Dual-Locked Enzyme-Activatable Bioorthogonal Fluorescence Turn-On Imaging of Senescent Cancer Cells.

IF 14.4 1区 化学 Q1 CHEMISTRY, MULTIDISCIPLINARY
Journal of the American Chemical Society Pub Date : 2024-08-14 Epub Date: 2024-08-05 DOI:10.1021/jacs.4c07286
Xinzhu Wang, Si Si Liew, Jingsheng Huang, Yuxuan Hu, Xin Wei, Kanyi Pu
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Abstract

Bioorthogonal pretargeting optical imaging shows the potential for enhanced diagnosis and prognosis. However, the bioorthogonal handles, known for being "always reactive", may engage in reactions at unintended sites with their counterparts, resulting in nonspecific fluorescence activation and diminishing detection specificity. Meanwhile, despite the importance of detecting senescent cancer cells in cancer therapy, current methods mainly rely on common single senescence-associated biomarkers, which lack specificity for differentiating between various types of senescent cells. Herein, we report a dual-locked enzyme-activatable bioorthogonal fluorescence (DEBOF) turn-on imaging approach for the specific detection of senescent cancer cells. A dual-locked bioorthogonal targeting agent (DBTA) and a bioorthogonally activatable fluorescent imaging probe (BAP) are synthesized as the biorthogonal pair. DBTA is a tetrazine derivative dually caged by two enzyme-cleavable moieties, respectively, associated with senescence and cancer, which ensures that its bioorthogonal reactivity ("clickability") is only triggered in the presence of senescent cancer cells. BAP is a fluorophore caged by trans-cyclooctane (TCO), whose fluorescence is only activated upon bioorthogonal reaction between its TCO and the decaged tetrazine of DBTA. As such, the DEBOF imaging approach differentiates senescent cancer cells from nonsenescent cancer cells or other senescent cells, allowing noninvasive tracking of the population fluctuation of senescent cancer cells in the tumor of living mice to guide cancer therapies. This study thus provides a general molecular strategy for biomarker-activatable in vivo bioorthogonal pretargeting imaging with the potential to be applied to other imaging modalities beyond optics.

Abstract Image

衰老癌细胞的双锁酶激活生物正交荧光开启成像。
生物正交前靶向光学成像具有增强诊断和预后的潜力。然而,以 "总是有反应 "著称的生物正交手柄可能会在非预期部位与对应物发生反应,从而导致非特异性荧光激活,降低检测的特异性。同时,尽管检测衰老癌细胞在癌症治疗中非常重要,但目前的方法主要依赖于常见的单一衰老相关生物标志物,缺乏区分不同类型衰老细胞的特异性。在此,我们报告了一种用于特异性检测衰老癌细胞的双锁定酶激活生物正交荧光(DEBOF)开启成像方法。我们合成了双锁定生物正交靶向剂(DBTA)和生物正交可激活荧光成像探针(BAP)作为生物正交对。DBTA 是一种四嗪衍生物,分别被两个与衰老和癌症有关的可酶解分子双重笼住,这确保了它的生物正交反应性("可点击性")只有在衰老癌细胞存在时才会被触发。BAP 是一种被反式环辛烷(TCO)笼住的荧光团,其荧光只有在其 TCO 与 DBTA 的脱醛四嗪发生生物正交反应时才会被激活。因此,DEBOF 成像方法可将衰老癌细胞与非衰老癌细胞或其他衰老细胞区分开来,从而可以无创追踪活体小鼠肿瘤中衰老癌细胞的种群波动,为癌症疗法提供指导。因此,这项研究为可激活生物标志物的体内生物正交前靶向成像提供了一种通用分子策略,有望应用于光学以外的其他成像模式。
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来源期刊
CiteScore
24.40
自引率
6.00%
发文量
2398
审稿时长
1.6 months
期刊介绍: The flagship journal of the American Chemical Society, known as the Journal of the American Chemical Society (JACS), has been a prestigious publication since its establishment in 1879. It holds a preeminent position in the field of chemistry and related interdisciplinary sciences. JACS is committed to disseminating cutting-edge research papers, covering a wide range of topics, and encompasses approximately 19,000 pages of Articles, Communications, and Perspectives annually. With a weekly publication frequency, JACS plays a vital role in advancing the field of chemistry by providing essential research.
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