Detection and Quantification of Tightly Bound Zn2+ in Blood Serum Using a Photocaged Chelator and a DNAzyme Fluorescent Sensor
Author(s) -
Shige Xing,
Yao Lin,
Liangyuan Cai,
Prem N. Basa,
Austin Shigemoto,
Chengbin Zheng,
Feng Zhang,
Shawn C. Burdette,
Yi Lu
Publication year - 2021
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.1c00140
Subject(s) - deoxyribozyme , chemistry , metal ions in aqueous solution , chelation , fluorescence , biomolecule , biosensor , metal , ion , combinatorial chemistry , nanotechnology , detection limit , inorganic chemistry , chromatography , biochemistry , organic chemistry , materials science , physics , quantum mechanics
DNAzymes have emerged as a powerful class of sensors for metal ions due to their high selectivity over a wide range of metal ions, allowing for on-site and real-time detection. Despite much progress made in this area, detecting and quantifying tightly bound metal ions, such as those in the blood serum, remain a challenge because the DNAzyme sensors reported so far can detect only mobile metal ions that are accessible to bind the DNAzymes. To overcome this major limitation, we report the use of a photocaged chelator, XDPAdeCage to extract the Zn 2+ from the blood serum and then release the chelated Zn 2+ into a buffer using 365 nm light for quantification by an 8-17 DNAzyme sensor. Protocols to chelate, uncage, extract, and detect metal ions in the serum have been developed and optimized. Because DNAzyme sensors for other metal ions have already been reported and more DNAzyme sensors can be obtained using in vitro selection, the method reported in this work will significantly expand the applications of the DNAzyme sensors from sensing metal ions that are not only free but also bound to other biomolecules in biological and environmental samples.
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