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使用具有改进降噪算法的压电板传感器进行灵敏度为100 zM的DNA杂交检测。

DNA hybridization detection with 100 zM sensitivity using piezoelectric plate sensors with an improved noise-reduction algorithm.

作者信息

Kirimli Ceyhun E, Shih Wei-Heng, Shih Wan Y

机构信息

Lakehead University, Department of Chemistry, Thunder Bay, Canada.

出版信息

Analyst. 2014 Jun 7;139(11):2754-63. doi: 10.1039/c4an00215f.

Abstract

We have examined real-time, in situ hybridization detection of target DNA (tDNA) in a buffer solution and in urine using 8 μm-thick lead magnesium niobate-lead titanate (PMN-PT) piezoelectric plate sensors (PEPSs) about 1.1-1.2 mm long and 0.45 mm wide with improved 3-mercaptopropyltrimethoxysilane (MPS) insulation and a new multiple-parabola (>50) resonance peak position fitting algorithm. With probe DNA (pDNA) immobilized on the PEPS surface and by monitoring the first width extension mode (WEM) resonance frequency shift we detected tDNA in real time at concentration as low as 1 × 10(-19) M in urine (100 zM) with a signal to noise ratio (SNR) of 13 without DNA isolation and amplification at room temperature in 30 min. The present multiple-parabola fitting algorithm increased the detection of SNR by about 10 times compared to those obtained using the raw data and by about 5 times compared to those obtained using single parabola fitting. The detection was validated by in situ follow-up detection and subsequent visualization of fluorescent reporter microspheres (FRMs) coated with reporter DNA complementary to the tDNA but different from the probe pDNA.

摘要

我们使用长度约为1.1 - 1.2毫米、宽度为0.45毫米的8微米厚铌镁酸铅 - 钛酸铅(PMN - PT)压电板传感器(PEPSs),并采用改进的3 - 巯基丙基三甲氧基硅烷(MPS)绝缘层和一种新的多抛物线(>50)共振峰位置拟合算法,对缓冲溶液和尿液中的目标DNA(tDNA)进行了实时原位杂交检测。将探针DNA(pDNA)固定在PEPS表面,通过监测第一宽度扩展模式(WEM)共振频率偏移,我们在室温下30分钟内无需DNA分离和扩增,就能实时检测尿液中低至1×10⁻¹⁹ M(100 zM)浓度的tDNA,信噪比(SNR)为13。与使用原始数据相比,当前的多抛物线拟合算法将SNR的检测提高了约10倍,与使用单抛物线拟合相比提高了约5倍。通过原位后续检测以及对涂有与tDNA互补但与探针pDNA不同的报告DNA的荧光报告微球(FRMs)的可视化,验证了该检测方法。

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