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Modification of the universally unmodified uridine-33 in a mitochondria-imported edited tRNA and the role of the anticodon arm structure on editing efficiency.

机译:线粒体导入的编辑tRNA中普遍未修饰的尿苷33的修饰以及反密码子臂结构对编辑效率的作用。

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摘要

Editing of tRNA has a wide phylogenetic distribution among eukaryotes and in some cases serves to expand the decoding capacity of the target tRNA. We previously described C-to-U editing of the wobble position of the imported tRNA(Trp) in Leishmania mitochondria, which is essential for decoding UGA codons as tryptophan. Here we show the complete set of nucleotide modifications in the anticodon arm of the mitochondrial and cytosolic tRNA(Trp) as determined by electrospray ionization mass spectrometry. This analysis revealed extensive mitochondria-specific posttranscriptional modifications, including the first example of thiolation of U33, the "universally unmodified" uridine. In light of the known rigidity imparted on sugar conformation by thiolation, our discovery of a thiolated U33 suggests that conformational flexibility is not a universal feature of the anticodon structural signature. In addition, the in vivo analysis of tRNA(Trp) variants presented shows a single base-pair reversal in the anticodon stem of tRNA(Trp) is sufficient to abrogate editing in vivo, indicating that subtle changes in anticodon structure can have drastic effects on editing efficiency.
机译:tRNA的编辑在真核生物中具有广泛的系统发育分布,在某些情况下可用于扩展目标tRNA的解码能力。我们先前描述了导入的tRNA(Trp)在利什曼原虫线粒体中的摆动位置的C到U编辑,这对于将UGA密码子解码为色氨酸至关重要。在这里,我们显示了通过电喷雾电离质谱法测定的线粒体和胞质tRNA(Trp)的反密码子臂中的核苷酸修饰的完整集合。该分析揭示了广泛的线粒体特异性转录后修饰,包括U33硫醇化的第一个实例,即“未修饰的尿苷”。鉴于通过硫醇化赋予糖构象的刚性,我们对硫醇化的U33的发现表明,构象柔韧性不是反密码子结构特征的普遍特征。此外,对tRNA(Trp)变异体进行的体内分析显示,tRNA(Trp)反密码子茎中的单个碱基对逆转足以消除体内编辑,表明反密码子结构的细微变化可对编辑效率。

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