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细菌特有的摆动修饰酶TilS的远端结构域有助于催化作用。

Distal Domains of the Bacterial-Exclusive Wobble-Modifying Enzyme TilS Contribute to Catalysis.

作者信息

Guinto Ferdiemar C, Robinson Samantha C, Alexander Rebecca W

机构信息

Department of Chemistry and Center for Molecular Signaling, Wake Forest University, Winston-Salem, North Carolina 27109, United States.

出版信息

ACS Omega. 2025 Mar 14;10(11):11618-11626. doi: 10.1021/acsomega.5c00897. eCollection 2025 Mar 25.

Abstract

tRNA lysidine synthetase (TilS) is a bacterial-specific wobble-modifying enzyme that acts on the isoleucine-accepting tRNA . TilS installs a lysine at the C34 position of the anticodon, generating the lysidine modification. The resulting LAU anticodon enables exclusive decoding of infrequently used AUA isoleucine codons, rejecting AUG methionine codons. Compared to other wobble-modifying enzymes that contact only the anticodon arm of their cognate tRNAs, TilS is distinct in containing additional domains outside of the N-terminal active site. For type I TilS enzymes such as the TilS (BcTilS) investigated here, appended domains contact the tRNA substrate along the body and through the acceptor stem, up to 60 Å away from the target C34. Among bacterial tRNAs, only unmodified tRNA and tRNA share an anticodon, suggesting that the appended domains of TilS provide substrate recognition strategies that other wobble-modifying enzymes do not need. Here, we investigate both protein and tRNA elements to understand the strategy by which TilS accepts its cognate tRNA substrate and rejects the near-cognate tRNA.

摘要

tRNA赖氨酸合成酶(TilS)是一种细菌特有的摆动修饰酶,作用于异亮氨酸接受tRNA。TilS在反密码子的C34位置安装一个赖氨酸,产生赖氨酸修饰。由此产生的LAU反密码子能够专一性解码不常用的AUA异亮氨酸密码子,而排斥AUG甲硫氨酸密码子。与其他仅接触同源tRNA反密码子臂的摆动修饰酶相比,TilS的独特之处在于其在N端活性位点之外还含有其他结构域。对于此处研究的I型TilS酶,如BcTilS,附加结构域沿着tRNA主体并通过受体茎与tRNA底物接触,距离目标C34可达60埃。在细菌tRNA中,只有未修饰的tRNA和tRNA共享一个反密码子,这表明TilS的附加结构域提供了其他摆动修饰酶不需要的底物识别策略。在此,我们研究蛋白质和tRNA元件,以了解TilS接受其同源tRNA底物并排斥近同源tRNA的策略。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7406/11947777/eb68a2504b09/ao5c00897_0001.jpg

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