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使用磁调制生物传感器快速灵敏地检测重复核酸序列

Rapid and Sensitive Detection of Repetitive Nucleic Acid Sequences Using Magnetically Modulated Biosensors.

作者信息

Margulis Michael, Danielli Amos

机构信息

Faculty of Engineering, The Institute of Nanotechnology and Advanced Materials, Bar-Ilan University, Max and Anna Webb Street, Ramat Gan 5290002, Israel.

出版信息

ACS Omega. 2019 Jul 8;4(7):11749-11755. doi: 10.1021/acsomega.9b01071. eCollection 2019 Jul 31.

Abstract

Repetitive DNA sequences are abundant in the genome of most biological species. These sequences are naturally "preamplified", which makes them a preferential target for a variety of biological assays. Current methods to detect specific DNA sequences are based on the quantitative polymerase chain reaction (PCR), which relies on target amplification by polymerase and uses a fluorescent resonance energy transfer (FRET)-based probe. Here, to rapidly detect a repetitive DNA sequence, we combine a highly sensitive magnetic modulation biosensing (MMB) system and a modified double-quenched FRET-based probe. The high numbers of copies of the female-specific I sequence of the domestic chicken (), combined with the low background fluorescence levels of the modified double-quenched probe and the high sensitivity of the MMB system, allow us to determine the chick sex in ovo within 13 min, with 100% sensitivity and specificity. Compared to quantitative PCR, the presented assay is 4-9 times faster. More broadly, by specifically tailoring the primers and probe, the proposed assay can detect any target DNA sequence, either repetitive or nonrepetitive.

摘要

重复DNA序列在大多数生物物种的基因组中都很丰富。这些序列会自然地“预扩增”,这使得它们成为各种生物学检测的优先目标。当前检测特定DNA序列的方法基于定量聚合酶链反应(PCR),该方法依靠聚合酶进行目标扩增,并使用基于荧光共振能量转移(FRET)的探针。在此,为了快速检测重复DNA序列,我们将高灵敏度磁调制生物传感(MMB)系统与一种改良的基于双淬灭FRET的探针相结合。家鸡雌性特异性I序列的大量拷贝,再加上改良双淬灭探针的低背景荧光水平以及MMB系统的高灵敏度,使我们能够在13分钟内对鸡胚进行性别鉴定,灵敏度和特异性均为100%。与定量PCR相比,本文所展示的检测方法快4至9倍。更广泛地说,通过专门定制引物和探针,所提出的检测方法可以检测任何目标DNA序列,无论是重复的还是非重复的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4c4d/6682110/426855aaddf1/ao-2019-01071y_0001.jpg

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