Near‐Infrared Bioorthogonally Activatable Fluorescence Probe for In Vivo Imaging of Immune Checkpoint in Cancer

材料科学 荧光 体内 免疫检查点 红外线的 纳米技术 癌症 荧光寿命成像显微镜 生物医学工程 光学 免疫疗法 医学 生物 内科学 物理 生物技术
作者
Jing Liu,Si Si Liew,Penghui Cheng,Xinzhu Wang,Dong‐Hao Li,Xin Wei,Yuxuan Hu,Kanyi Pu
出处
期刊:Advanced Functional Materials [Wiley]
卷期号:35 (43) 被引量:5
标识
DOI:10.1002/adfm.202508396
摘要

Abstract Real‐time in vivo imaging of immune checkpoints is important for the guidance and prognosis of cancer immunotherapy. Although activatable optical probes have the advantages of high specificity and sensitivity as compared with “always‐on” probes, it is nearly impossible to adopt the reactivity‐based design approach for the detection of checkpoint proteins because they generally lack enzymatic activity. Herein, bioorthogonal‐reaction‐enabled fluorescence turn‐on detection of immune checkpoint in cancer is reported. This approach involves a bioorthogonally activatable near‐infrared fluorescence probe (BAP) and a transcyclooctene (TCO) tagged immune checkpoint antibody (αPDL1 TCO ). BAP is a hemicyanine fluorophore whose hydroxyl group is caged by tetrazine. Upon reaction with the TCOs of αPDL1 TCO , the tetrazine moiety of BAP is cleaved to release the uncaged hemicyanine with a fluorescence turn‐on response. BAP not only allows to specifically detect and track the fluctuation of PDL1 expression level in a murine colon cancer model during therapy but also shows a higher signal‐to‐background ratio than the “always‐on” fluorophore conjugated‐antibody, and a higher detection sensitivity than flow cytometric analysis of biopsied tumor tissues. It is expected that the design strategy of this bioorthogonally activatable probe can be applied for specific detection of other disease‐related protein biomarkers without enzymatic reactivity.
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