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环滚动扩增Förster 共振能量转移(RCA-FRET)用于无洗涤实时单蛋白成像。

Rolling Circle Amplification Förster Resonance Energy Transfer (RCA-FRET) for Washing-Free Real-Time Single-Protein Imaging.

机构信息

nanoFRET.com, Laboratoire COBRA (Chimie Organique, Bioorganique, Réactivité et Analyse), Université de Rouen Normandie, CNRS, INSA, 76821 Mont-Saint-Aignan, France.

Institute for Integrative Biology of the Cell (I2BC), Université Paris-Saclay, CNRS, CEA, 91405 Orsay Cedex, France.

出版信息

Anal Chem. 2021 Jan 26;93(3):1842-1850. doi: 10.1021/acs.analchem.0c04828. Epub 2020 Dec 27.

DOI:10.1021/acs.analchem.0c04828
PMID:33356162
Abstract

Fluorescence signal enhancement isothermal nucleic acid amplification is an important approach for sensitive imaging of intra- or extracellular nucleic acid or protein biomarkers. Rolling circle amplification (RCA) is frequently applied for fluorescence imaging but faces limitations concerning multiplexing, dynamic range, and the required multiple washing steps before imaging. Here, we show that Förster resonance energy transfer (FRET) between fluorescent dyes and between lanthanide (Ln) complexes and dyes that hybridize to β-actin-specific RCA products in HaCaT cells can afford washing-free imaging of single β-actin proteins. Proximity-dependent FRET could be monitored directly after or during (real-time monitoring) dye or Ln DNA probe incubation and could efficiently distinguish between photoluminescence from β-actin-specific RCA and DNA probes freely diffusing in solution or nonspecifically attached to cells. Moreover, time-gated FRET imaging with the Ln-dye FRET pairs efficiently suppressed sample autofluorescence and improved the signal-to-background ratio. Our results present an important proof of concept of RCA-FRET imaging with a strong potential to advance RCA toward easier sample preparation, higher-order multiplexing, autofluorescence-free detection, and increased dynamic range by real-time monitoring of RCA.

摘要

荧光信号增强等温核酸扩增是一种用于灵敏检测细胞内或细胞外核酸或蛋白质生物标志物的重要方法。滚环扩增(RCA)常用于荧光成像,但在多重检测、动态范围以及成像前需要进行多次洗涤等方面存在局限性。在这里,我们展示了在 HaCaT 细胞中,荧光染料之间以及镧系(Ln)配合物与杂交到 β-肌动蛋白特异性 RCA 产物上的染料之间的Förster 共振能量转移(FRET)可以实现对单个 β-肌动蛋白蛋白的免洗成像。在染料或 Ln DNA 探针孵育后或期间(实时监测)可以直接监测到依赖于距离的 FRET,并且可以有效地将 β-肌动蛋白特异性 RCA 产生的光致发光与在溶液中自由扩散或非特异性附着在细胞上的 DNA 探针区分开来。此外,采用 Ln-染料 FRET 对的时间门控 FRET 成像有效地抑制了样品自体荧光,并提高了信号与背景的比值。我们的研究结果提供了一个重要的 RCA-FRET 成像概念验证,具有很大的潜力通过实时监测 RCA 来推动 RCA 朝着更简单的样品制备、更高阶的多重检测、无自体荧光检测和更大的动态范围方向发展。

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