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一种基于氧化石墨烯的荧光纳米传感器,可用于端粒酶活性的原位“开启”检测。

A facile graphene oxide-based fluorescent nanosensor for the in situ "turn-on" detection of telomerase activity.

机构信息

College of Chemistry, Nanchang University, Nanchang 330031, China.

出版信息

Analyst. 2018 May 15;143(10):2334-2341. doi: 10.1039/c8an00402a.

Abstract

A facile and sensitive method for the quantitative detection of telomerase and in situ imaging of intracellular telomerase is developed by using a graphene oxide (GO)-based fluorescent nanosensor. The nanosensor consists of a fluorescent DNA (P1) adsorbed on the GO surface. Here, GO serves not only as a fluorescence quencher but also as a carrier to successfully transport P1 into cancer cells as a signal reporter. P1 is a dye-labeled single-stranded DNA complementary to the telomeric repeated sequence, and initially the combination of P1 and GO exhibits minimal background fluorescence. When telomerase extends its repeat units of TTAGGG on the 3'-end of the primer-DNA, the fluorescence of P1 is subsequently recovered because the telomeric repeated sequence can hybridize with P1 and liberate it from the GO surface. This method enables the determination of telomerase activity down to 10 cells. For the in situ detection of telomerase, upon endocytosis of the P1/GO combinatorial probe into living cancer cells, the intracellular telomerase extends its primer to produce the telomeric repeated sequence and then turns on the fluorescence of P1, which can be directly monitored by confocal laser scanning microscopy. The feasibility of the assay is further investigated by treating with telomerase-related drugs, and the results demonstrate its potential in antitumor drug screening and cancer therapy evaluation.

摘要

一种基于氧化石墨烯(GO)的荧光纳米传感器被开发用于端粒酶的定量检测和细胞内端粒酶的原位成像,该方法简单灵敏。该纳米传感器由吸附在 GO 表面上的荧光 DNA(P1)组成。在这里,GO 不仅用作荧光猝灭剂,还用作载体,成功地将 P1 作为信号报告物运输到癌细胞中。P1 是一种与端粒重复序列互补的染料标记的单链 DNA,最初 P1 与 GO 的结合表现出最小的背景荧光。当端粒酶在引物-DNA 的 3'端延伸其 TTAGGG 重复单元时,P1 的荧光随后恢复,因为端粒重复序列可以与 P1 杂交并将其从 GO 表面释放出来。该方法能够检测到低至 10 个细胞的端粒酶活性。对于端粒酶的原位检测,当 P1/GO 组合探针被内吞进入活的癌细胞后,细胞内的端粒酶将其引物延伸产生端粒重复序列,然后打开 P1 的荧光,通过共聚焦激光扫描显微镜可以直接监测到 P1 的荧光。通过用端粒酶相关药物进行处理进一步研究了该测定法的可行性,结果表明其在抗肿瘤药物筛选和癌症治疗评估方面具有潜力。

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