Accurate Molecular Sensing based on a Modular and Customizable CRISPR/Cas‐Assisted Nanopore Operational Nexus (CANON)

清脆的 模块化设计 纳米孔测序 反式激活crRNA 纳米孔 计算机科学 DNA 核酸 化学 Cas9 纳米技术 计算生物学 DNA测序 材料科学 生物 生物化学 基因 操作系统
作者
Huaning Wang,Rujian Zhao,Bing Zhang,Yao Xiao,Chunmiao Yu,Yesheng Wang,Chunxu Yu,Yidan Tang,Yanru Li,Baiyang Lu,Bingling Li
出处
期刊:Angewandte Chemie [Wiley]
卷期号:64 (13): e202423473-e202423473 被引量:8
标识
DOI:10.1002/anie.202423473
摘要

Solid-state nanopore is a promising single molecular detection technique, but is largely limited by relatively low resolution to small-size targets and laborious design of signaling probes. Here we establish a universal, CRISPR/Cas-Assisted Nanopore Operational Nexus (CANON), which can accurately transduce different targeting sources/species into different DNA structural probes via a "Signal-ON" mode. Target recognition activates the cleavage activity of a Cas12a/crRNA system and then completely digest the blocker of an initiator. The unblocked initiator then triggers downstream DNA assembly reaction and generate a large-size structure easy for nanopore detection. Such integration of Cas12a/crRNA with DNA assembly establishes an accurate correspondence among the input targets, output DNA structures, and the ultimate nanopore signals. We demonstrated dsDNA, long RNA (i.e., Flu virus gene), short microRNA (i.e., let-7d) and non-nucleic acids (i.e., Pb2+) as input paradigms. Various structural assembly reactions, such as hybridization chain reaction (HCR), G-HCR and duplex polymerization strategy (DPS), are adapted as outputs for nanopore signaling. Simultaneous assay is also verified via transferring FluA and FluB genes into HCR and G-HCR, respectively. CANON is thus a modular sensing platform holding multiple advantages such as high accuracy, high resolution and high universality, which can be easily customized into various application scenes.
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