Colorimetric detection of microRNA based on DNAzyme and nuclease-assisted catalytic hairpin assembly signal amplification

被引:30
|
作者
Zhang, Hongmei [1 ,2 ]
Wang, Kuiyu [1 ,2 ]
Bu, Shengjun [2 ]
Li, Zhongyi [2 ]
Ju, Chuanjing [3 ,4 ]
Wan, Jiayu [2 ]
机构
[1] Heilongjiang Bayi Agr Univ, Daqing 163319, Peoples R China
[2] Acad Mil Med Sci, Inst Mil Vet, Changchun 130122, Jilin, Peoples R China
[3] FAW, Gen Hosp, Changchun 130011, Jilin, Peoples R China
[4] Jilin Univ, Hosp 4, Changchun 130011, Jilin, Peoples R China
关键词
MicroRNAs detection; Duplex-specific nuclease; Catalytic hairpin assembly; DNAzyme; DUPLEX-SPECIFIC NUCLEASE; SENSITIVE DETECTION; ASSAY; STRATEGY; SENSOR; PROBE;
D O I
10.1016/j.mcp.2018.02.002
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Accurate and quantitative analysis of microRNA (miRNA) expression is critical for the diagnostics and theranostics of a disease. Herein, a proof-of-concept of a colorimetric horseradish peroxidase-mimicking DNAzyme (HRP-DNAzyme) biosensor for miRNA assay based on nuclease-assisted catalytic hairpin assembly (CHA) signal amplification was demonstrated. Duplex-specific nuclease (DSN) was employed to cleave the single-stranded DNA (ssDNA) chimeric probe (CP) on the magnetic bead (MB) surface via hybridization of the CP and target miRNA. The regenerated miRNA can cleave a large number of ssDNA CP to produce CHA initiator sequence fragments. The CP consists of two main regions: a target miRNA recognition DNA sequence at the 5' end and a CHA initiator (CI) sequence at the 3' end. The catalyzed assembly process of CHA produces a large amount of G-rich DNA. In the presence of hemin, the G-rich DNA forms G-quadruplex/hemin complex and mimics the horseradish peroxidase activity, which catalyzes a colorimetric reaction. For the proof-of-concept, microRNA-21 (miR-21) was selected as the model target to authenticate this strategy as a versatile assay platform. The proposed strategy allowed quantitation of the sequence specificity of miRNA-21 with a detection limit of 9.2 fM in a dynamic range from 10 fM-1 nM, with an excellent ability to discriminate the differences in miRNAs. Additionally, the miRNA assay in real samples was satisfactory, thereby confirming its applicability. Therefore, this method exhibited a great potential as a miRNA quantification method in biomedical research and clinical diagnosis.
引用
收藏
页码:13 / 18
页数:6
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