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第10章 使用磷酸泛酰巯基乙胺基转移酶进行酶的翻译后激活、位点特异性蛋白质标记以及从细菌基因组中鉴定天然产物生物合成基因簇

Chapter 10 using phosphopantetheinyl transferases for enzyme posttranslational activation, site specific protein labeling and identification of natural product biosynthetic gene clusters from bacterial genomes.

作者信息

Sunbul Murat, Zhang Keya, Yin Jun

机构信息

Department of Chemistry, The University of Chicago, Chicago, Illinois, USA.

出版信息

Methods Enzymol. 2009;458:255-75. doi: 10.1016/S0076-6879(09)04810-1.

Abstract

Phosphopantetheinyl transferases (PPTases) covalently attach the phosphopantetheinyl group derived from coenzyme A (CoA) to acyl carrier proteins or peptidyl carrier proteins as part of the enzymatic assembly lines of fatty acid synthases (FAS), polyketide synthases (PKS), and nonribosomal peptide synthetases (NRPS). PPTases have demonstrated broad substrate specificities for cross-species modification of carrier proteins embedded in PKS or NRPS modules. PPTase Sfp from Bacillus subtilis and AcpS from Escherichia coli also transfer small molecules of diverse structures from their CoA conjugates to the carrier proteins. Short peptide tags have thus been developed as efficient substrates of Sfp and AcpS for site-specific labeling of the peptide-tagged fusion proteins with biotin or organic fluorophores. This chapter discusses the use of PPTases for in vivo and in vitro modification of PKS and NRPS enzymes and for site-specific protein labeling. We also describe a phage selection method based on PPTase-catalyzed carrier protein modification for the identification of PKS or NRPS genes from bacterial genomes.

摘要

磷酸泛酰巯基乙胺基转移酶(PPTases)将源自辅酶A(CoA)的磷酸泛酰巯基乙胺基团共价连接到酰基载体蛋白或肽基载体蛋白上,作为脂肪酸合酶(FAS)、聚酮合酶(PKS)和非核糖体肽合成酶(NRPS)酶促装配线的一部分。PPTases已证明对嵌入PKS或NRPS模块中的载体蛋白进行跨物种修饰具有广泛的底物特异性。来自枯草芽孢杆菌的PPTase Sfp和来自大肠杆菌的AcpS也将各种结构的小分子从其CoA缀合物转移到载体蛋白上。因此,短肽标签已被开发为Sfp和AcpS的有效底物,用于用生物素或有机荧光团对肽标签融合蛋白进行位点特异性标记。本章讨论了PPTases在体内和体外对PKS和NRPS酶进行修饰以及用于位点特异性蛋白质标记的用途。我们还描述了一种基于PPTase催化的载体蛋白修饰的噬菌体选择方法,用于从细菌基因组中鉴定PKS或NRPS基因。

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