Amplification-free detection of bacterial genes using a signaling probe-based DNA microarray

被引:16
作者
Taguchi, Tomoyuki [1 ]
Ishikawa, Machi [2 ]
Ichikawa, Momoko [2 ]
Tadenuma, Takashi [1 ]
Hirakawa, Yuko [1 ,2 ]
Yoshino, Tomoko [2 ]
Maeda, Yoshiaki [2 ]
Takeuchi, Hiyori [2 ]
Nojima, Daisuke [1 ]
Tanaami, Takeo [1 ]
Matsunaga, Tadashi [2 ,3 ]
Tanaka, Tsuyoshi [2 ]
机构
[1] Yokogawa Elect Corp, 2-9-32 Naka Cho, Musashino, Tokyo 1808750, Japan
[2] Tokyo Univ Agr & Technol, Inst Engn, Div Biotechnol & Life Sci, 2-24-16 Naka Cho, Koganei, Tokyo 1848588, Japan
[3] Japan Agcy Marine Earth Sci & Technol JAMSTEC, 2-15 Natsushima Cho, Yokosuka, Kanagawa 2370061, Japan
关键词
Signaling probes; DNA microarray; Amplification-free detection; 16S rDNA; 16S rRNA; FRET; AUTOMATED MICROARRAY; MASS-SPECTROMETRY; RAPID DETECTION; PERFORMANCE; SYSTEM; SENSOR; ACID; TIME;
D O I
10.1016/j.bios.2021.113659
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
In this study, we developed a novel DNA microarray system that does not require fluorophore-labeling, amplification, or washing of the target nucleic acid fragments. Two types of DNA probes (so-called "signaling probes") labeled with a fluorescence dye (Cy3) and quencher molecule (BHQ2) were spotted on the DNA microarray such that fluorescent signals of Cy3 could be quenched by BHQ2 due to duplex formation between the probes. The addition of the target DNA or RNA fragments disrupted the duplex formed by the probes, resulting in the generation of fluorescence signals. We examined the assay conditions of the signaling probe-based DNA microarray, including the design of the probes, hybridization temperatures, and methods for fragmentation of target molecules. Since this approach does not require time-consuming processes, including labeling, amplification, and washing, the assay achieved specific detection of 16S rDNA and 16S rRNA extracted from Escherichia coli within 60 min, which was significantly rapid compared to conventional PCR-dependent DNA microarrays.
引用
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页数:8
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