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A molecular design strategy toward enzyme-activated probes with near-infrared I and II fluorescence for targeted cancer imaging

机译:一种针对具有靶向目标的癌症成像的具有近红外I和II荧光的酶激活探针的分子设计策略

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摘要

The advance of cancer imaging requires innovations to establish novel fluorescent scaffolds that are excitable and emit in the near-infrared region with favorable Stokes shifts. Nevertheless, the lack of probes with these optimized optical properties presents a major bottleneck in targeted cancer imaging. By coupling of boron dipyrromethene platforms to enzymic substrates via a self-immolative benzyl thioether linker, we here report a strategy toward enzyme-activated fluorescent probes to satisfy these requirements. This strategy is applicable to generate various BODIPY-based probes across the NIR spectrum via introducing diverse electron-withdrawing substituents at the 3-position of the BODIPY core through a vinylene unit. As expected, such designed probes show advantages of two-channel ratiometric fluorescence and light-up NIR (I and II) emission with large Stokes shifts upon enzyme activation, enabling targeted cancer cell imaging and accurate tumor location by real-time monitoring of enzyme activities. This strategy is promising in engineering activatable molecular probes suitable for precision medicine.
机译:癌症影像学的发展要求创新以建立新型的荧光支架,该支架可激发并在近红外区域发射,并具有良好的斯托克斯位移。然而,缺乏具有这些优化的光学性质的探针在靶向癌症成像中存在主要瓶颈。通过自消灭的苄基硫醚连接基,将硼二吡咯亚甲基平台偶联至酶促底物上,我们在此报告了一种针对酶活化荧光探针的策略,以满足这些要求。通过在亚乙炔单元的BODIPY核的3位引入不同的吸电子取代基,该策略适用于在整个NIR光谱中生成各种基于BODIPY的探针。如预期的那样,这种设计的探针显示出两通道比例荧光和NIR(I和II)发光的优点,并在酶激活时具有大的斯托克斯位移,从而可以通过实时监测酶活性来进行靶向的癌细胞成像和准确的肿瘤定位。这种策略在工程学上适用于精密医学的可激活分子探针中很有希望。

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