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基于近红外荧光杂交链式反应的 miR-21 光声对比剂

A Photoacoustic Contrast Agent for miR-21 via NIR Fluorescent Hybridization Chain Reaction.

机构信息

Department of NanoEngineering, University of California, San Diego, La Jolla, California 92093. United States.

Department of Radiology, University of California, San Diego, La Jolla, California 92093. United States.

出版信息

Bioconjug Chem. 2022 Jun 15;33(6):1080-1092. doi: 10.1021/acs.bioconjchem.1c00375. Epub 2021 Aug 18.

Abstract

Nucleic acids are well-established biomarkers of cancer with immense value in diagnostics and basic research. However, strategies to monitor these species in tissue can be challenging due to the need for amplification of imaging signal from low analyte concentrations with high specificity. Photoacoustic (PA) imaging is gaining traction for molecular imaging of proteins, small biomolecules, and nucleic acids by coupling pulsed near-infrared (NIR) excitation with broadband acoustic detection. This work introduces a PA nucleic acid contrast agent that harnesses NIR fluorophore and quencher-tagged hybridization chain reaction (HCR) for signal amplification. This HCR probe was designed to enable contact quenching between NIR dye-quencher pairs by coercing their direct alignment when miR-21, a microRNA cancer biomarker, is detected. The probe demonstrated a ratiometric PA limit of detection of 148 pM miR-21, sequence specificity against one- and two-base mutations, and selectivity over other microRNAs. It was further tested in live human ovarian cancer (SKOV3) and noncancerous (HEK 293T) cells to exemplify PA activation based on differences in endogenous miR-21 regulation ( = 0.0002). The probe was lastly tested in tissue mimicking phantoms to exemplify sustained contrast in centimeter-range depths and 85.3% photostability after 15 min of laser irradiation. The probe's miR-21-specific activation and its ability to maintain contrast in biologically relevant absorbing and scattering media support its consideration for live-cell PA microscopy and potential cancer diagnostics. Results from this probe also underscore the combined detection power between ratiometric PA signaling and strand amplification for more sensitive DNA-based PA sensors.

摘要

核酸是癌症的既定生物标志物,在诊断和基础研究中具有巨大的价值。然而,由于需要高特异性地从低分析物浓度放大成像信号,因此在组织中监测这些物质的策略可能具有挑战性。光声(PA)成像通过将脉冲近红外(NIR)激发与宽带声检测相结合,正在成为蛋白质、小分子和核酸的分子成像的有力工具。本工作引入了一种 PA 核酸对比剂,该对比剂利用 NIR 荧光团和淬灭剂标记的杂交链式反应(HCR)进行信号放大。该 HCR 探针的设计目的是通过在检测 microRNA 癌症生物标志物 miR-21 时强制其直接对齐,实现 NIR 染料-淬灭对之间的接触淬灭。该探针表现出 miR-21 的比率光声检测限为 148 pM,对单碱基和双碱基突变具有序列特异性,并且对其他 microRNAs 具有选择性。进一步在活的人卵巢癌细胞(SKOV3)和非癌细胞(HEK 293T)中进行了测试,以说明基于内源性 miR-21 调节的 PA 激活差异( = 0.0002)。最后,该探针在组织模拟体模中进行了测试,以说明在厘米范围内的深度具有持续的对比度,并且在 15 分钟的激光照射后具有 85.3%的光稳定性。该探针对 miR-21 的特异性激活及其在生物相关吸收和散射介质中保持对比度的能力支持其用于活细胞 PA 显微镜和潜在癌症诊断的考虑。该探针的结果还强调了比率光声信号和链扩增的组合检测能力,可用于更灵敏的基于 DNA 的 PA 传感器。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9c10/9122088/fb9ecd979c97/nihms-1803436-f0001.jpg

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