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活的哺乳动物细胞中合成mRNA输入介导的核酸链置换

Nucleic Acid Strand Displacement with Synthetic mRNA Inputs in Living Mammalian Cells.

作者信息

Chatterjee Gourab, Chen Yuan-Jyue, Seelig Georg

机构信息

Department of Bioengineering , University of Washington , Seattle , Washington 98105 , United States.

Department of Electrical Engineering , University of Washington , Seattle , Washington 98195 , United States.

出版信息

ACS Synth Biol. 2018 Dec 21;7(12):2737-2741. doi: 10.1021/acssynbio.8b00288. Epub 2018 Nov 20.

DOI:10.1021/acssynbio.8b00288
PMID:30441897
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7254870/
Abstract

Strand displacement reactions are widely used in DNA nanotechnology as a building block for engineering molecular computers and machines. Here, we demonstrate that strand displacement-based probes can be triggered by RNA expressed in mammalian cells, thus taking a step toward adapting the DNA nanotechnology toolbox to a cellular environment. We systematically compare different probe architectures in order to identify a design that works robustly in living cells. Our optimized strand displacement probe combines chemically modified nucleic acids that enhance stability to degradation by cellular nucleases with structural elements that improve probe retention in the cytoplasm. We visualize probe binding to individual mRNA carrying 96 repeats of a target sequence in the 3'UTR. We find that RNA counts based on live cell imaging using a strand displacement probe are comparable to counts from independent measurement based on fluorescence in situ hybridization experiments. We used probes with scrambled toeholds and scrambled binding domains to demonstrate that target recognition indeed occurs through toehold-mediated strand displacement. Our results demonstrate that strand displacement probes can work reliably in mammalian cells and lay the groundwork for future applications of such probes for live-cell imaging and molecular computing.

摘要

链置换反应在DNA纳米技术中被广泛用作构建分子计算机和机器的基础模块。在此,我们证明基于链置换的探针可被哺乳动物细胞中表达的RNA触发,从而朝着使DNA纳米技术工具箱适应细胞环境迈出了一步。我们系统地比较了不同的探针结构,以确定一种能在活细胞中稳定发挥作用的设计。我们优化后的链置换探针结合了化学修饰的核酸,这种核酸可增强对细胞核酸酶降解的稳定性,以及能提高探针在细胞质中保留率的结构元件。我们可视化了探针与3'UTR中携带96个目标序列重复片段的单个mRNA的结合情况。我们发现,基于链置换探针的活细胞成像得出的RNA计数与基于荧光原位杂交实验的独立测量结果相当。我们使用了具有随机化起始区和随机化结合域的探针,以证明目标识别确实是通过起始区介导的链置换发生的。我们的结果表明,链置换探针能在哺乳动物细胞中可靠地发挥作用,为这类探针未来用于活细胞成像和分子计算奠定了基础。