A lifetime-sensitive fluorescence anisotropy probe for DNA-based bioassays: The case of SYBR Green
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作者:
Chovelon, Benoit
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Univ Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
CNRS, DPM UMR 5063, F-38041 Grenoble, France
CHU Grenoble Site Nord, Inst Biol & Pathol, Dept Biochim Toxicol & Pharmacol, F-38041 Grenoble, FranceUniv Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
Chovelon, Benoit
[1
,2
,3
]
Fiore, Emmanuelle
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Univ Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
CNRS, DPM UMR 5063, F-38041 Grenoble, FranceUniv Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
Fiore, Emmanuelle
[1
,2
]
Faure, Patrice
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CHU Grenoble Site Nord, Inst Biol & Pathol, Dept Biochim Toxicol & Pharmacol, F-38041 Grenoble, France
Univ Grenoble Alpes, Lab Hypoxy Physiopathol Study, INSERM, U1042, F-38700 La Tronche, FranceUniv Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
Faure, Patrice
[3
,4
]
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Peyrin, Eric
[1
,2
]
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Ravelet, Corinne
[1
,2
]
机构:
[1] Univ Grenoble Alpes, DPM UMR 5063, F-38041 Grenoble, France
[2] CNRS, DPM UMR 5063, F-38041 Grenoble, France
[3] CHU Grenoble Site Nord, Inst Biol & Pathol, Dept Biochim Toxicol & Pharmacol, F-38041 Grenoble, France
[4] Univ Grenoble Alpes, Lab Hypoxy Physiopathol Study, INSERM, U1042, F-38700 La Tronche, France
In standard steady-state fluorescence anisotropy (FA) DNA-based assays, the ligand binding to a given receptor is typically signalled by the rotational correlation time changes of the tracer. Herein, we report a radically different strategy that relies on the peculiar excited state lifetime features of the SYBR Green (SG) dye. This DNA-binding probe exhibits a drastically short lifetime in solution, leading toe high FA signal. Its complexation to oligonucleotides determines a singular and very large depolarization depending on the concerted effects of extreme lifetime enhancement and resonance energy homotransfer. On the basis of ligand-induced changes in the molar fractions of bound and free forms of SG, the approach provides an unprecedented means for the FA monitoring of the ligand binding to short DNA molecules, allowing the elaboration of a variety of intercalator displacement assays and label-free biosensors that involve diverse DNA structures (duplex, hairpin, G-quadruplex and single-stranded), ligand types (ion, small organic molecule and protein) and binding modes (intercalation, minor groove, allosteric switch). These findings open up promising avenues in the design of a new generation of FA assays.
机构:
S China Normal Univ, Coll Biophoton, MOE Key Lab Laser Life Sci, Guangzhou 510631, Guangdong, Peoples R ChinaS China Normal Univ, Coll Biophoton, MOE Key Lab Laser Life Sci, Guangzhou 510631, Guangdong, Peoples R China
Zhu, Xiao
Xing, Da
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S China Normal Univ, Coll Biophoton, MOE Key Lab Laser Life Sci, Guangzhou 510631, Guangdong, Peoples R ChinaS China Normal Univ, Coll Biophoton, MOE Key Lab Laser Life Sci, Guangzhou 510631, Guangdong, Peoples R China
Xing, Da
OPTICS IN HEALTH CARE AND BIOMEDICAL OPTICS V,
2012,
8553