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A rapid, inexpensive yeast-based dual-fluorescence assay of programmed—1 ribosomal frameshifting for high-throughput screening

机译:一种快速,廉价的基于酵母的双荧光检测程序,用于程序化的1核糖体移码,可进行高通量筛选

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摘要

Programmed −1 ribosomal frameshifting (−1 PRF) is a mechanism that directs elongating ribosomes to shift-reading frame by 1 base in the 5′ direction that is utilized by many RNA viruses. Importantly, rates of −1 PRF are fine-tuned by viruses, including Retroviruses, Coronaviruses, Flavivriuses and in two endogenous viruses of the yeast Saccharomyces cerevisiae, to deliver the correct ratios of different viral proteins for efficient replication. Thus, −1 PRF presents a novel target for antiviral therapeutics. The underlying molecular mechanism of −1 PRF is conserved from yeast to mammals, enabling yeast to be used as a logical platform for high-throughput screens. Our understanding of the strengths and pitfalls of assays to monitor −1 PRF have evolved since the initial discovery of −1 PRF. These include controlling for the effects of drugs on protein expression and mRNA stability, as well as minimizing costs and the requirement for multiple processing steps. Here we describe the development of an automated yeast-based dual fluorescence assay of −1 PRF that provides a rapid, inexpensive automated pipeline to screen for compounds that alter rates of −1 PRF which will help to pave the way toward the discovery and development of novel antiviral therapeutics.
机译:程序化的-1核糖体移码(-1 PRF)是一种机制,可将延伸的核糖体沿许多RNA病毒利用的5'方向以1个碱基移位阅读框。重要的是,-1 PRF的比率可通过病毒(包括逆转录病毒,冠状病毒,黄病毒和酿酒酵母)的两种内源性病毒进行微调,以提供正确比例的不同病毒蛋白进行有效复制。因此,-1 PRF提出了抗病毒治疗的新目标。 -1 PRF的基本分子机制从酵母到哺乳动物都是保守的,使酵母可用作高通量筛选的逻辑平台。自从首次发现-1 PRF以来,我们对监测-1 PRF的检测方法的优势和陷阱的了解已经发展。这些措施包括控制药物对蛋白质表达和mRNA稳定性的影响,以及最小化成本和对多个加工步骤的需求。在这里,我们描述了基于自动酵母的-1 PRF双重荧光测定法的开发,该测定法提供了一种快速,廉价的自动化管道来筛选改变-1 PRF速率的化合物,这将有助于为发现和开发P-1铺平道路。新型抗病毒疗法。

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