PCR-coupled Paper-based Surface-enhanced Raman Scattering (SERS) Sensor for Rapid and Sensitive Detection of Respiratory Bacterial DNA

被引:56
|
作者
Lee, Hyo Geun [1 ,2 ]
Choi, Wook [1 ]
Yang, Seung Yun [2 ]
Kim, Dong-Ho [1 ]
Park, Sung-Gyu [1 ]
Lee, Min-Young [3 ,4 ]
Jung, Ho Sang [1 ]
机构
[1] Korea Inst Mat Sci KIMS, Adv Nanosurface Dept, Chang Won 51508, Gyeongnam, South Korea
[2] Pusan Natl Univ, Life & Ind Convergence Inst, Dept Biomat Sci, 1268-50 Samnangjin Ro, Miryang 50463, Gyeongnam, South Korea
[3] Samsung Med Ctr, Biomed Engn Res Ctr, 81 Irwon Ro, Seoul 06351, South Korea
[4] Sungkyunkwan Univ, Samsung Adv Inst Hlth Sci & Technol SAIHST, Dept Med Device Management & Res, 81 Irwon Ro, Seoul 06351, South Korea
关键词
Bacterial DNA detection; Surface Enhanced Raman Scattering; Point-of-Care test (POCT); Molecular Diagnostics; COMMUNITY-ACQUIRED PNEUMONIA; REAL-TIME PCR; STREPTOCOCCUS-PNEUMONIAE; MYCOPLASMA-PNEUMONIAE; INVERSE SENSITIVITY; GOLD NANOPARTICLES; ASSAY; MUTATIONS; SUBSTRATE; ELISA;
D O I
10.1016/j.snb.2020.128802
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
A paper-based surface-enhanced Raman scattering (SERS) substrate composed of silver-nanowires (AgNWs) was coupled with polymerase chain reaction (PCR) for rapid and sensitive determination of respiratory bacterial DNA. EvaGreen dye, which is a DNA intercalating molecule, was introduced to the low-cycled PCR product, and the difference in dye intercalation in the DNA structure was quantified by Raman spectroscopy to verify the presence of a target gene. Mycoplasma pneumoniae (M. Pne), was selected as a target for the sensing demonstration. At various gene concentrations and amplification cycles, detection capability of fluorescence-based realtime PCR (RT-PCR) and the PCR-coupled SERS method were compared to develop a DNA detection system capable of low-cycle amplification and sensitive DNA sensing. After 10 cycles, the PCR-coupled SERS method showed enhanced detection capability with a DNA detection limit of 3.12 pg/mu L. Then, the SERS substrate was prepared as a rapid kit that included a test line and negative and positive control lines. Target DNA after 10 cycles of amplification was successfully discriminated compared to non-target DNA and it was statistically relevant. The developed system is expected to be used as a detection method for various bacteria and viruses, and also be integrated with diverse POC diagnostic systems.
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页数:10
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