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具有额外染料结合位点的单链DNA探针配对适体传感器,以增强其在目标化合物存在时的荧光响应。

Single-stranded DNA probe paired aptasensor with extra dye binding sites to enhance its fluorescence response in the presence of a target compound.

作者信息

Cho Seo Won, Lim Hyun Jeong, Chua Beelee, Son Ahjeong

机构信息

Department of Environmental Science and Engineering, Ewha Womans University 52 Ewhayeodae-gil, Seodaemun-gu Seoul 03760 Republic of Korea

Department of Civil and Environmental Engineering, University of Wisconsin-Madison Madison WI 53706 USA.

出版信息

RSC Adv. 2021 Jun 21;11(35):21796-21804. doi: 10.1039/d1ra00971k. eCollection 2021 Jun 15.

Abstract

The purpose of this study is to investigate the possibility of improving the performance of a DNA binding dye water quenching based aptasensor without changing or truncating the aptamer. To demonstrate the possibility of increasing the change in fluorescence of the aptasensor by pairing it with a suitable ssDNA probe, three ssDNA probes (probe 1, 2, and 3) were employed and the fluorescence from the bound dyes was measured. This showed that ssDNA probe 2 created the most additional binding sites. By varying the target compound concentration (0, 0.05, 0.5, 5, 50, and 500 mg L 4--nonylphenol), the corresponding change in the fluorescence signal of the unpaired and ssDNA probe paired aptasensors were measured and compared over a range of emission wavelengths. The response of all three ssDNA probe paired aptasensors showed good fit ( = 0.88-0.92) to a logarithmic response. The sensitivity of the aptasensor paired with ssDNA probe 2 was improved by ∼60%, whereas that of the aptasensor paired with ssDNA probe 3 was only improved by a marginal ∼3%. This study is a demonstration of using an appropriate ssDNA probe to increase the number of binding sites and hence the performance of a DNA binding dye and water quenched aptasensor. It is a possibility that can be extended to similar aptasensors without having to change or truncate the aptamer.

摘要

本研究的目的是在不改变或截断适配体的情况下,研究提高基于DNA结合染料水猝灭的适配体传感器性能的可能性。为了证明通过将适配体传感器与合适的单链DNA探针配对来增加其荧光变化的可能性,使用了三种单链DNA探针(探针1、2和3),并测量了结合染料的荧光。结果表明,单链DNA探针2产生了最多的额外结合位点。通过改变目标化合物浓度(0、0.05、0.5、5、50和500 mg L⁻¹——壬基酚),在一系列发射波长范围内测量并比较了未配对和与单链DNA探针配对的适配体传感器荧光信号的相应变化。所有三种与单链DNA探针配对的适配体传感器的响应均显示出与对数响应的良好拟合(R² = 0.88 - 0.92)。与单链DNA探针2配对的适配体传感器的灵敏度提高了约60%,而与单链DNA探针3配对的适配体传感器的灵敏度仅提高了约3%。本研究证明了使用合适的单链DNA探针来增加结合位点数量,从而提高DNA结合染料和水猝灭适配体传感器的性能。这种可能性可以扩展到类似的适配体传感器,而无需改变或截断适配体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/231b/9034146/c6db2984f5c7/d1ra00971k-f1.jpg

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