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pH-responsive ZnO nanoprobe mediated DNAzyme signal amplification strategy for sensitive detection and live cell imaging of multiple microRNAs

机译:pH响应的ZnO纳米探针介导的DNA酶信号放大策略,用于多种microRNA的灵敏检测和活细胞成像

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Here, a pH-responsive ZnO nanoprobe mediated DNAzyme signal amplification strategy was proposed for sensitive detection and live cell imaging of multiple microRNAs. The nanoprobe including ZnO nanoparticles (ZnO NPs) core as carrier and cofactor provider and polydopamine shell for adsorption the functional hairpin DNAs was designed. When nanoprobe entered the cell through endocytosis, the acidic environment of the cell could decompose the ZnO NPs core to release the functional hairpin DNAs and Zn2+. The Zn2+ could act as cofactor for the DNAzyme cleavage amplification reaction, avoiding additional cell delivery processes. The recognition hairpin DNAs (H1 and H3) recognized microRNA and exposed the DNAzyme. The DNAzyme cleaved cyclically the reporter hairpin DNAs (H2 and H4), producing enhanced fluorescent signal for miR-21 and miR-373 detection with the detection limit of 54 pM and 38 pM, respectively. Expression levels of miR-21 in Hela, HepG-2 and L02 cells were differentiated. Furthermore, simultaneous imaging of miR-21 and miR-373 in same living cells was achieved. These results indicated this strategy could have a potential application in microRNAs assays for the accurate diagnosis and therapy of cancer.
机译:在此,提出了一种pH敏感的ZnO纳米探针介导的DNA酶信号放大策略,用于多种microRNA的灵敏检测和活细胞成像。设计了以ZnO纳米颗粒(ZnO NPs)核为载体和辅因子提供者,并用聚多巴胺壳吸附功能性发夹DNA的纳米探针。当纳米探针通过内吞作用进入细胞时,细胞的酸性环境会分解ZnO NPs核心,释放出功能性发夹DNA和Zn2 +。 Zn2 +可以作为辅酶进行DNAzyme裂解扩增反应,避免额外的细胞递送过程。识别发夹DNA(H1和H3)识别微小RNA,并暴露DNA酶。 DNAzyme周期性切割报告子发夹DNA(H2和H4),产生增强的荧光信号用于miR-21和miR-373检测,检测限分别为54 pM和38 pM。区分了HeR,HepG-2和L02细胞中miR-21的表达水平。此外,在相同的活细胞中实现了miR-21和miR-373的同步成像。这些结果表明该策略可能在microRNA分析中具有潜在的应用价值,可用于癌症的准确诊断和治疗。

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