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Switching the activity of Cas12a using guide RNA strand displacement circuits

机译:使用指导RNA链置换电路切换Cas12a的活性

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The CRISPR effector protein Cas12a has been used for a wide variety of applications such as in vivo gene editing and regulation or in vitro DNA sensing. Here, we add programmability to Cas12a-based DNA processing by combining it with strand displacement-based reaction circuits. We first establish a viable strategy for augmenting Cas12a guide RNAs (gRNAs) at their 5' end and then use such 5' extensions to construct strand displacement gRNAs (SD gRNAs) that can be activated by single-stranded RNA trigger molecules. These SD gRNAs are further engineered to exhibit a digital and orthogonal response to different trigger RNA inputs-including full length mRNAs-and to function as multi-input logic gates. We also demonstrate that SD gRNAs can be designed to work inside bacterial cells. Using such in vivo SD gRNAs and a DNase inactive version of Cas12a (dCas12a), we demonstrate logic gated transcriptional control of gene expression in E. coli.
机译:CRISPR效应蛋白Cas12a已用于多种应用,例如体内基因编辑和调控或体外DNA传感。在这里,我们将其与基于链置换的反应电路相结合,为基于Cas12a的DNA处理增加了可编程性。我们首先建立了在其5'端增强Cas12a指导RNA(gRNA)的可行策略,然后使用此类5'延伸构建可被单链RNA触发分子激活的链置换gRNA(SD gRNA)。这些SD gRNA被进一步工程化,以显示对不同触发RNA输入(包括全长mRNA)的数字响应和正交响应,并充当多输入逻辑门。我们还证明了SD gRNA可以设计为在细菌细胞内部工作。使用这种体内SD gRNA和Cas12a(dCas12a)的DNase无效版本,我们证明了大肠杆菌中基因表达的逻辑门控转录控制。

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