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鉴别器碱基堆积相互作用的重要性:A73微螺旋(丙氨酸)变体的分子动力学分析

Importance of discriminator base stacking interactions: molecular dynamics analysis of A73 microhelix(Ala) variants.

作者信息

Nagan M C, Beuning P, Musier-Forsyth K, Cramer C J

机构信息

Department of Chemistry and Supercomputer Institute, University of Minnesota, Minneapolis 55455-0431, USA.

出版信息

Nucleic Acids Res. 2000 Jul 1;28(13):2527-34. doi: 10.1093/nar/28.13.2527.

Abstract

Transfer of alanine from Escherichia coli alanyl-tRNA synthetase (AlaRS) to RNA minihelices that mimic the amino acid acceptor stem of tRNA(Ala) has been shown, by analysis of variant minihelix aminoacylation activities, to involve a transition state sensitive to changes in the 'discriminator' base at position 73. Solution NMR has indicated that this single-stranded nucleotide is predominantly stacked onto G1 of the first base pair of the alanine acceptor stem helix. We report the activity of a new variant with the adenine at position 73 substituted by its non-polar isostere 4-methylindole (M). Despite lacking N7, this analog is well tolerated by AlaRS. Molecular dynamics (MD) simulations show that the M substitution improves position 73 base stacking over G1, as measured by a stacking lifetime analysis. Additional MD simulations of wild-type microhelix(Ala) and six variants reveal a positive correlation between N73 base stacking propensity over G1 and aminoacylation activity. For the two DeltaN7 variants simulated we found that the propensity to stack over G1 was similar to the analogous variants that contain N7 and we conclude that the decrease in aminoacylation efficiency observed upon deletion of N7 is likely due to loss of a direct stabilizing interaction with the synthetase.

摘要

通过对变体小螺旋氨酰化活性的分析表明,丙氨酸从大肠杆菌丙氨酰 - tRNA合成酶(AlaRS)转移至模拟tRNA(Ala)氨基酸接受茎的RNA小螺旋的过程,涉及对73位“鉴别”碱基变化敏感的过渡态。溶液核磁共振表明,这个单链核苷酸主要堆积在丙氨酸接受茎螺旋第一个碱基对的G1上。我们报道了一个新变体的活性,该变体中73位的腺嘌呤被其非极性等排体4 - 甲基吲哚(M)取代。尽管缺乏N7,但该类似物能被AlaRS很好地耐受。分子动力学(MD)模拟表明,通过堆积寿命分析测量,M取代改善了73位碱基相对于G1的堆积。对野生型微螺旋(Ala)和六个变体的额外MD模拟揭示了73位碱基相对于G1的堆积倾向与氨酰化活性之间存在正相关。对于模拟的两个缺失N7的变体,我们发现其相对于G1的堆积倾向与含有N7的类似变体相似,并且我们得出结论,删除N7后观察到的氨酰化效率降低可能是由于与合成酶直接稳定相互作用的丧失。

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