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从宏基因组 DNA 文库中筛选和鉴定一种新型酯酶 EstPE。

Screening and identification of a novel esterase EstPE from a metagenomic DNA library.

机构信息

Department of Biological Sciences, College of Natural Sciences, Chonnam National University, Gwangju, 500-757, Republic of Korea.

出版信息

J Microbiol. 2011 Feb;49(1):7-14. doi: 10.1007/s12275-011-0201-7. Epub 2011 Mar 3.

Abstract

Esterases represent a large family of hydrolases with broad substrate specificity and functional sequence space. Although many attempts to screen new esterases have been conducted, there have been few reports conducted to discriminate unique enzymes from typical ones based on novel structure and function. In this study, we discovered an esterase and a novel family through a successive assay of whole cells and crude lysates (oxidative open condition). The screened putative esterases from the metagenomic DNA of salted shrimp consisted of 753 bp encoding 27 kDa of polypeptide, namely PE esterase. Sequence analyses revealed that an identical gene was reported from whole genome sequencing of Stenotrophomonas maltophilia K279a. However, its biochemical and phylogenetic characteristics have not yet been evaluated. PE esterase was overexpressed only by the MBP fusion state in E. coli and was easily purified using an affinity column. This enzyme showed a typical spectrum of substrate specificity and possessed the consensus motifs, Ser-Asp-His and GXSXG, which are essential for most esterase/lipase superfamilies. Interestingly, the entire organization of the ORF and consensus sequence around the active site were distinct from the related enzymes, and its structure could be affected by a reducing agent, DTT.

摘要

酯酶是一类具有广泛底物特异性和功能序列空间的水解酶大家族。尽管已经有许多筛选新酯酶的尝试,但很少有报道根据新的结构和功能从典型酶中区分出独特的酶。在这项研究中,我们通过全细胞和粗提物(氧化开放条件)的连续测定发现了一种酯酶和一个新家族。从腌制虾的宏基因组 DNA 中筛选出的推定酯酶由编码 27 kDa 多肽的 753 bp 组成,即 PE 酯酶。序列分析表明,在嗜麦芽寡养单胞菌 K279a 的全基因组测序中也报道了相同的基因。然而,其生化和系统发育特征尚未得到评估。PE 酯酶仅在大肠杆菌中以 MBP 融合状态过表达,并且可以使用亲和柱轻松纯化。该酶表现出典型的底物特异性谱,并具有大多数酯酶/脂肪酶超家族所必需的保守基序 Ser-Asp-His 和 GXSXG。有趣的是,ORF 的整个组织和活性位点周围的保守序列与相关酶明显不同,其结构可能受到还原剂 DTT 的影响。

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