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Real-time apta-PCR for 20 000-fold improvement in detection limit

机译:实时荧光定量 apta-PCR 将检测限提高 20 000 倍

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摘要

A real-time apta-PCR for the ultrasensitive detection of thrombin is reported, where the thrombin aptamer acts not only as a biomolecular recognition element, but also as a label for amplification via real-time PCR. Aptamers can be easily converted to a reporter agent for detection by real-time PCR, simply via flanking of the aptamer's recognition moiety with primer sequences. The reported technique has the advantage of the ultrasensitivity achievable with immuno-PCR, but without the complications of addition of a DNA label, and is a technique generically applicable to all aptamers. Here, we use a sandwich format, where two existing thrombin binding aptamers with distinct binding epitopes have been utilised to capture and detect thrombin in a streptavidin-coated microtiter plate. The amount of thrombin is calculated from real-time PCR analysis of eluted captured reporter aptamer. However, the technique can also be used for aptamer-antibody sandwiches, or simply with single aptamers. A greater than 20 000-fold increase in sensitivity is achieved, highlighting the potential of this approach for the detection of very low levels of target analytes. The use of the aptamer itself as the reporter molecule eliminates the necessity of laborious enzyme/DNA labelling, facilitating a significantly more straightforward assay with a vastly enhanced sensitivity.
机译:报道了一种用于超灵敏检测凝血酶的实时 apta-PCR,其中凝血酶适配体不仅可作为生物分子识别元件,还可以作为通过实时荧光定量 PCR 扩增的标记物。核酸适配体可以很容易地转化为报告因子,以便通过实时荧光定量PCR进行检测,只需将适配体的识别部分与引物序列进行侧翼即可。所报道的技术具有免疫PCR可实现的超灵敏度的优点,但没有添加DNA标记的复杂性,并且是一种普遍适用于所有适配体的技术。在这里,我们使用三明治形式,其中两种现有的凝血酶结合适配体具有不同的结合表位,用于捕获和检测链霉亲和素包被的微量滴定板中的凝血酶。凝血酶的量是通过洗脱捕获的报告适配体的实时PCR分析计算的。然而,该技术也可用于适配体抗体三明治,或仅用于单个适配体。灵敏度提高了 20 000 倍以上,凸显了这种方法在检测极低水平目标分析物方面的潜力。使用适配体本身作为报告分子,消除了费力的酶/DNA标记的必要性,促进了更直接的检测,灵敏度大大提高。

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