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Sensitive detection of p53 DNA based on spatially confined fluorescence resonance energy transfer and multivalent assembly of branched DNAElectronic supplementary information (ESI) available. See DOI: 10.1039/d1ay01110c

Authors :
Liu, Yeling
Sun, Xia
Yuan, Hui
Liu, Bingxin
Zhou, Bingqian
Chen, Xuening
Li, Xia
Xue, Qingwang
Source :
Analytical Methods; 2021, Vol. 13 Issue: 37 p4314-4319, 6p
Publication Year :
2021

Abstract

A key challenge for the discrete distribution-based Förster resonance energy transfer system (D-FRET) is the reduced intensity and stability of signal probes in complex biological matrices. Here, we present a spatially confined FRET (SC-FRET) probe with a stable structure and strong signal output. It consists of multivalent FRET pairs labeled with FAM or TAMRA. In this assay, p53 DNA was chosen as a model hairpin probe (HP), and two kinds of branched DNA probes (ssDNA-FAM, ssDNA-TAMRA) were involved. Under the action of p53 DNA, the unfolded HP acts as a primer to initiate polymerization extension of KFP polymerase and cleavage of Nb.BbvCI endonuclease, which produces plenty of ssDNA (primer-DNA). The branched DNA is designed to have the same binding core and different sticky ends, the core part of which can self-assemble to form X-shaped branched DNA (X-FAM or X-TAMRA), and the sticky ends of which are complementary to the primer-DNA. Therefore, the primer-DNAs released during the polymerization cleavage process will combine a large number of X-FAM and X-TAMRA in a limited space through complementary base pairing. Fluorescence was transferred from FAM to TAMRA, and a strong FRET response was generated by the locational effects. The proposed SC-FRET system based on the multivalent assembly of branched DNA exhibited a strong FRET response with an LOD of 0.01394 pM. Importantly, it also showed a high-contrast and stable FRET response in HeLa cells. Its superior biological stability is attributed to the large steric hindrance of the compact and rigid frame of the SC-FRET probe, which helps prevent intracellular degradation and provides a powerful tool for biomedical research.

Details

Language :
English
ISSN :
17599660 and 17599679
Volume :
13
Issue :
37
Database :
Supplemental Index
Journal :
Analytical Methods
Publication Type :
Periodical
Accession number :
ejs57937461
Full Text :
https://doi.org/10.1039/d1ay01110c