Singlet oxygen-based photoelectrochemical detection of DNA

被引:23
|
作者
Shanmugam, Saranya Thiruvottriyur [1 ,2 ]
Trashin, Stanislav [1 ,2 ]
De Wael, Karolien [1 ,2 ]
机构
[1] Univ Antwerp, Dept Bioengn, A Sense Lab, Groenenborgerlaan 171, B-2020 Antwerp, Belgium
[2] Univ Antwerp, NANOlab Ctr Excellence, Groenenborgerlaan 171, B-2020 Antwerp, Belgium
来源
关键词
Photoelectrochemistry; Singlet oxygen; Nucleic acids; DNA detection; METHYLENE-BLUE; ELECTROCHEMICAL DETECTION; QUANTUM YIELDS; FURFURYL ALCOHOL; LABEL-FREE; BIOSENSOR; MECHANISM; OXIDATION; BIOMARKER; MICRORNA;
D O I
10.1016/j.bios.2021.113652
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
The current work, designed for the photoelectrochemical detection of DNA, evaluates light-responsive DNA probes carrying molecular photosensitizers generating singlet oxygen (O-1(2)). We take advantage of their chromophore's ability to produce O-1(2) upon photoexcitation and subsequent photocurrent response. Type I, fluorescent and type II photosensitizers were studied using diode lasers at 406 nm blue, 532 nm green and 659 nm red lasers in the presensce and absence of a redox reporter, hydroquinone (HQ). Only type II photosensitizers (producing O-1(2)) resulted in a noticeable photocurrent in 1-4 nA range upon illumination, in particular, dissolved DNA probes labeled with chlorin e6 and erythrosine were found to give a well-detectable photocurrent response in the presence of HQ. Whereas, Type I photosensitizers and fluorescent chromophores generate negligible photocurrents (<0.15 nA). The analytical performance of the sensing system was evaluated using a magnetic beads-based DNA assay on disposable electrode platforms, with a focus to enhance the sensitivity and robustness of the technique in detecting complementary DNA targets. Amplified photocurrent responses in the range of 70-100 nA were obtained and detection limits of 17 pM and 10 pM were achieved using magnetic beads-captured chlorin e6 and erythrosine labeled DNA probes respectively. The presented novel photoelectrochemical detection can further be optimized and employed in applications for which enzymatic amplification such as polymerase chain reaction (PCR) is not applicable owing to their limitations and as an effective alternative to colorimetric detection when rapid detection of specific nucleic acid targets is required.
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收藏
页数:9
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