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Nucleic Acid Sandwich Hybridization Assay with Quantum Dot-Induced Fluorescence Resonance Energy Transfer for Pathogen Detection

机译:量子点诱导荧光共振能量转移的核酸夹心杂交检测病原体

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摘要

This paper reports a nucleic acid sandwich hybridization assay with a quantum dot (QD)-induced fluorescence resonance energy transfer (FRET) reporter system. Two label-free hemagglutinin H5 sequences (60-mer DNA and 630-nt cDNA fragment) of avian influenza viruses were used as the targets in this work. Two oligonucleotides (16 mers and 18 mers) that specifically recognize two separate but neighboring regions of the H5 sequences were served as the capturing and reporter probes, respectively. The capturing probe was conjugated to QD655 (donor) in a molar ratio of 10:1 (probe-to-QD), and the reporter probe was labeled with Alexa Fluor 660 dye (acceptor) during synthesis. The sandwich hybridization assay was done in a 20 μL transparent, adhesive frame-confined microchamber on a disposable, temperature-adjustable indium tin oxide (ITO) glass slide. The FRET signal in response to the sandwich hybridization was monitored by a homemade optical sensor comprising a single 400 nm UV light-emitting diode (LED), optical fibers, and a miniature 16-bit spectrophotometer. The target with a concentration ranging from 0.5 nM to 1 μM was successfully correlated with both QD emission decrease at 653 nm and dye emission increase at 690 nm. To sum up, this work is beneficial for developing a portable QD-based nucleic acid sensor for on-site pathogen detection.
机译:本文报道了一种利用量子点(QD)诱导的荧光共振能量转移(FRET)报告系统进行的核酸夹心杂交检测方法。禽流感病毒的两个无标记血凝素H5序列(60-mer DNA和630-nt cDNA片段)被用作这项工作的目标。特异性识别H5序列的两个单独但相邻区域的两个寡核苷酸(16聚体和18聚体)分别用作捕获探针和报告探针。将捕获探针以10:1(探针与QD)的摩尔比与QD655(供体)结合,并在合成过程中用Alexa Fluor 660染料(受体)标记报告探针。三明治杂交测定法是在一次性的,温度可调节的铟锡氧化物(ITO)载玻片上的20μL透明,粘着框架限定的微腔中进行的。通过自制的光学传感器监测响应三明治杂交的FRET信号,该传感器包括一个400 nm的紫外线发光二极管(LED),光纤和一个微型16位分光光度计。浓度范围从0.5 nM到1μM的目标与653 nm处QD发射减少和690 nm处染料发射增加成功相关。综上所述,这项工作对于开发用于现场病原体检测的基于QD的便携式核酸传感器是有益的。

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