Fluorometric determination of microRNA based on strand displacement amplification and rolling circle amplification

被引:0
|
作者
Yunlei Zhou
Bingchen Li
Minghui Wang
Jun Wang
Huanshun Yin
Shiyun Ai
机构
[1] Shandong Agricultural University,College of Chemistry and Material Science
[2] Shandong Agricultural University,College of Resources and Environment, Key Laboratory of Agricultural Environment in Universities of Shandong
来源
Microchimica Acta | 2017年 / 184卷
关键词
MicroRNA detection; Fluorescence assay; Signal amplification; SYBR Green II; DNA polymerase; Breast cancer; Serum samples;
D O I
暂无
中图分类号
学科分类号
摘要
The authors describe a fluorometric assay for microRNA. It is based on two-step amplification involving (a) strand displacement replication and (b) rolling circle amplification. The strand displacement amplification system is making use of template DNA (containing a sequence that is complementary to microRNA-21) and nicking enzyme sites. After hybridization, the microRNA strand becomes extended by DNA polymerase chain reaction and then cleaved by the nicking enzyme. The DNA thus produced acts as a primer in rolling circle amplification. Then, the DNA probe SYBR Green II is added to bind to ssDNA to generate a fluorescent signal which increases with increasing concentration of microRNA. The method has a wide detection range that covers the10 f. to 0.1 nM microRNA concentration range and has a detection limit as low as 1.0 fM. The method was successfully applied to the determination of microRNA-21 in the serum of healthy and breast cancer patients.
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页码:4359 / 4365
页数:6
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