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基于快速引发级联放大反应的活细胞中端粒酶活性的高灵敏检测。

Highly sensitive monitoring of telomerase activity in living cells based on rapidly triggered cascade amplification reaction.

机构信息

Research Center for Analytical Sciences, Northeastern University, Shenyang, 110819, PR China.

Research Center for Analytical Sciences, Northeastern University, Shenyang, 110819, PR China.

出版信息

Biosens Bioelectron. 2022 Nov 15;216:114645. doi: 10.1016/j.bios.2022.114645. Epub 2022 Aug 19.

DOI:10.1016/j.bios.2022.114645
PMID:36029663
Abstract

Telomerase is an important potential biomarker for the study of tumor progression. Herein, we designed a cascade-amplification-reaction-based nanoprobe for intracellular telomerase detection based on the integration of rolling circle amplification (RCA) and catalytic hairpin assembly (CHA) onto MnO nanosheets. Firstly, MnO nanosheets rapidly delivered and released signal amplification units into cells, and very short telomerase extension products formed RCA circular templates and initiated the exponential RCA, producing enriched telomere sequence amplification products. Then the amplification products specifically triggered the CHA process and numerous H1/H2 complexes were formed, realizing the exponential amplification of fluorescence signals. The detection limit is as low as 1 LoVo cell for telomerase activity in cell extract. We further designed a microfluidic chip with six independent cell culture regions for in situ fluorescence imaging. Simultaneous detection of six types of cells was realized on the chip, and only 1-2 μL of cell suspension and reagents are needed. Our detection method features faster response speed and stronger fluorescence signal. Telomerase in living cells showed strong fluorescence signal within 1.5 h, and tumor cells were effectively distinguished from normal cells. Telomerase activities of different types of tumor cells and activity changes were both monitored conveniently. These results demonstrate that this method holds the potential for the sensitive detection of low abundance biomarkers in living cells, and will contribute to cancer diagnosis, cancer treatment and telomerase-related drug screening.

摘要

端粒酶是研究肿瘤进展的重要潜在生物标志物。在此,我们设计了一种基于级联放大反应的纳米探针,用于基于滚环扩增(RCA)和催化发夹组装(CHA)集成到 MnO 纳米片中的细胞内端粒酶检测。首先,MnO 纳米片快速将信号放大单元递送到细胞中,并迅速释放出来,非常短的端粒酶延伸产物形成 RCA 圆形模板,并启动指数 RCA,产生丰富的端粒序列扩增产物。然后,扩增产物特异性触发 CHA 过程,形成大量 H1/H2 复合物,实现荧光信号的指数放大。端粒酶活性在细胞提取物中的检测限低至 1 个 LoVo 细胞。我们进一步设计了具有六个独立细胞培养区的微流控芯片,用于原位荧光成像。在芯片上实现了六种类型细胞的同时检测,仅需要 1-2μL 的细胞悬浮液和试剂。我们的检测方法具有更快的响应速度和更强的荧光信号。活细胞中的端粒酶在 1.5 小时内显示出强荧光信号,并且可以有效地将肿瘤细胞与正常细胞区分开来。还可以方便地监测不同类型肿瘤细胞的端粒酶活性及其变化。这些结果表明,该方法具有在活细胞中灵敏检测低丰度生物标志物的潜力,并将有助于癌症诊断、癌症治疗和端粒酶相关药物筛选。

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