Bioluminescent Protein–Inhibitor Pair in the Design of a Molecular Aptamer Beacon Biosensing System
Author(s) -
Angeliki Moutsiopoulou,
David Broyles,
Hamdi Joda,
Emre Dikici,
Avinash Kaur,
Angel E. Kaifer,
Sylvia Daunert,
Sapna K. Deo
Publication year - 2020
Publication title -
analytical chemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.117
H-Index - 332
eISSN - 1520-6882
pISSN - 0003-2700
DOI - 10.1021/acs.analchem.0c00518
Subject(s) - bioluminescence , molecular beacon , chemistry , aptamer , biosensor , luciferase , substrate (aquarium) , quenching (fluorescence) , detection limit , combinatorial chemistry , biophysics , fluorescence , biochemistry , microbiology and biotechnology , chromatography , oligonucleotide , physics , dna , transfection , oceanography , quantum mechanics , gene , biology , geology
Although bioluminescent molecular beacons designed around resonance quenchers have shown higher signal-to-noise ratios and increased sensitivity compared with fluorescent beacon systems, bioluminescence quenching is still comparatively inefficient. A more elegant solution to inefficient quenching can be realized by designing a competitive inhibitor that is structurally very similar to the native substrate, resulting in essentially complete substrate exclusion. In this work, we designed a conjugated anti-interferon-γ (IFN-γ) molecular aptamer beacon (MAB) attached to a bioluminescent protein, Gaussia luciferase (GLuc), and an inhibitor molecule with a similar structure to the native substrate coelenterazine. To prove that a MAB can be more sensitive and have a better signal-to-noise ratio, a bioluminescence-based assay was developed against IFN-γ and provided an optimized, physiologically relevant detection limit of 1.0 nM. We believe that this inhibitor approach may provide a simple alternative strategy to standard resonance quenching in the development of high-performance molecular beacon-based biosensing systems.
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