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将DNA共价固定在丝网印刷电极网络上,用于直接无标记检测p53序列的杂交。

DNA covalent immobilization onto screen-printed electrode networks for direct label-free hybridization detection of p53 sequences.

作者信息

Marquette C A, Lawrence M F, Blum L J

机构信息

Laboratoire de Génie Enzymatique et Biomoléculaire, UMR CNRS 5013 Bat. CPE Université Claude Bernard Lyon 1, Villeurbanne, France.

出版信息

Anal Chem. 2006 Feb 1;78(3):959-64. doi: 10.1021/ac051585o.

DOI:10.1021/ac051585o
PMID:16448075
Abstract

A new electrochemical biochip for the detection of DNA sequences was developed. The entire biochip-i.e., working, reference, and counter electrodes-was constructed based on the screen-printing technique and exhibits eight working electrodes that could be individually addressed and grafted through a simple electrochemical procedure. Screen-printed electrode networks were functionalized electrochemically with 1-ethyl-3-(3dimethylaminopropyl)carbodidiimide according to a simple procedure. Single-stranded DNA with a C6-NH(2) linker at the 5'-end was then covalently bound to the surface to act as probe for the direct, nonlabeled, detection of complementary strands in a conductive liquid medium. In the present system, the study was focused on a particular codon (273) localized in the exon 8 of the p53 gene (20 mer, TTGAGGTGCATGTTTGTGCC). The integrity of the immobilized probes and its ability to capture target sequences was monitored through chemiluminescent detection following the hybridization of a peroxidase-labeled target. The grafting of the probe at the electrode surface was shown to generate significant shifts of the Nyquist curves measured in the 10-kHz to 80-Hz range. These variations of the faradaic impedance were found to be related to changes of the double layer capacitance of the electrochemical system's equivalent circuit. Similarly, hybridization of complementary strands was monitored through the measurements of these shifts, which enabled the detection of target sequences from 1 to 200 nM. Discrimination between complementary, noncomplementary, and single-nucleotide mismatch targets was easily accomplished.

摘要

开发了一种用于检测DNA序列的新型电化学生物芯片。整个生物芯片,即工作电极、参比电极和对电极,基于丝网印刷技术构建,具有八个工作电极,这些电极可通过简单的电化学程序单独寻址和接枝。丝网印刷电极网络根据简单程序用1-乙基-3-(3-二甲氨基丙基)碳二亚胺进行电化学功能化。然后将5'-端带有C6-NH(2)接头的单链DNA共价结合到表面,作为在导电液体介质中直接、无标记检测互补链的探针。在本系统中,研究集中在位于p53基因外显子8中的一个特定密码子(273)(20聚体,TTGAGGTGCATGTTTGTGCC)。通过过氧化物酶标记的靶标杂交后的化学发光检测,监测固定化探针的完整性及其捕获靶标序列的能力。结果表明,探针在电极表面的接枝会使在10 kHz至80 Hz范围内测量的奈奎斯特曲线发生显著偏移。发现这些法拉第阻抗的变化与电化学系统等效电路的双层电容变化有关。同样,通过测量这些偏移来监测互补链的杂交,从而能够检测1至200 nM的靶标序列。互补、非互补和单核苷酸错配靶标之间的区分很容易实现。

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