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大肠杆菌甲硫氨酰 - tRNA甲酰转移酶16个氨基酸插入模块中保守的精氨酸与起始tRNA中进行甲酰化的决定因素之间的功能相互作用。

Functional interaction of an arginine conserved in the sixteen amino acid insertion module of Escherichia coli methionyl-tRNA formyltransferase with determinants for formylation in the initiator tRNA.

作者信息

Ramesh V, Gite S, RajBhandary U L

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge 02139, USA.

出版信息

Biochemistry. 1998 Nov 10;37(45):15925-32. doi: 10.1021/bi981873x.

DOI:10.1021/bi981873x
PMID:9843398
Abstract

Formylation of initiator methionyl-tRNA by methionyl-tRNA formyltransferase (MTF) is important for initiation of protein synthesis in eubacteria. The determinants for formylation are clustered mostly in the acceptor stem of the initiator tRNA. Previous studies suggested that a 16 amino acid insertion loop, present in all eubacterial MTF's (residues 34-49 in the E. coli enzyme), plays an important role in specific recognition of the initiator tRNA. Here, we have analyzed the effect of site-specific mutations of amino acids within this region. We show that an invariant arginine at position 42 within the loop plays a very important role both in the steps of substrate binding and in catalysis. The kinetic parameters of the R42K and R42L mutant enzymes using acceptor stem mutant initiator tRNAs as substrates suggest that arginine 42 makes functional contacts with the determinants at the 3:70 and possibly also the 2:71 base pairs in the acceptor stem of the initiator tRNA. The kinetic parameters of the G41R/R42L double mutant enzyme are essentially the same as those of R42L mutant, suggesting that the requirement for arginine at position 42 cannot be fulfilled by an arginine at position 41. Along with other data, this result suggests that the insertion loop, which is normally unstructured and flexible, adopts a defined conformation upon binding to the tRNA.

摘要

甲硫氨酰 - tRNA甲酰基转移酶(MTF)对起始甲硫氨酰 - tRNA的甲酰化作用对于真细菌中蛋白质合成的起始至关重要。甲酰化的决定因素大多集中在起始tRNA的受体茎中。先前的研究表明,所有真细菌MTF中都存在的一个16个氨基酸的插入环(大肠杆菌酶中的第34 - 49位残基)在起始tRNA的特异性识别中起重要作用。在这里,我们分析了该区域内氨基酸位点特异性突变的影响。我们发现,环内第42位的一个不变精氨酸在底物结合步骤和催化过程中都起着非常重要的作用。使用受体茎突变起始tRNA作为底物的R42K和R42L突变酶的动力学参数表明,精氨酸42与起始tRNA受体茎中3:70以及可能还有2:71碱基对处的决定因素进行功能性接触。G41R/R42L双突变酶的动力学参数与R42L突变酶基本相同,这表明第42位对精氨酸的需求不能由第41位的精氨酸来满足。连同其他数据,该结果表明,通常无结构且灵活的插入环在与tRNA结合时会采取确定的构象。

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