适体
卵巢癌
双模
糖蛋白
对偶(语法数字)
药品
P-糖蛋白
癌症研究
多重耐药
抗药性
医学
肿瘤科
内科学
药理学
分子生物学
生物
癌症
多重耐药
工程类
遗传学
哲学
航空航天工程
语言学
作者
Chaobin Pang,Heng Xu,Jichao Xu,Lei Zhang,Jinhua Wang,Su Jing
出处
期刊:Analyst
[Royal Society of Chemistry]
日期:2024-01-01
卷期号:149 (15): 3928-3938
被引量:2
摘要
Drug resistance presents a significant obstacle in treating human ovarian cancer. The development of effective methods for detecting drug-resistant cancer cells is pivotal for tailoring personalized therapies and prognostic assessments. In this investigation, we introduce a dual-mode detection technique employing a fluorogenic aptamer probe for the qualification of P-glycoprotein (P-gp) in drug-resistant ovarian cancer cells. The probe, initially in an "off" state due to the proximity of a quencher to the fluorophore, exhibits increased fluorescence intensity upon binding with the target. The fluorescence enhancement shows a linear correlation with both the concentration of P-gp and the presence of P-gp in drug-resistant ovarian cancer cells. This correlation is quantifiable, with detection limits of 1.56 nM and 110 cells per mL. In an alternate mode, the optimized fluorophores, attached to the aptamer, form larger complexes upon binding to the target protein, which diminishes the rotation speed, thereby augmenting fluorescence polarization. The alteration in fluorescence polarization enables the quantitative analysis of P-gp in the cells, ranging from 100 to 1500 cells per milliliter, with a detection limit of 40 cells per mL. Gene expression analyses, protein expression studies, and immunofluorescence imaging further validated the reliability of our aptamer-based probe for its specificity towards P-gp in drug-resistant cancer cells. Our findings underscore that the dual-mode detection approach promises to enhance the diagnosis and treatment of multidrug-resistant ovarian cancer.
科研通智能强力驱动
Strongly Powered by AbleSci AI