promiscuous beta-lactam hydrolytic activity. Site-directed mutagenesis studies also revealed that in addition to Ser103 and Lys106 residues, the Tyr219 residue also plays a catalytic role in EstC. The organic solvent stability and the specificity towards esters of tertiary alcohols linalyl acetate (3,7-dimethyl-1,6-octadien-3-yl acetate) make EstC potentially useful in biocatalysis.

摘要

认识到大多数微生物在实验室条件下无法作为分离物进行培养,促使人们采用不依赖培养的宏基因组学方法,这是一种发现新型生物催化剂的新技术。构建了渗滤液fosmid鸟枪法宏基因组文库,随后在三丁酸甘油酯琼脂培养基上筛选酯解活性。对一个酯酶阳性的fosmid克隆进行核苷酸测序和翻译分析,鉴定出一个1281 bp的酯酶基因(estC),其编码一个427个氨基酸的蛋白质(EstC),翻译后的分子量为46.3 kDa。EstC的一级结构包含一个信号前导肽(29个氨基酸),可被切割形成一个398个氨基酸、分子量为43.3 kDa的成熟蛋白质。同源性搜索显示,EstC属于VIII族酯酶,该族酯酶利用S-x-x-K基序中的丝氨酸残基作为催化亲核试剂。底物特异性研究表明,EstC更倾向于对短至中等酰基链长度的对硝基苯酯,这是“真正的”羧酸酯酶的典型特征。此外,EstC是VIII族酯酶中第一个具有前导肽和可检测的混杂β-内酰胺水解活性的成员。定点诱变研究还表明,除了Ser103和Lys106残基外,Tyr219残基在EstC中也起催化作用。EstC的有机溶剂稳定性以及对叔醇乙酸芳樟酯(3,7-二甲基-1,6-辛二烯-3-基乙酸酯)酯的特异性使其在生物催化中具有潜在的应用价值。

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