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[马蓝及其他78种植物中分支酸合酶的生物信息分析]

[Bioinformation analysis of chorismate synthase in Baphicacantus cusia and other 78 species of plants].

作者信息

Yu Jian, Ye Qi, Ning Shu-Ju, Li Qing, Tan He-Xin, Feng Jing-Xian, Chen Rui-Bing, Ma Xiao-Li, Gong Pei-Min, Zhao Xuan-Xuan, Zhang Lei, Wei Dao-Zhi

机构信息

College of Life Science, Fujian Agriculture and Forestry University, Fuzhou 350002, China.

Fujian Provincial Key Laboratory of Agroecological Processing and Safety Monitoring, Fuzhou 350002, China.

出版信息

Zhongguo Zhong Yao Za Zhi. 2018 Feb;43(4):721-730. doi: 10.19540/j.cnki.cjcmm.20180105.002.

Abstract

Chorismate synthase(CS, EC:4.2.3.5) catalyses 5-enolpyruvy-shikimate-3-phosphate to form chorismate, which is the essential enzyme for chorismate biosynthesis in organisms. The amino acid sequences of CS from 79 species of higher plants were reported in GenBank at present. 125 amino acid sequences of CS from Baphicacanthus cusia and other 78 species of plants were predicted and analyzed by using various bioinformatics software, including the composition of amino acid sequences, signal peptide, leader peptide, hydrophobic/hydrophilic, transmembrane structure, coiled-coil domain, protein secondary structure, tertiary structure and functional domains. The phylogenetic tree of CS protein family was constructed and divided into eight groups by phylogenetic analysis. The homology comparison indicated that B. cusia shared a high homology with several plants such as Sesamum indicum, Nicotiana tabacum, Solanum tuberosum and so on. The open reading frame(ORF) of all samples is about 1 300 bp, the molecular weight is about 50 kDa, the isoelectric point(pI) is 5.0-8.0 which illustrated that CS protein is slightly basic. The ORF of CS we cloned in B. cusia is 1 326 bp, the amino acid residues are 442, the molecular weight is 47 kDa and pI is 8.11. The CS in B.cusia showed obvious hydrophobicity area and hydrophilicity area, no signal peptide, and may exists transmembrane structure areas. The main secondary structures of CS protein are random coil and Alpha helix, also contain three main structural domains which are an active structural domain, a PLN02754 conserved domain and a FMN binding site. The acquired information in this study would provide certain scientific basis for further study on structure-activity relationship and structure modification of CS in plants in the future.

摘要

分支酸合酶(CS,EC:4.2.3.5)催化5-烯醇丙酮酸莽草酸-3-磷酸形成分支酸,它是生物体中分支酸生物合成的关键酶。目前GenBank中已报道了79种高等植物的CS氨基酸序列。利用多种生物信息学软件对马蓝及其他78种植物的125条CS氨基酸序列进行了预测和分析,包括氨基酸序列组成、信号肽、前导肽、疏水/亲水性、跨膜结构、卷曲螺旋结构域、蛋白质二级结构、三级结构和功能结构域。构建了CS蛋白家族的系统发育树,并通过系统发育分析将其分为八组。同源性比较表明,马蓝与芝麻、烟草、马铃薯等多种植物具有较高的同源性。所有样本的开放阅读框(ORF)约为1300 bp,分子量约为50 kDa,等电点(pI)为5.0 - 8.0,表明CS蛋白略显碱性。我们克隆的马蓝CS的ORF为1326 bp,氨基酸残基为442个,分子量为47 kDa,pI为8.11。马蓝中的CS表现出明显的疏水区和亲水区,无信号肽,可能存在跨膜结构区域。CS蛋白的主要二级结构为无规卷曲和α螺旋,还包含三个主要结构域,即一个活性结构域、一个PLN02754保守结构域和一个FMN结合位点。本研究获得的信息将为今后进一步研究植物中CS的构效关系和结构修饰提供一定的科学依据。

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