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利用阳离子共轭聚合物对单核苷酸多态性进行荧光和可视化检测。

Fluorescence and visual detection of single nucleotide polymorphism using cationic conjugated polyelectrolyte.

机构信息

Department of Chemical and Biomolecular Engineering, 4 Engineering Drive 4, National University of Singapore, Singapore 117567, Singapore.

出版信息

Langmuir. 2012 Jan 10;28(1):889-95. doi: 10.1021/la203714e. Epub 2011 Dec 5.

DOI:10.1021/la203714e
PMID:22047010
Abstract

We report a simple assay for visual detection of single nucleotide polymorphisms (SNPs) with good sensitivity and selectivity. The selectivity is determined by Escherichia coli (E. coli) DNA ligase mediated circular formation upon recognition of the point mutation on DNA targets. Rolling cycle amplification (RCA) of the perfect-matched DNA target is then initiated using the in situ formed circular template in the presence of Phi29 enzyme. Due to amplification of the DNA target, the RCA product has a tandem-repeated sequence, which is significantly longer than that for the SNP strand. Direct addition of a cationic conjugated polymer of poly[9,9'-bis(6'-(N,N,N-trimethylammonium)hexyl)fluorene-co-9,9'-bis(2-(2-(2-(N,N,N-trimethylammonium)ethoxyl)-ethoxy)-ethyl)fluorene tetrabromide] containing 20 mol% 2,1,3-benzothiadiazole (PFBT(20)) into the RCA solution leads to blue-whitish fluorescent color for SNP strand and yellowish fluorescent color for amplified DNA, due to PFBT(20)/DNA complexation induced intrachain/interchain energy transfer. To further improve the contrast for visual detection, FAM-labeled peptide nucleic acid (PNA) was hybridized to each amplified sequence, which is followed by the addition of poly{2,7-[9,9-bis(6'-N,N,N-trimethylammoniumhexyl)]fluorene-co-2,5-difluoro-1,4-phenylene dibromide} (PFP). The PNA/DNA hybridization brings PFP and FAM-PNA into close proximity for energy transfer, and the solution fluorescent color appears green in the presence of target DNA with a detection limit of 1 nM, which is significantly improved as compared to that for most reported visual SNP assay.

摘要

我们报道了一种简单的用于视觉检测单核苷酸多态性(SNP)的分析方法,该方法具有良好的灵敏度和选择性。该选择性是通过大肠杆菌(E. coli)DNA 连接酶在识别 DNA 靶标上的点突变时介导的环形形成来确定的。然后,在Phi29 酶存在下,使用原位形成的环形模板启动完美匹配的 DNA 靶标的滚环扩增(RCA)。由于 DNA 靶标的扩增,RCA 产物具有串联重复序列,其长度明显长于 SNP 链。阳离子共轭聚合物聚[9,9'-双(6'-(N,N,N-三甲基铵)己基)芴-共-9,9'-双(2-(2-(2-(N,N,N-三甲基铵)乙氧基)-乙氧基)-乙基)芴四溴化物](PFBT(20))直接添加到 RCA 溶液中,导致 SNP 链呈蓝白色荧光,扩增 DNA 呈黄色荧光,这是由于 PFBT(20)/DNA 复合物诱导的链内/链间能量转移。为了进一步提高视觉检测的对比度,将 FAM 标记的肽核酸(PNA)杂交到每个扩增序列上,然后加入聚{2,7-[9,9-双(6'-N,N,N-三甲基己基)芴-共-2,5-二氟-1,4-亚苯基二溴化物}(PFP)。PNA/DNA 杂交使 PFP 和 FAM-PNA 靠近以进行能量转移,并且在存在靶 DNA 的情况下溶液荧光颜色呈现绿色,检测限为 1 nM,与大多数报道的视觉 SNP 分析相比,这一检测限有了显著提高。

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