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使用 EF-P 反应性人工起始 tRNA 对非天然氨基酸进行翻译起始。

Translation initiation with exotic amino acids using EF-P-responsive artificial initiator tRNA.

机构信息

Department of Chemistry, Graduate School of Science, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan.

出版信息

Nucleic Acids Res. 2023 Aug 25;51(15):8169-8180. doi: 10.1093/nar/gkad496.

Abstract

Translation initiation using noncanonical initiator substrates with poor peptidyl donor activities, such as N-acetyl-l-proline (AcPro), induces the N-terminal drop-off-reinitiation event. Thereby, the initiator tRNA drops-off from the ribosome and the translation reinitiates from the second amino acid to yield a truncated peptide lacking the N-terminal initiator substrate. In order to suppress this event for the synthesis of full-length peptides, here we have devised a chimeric initiator tRNA, referred to as tRNAiniP, whose D-arm comprises a recognition motif for EF-P, an elongation factor that accelerates peptide bond formation. We have shown that the use of tRNAiniP and EF-P enhances the incorporation of not only AcPro but also d-amino, β-amino and γ-amino acids at the N-terminus. By optimizing the translation conditions, e.g. concentrations of translation factors, codon sequence and Shine-Dalgarno sequence, we could achieve complete suppression of the N-terminal drop-off-reinitiation for the exotic amino acids and enhance the expression level of full-length peptide up to 1000-fold compared with the use of the ordinary translation conditions.

摘要

利用 N-乙酰-L-脯氨酸(AcPro)等肽供体活性差的非典型起始底物进行翻译起始,会诱导 N 端脱落-重新起始事件。因此,起始 tRNA 从核糖体上脱落,翻译从第二个氨基酸重新开始,从而产生缺乏 N 端起始底物的截短肽。为了抑制这种事件以合成全长肽,我们设计了一种嵌合起始 tRNA,称为 tRNAiniP,其 D 臂包含一个对 EF-P 的识别基序,EF-P 是一种加速肽键形成的延伸因子。我们已经表明,使用 tRNAiniP 和 EF-P 不仅可以增强 AcPro 的掺入,还可以增强 N 端的 D-氨基酸、β-氨基酸和 γ-氨基酸的掺入。通过优化翻译条件,例如翻译因子的浓度、密码子序列和 Shine-Dalgarno 序列,我们可以完全抑制非天然氨基酸的 N 端脱落-重新起始,并将全长肽的表达水平提高 1000 倍,与使用普通翻译条件相比。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b006/10450175/057c7f5b665f/gkad496figgra1.jpg

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