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Tracking of STAT3 signaling for anticancer drug-discovery based on localized surface plasmon resonance

机译:基于局部表面等离振子共振的STAT3信号追踪抗癌药物发现

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摘要

Signal transducer and activator of transcription 3 (STAT3) protein signaling is crucial for the survival, invasion, and growth of human cancer cells; thus, STAT3 protein is an ideal target for a new drug screening system. Herein, we developed a label-free sensor for anticancer drug-discovery based on the localized surface plasmon resonance (LSPR) shift response by tracking of STAT3 signaling including phosphorylation and dimerization. This enables ultrasensitive monitoring of the molecular interactions that occur on the surface of single gold nanoparticles. The red shift of the LSPR lambda(max) was observed as 3.46 nm and 9.00 nm, respectively, indicating phosphorylation and dimerization of the STAT3 signaling pathway. In screening of anticancer candidates, the system worked well in the presence of STA-21 which inhibits STAT3 dimerization. The LSPR lambda max shift in the inhibition condition is three times lower than that in the absence of an inhibitor. Interestingly, the system reveals high specificity, reproducibility and compatibility with real samples (MCF-7 cell line). Therefore, these results demonstrated that this system has strong potential to be an accurate and effective sensor for tracking of signaling pathways and drug screening of anticancer candidates for anticancer therapy.
机译:信号转导和转录激活因子3(STAT3)蛋白信号对于人类癌细胞的存活,侵袭和生长至关重要。因此,STAT3蛋白是新药筛选系统的理想靶标。本文中,我们通过跟踪包括磷酸化和二聚化在内的STAT3信号,基于局部表面等离子体共振(LSPR)位移响应,开发了一种用于抗癌药物发现的无标记传感器。这使得能够对单个金纳米颗粒表面上发生的分子相互作用进行超灵敏监测。观察到LSPR lambda(max)的红移为3.46 nm和9.00 nm,表明STAT3信号通路的磷酸化和二聚化。在筛选候选抗癌药物时,该系统在抑制STAT3二聚化的STA-21存在下运行良好。抑制条件下的LSPRλ最大位移比不存在抑制剂时的低三倍。有趣的是,该系统显示出与真实样品(MCF-7细胞系)的高度特异性,可重复性和兼容性。因此,这些结果表明,该系统具有强大的潜力,可以成为跟踪信号通路和进行抗癌候选药物筛选的准确有效的传感器。

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