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荧光遮蔽纳米粒子簇用于实时监测肿瘤进展。

Fluorescence-Shadowing Nanoparticle Clusters for Real-Time Monitoring of Tumor Progression.

机构信息

Department of Biomedical Materials Engineering, Kangwon National University, Chuncheon 24341, Republic of Korea.

Kangwon Radiation Convergence Research Support Center, Kangwon National University, Chuncheon 24341, Republic of Korea.

出版信息

Biomacromolecules. 2022 Aug 8;23(8):3130-3141. doi: 10.1021/acs.biomac.2c00169. Epub 2022 Apr 22.

Abstract

Monitoring tumor progression is important for elucidating appropriate therapeutic strategies in response to anticancer therapeutics. To fluorescently monitor the levels of tumor-specific enzymes, we prepared matrix metalloprotease (MMP)-responsive gold nanoparticle (AuNP) clusters to sense tumor microenvironments. Specifically, AuNPs and quantum dots (QDs) were surface-engineered with two poly(ethylene glycol) [PEG] shells and cyclooctyne moieties, respectively, for the copper-free click reaction. Upon "peeling off" of the secondary shell from the double-PEGylated AuNPs under MMP-rich conditions, shielded azide moieties of the AuNPs were displayed toward the QD, and those two particles were clicked into nanoparticle clusters. This consequently resulted in a dramatic size increase and fluorescence quenching of QDs via fluorescence energy transfer (FRET) due to the molecular proximity of the particles. We observed that FRET efficiency was modulated via changes in MMP levels and exposure time. Cancer cell numbers exhibited a strong correlation with FRET efficiency, and studies that employed solid tumor models accordingly showed that FRET efficiency was dependent on the tumor size. Thus, we envision that this platform can be tailored and optimized for tumor monitoring based on MMP levels in solid tumors.

摘要

监测肿瘤进展对于阐明针对抗癌治疗的适当治疗策略非常重要。为了荧光监测肿瘤特异性酶的水平,我们制备了基质金属蛋白酶(MMP)响应性金纳米颗粒(AuNP)簇来感知肿瘤微环境。具体而言,AuNP 和量子点(QD)分别用两个聚乙二醇(PEG)壳和环辛炔部分进行表面工程化,用于无铜点击反应。在 MMP 丰富的条件下,从双 PEG 化 AuNP 上“剥离”二级壳后,AuNP 的屏蔽叠氮部分朝向 QD 显示,这两个粒子被点击成纳米颗粒簇。这导致由于粒子的分子接近,QD 的尺寸急剧增加和荧光猝灭通过荧光能量转移(FRET)。我们观察到 FRET 效率通过 MMP 水平和暴露时间的变化进行调节。癌细胞数量与 FRET 效率具有很强的相关性,因此,我们的研究采用了实体瘤模型,表明 FRET 效率取决于肿瘤大小。因此,我们设想可以根据实体瘤中的 MMP 水平对该平台进行定制和优化,以用于肿瘤监测。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d4b6/9364936/82d58f64b3ea/bm2c00169_0002.jpg

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