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基于 λ 外切酶辅助信号扩增的 DNA 电化学生物传感器检测表皮生长因子受体基因状态。

Detection of Epidermal Growth Factor Receptor Gene Status via a DNA Electrochemical Biosensor Based on Lambda Exonuclease-assisted Signal Amplification.

机构信息

Department of Pharmacy, First Affiliated Hospital of Fujian Medical University, Fuzhou, Fujian, 350005, PR, China.

Department of Pharmaceutical Analysis, Fujian Medical University, Fuzhou, Fujian, 350004, PR, China.

出版信息

Anal Sci. 2020 Jun 10;36(6):697-701. doi: 10.2116/analsci.19P422. Epub 2019 Dec 20.

DOI:10.2116/analsci.19P422
PMID:31866610
Abstract

Based on our previous work, we have constructed a new electrochemical biosensor to detect epidermal growth factor receptor (EGFR) gene mutation, which was a significant therapeutic effect predictor of target drugs for non-small cell lung cancer. In order to lower the detection limit to detect the small amount of EGFR gene status, we have employed lambda exonuclease (λ-Exo) to form a hybridization-digestion cycle. The reaction stages are depicted as follows: the target DNA hybridized with auxiliary DNA which had been modified with the λ-Exo recognition site; then, the double strands were cleaved by λ-Exo. The target DNA was released completely, and continued to hybridize with remaining auxiliary DNA, which formed a recycle for target reutilization. Finally, we detected the remaining auxiliary DNA to evaluate the amount or status of the EGFR gene. The reutilization of target DNA will help to achieve an enlarged signal with a small amount of target DNA, and the detection limit of the biosensor decreased down to 10 pM. Meanwhile, our assay can differentiate wild genes from the mutational gene of EGFR with excellent specificity. Our signal amplification method provides a research foundation for the detection system of the electrochemical biosensor by employing exonuclease, and impels the biosensor to be developed as a suitable method for EGFR detection in clinical applications.

摘要

基于我们之前的工作,我们构建了一种新的电化学生物传感器来检测表皮生长因子受体(EGFR)基因突变,这是预测非小细胞肺癌靶向药物治疗效果的重要指标。为了降低检测限以检测少量 EGFR 基因状态,我们利用λ核酸外切酶(λ-Exo)形成杂交-消化循环。反应阶段如下:目标 DNA 与带有 λ-Exo 识别位点的辅助 DNA 杂交;然后,双链被 λ-Exo 切割。目标 DNA 被完全释放,并继续与剩余的辅助 DNA 杂交,形成目标再利用的循环。最后,我们检测剩余的辅助 DNA 来评估 EGFR 基因的数量或状态。目标 DNA 的再利用有助于实现少量目标 DNA 的信号放大,生物传感器的检测限降低到 10 pM。同时,我们的测定法具有优异的特异性,可以区分野生基因和 EGFR 的突变基因。我们的信号放大方法为采用核酸外切酶的电化学生物传感器检测系统提供了研究基础,并推动生物传感器发展成为临床应用中 EGFR 检测的合适方法。

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