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一种通用的 DNA 探针设计,通过生成银纳米簇实现比率荧光检测。

A universal design for a DNA probe providing ratiometric fluorescence detection by generation of silver nanoclusters.

机构信息

Department of Mechanical Engineering, University of California Santa Barbara, USA.

出版信息

Nanoscale. 2016 Aug 14;8(30):14489-96. doi: 10.1039/c6nr03827a. Epub 2016 Jul 13.

DOI:10.1039/c6nr03827a
PMID:27406901
Abstract

DNA-stabilized silver nanoclusters (AgNCs), the fluorescence emission of which can rival that of typical organic fluorophores, have made possible a new class of label-free molecular beacons for the detection of single-stranded DNA. Like fluorophore-quencher molecular beacons (FQ-MBs) AgNC-based molecular beacons (AgNC-MBs) are based on a single-stranded DNA that undergoes a conformational change upon binding a target sequence. The new conformation exposes a stretch of single-stranded DNA capable of hosting a fluorescent AgNC upon reduction in the presence of Ag(+) ions. The utility of AgNC-MBs has been limited, however, because changing the target binding sequence unpredictably alters cluster fluorescence. Here we show that the original AgNC-MB design depends on bases in the target-binding (loop) domain to stabilize its AgNC. We then rationally alter the design to overcome this limitation. By separating and lengthening the AgNC-stabilizing domain, we create an AgNC-hairpin probe with consistent performance for arbitrary target sequence. This new design supports ratiometric fluorescence measurements of DNA target concentration, thereby providing a more sensitive, responsive and stable signal compared to turn-on AgNC probes. Using the new design, we demonstrate AgNC-MBs with nanomolar sensitivity and singe-nucleotide specificity, expanding the breadth of applicability of these cost-effective probes for biomolecular detection.

摘要

DNA 稳定的银纳米簇(AgNCs)的荧光发射可以与典型的有机荧光团相媲美,为单链 DNA 的检测提供了一类新的无标记分子信标。与荧光团猝灭分子信标(FQ-MBs)一样,基于 AgNC 的分子信标(AgNC-MBs)基于单链 DNA,在与目标序列结合时会发生构象变化。新的构象暴露了一段单链 DNA,在 Ag(+) 离子存在下可以还原容纳荧光 AgNC。然而,AgNC-MBs 的实用性受到限制,因为改变目标结合序列会不可预测地改变簇的荧光。在这里,我们表明原始的 AgNC-MB 设计依赖于靶结合(环)域中的碱基来稳定其 AgNC。然后,我们合理地改变设计以克服这一限制。通过分离和延长 AgNC 稳定域,我们创建了具有一致性能的 AgNC 发夹探针,适用于任意目标序列。这种新设计支持 DNA 目标浓度的比率荧光测量,从而与开环 AgNC 探针相比提供更灵敏、响应更快和更稳定的信号。使用新设计,我们展示了具有纳摩尔灵敏度和单核苷酸特异性的 AgNC-MBs,扩展了这些具有成本效益的探针在生物分子检测中的广泛适用性。

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