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用于被转录后修饰酶识别的tRNA的替代三级结构。

Alternative tertiary structure of tRNA for recognition by a posttranscriptional modification enzyme.

作者信息

Ishitani Ryuichiro, Nureki Osamu, Nameki Nobukazu, Okada Norihiro, Nishimura Susumu, Yokoyama Shigeyuki

机构信息

Department of Biophysics and Biochemistry, Graduate School of Science, University of Tokyo, Hongo, Bunkyo-ku, Tokyo 113-0033, Japan.

出版信息

Cell. 2003 May 2;113(3):383-94. doi: 10.1016/s0092-8674(03)00280-0.

Abstract

Transfer RNA (tRNA) canonically has the clover-leaf secondary structure with the acceptor, D, anticodon, and T arms, which are folded into the L-shaped tertiary structure. To strengthen the L form, posttranscriptional modifications occur on nucleotides buried within the core, but the modification enzymes are paradoxically inaccessible to them in the L form. In this study, we determined the crystal structure of tRNA bound with archaeosine tRNA-guanine transglycosylase, which modifies G15 of the D arm in the core. The bound tRNA assumes an alternative conformation ("lambda form") drastically different from the L form. All of the D-arm secondary base pairs and the canonical tertiary interactions are disrupted. Furthermore, a helical structure is reorganized, while the rest of the D arm is single stranded and protruded. Consequently, the enzyme precisely locates the exposed G15 in the active site, by counting the nucleotide number from G1 to G15 in the lambda form.

摘要

转运RNA(tRNA)通常具有带有受体臂、D臂、反密码子臂和T臂的三叶草形二级结构,这些臂折叠成L形三级结构。为了强化L形结构,转录后修饰发生在核心区域内埋藏的核苷酸上,但矛盾的是,修饰酶在L形结构中无法接近这些核苷酸。在本研究中,我们确定了与古氨酰tRNA-鸟嘌呤转糖基酶结合的tRNA的晶体结构,该酶修饰核心区域D臂上的G15。结合的tRNA呈现出与L形结构截然不同的另一种构象(“λ形”)。所有D臂二级碱基对和典型的三级相互作用均被破坏。此外,一个螺旋结构被重新组织,而D臂的其余部分是单链且突出的。因此,该酶通过在λ形结构中从G1到G15计数核苷酸数量,精确地将暴露的G15定位在活性位点。

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