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DNA 程序化量子点聚合用于癌症细胞的超高灵敏分子成像。

DNA-Programmed Quantum Dot Polymerization for Ultrasensitive Molecular Imaging of Cancer Cells.

机构信息

The Key Lab of Health Chemistry and Molecular Diagnosis of Suzhou, College of Chemistry, Chemical Engineering and Materials Science, Soochow University , Suzhou, 215123, P. R. China.

出版信息

Anal Chem. 2016 Oct 4;88(19):9355-9358. doi: 10.1021/acs.analchem.6b02864. Epub 2016 Sep 22.


DOI:10.1021/acs.analchem.6b02864
PMID:27649276
Abstract

Inorganic nanocrystals, such as quantum dots (QDs), hold great promise as molecular imaging contrast agents because of their superior optical properties. However, the molecular imaging sensitivity of these probes is far from optimized due to the lack of efficient and general method for molecular engineering of nanocrystal into effective bioprobes for signal-amplified imaging. Herein, we develop a strategy to boost the molecular imaging sensitivity of QDs over the limit by copolymerizing QDs and cell-binding aptamers into linear QD-aptamer polymers (QAPs) through DNA-programmed hybridization chain reaction. We show that the cancer cells treated with QAPs exhibit much stronger photoluminescence (PL) signal than those treated with QD-aptamer monomers (QAMs) because of multivalent binding and multi-QD-based signal amplification. The enhanced cell binding and imaging capacity of QAPs significantly improves imaging-based discrimination between different cancer cell types. This approach adds a new dimension for engineering inorganic nanoparticles into effective bioprobes for biomedical applications.

摘要

无机纳米晶体,如量子点 (QD),由于其优越的光学性质,有望成为分子成像对比剂。然而,由于缺乏将纳米晶体有效分子工程成用于信号放大成像的有效生物探针的通用方法,这些探针的分子成像灵敏度远未得到优化。在此,我们通过 DNA 编程的杂交链式反应,将 QD 与细胞结合适体共聚成线性 QD-适体聚合物 (QAP),从而提高 QD 的分子成像灵敏度,超越了极限。我们表明,用 QAP 处理的癌细胞表现出比用 QD-适体单体 (QAM) 处理的癌细胞强得多的光致发光 (PL) 信号,因为多价结合和多 QD 基于信号放大。QAP 的增强的细胞结合和成像能力显著提高了基于成像的不同癌细胞类型之间的区分能力。该方法为将无机纳米粒子工程成用于生物医学应用的有效生物探针增添了新维度。

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[3]
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[4]
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[5]
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[6]
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[7]
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[8]
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[9]
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[10]
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