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肽合成酶中的ATP结合:通过用2-叠氮基三磷酸腺苷对短杆菌酪肽合成酶1进行光亲和标记来确定腺嘌呤部分的接触位点。

ATP binding in peptide synthetases: determination of contact sites of the adenine moiety by photoaffinity labeling of tyrocidine synthetase 1 with 2-azidoadenosine triphosphate.

作者信息

Pavela-Vrancic M, Pfeifer E, van Liempt H, Schäfer H J, von Döhren H, Kleinkauf H

机构信息

Institut für Biochemie und Molekulare Biologie, Technische Universität Berlin, FRG.

出版信息

Biochemistry. 1994 May 24;33(20):6276-83. doi: 10.1021/bi00186a030.

DOI:10.1021/bi00186a030
PMID:8193142
Abstract

Characterization of the nucleotide binding domain in peptide synthetases was approached by photoaffinity labeling of tyrocidine synthetase 1 (TY1) with 2-azidoadenosine triphosphate (2-azido-ATP). Exposure of TY1 in the presence of photolabel to irradiation with ultraviolet light resulted in a time-dependent covalent modification of the enzyme with a concomitant loss of catalytic activity. Inactivation was not observed if incubation was performed in the absence of either light or the nucleotide analogue. Specificity of labeling was indicated by the ability of 2-azido-ATP to serve as a substrate in the amino acid activation reaction. The modified protein was subjected to tryptic digestion, and the fragments labeled by the nucleotide analogue were purified by reverse-phase high-performance liquid chromatography. Sequence analysis identified three tryptic peptides corresponding to residues G373-K384, W405-R416, and L483-K494, derived from the N-terminal half of the TY1 sequence. As this region shows similarity to strongly conserved regions in other peptide synthetases and acyl-CoA synthetases, it is considered to be the region catalyzing aminoacyl adenylate formation. The identified sequences appear to define components of the nucleotide binding domain found in close proximity to the adenine ring in ATP. Conservation of primary structure and homology to other carboxyl-activating enzymes of this superfamily, including peptide synthetases, insect luciferases, and acyl-CoA synthetases, is discussed.

摘要

通过用2-叠氮基三磷酸腺苷(2-azido-ATP)对短杆菌酪肽合成酶1(TY1)进行光亲和标记,来研究肽合成酶中核苷酸结合结构域的特性。在光标记存在的情况下,用紫外线照射TY1,会导致该酶发生时间依赖性的共价修饰,同时催化活性丧失。如果在没有光或核苷酸类似物的情况下进行孵育,则未观察到失活现象。2-叠氮基-ATP作为氨基酸活化反应底物的能力表明了标记的特异性。将修饰后的蛋白质进行胰蛋白酶消化,并用反相高效液相色谱法纯化被核苷酸类似物标记的片段。序列分析鉴定出三个对应于G373-K384、W405-R416和L483-K494残基的胰蛋白酶肽段,它们来自TY1序列的N端一半。由于该区域与其他肽合成酶和酰基辅酶A合成酶中高度保守的区域相似,因此被认为是催化氨酰腺苷酸形成的区域。所鉴定的序列似乎定义了在ATP中靠近腺嘌呤环处发现的核苷酸结合结构域的组成部分。讨论了该超家族其他羧基活化酶(包括肽合成酶、昆虫荧光素酶和酰基辅酶A合成酶)的一级结构保守性和同源性。

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