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谷氨酰胺-tRNA还原酶的结构与功能,植物和原核生物中四吡咯生物合成的首个酶。

Structure and function of glutamyl-tRNA reductase, the first enzyme of tetrapyrrole biosynthesis in plants and prokaryotes.

作者信息

Schubert Wolf-Dieter, Moser Jürgen, Schauer Stefan, Heinz Dirk W, Jahn Dieter

机构信息

Department of Structural Biology, German Research Center for Biotechnology, Mascheroder Weg 1, 38104, Braunschweig, Germany.

出版信息

Photosynth Res. 2002;74(2):205-15. doi: 10.1023/A:1020963711861.

Abstract

Glutamyl-tRNA reductase (GluTR) catalyzes the first step of tetrapyrrole biosynthesis in plants, archaea and most bacteria. The catalytic mechanism of the enzyme was elucidated both by biochemical data and the determination of the high-resolution crystal structure of the enzyme from the archaeon Methanopyrus kandleri in complex with a competitive inhibitor. The dimeric enzyme has an unusual V-shaped architecture where each monomer consists of three domains linked by a long 'spinal' alpha-helix. The central catalytic domain specifically recognizes the glutamate moiety of the substrate. It bears a conserved cysteine poised to nucleophilically attack the activated aminoacyl bond of glutamyl-tRNA. Subsequently, the thioester intermediate is reduced to the product glutamate-1-semialdehyde via hydride transfer from NADPH supplied by the second domain. A structure-based sequence alignment indicates that catalytically essential amino acids are conserved throughout all GluTRs. Thus the catalytic mechanism derived for M. kandleri is common to all including plant GluTRs. Mutations described to influence the catalytic efficiency of the barley enzyme can therefore be explained.

摘要

谷氨酰胺-tRNA还原酶(GluTR)催化植物、古细菌和大多数细菌中四吡咯生物合成的第一步。通过生化数据以及对来自古细菌坎氏甲烷嗜热菌的该酶与竞争性抑制剂复合物的高分辨率晶体结构的测定,阐明了该酶的催化机制。二聚体酶具有不寻常的V形结构,其中每个单体由通过长的“脊柱状”α螺旋连接的三个结构域组成。中央催化结构域特异性识别底物的谷氨酸部分。它有一个保守的半胱氨酸,准备亲核攻击谷氨酰胺-tRNA的活化氨酰键。随后,硫酯中间体通过来自第二个结构域提供的NADPH的氢化物转移被还原为产物谷氨酸-1-半醛。基于结构的序列比对表明,催化必需氨基酸在所有GluTR中都是保守的。因此,为坎氏甲烷嗜热菌推导的催化机制对包括植物GluTR在内的所有酶都是通用的。因此,可以解释所描述的影响大麦酶催化效率的突变。

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