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一种细菌氨酰-tRNA合成酶和一种家蚕氨酰-tRNA合成酶具有一个共同的表位,该表位定位于各自的催化结构域。

A bacterial and silkworm aminoacyl-tRNA synthetase have a common epitope which maps to the catalytic domain of each.

作者信息

Regan L, Dignam J D, Schimmel P

出版信息

J Biol Chem. 1986 Apr 25;261(12):5241-4.

PMID:2420799
Abstract

We report here the identification of a common immunological determinant in Escherichia coli and Bombyx mori (silkworm) alanine tRNA synthetases. The E. coli protein is a tetramer of identical Mr = 95,000 chains, and the silkworm enzyme is a monomer of Mr = 115,000. Antibodies against the silkworm enzyme react with E. coli Ala-tRNA synthetase. Analysis of 10 fragments of the E. coli enzyme has mapped the cross-reacting epitope to between amino acids 350 and 385. This is within the part of the enzyme which is essential for alanyladenylate synthesis. The anti-B. mori Ala-tRNA synthetase antibodies which cross-react with the E. coli enzyme were affinity-purified. They react specifically with the catalytic domain of the silkworm enzyme and not with the remaining dispensable segment of 500 amino acids. The results support the concept that the core catalytic structural elements, and not the dispensable portions, are the most related among the synthetases.

摘要

我们在此报告在大肠杆菌和家蚕丙氨酸tRNA合成酶中鉴定出一种共同的免疫决定簇。大肠杆菌的该蛋白是由相同的Mr = 95,000链组成的四聚体,而家蚕的酶是Mr = 115,000的单体。抗家蚕酶的抗体与大肠杆菌丙氨酸tRNA合成酶发生反应。对大肠杆菌酶的10个片段进行分析,已将交叉反应表位定位在氨基酸350至385之间。这位于该酶中对丙氨酰腺苷酸合成至关重要的部分内。与大肠杆菌酶发生交叉反应的抗家蚕丙氨酸tRNA合成酶抗体经亲和纯化。它们与家蚕酶的催化结构域特异性反应,而不与其余500个氨基酸的可去除片段反应。结果支持了这样的概念,即合成酶之间最相关的是核心催化结构元件,而不是可去除部分。

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