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Multiplexed miRNA northern blots via hybridization chain reaction

机译:通过杂交链反应的多重miRNA Northern印迹

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摘要

Northern blots enable detection of a target RNA of interest in a biological sample using standard benchtop equipment. miRNAs are the most challenging targets as they must be detected with a single short nucleic acid probe. With existing approaches, it is cumbersome to perform multiplexed blots in which several RNAs are detected simultaneously, impeding the study of interacting regulatory elements. Here, we address this shortcoming by demonstrating multiplexed northern blotting based on the mechanism of hybridization chain reaction (HCR). With this approach, nucleic acid probes complementary to RNA targets trigger chain reactions in which fluorophore-labeled DNA hairpins self-assemble into tethered fluorescent amplification polymers. The programmability of HCR allows multiple amplifiers to operate simultaneously and independently within a blot, enabling straightforward multiplexing. We demonstrate simultaneous detection of three endogenous miRNAs in total RNA extracted from 293T and HeLa cells. For a given target, HCR signal scales linearly with target abundance, enabling relative and absolute quantitation. Using non-radioactive HCR, sensitive and selective miRNA detection is achieved using 2′OMe-RNA probes. The HCR northern blot protocol takes ∼1.5 days independent of the number of target RNAs.
机译:Northern印迹可以使用标准台式设备检测生物样品中的目标靶RNA。 miRNA是最具挑战性的靶标,因为必须使用单个短核酸探针对其进行检测。使用现有的方法,进行同时检测多个RNA的多重印迹是麻烦的,这阻碍了相互作用调节元件的研究。在这里,我们通过展示基于杂交链反应(HCR)机理的多重Northern blotting解决了这一缺点。使用这种方法,与RNA互补的核酸探针可触发链反应,在链反应中,荧光团标记的DNA发夹会自动组装成束缚的荧光扩增聚合物。 HCR的可编程性允许多个放大器在印迹内同时独立运行,从而实现简单的多路复用。我们展示了同时检测从293T和HeLa细胞提取的总RNA中的三个内源性miRNA。对于给定的目标,HCR信号随目标丰度线性变化,从而实现相对和绝对定量。使用非放射性HCR,使用2'OMe-RNA探针可实现灵敏且选择性的miRNA检测。 HCR Northern印迹实验需要约1.5天,与目标RNA的数量无关。

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