Department of Microbiology, Bose Institute, P-1/12 CIT Scheme VII M, Kolkata, 700054, India.
Microb Cell Fact. 2020 Mar 24;19(1):77. doi: 10.1186/s12934-020-01336-x.
Microbes are rich sources of enzymes and esterases are one of the most important classes of enzymes because of their potential for application in the field of food, agriculture, pharmaceuticals and bioremediation. Due to limitations in their cultivation, only a small fraction of the complex microbial communities can be cultured from natural habitats. Thus to explore the catalytic potential of uncultured organisms, the metagenomic approach has turned out to be an effective alternative method for direct mining of enzymes of interest. Based on activity-based screening method, an esterase-positive clone was obtained from metagenomic libraries.
Functional screening of a soil metagenomic fosmid library, followed by transposon mutagenesis led to the identification of a 1179 bp esterase gene, estM2, that encodes a 392 amino acids long protein (EstM2) with a translated molecular weight of 43.12 kDa. Overproduction, purification and biochemical characterization of the recombinant protein demonstrated carboxylesterase activity towards short-chain fatty acyl esters with optimal activity for p-nitrophenyl butyrate at pH 8.0 and 37 °C. Amino acid sequence analysis and subsequent phylogenetic analysis suggested that EstM2 belongs to the family VIII esterases that bear modest similarities to class C β-lactamases. EstM2 possessed the conserved S-x-x-K motif of class C β-lactamases but did not exhibit β-lactamase activity. Guided by molecular docking analysis, EstM2 was shown to hydrolyze a wide range of di- and monoesters of alkyl-, aryl- and benzyl-substituted phthalates. Thus, EstM2 displays an atypical hydrolytic potential of biotechnological significance within family VIII esterases.
This study has led to the discovery of a new member of family VIII esterases. To the best of our knowledge, this is the first phthalate hydrolase (EstM2), isolated from a soil metagenomic library that belongs to a family possessing β-lactamase like catalytic triad. Based on its catalytic potential towards hydrolysis of both phthalate diesters and phthalate monoesters, this enzyme may find use to counter the growing pollution caused by phthalate-based plasticizers in diverse geological environment and in other aspects of biotechnological applications.
微生物是丰富的酶源,酯酶是最重要的酶类之一,因为它们具有在食品、农业、制药和生物修复等领域应用的潜力。由于其培养的局限性,只能从自然栖息地培养出复杂微生物群落的一小部分。因此,为了探索未培养生物的催化潜力,宏基因组方法已成为直接挖掘感兴趣酶的有效替代方法。基于基于活性的筛选方法,从宏基因组文库中获得了一个酯酶阳性克隆。
对土壤宏基因组 fosmid 文库进行功能筛选,然后进行转座子诱变,鉴定出一个 1179bp 的酯酶基因 estM2,该基因编码一个 392 个氨基酸长的蛋白质(EstM2),其翻译分子量为 43.12kDa。重组蛋白的大量表达、纯化和生化特性表明,该酶对短链脂肪酸酯具有羧酸酯酶活性,在 pH8.0 和 37°C 时对 p-硝基苯丁酸的活性最佳。氨基酸序列分析和随后的系统发育分析表明,EstM2 属于家族 VIII 酯酶,与 C 类β-内酰胺酶有一定的相似性。EstM2 具有 C 类β-内酰胺酶的保守 S-x-x-K 基序,但没有表现出β-内酰胺酶活性。通过分子对接分析指导,表明 EstM2 能够水解多种烷基、芳基和苄基取代的邻苯二甲酸的二酯和单酯。因此,EstM2 在家族 VIII 酯酶中表现出一种非典型的具有生物技术意义的水解潜力。
本研究发现了一种新的家族 VIII 酯酶成员。据我们所知,这是第一个从土壤宏基因组文库中分离出的属于具有β-内酰胺酶样催化三联体的邻苯二甲酸酯水解酶(EstM2)。基于其对邻苯二甲酸二酯和邻苯二甲酸单酯水解的催化潜力,该酶可能在不同地质环境和生物技术应用的其他方面用于对抗由邻苯二甲酸酯类增塑剂造成的日益严重的污染。
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