Tungsten disulfide nanosheet and exonuclease III co-assisted amplification strategy for highly sensitive fluorescence polarization detection of DNA glycosylase activity

被引:31
作者
Zhao, Jingjin [1 ]
Ma, Yefei [1 ]
Kong, Rongmei [2 ]
Zhang, Liangliang [1 ]
Yang, Wen [1 ]
Zhao, Shulin [1 ]
机构
[1] Guangxi Normal Univ, Educ Minist, Key Lab Chem & Mol Engn Med Resources, Guilin 541004, Peoples R China
[2] Qufu Normal Univ, Coll Chem & Chem Engn, Key Lab Life Organ Anal, Qufu 273165, Shandong, Peoples R China
关键词
Tungsten disulfide nanosheet; Exonuclease III; Fluorescence polarization; DNA glycosylase; BASE-EXCISION-REPAIR; SIGNAL-AMPLIFICATION; WS2; NANOSHEET; ENZYME-ACTIVITY; ANISOTROPY DETECTION; GOLD NANOPARTICLES; SENSING PLATFORM; NICKING ENZYME; URACIL REMOVAL; NUCLEIC-ACID;
D O I
10.1016/j.aca.2015.07.006
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Herein, we introduced a tungsten disulfide (WS2) nanosheet and exonuclease III (Exo III) co-assisted signal amplification strategy for highly sensitive fluorescent polarization (FP) assay of DNA glycosylase activity. Two DNA glycosylases, uracil-DNA glycosylase (UDG) and human 8-oxoG DNA glycosylase 1 (hOGG1), were tested. A hairpin-structured probe (HP) which contained damaged bases in the stem was used as the substrate. The removal of damaged bases from substrate by DNA glycosylase would lower the melting temperature of HP. The HP was then opened and hybridized with a FAM dye-labeled single strand DNA (DP), generating a duplex with a recessed 30-terminal of DP. This design facilitated the Exo III-assisted amplification by repeating the hybridization and digestion of DP, liberating numerous FAM fluorophores which could not be adsorbed on WS2 nanosheet. Thus, the final system exhibited a small FP signal. However, in the absence of DNA glycosylases, no hybridization between DP and HP was occurred, hampering the hydrolysis of DP by Exo III. The intact DP was then adsorbed on the surface of WS2 nanosheet that greatly amplified the mass of the labeled-FAM fluorophore, resulting in a large FP value. With the co-assisted amplification strategy, the sensitivity was substantially improved. In addition, this method was applied to detect UDG activity in cell extracts. The study of the inhibition of UDG was also performed. Furthermore, this method is simple in design, easy in implementation, and selective, which holds potential applications in the DNA glycosylase related mechanism research and molecular diagnostics. (C) 2015 Elsevier B.V. All rights reserved.
引用
收藏
页码:216 / 223
页数:8
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