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自猝灭荧光和拉曼探针用于活细胞中 γ-谷氨酰转肽酶的实时成像和定量。

Self-Immolative Fluorescent and Raman Probe for Real-Time Imaging and Quantification of γ-Glutamyl Transpeptidase in Living Cells.

机构信息

Smart Hybrid Materials Laboratory (SHMs), Advanced Membranes and Porous Materials Center , King Abdullah University of Science and Technology (KAUST) , Thuwal 23955-6900 , Saudi Arabia.

出版信息

ACS Appl Mater Interfaces. 2019 Aug 7;11(31):27529-27535. doi: 10.1021/acsami.9b07186. Epub 2019 Jul 24.

Abstract

Characterizing over-expressed enzymes or biomarkers in living cells is critical for the molecular understanding of disease pathology and consequently for designing precision medicines. Herein, a "switch-on" probe is designed to selectively detect γ-glutamyl transpeptidase (GGT) in living cells via a unique ensemble of enhanced fluorescence and surface-enhanced Raman scattering (SERS). In the presence of GGT, the γ-glutamyl bond in the probe molecule is cleaved, thereby activating a fluorescent probe molecule as well as a Raman reporter molecule. Consequently, the detection of GGT is achieved based on both plasmonic fluorescent enhancement and SERS with a detection limit as low as 1.2 × 10 U/L (normal range for GGT levels in the blood is 9-48 U/L). The main advantage of this platform is that on the occasion of fluorescence signal interference, especially in the presence of free metal ions in cells, the SERS signals still hold high stability as a backup. This work highlights the benefits of the marriage of two complimentary sensing techniques into one platform that can overcome the major obstacles of detection of real-time biomarkers and imaging in living cells.

摘要

在活细胞中对过表达的酶或生物标志物进行特征描述,对于深入了解疾病病理学,从而设计精准药物至关重要。本文设计了一种“开启型”探针,通过独特的增强荧光和表面增强拉曼散射(SERS)组合,选择性地在活细胞中检测γ-谷氨酰转肽酶(GGT)。在 GGT 的存在下,探针分子中的γ-谷氨酰键被切断,从而激活荧光探针分子和拉曼报告分子。因此,基于等离子体荧光增强和 SERS 实现了 GGT 的检测,检测限低至 1.2×10 U/L(血液中 GGT 水平的正常范围为 9-48 U/L)。该平台的主要优势在于,在荧光信号干扰的情况下,特别是在细胞中存在游离金属离子的情况下,SERS 信号仍然保持高度稳定性,作为备份。这项工作突出了将两种互补传感技术结合到一个平台中的优势,该平台可以克服在活细胞中实时生物标志物检测和成像的主要障碍。

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