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拓宽工具包,用于定量评估酵母中非标准氨基酸的掺入。

Broadening the Toolkit for Quantitatively Evaluating Noncanonical Amino Acid Incorporation in Yeast.

机构信息

Chemical and Biological Engineering Department, Tufts University, Medford, Massachusetts 02155, United States.

Biomedical Engineering Department, Tufts University, Medford, Massachusetts 02155, United States.

出版信息

ACS Synth Biol. 2021 Nov 19;10(11):3094-3104. doi: 10.1021/acssynbio.1c00370. Epub 2021 Nov 3.

Abstract

Genetic code expansion is a powerful approach for advancing critical fields such as biological therapeutic discovery. However, the machinery for genetically encoding noncanonical amino acids (ncAAs) is only available in limited plasmid formats, constraining potential applications. In extreme cases, the introduction of two separate plasmids, one containing an orthogonal translation system (OTS) to facilitate ncAA incorporation and a second for expressing a ncAA-containing protein of interest, is not possible due to a lack of the available selection markers. One strategy to circumvent this challenge is to express the OTS and protein of interest from a single vector. For what we believe is the first time in yeast, we describe here several sets of single plasmid systems (SPSs) for performing genetic code manipulation and compare the ncAA incorporation capabilities of these plasmids against the capabilities of previously described dual plasmid systems (DPSs). For both dual fluorescent protein reporters and yeast display reporters tested with multiple OTSs and ncAAs, measured ncAA incorporation efficiencies with SPSs were determined to be equal to efficiencies determined with DPSs. Click chemistry on yeast cells displaying ncAA-containing proteins was also shown to be feasible in both formats, although differences in reactivity between formats suggest the need for caution when using such approaches. Additionally, we investigated whether these reporters would support the separation of yeast strains known to exhibit distinct ncAA incorporation efficiencies. Model sorts conducted with mixtures of two strains transformed with the same SPS or DPS both led to the enrichment of a strain known to support a higher efficiency ncAA incorporation, suggesting that these reporters will be suitable for conducting screens for strains exhibiting enhanced ncAA incorporation efficiencies. Overall, our results confirm that SPSs are well behaved in yeast and provide a convenient alternative to DPSs. SPSs are expected to be invaluable for conducting high-throughput investigations of the effects of genetic or genomic changes on ncAA incorporation efficiency and, more fundamentally, the eukaryotic translation apparatus.

摘要

遗传密码扩展是推进生物治疗发现等关键领域的强大方法。然而,用于遗传编码非标准氨基酸(ncAA)的机制仅可用于有限的质粒格式,限制了潜在的应用。在极端情况下,由于缺乏可用的选择标记,不可能引入两个单独的质粒,一个质粒包含一个正交翻译系统(OTS)以促进 ncAA 掺入,另一个质粒用于表达含有 ncAA 的感兴趣的蛋白质。规避这一挑战的一种策略是从单个载体表达 OTS 和感兴趣的蛋白质。据我们所知,这是酵母中首次描述了几套用于进行遗传密码操作的单质粒系统(SPS),并比较了这些质粒与先前描述的双质粒系统(DPS)的 ncAA 掺入能力。对于经过多个 OTS 和 ncAA 测试的双荧光蛋白报告子和酵母展示报告子,SPS 测量的 ncAA 掺入效率被确定与 DPS 确定的效率相等。在这两种格式中,也证明了在含有 ncAA 的蛋白质的酵母细胞上进行点击化学是可行的,尽管格式之间的反应性差异表明在使用此类方法时需要谨慎。此外,我们研究了这些报告子是否会支持分离已知具有不同 ncAA 掺入效率的酵母菌株。使用相同的 SPS 或 DPS 转化的两种菌株的混合物进行的模型分类都导致了已知支持更高效率 ncAA 掺入的菌株的富集,这表明这些报告子将适合用于筛选具有增强的 ncAA 掺入效率的菌株。总的来说,我们的结果证实了 SPS 在酵母中表现良好,并为 DPS 提供了一种方便的替代方案。SPS 有望成为进行遗传或基因组变化对 ncAA 掺入效率影响的高通量研究的宝贵工具,更根本的是,对真核翻译装置的研究。

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