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A discriminator code–based DTD surveillance ensures faithful glycine delivery for protein biosynthesis in bacteria

机译:基于区分代码的DTD监控可确保忠实地递送甘氨酸,从而实现细菌中蛋白质的生物合成

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摘要

D-aminoacyl-tRNA deacylase (DTD) acts on achiral glycine, in addition to D-amino acids, attached to tRNA. We have recently shown that this activity enables DTD to clear non-cognate Gly-tRNAAla with 1000-fold higher efficiency than its activity on Gly-tRNAGly, indicating tRNA-based modulation of DTD (Pawar et al., 2017). Here, we show that tRNA’s discriminator base predominantly accounts for this activity difference and is the key to selection by DTD. Accordingly, the uracil discriminator base, serving as a negative determinant, prevents Gly-tRNAGly misediting by DTD and this protection is augmented by EF-Tu. Intriguingly, eukaryotic DTD has inverted discriminator base specificity and uses only G3•U70 for tRNAGly/Ala discrimination. Moreover, DTD prevents alanine-to-glycine misincorporation in proteins rather than only recycling mischarged tRNAAla. Overall, the study reveals the unique co-evolution of DTD and discriminator base, and suggests DTD’s strong selection pressure on bacterial tRNAGlys to retain a pyrimidine discriminator code.
机译:D-氨基酰基-tRNA脱酰基酶(DTD)除连接至tRNA的D-氨基酸外,还作用于非手性甘氨酸。最近我们发现,这种活性使DTD能够清除非同源Gly-tRNA Ala ,其效率比其对Gly-tRNA Gly 的活性高1000倍,表明tRNA-基于DTD的调制(Pawar et al。,2017)。在这里,我们证明tRNA的区分基主要是造成这种活性差异的原因,并且是DTD选择的关键。因此,尿嘧啶鉴别基作为负决定因子,防止了Dly对Gly-tRNA Gly 的错误编辑,而EF-Tu增强了这种保护作用。有趣的是,真核生物DTD具有反向的鉴别器碱基特异性,并且仅使用G3•U70进行tRNA Gly / Ala 鉴别。此外,DTD可以防止蛋白质中丙氨酸与甘氨酸的错误掺入,而不仅可以回收带错电荷的tRNA Ala 。总体而言,这项研究揭示了DTD和鉴别基的独特共同进化,并暗示DTD对细菌tRNA Gly 的强大选择压力,以保留嘧啶鉴别码。

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