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通过探针延伸开发超灵敏电化学生物传感器,用于检测人血清中的基因组 DNA。

Ultrasensitive Electrochemical Biosensor Developed by Probe Lengthening for Detection of Genomic DNA in Human Serum.

机构信息

The Centralab , The First Affiliated Hospital of Fujian Medical University , Fuzhou 350005 , China.

Department of Pharmaceutical Analysis, Higher Educational Key Laboratory for Nano Biomedical Technology of Fujian Province, Faculty of Pharmacy , Fujian Medical University , Fuzhou 350122 , China.

出版信息

Anal Chem. 2019 Apr 2;91(7):4552-4558. doi: 10.1021/acs.analchem.8b05692. Epub 2019 Mar 14.

DOI:10.1021/acs.analchem.8b05692
PMID:30838849
Abstract

As an alternative to most of the reported nucleic acid amplification-based electrochemical DNA biosensors used for detection of trace levels of genomic DNA, we herein present a novel detection concept. The proposed system involves the conversion of two short double-stranded DNAs (dsDNAs), labeled with a thiol-tag or biotin-tag, into a single integrated dsDNA containing thiol and biotin at both terminals in the presence of target DNA through ligase chain reaction (LCR) and followed by the immobilization of these integrated dsDNAs on a bovine serum albumin (BSA)-modified gold electrode surface. Owing to rapid depletion of the two short dsDNAs via LCR, the integrated dsDNAs were generated in an exponential manner so that this sensoring approach offered a limit of detection of 25 yoctomoles (15 copies in 50 μL sample volumes), a high discrimination of single-base mismatch and a wide linear concentration range (across 6 orders of magnitude) for target DNA. Significantly, the proposed sensor, which has simplicity in operation and ease of miniaturization, detected the target of interest in total nucleic acid extracts derived from clinical serum samples with excellent results, thereby demonstrating its considerable diagnostic potential in fields ranging from virus detection to the diagnosis of genetic diseases.

摘要

与大多数用于痕量基因组 DNA 检测的基于核酸扩增的电化学生物 DNA 生物传感器不同,我们在此提出了一种新的检测概念。该系统涉及在目标 DNA 的存在下,通过连接酶链反应 (LCR) 将两个带有硫醇标记或生物素标记的短双链 DNA (dsDNA) 转化为含有两端硫醇和生物素的单个整合 dsDNA,然后将这些整合 dsDNA 固定在牛血清白蛋白 (BSA) 修饰的金电极表面上。由于 LCR 快速耗尽了两个短 dsDNA,因此整合的 dsDNA 以指数方式产生,因此这种传感方法的检测限为 25 zeptomoles(50 μL 样品体积中的 15 个拷贝),对单碱基错配具有高度的区分度,并且对目标 DNA 的线性浓度范围很宽(跨越 6 个数量级)。重要的是,该传感器操作简单,易于小型化,可从临床血清样本的总核酸提取物中检测到感兴趣的靶标,从而证明了其在从病毒检测到遗传疾病诊断等领域的巨大诊断潜力。

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