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丙氨酰 - tRNA合成酶晶体结构及用于受体茎识别的设计

Alanyl-tRNA synthetase crystal structure and design for acceptor-stem recognition.

作者信息

Swairjo Manal A, Otero Francella J, Yang Xiang-Lei, Lovato Martha A, Skene Robert J, McRee Duncan E, Ribas de Pouplana Lluis, Schimmel Paul

机构信息

Skaags Institute for Chemical Biology, Departments of Molecular Biology and Chemistry, The Scripps Research Institute, BCC-379, 10550 North Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

Mol Cell. 2004 Mar 26;13(6):829-41. doi: 10.1016/s1097-2765(04)00126-1.

Abstract

Early work on aminoacylation of alanine-specific tRNA (tRNA(Ala)) by alanyl-tRNA synthetase (AlaRS) gave rise to the concept of an early "second genetic code" imbedded in the acceptor stems of tRNAs. A single conserved and position-specific G:U base pair in the tRNA acceptor stem is the key identity determinant. Further understanding has been limited due to lack of a crystal structure of the enzyme. We determined a 2.14 A crystal structure of the 453 amino acid catalytic fragment of Aquifex aeolicus AlaRS. It contains the catalytic domain characteristic of class II synthetases, a helical domain with a hairpin motif critical for acceptor-stem recognition, and a C-terminal domain of a mixed alpha/beta fold. Docking of tRNA(Ala) on AlaRS shows critical contacts with the three domains, consistent with previous mutagenesis and functional data. It also suggests conformational flexibility within the C domain, which might allow for the positional variation of the key G:U base pair seen in some tRNA(Ala)s.

摘要

早期关于丙氨酰 - tRNA合成酶(AlaRS)对丙氨酸特异性tRNA(tRNA(Ala))进行氨酰化的研究催生了一个概念,即一种早期的“第二遗传密码”嵌入在tRNA的受体茎中。tRNA受体茎中一个单一的保守且位置特异的G:U碱基对是关键的识别决定因素。由于缺乏该酶的晶体结构,进一步的了解受到了限制。我们确定了嗜热栖热菌AlaRS的453个氨基酸催化片段的2.14 Å晶体结构。它包含II类合成酶特有的催化结构域、一个对受体茎识别至关重要的具有发夹基序的螺旋结构域以及一个混合α/β折叠的C末端结构域。将tRNA(Ala)对接在AlaRS上显示出与这三个结构域的关键接触,这与先前的诱变和功能数据一致。它还表明C结构域内存在构象灵活性,这可能允许在一些tRNA(Ala)中看到的关键G:U碱基对的位置变化。

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