A Facile Platform to Engineer Escherichia coli Tyrosyl-tRNA Synthetase Adds New Chemistries to the Eukaryotic Genetic Code, Including a Phosphotyrosine Mimic

大肠杆菌 生物结合 突变体 遗传密码 转移RNA 合成生物学 细菌接合 生物 生物化学 选择(遗传算法) 计算生物学 氨酰tRNA合成酶 氨基酸 化学 组合化学 基因 核糖核酸 计算机科学 人工智能
作者
Katherine T. Grasso,Soumya Jyoti Singha Roy,Arianna O. Osgood,Megan Jin Rae Yeo,Chintan Soni,Christen M. Hillenbrand,Elise D. Ficaretta,Abhishek Chatterjee
出处
期刊:ACS central science [American Chemical Society]
卷期号:8 (4): 483-492 被引量:17
标识
DOI:10.1021/acscentsci.1c01465
摘要

The Escherichia coli tyrosyl-tRNA synthetase (EcTyrRS)/tRNAEcTyr pair offers an attractive platform for genetically encoding new noncanonical amino acids (ncAA) in eukaryotes. However, challenges associated with a eukaryotic selection system, which is needed to engineer the platform, have impeded its success in the past. Recently, using a facile E. coli-based selection system, we showed that EcTyrRS could be engineered in a strain where the endogenous tyrosyl pair was substituted with an archaeal counterpart. However, significant cross-reactivity between the UAG-suppressing tRNACUAEcTyr and the bacterial glutaminyl-tRNA synthetase limited the scope of this strategy, preventing the selection of moderately active EcTyrRS mutants. Here we report an engineered tRNACUAEcTyr that overcomes this cross-reactivity. Optimized selection systems based on this tRNA enabled the efficient enrichment of both strongly and weakly active ncAA-selective EcTyrRS mutants. We also developed a wide dynamic range (WiDR) antibiotic selection to further enhance the activities of the weaker first-generation EcTyrRS mutants. We demonstrated the utility of our platform by developing several new EcTyrRS mutants that efficiently incorporated useful ncAAs in mammalian cells, including photoaffinity probes, bioconjugation handles, and a nonhydrolyzable mimic of phosphotyrosine.
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