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可编程DNA电路辅助检测循环细胞外囊泡PD-L1用于肺癌诊断和免疫治疗反应预测

Programmable DNA Circuit-Facilitated Determination of Circulating Extracellular Vesicle PD-L1 for Lung Cancer Diagnosis and Immunotherapy Response Prediction.

作者信息

Bo Bing, Li Wei, Li Jiayu, Han Chaonan, Fang Qiyu, Yang Menghang, Ni Jian, Zhou Caicun

机构信息

Department of Medical Oncology, Shanghai Pulmonary Hospital, School of Medicine, Tongji University, Shanghai 200433, China.

Department of Lung Cancer and Immunology, Shanghai Pulmonary Hospital, School of Medicine, Tongji University, Shanghai 200433, China.

出版信息

ACS Appl Mater Interfaces. 2023 Apr 12;15(14):17696-17704. doi: 10.1021/acsami.3c01607. Epub 2023 Mar 28.

Abstract

Circulating extracellular vesicle (EV) PD-L1 is correlated with the occurrence and progression of lung cancer and has great potential as a valuable diagnostic and immunotherapy predictive biomarker. In this work, we propose a fluorescent biosensing method for the sensitive and accurate determination of circulating EV PD-L1. Specifically, after the phosphatidylserine-targeting peptide-assisted magnetic enrichment, a programmable DNA circuit is designed to translate the presence of PD-L1 to the appearance of numerous duplex DNA probes on the circulating EV surface. Upon fructose treatment, these newly formed duplex DNA probes are released from the EV surface to activate the trans-cleavage activity of CRISPR/Cas12a system, which finally produces a significant fluorescence signal. Experimental results reveal that the method not only enables sensitive determination of EV PD-L1 with a detection limit of 67 particles/mL but also demonstrates the potential use in the diagnosis and immunotherapy response prediction of lung cancer in a principle-of-proof study. Therefore, the method may provide a useful tool for EV PD-L1 determination, which may provide valuable information for the precise diagnosis and personalized treatment of lung cancer patients.

摘要

循环细胞外囊泡(EV)中的程序性死亡配体1(PD-L1)与肺癌的发生和进展相关,具有作为有价值的诊断和免疫治疗预测生物标志物的巨大潜力。在本研究中,我们提出了一种荧光生物传感方法,用于灵敏且准确地测定循环EV中的PD-L1。具体而言,在磷脂酰丝氨酸靶向肽辅助磁富集后,设计了一种可编程DNA电路,将PD-L1的存在转化为循环EV表面大量双链DNA探针的出现。经果糖处理后,这些新形成的双链DNA探针从EV表面释放,激活CRISPR/Cas12a系统的反式切割活性,最终产生显著的荧光信号。实验结果表明,该方法不仅能够以67个颗粒/毫升的检测限灵敏地测定EV PD-L1,还在一项原理验证研究中证明了其在肺癌诊断和免疫治疗反应预测中的潜在应用。因此,该方法可能为EV PD-L1的测定提供一种有用的工具,可为肺癌患者的精确诊断和个性化治疗提供有价值的信息。

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