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Enzyme-Directed Assembly of Nanoparticles in Tumors Monitored by In Vivo Whole Animal and Ex Vivo Super Resolution Fluorescence Imaging

机译:体内整个动物和体内超分辨率荧光成像监测的肿瘤中酶的纳米颗粒组装。

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摘要

Matrix metalloproteinase enzymes, overexpressed in HT-1080 human fibrocarcinoma tumors, were used to guide the accumulation and retention of an enzyme-responsive nanoparticle in a xenograft mouse model. The nanoparticles were prepared as micelles from amphiphilic block copolymers bearing a simple hydrophobic block, and a hydrophilic peptide brush. The polymers were end-labeled with Alexa Fluor 647 dyes leading to the formation of labeled micelles upon dialysis of the polymers from DMSO to aqueous buffer. This dye-labeling strategy allowed the presence of the retained material to be visualized via whole animal imaging in vivo, and in ex vivo organ analysis following intratumoral injection into HT-1080 xenograft tumors. We propose that the material is retained by virtue of an enzyme-induced accumulation process whereby particles change morphology from 20 nm spherical micelles to micron-scale aggregates, kinetically trapping them within the tumor. This hypothesis is tested here via an unprecedented super resolution fluorescence analysis of ex vivo tissue slices confirming a particle size increase occurs concomitantly with extended retention of responsive particles compared to unresponsive controls.
机译:在HT-1080人纤维癌肿瘤中过表达的基质金属蛋白酶被用来指导异种移植小鼠模型中酶反应性纳米颗粒的积累和保留。纳米颗粒由带有简单疏水嵌段的两亲嵌段共聚物和亲水肽刷制成胶束。用Alexa Fluor 647染料对聚合物进行末端标记,导致在将聚合物从DMSO渗析至水性缓冲液后,形成标记的胶束。这种染料标记策略允许通过体内全动物成像以及瘤内注射入HT-1080异种移植肿瘤后的离体器官分析来观察保留材料的存在。我们建议通过酶诱导的积累过程来保留材料,从而使颗粒的形态从20 nm球形胶束变为微米级聚集体,从而将它们动态地捕获在肿瘤内。在此通过对离体组织切片进行前所未有的超分辨率荧光分析测试了这一假设,从而证实了与无反应的对照相比,随着反应颗粒的保留时间延长,同时发生了粒径增加。

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