从假单胞菌属 WU-0701 中鉴定参与反式乌头酸同化的顺乌头酸异构酶的酶学特性和基因。

Enzymatic characterization and gene identification of aconitate isomerase, an enzyme involved in assimilation of trans-aconitic acid, from Pseudomonas sp. WU-0701.

机构信息

Department of Applied Chemistry, Faculty of Science and Engineering, Waseda University, Shinjuku-ku, Japan.

出版信息

FEBS J. 2015 Nov;282(22):4257-67. doi: 10.1111/febs.13494. Epub 2015 Sep 12.

DOI:10.1111/febs.13494

PMID:26293748

Abstract

UNLABELLED

trans-Aconitic acid is an unsaturated organic acid that is present in some plants such as soybean and wheat; however, it remains unclear how trans-aconitic acid is degraded and/or assimilated by living cells in nature. From soil, we isolated Pseudomonas sp. WU-0701 assimilating trans-aconitic acid as a sole carbon source. In the cell-free extract of Pseudomonas sp. WU-0701, aconitate isomerase (AI; EC 5.3.3.7) activity was detected. Therefore, it seems likely that strain Pseudomonas sp. WU-0701 converts trans-aconitic acid to cis-aconitic acid with AI, and assimilates this via the tricarboxylic acid cycle. For the characterization of AI from Pseudomonas sp. WU-0701, we performed purification, determination of enzymatic properties and gene identification of AI. The molecular mass of AI purified from cell-free extract was estimated to be ~ 25 kDa by both SDS/PAGE and gel filtration analyses, indicating that AI is a monomeric enzyme. The optimal pH and temperature of purified AI for the reaction were 6.0 °C and 37 °C, respectively. The gene ais encoding AI was cloned on the basis of the N-terminal amino acid sequence of the protein, and Southern blot analysis revealed that only one copy of ais is located on the bacterial genome. The gene ais contains an ORF of 786 bp, encoding a polypeptide of 262 amino acids, including the N-terminal 22 amino acids as a putative periplasm-targeting signal peptide. It is noteworthy that the amino acid sequence of AI shows 90% and 74% identity with molybdenum ABC transporter substrate-binding proteins of Pseudomonas psychrotolerans and Xanthomonas albilineans, respectively. This is the first report on purification to homogeneity, characterization and gene identification of AI.

DATABASE

The nucleotide sequence of ais described in this article is available in the DDBJ/EMBL/GenBank nucleotide sequence databases under the Accession No. LC010980.

摘要

未标记

反丁烯二酸是一种不饱和有机酸，存在于大豆和小麦等一些植物中；然而，目前尚不清楚反丁烯二酸在自然界中是如何被活细胞降解和/或同化的。我们从土壤中分离到一株可同化反丁烯二酸作为唯一碳源的假单胞菌 sp. WU-0701。在假单胞菌 sp. WU-0701 的无细胞提取物中检测到顺乌头酸异构酶 (AI; EC 5.3.3.7) 活性。因此，似乎假单胞菌 sp. WU-0701 菌株通过 AI 将反丁烯二酸转化为顺丁烯二酸，并通过三羧酸循环同化它。为了对来自假单胞菌 sp. WU-0701 的 AI 进行表征，我们进行了 AI 的纯化、酶学性质测定和基因鉴定。通过 SDS/PAGE 和凝胶过滤分析，估计从无细胞提取物中纯化的 AI 的分子量约为 25 kDa，表明 AI 是一种单体酶。纯化的 AI 反应的最适 pH 和温度分别为 6.0°C 和 37°C。根据蛋白质的 N 末端氨基酸序列克隆了编码 AI 的 ais 基因，Southern blot 分析表明 ais 仅位于细菌基因组上的一个拷贝。ais 基因包含一个 786 bp 的 ORF，编码一个 262 个氨基酸的多肽，包括 N 末端 22 个氨基酸作为潜在的周质靶向信号肽。值得注意的是，AI 的氨基酸序列与嗜冷假单胞菌和黄单胞菌的钼 ABC 转运体底物结合蛋白分别具有 90%和 74%的同一性。这是首次对 AI 进行纯化成均相、特性鉴定和基因鉴定的报道。