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一种基于荧光点亮适体转录的超灵敏无标记核糖核酸酶H检测方法。

An ultrasensitive label-free RNase H assay based on transcription of fluorogenic light-up aptamer.

作者信息

Lee Jinhwan, Kim Hansol, Li Yan, Lee Seoyoung, Park Hyun Gyu

机构信息

Department of Chemical and Biomolecular Engineering (BK21 Four), Korea Advanced Institute of Science and Technology (KAIST) 291 Daehak-ro, Yuseong-gu Daejeon 34141 Republic of Korea

出版信息

Nanoscale Adv. 2024 Mar 7;6(7):1926-1931. doi: 10.1039/d3na00975k. eCollection 2024 Mar 26.

Abstract

Herein, we proposed a label-free method to identify RNase H activity by utilizing transcription of fluorogenic light-up aptamers. In this work, we employed the specially designed two pivotal components of the hairpin substrate probe (HP) containing an RNA/DNA chimeric stem region and the template probe (TP) as a transcription template, and the RNase H activity was made to lead to the formation of a complete ds T7 promoter. T7 RNA polymerase could then promote transcription to generate numerous light-up RNA aptamers that result in significant fluorescence enhancements upon binding to the cognate fluorogenic dye. By leveraging this deliberate design principle, we identified RNase H activity ultrasensitively as low as 0.000156 U mL with excellent specificity against non-target enzymes. We further demonstrated that the strategy can also reliably identify RNase H activity in heterogeneous biological samples such as cell lysates, ensuring its robust practical applicability. This work would provide invaluable insight for the development of innovative biosensing systems utilizing transcription of light-up aptamers, and it could be broadened to construct other assays by appropriately redesigning the HPs.

摘要

在此,我们提出了一种无标记方法,通过利用荧光点亮适体的转录来鉴定核糖核酸酶H(RNase H)的活性。在这项工作中,我们使用了特别设计的发夹底物探针(HP)的两个关键组成部分,其中包含一个RNA/DNA嵌合茎区和作为转录模板的模板探针(TP),并且使RNase H的活性导致形成完整的双链T7启动子。然后,T7 RNA聚合酶可以促进转录以产生大量的点亮RNA适体,这些适体在与同源荧光染料结合时会导致显著的荧光增强。通过利用这种精心设计的原理,我们以低至0.000156 U/mL的超灵敏度鉴定了RNase H的活性,并且对非靶标酶具有出色的特异性。我们进一步证明,该策略还可以可靠地鉴定细胞裂解液等异质生物样品中的RNase H活性,确保其强大的实际适用性。这项工作将为利用点亮适体转录开发创新的生物传感系统提供宝贵的见解,并且通过适当重新设计HP,可以将其扩展以构建其他检测方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e571/10964761/f074bcac461b/d3na00975k-f1.jpg

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