Label-Free Cross-Priming Amplification Coupled With Endonuclease Restriction and Nanoparticles-Based Biosensor for Simultaneous Detection of Nucleic Acids and Prevention of Carryover Contamination

被引:4
|
作者
Wang, Yi [1 ]
Sun, Lin [1 ]
Li, Jie-qiong [1 ]
Wang, Ze-ming [1 ]
Jiao, Wei-wei [1 ]
Xiao, Jing [1 ]
Shen, Chen [1 ]
Xu, Fang [1 ]
Qi, Hui [1 ]
Wang, Yong-hong [1 ]
Guo, Ya-jie [1 ]
Shen, A-dong [1 ]
机构
[1] Capital Medial Univ, Natl Clin Res Ctr Resp Dis,Key Lab Major Dis Chil, Beijing Key Lab Pediat Resp Infect Dis,Beijing Ch, Beijing Pediat Res Inst,Natl Ctr Childrens Hlth,M, Beijing, Peoples R China
来源
FRONTIERS IN CHEMISTRY | 2019年 / 7卷
关键词
cross-priming amplification; endonuclease restriction; lateral flow biosensor; S; aureus; limit of detection; LATERAL FLOW BIOSENSOR; ISOTHERMAL AMPLIFICATION; RAPID DETECTION;
D O I
10.3389/fchem.2019.00322
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Here, we reported on a label-free cross-priming amplification (CPA) scheme that utilized endonuclease restriction for simultaneous detection of nucleic acids and elimination of carryover contamination. Reaction mixtures were detected in a nanoparticle-based lateral flow biosensor (LFB). The assay exhibited attractive traits in that it did not require the use of labeled primers or labeled probes, and thus, the technique could prevent undesired results arising from unwanted hybridization between labeled primers or between a probe and labeled primer. Isothermal amplification and endonuclease restriction digestion were conducted in a single pot, and the use of a closed-tube amplification removed false-positive results due to contaminants. To validate the assay's applicability, we employed the novel technique to detect the pathogen Staphylococcus aureus in pure cultures and artificial blood samples. The assay could detect target bacterium in pure culture with a 100 fg.mu L-1 detection limit, and in spiked blood samples with a 700 cfu.mL(-1) detection limit. The whole process, including sample procedure (20-min), isothermal amplification (60-min), endonuclease digestion (10-min) and result reporting (within 2-min), could be finished within 95-min. As a poof-of-concept assay, the technique devised in the current report could be employed for detecting various other sequences if the specific CPA primers were available.
引用
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页数:11
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