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A novel screening method for competitive FRET-aptamers applied to E. coli assay development

机译:一种用于竞争性FRET适配子的新型筛选方法,用于大肠杆菌测定开发

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摘要

A novel high-throughput screening method is described in which a family of DNA aptamers selected against E. coli outer membrane proteins (OMPs) is subjected to PCR in the presence of fluorophore-dUTP conjugates using Deep Vent? exo- polymerase. The fluorophore-doped aptamers and their complementary strands are then heated to render them single-stranded and screened in filter well microtiter plates for fluorescence resonance energy transfer (FRET) assay potential. Using this system, a superior competitive FRET-aptamer designated EcO 4R was identified and the location of its putative binding pocket was determined by individually testing FRET potential in each of the secondary loop structures. By labeling the binding pocket with Alexa Fluor (AF) 647 and binding the aptamer to heavily Black Hole Quencher-3 (BHQ-3)-labeled E. coli bacteria, detection of as few as 30 live unlabeled E. coli per ml was achieved in a competitive displacement FRET assay format. The far red fluorescence emission enables detection in largely blue-green autofluorescent matrices. In addition, the competitive transfer of AF 647-EcO-4R aptamer to unlabeled E. coli cells after a 15 min equilibration period was verified by fluorescence microscopy. The present study also demonstrated that high aptamer affinity is not well correlated with competitive FRET potential.
机译:描述了一种新颖的高通量筛选方法,其中在存在荧光团-dUTP缀合物的情况下,使用Deep Vent?将针对大肠杆菌外膜蛋白(OMPs)选择的DNA适体家族进行PCR。外聚合酶。然后将荧光团掺杂的适体及其互补链加热,使其成为单链,并在滤池微量滴定板中进行筛选,以进行荧光共振能量转移(FRET)分析。使用该系统,鉴定出了称为EcO 4R的极具竞争力的FRET适体,并通过单独测试每个次级环结构中的FRET电位来确定其推定结合口袋的位置。通过用Alexa Fluor(AF)647标记结合口袋,并将适体与黑洞Quencher-3(BHQ-3)标记的大量大肠杆菌结合,每毫升可检测到多达30个未标记的活大肠杆菌以竞争性置换FRET分析形式进行。远红色荧光发射使您可以在很大程度上是蓝绿色的自发荧光基质中进行检测。另外,在15分钟的平衡期后,通过荧光显微镜验证了AF 647-EcO-4R适体向未标记的大肠杆菌细胞的竞争性转移。本研究还表明,高适体亲和力与竞争性FRET潜能没有很好的相关性。

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