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转运RNA的T臂是转运RNA(5-甲基尿苷54)-甲基转移酶的底物。

The T-arm of tRNA is a substrate for tRNA (m5U54)-methyltransferase.

作者信息

Gu X R, Santi D V

机构信息

Department of Biochemistry, University of California, San Francisco 94143.

出版信息

Biochemistry. 1991 Mar 26;30(12):2999-3002. doi: 10.1021/bi00226a003.

Abstract

Fragments of Escherichia coli FUra-tRNA(1Val) as small as 15 nucleotides form covalent complexes with tRNA (m5U54)-methyltransferase (RUMT). The sequence essential for binding includes position 52 of the T-stem and the T-loop and extends toward the 3' acceptor end of FUra-tRNA. The in vitro synthesized 17mer T-arm of E. coli tRNA(1Val), composed of the seven-base T-loop and 5-base-pair stem, is a good substrate for RUMT. The Km is decreased 5-fold and kcat is decreased 2-fold compared to the entire tRNA. The T-arm structure could be further reduced to an 11mer containing the loop and two base pairs and still retain activity; the Km was similar to that of the 17mer T-arm, whereas kcat was decreased an additional 20-fold. The data indicate that the primary specificity determinants for the RUMT-tRNA interaction are contained within the primary and secondary structure of the T-arm of tRNA.

摘要

小至15个核苷酸的大肠杆菌FUra - tRNA(1Val)片段可与tRNA (m5U54)-甲基转移酶(RUMT)形成共价复合物。结合所必需的序列包括T茎环的第52位,并向FUra - tRNA的3'受体末端延伸。体外合成的大肠杆菌tRNA(1Val)的17聚体T臂,由7个碱基的T环和5个碱基对的茎组成,是RUMT的良好底物。与整个tRNA相比,Km降低了5倍,kcat降低了2倍。T臂结构可进一步简化为包含环和两个碱基对的11聚体,仍保留活性;Km与17聚体T臂相似,而kcat又降低了20倍。数据表明,RUMT与tRNA相互作用的主要特异性决定因素包含在tRNA T臂的一级和二级结构中。

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