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Kinetic analysis of aptazyme-regulated gene expression in a cell-free translation system: Modeling of ligand-dependent and -independent expression

机译:在无细胞翻译系统中由aptazyme调节的基因表达的动力学分析:配体依赖性和非依赖性表达的建模

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摘要

Aptazymes are useful as RNA-based switches of gene expression responsive to several types of compounds. One of the most important properties of the switching ability is the signaloise (S/N) ratio, i.e., the ratio of gene expression in the presence of ligand to that in the absence of ligand. The present study was performed to gain a quantitative understanding of how the aptazyme S/N ratio is determined by factors involved in gene expression, such as transcription, RNA self-cleavage, RNA degradation, protein translation, and their ligand dependencies. We performed switching of gene expression using two on-switch aptazymes with different properties in a cell-free translation system, and constructed a kinetic model that quantitatively describes the dynamics of RNA and protein species involved in switching. Both theoretical and experimental analyses consistently demonstrated that factors determining both the absolute value and the dynamics of the S/N ratio are highly dependent on the routes of translation in the absence of ligand: translation from the ligand-independently cleaved RNA or leaky translation from the noncleaved RNA. The model obtained here is useful to assess the factors that restrict the S/N ratio and to improve aptazymes more efficiently.
机译:Aptazymes可用作响应多种类型化合物的基因表达的基于RNA的开关。切换能力的最重要特性之一是信噪比(S / N),即在存在配体的情况下与不存在配体的情况下的基因表达比率。进行本研究是为了定量了解适体酶的信噪比(S / N)是由基因表达所涉及的因素决定的,例如转录,RNA自切割,RNA降解,蛋白质翻译及其配体依赖性。我们在无细胞翻译系统中使用两个具有不同特性的开关核酸酶进行了基因表达的转换,并构建了一个动力学模型,定量描述了涉及转换的RNA和蛋白质种类的动力学。理论和实验分析均一致地表明,决定S / N比的绝对值和动态的因素都高度依赖于在没有配体的情况下的翻译途径:来自配体的独立切割的RNA的翻译或来自SRNA的泄漏翻译。未切割的RNA。此处获得的模型可用于评估限制信噪比的因素,并更有效地改善aptazyme。

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