Cyclometalated Iridium(III) Complex-Sensitized NiO-Based-Cathodic Photoelectrochemical Platform for DNA Methyltransferase Assay

被引:9
作者
Cai, Yueyuan [1 ]
Zhang, Yingtao [1 ]
Wang, Huan [1 ]
Lin, Xiaojia [1 ]
Yu, Kunpeng [1 ]
Li, Chunxiang [1 ]
Jie, Guifen [1 ]
机构
[1] Qingdao Univ Sci & Technol, Key Lab Opt Elect Sensing & Analyt Chem Life Sci, Shandong Key Lab Biochem Anal,MOE, Key Lab Analyt Chem Life Sci Univ Shandong,Coll C, Qingdao 266042, Peoples R China
关键词
cyclometalated Ir(III) complex-sensitized NiO; photocathodic bioanalysis; catalytic hairpin assembly; DNA adenine methyltransferase; hybridization chain reaction; ULTRASENSITIVE DETECTION; IMMUNOSENSING PLATFORM; SIGNAL AMPLIFICATION; STRAND DISPLACEMENT; HOLE INJECTION; EXCITED-STATE; DYE; LIGHT; PHOTOCATHODE; GENERATION;
D O I
10.1021/acsabm.1c00445
中图分类号
TB3 [工程材料学];
学科分类号
0805 ; 080502 ;
摘要
This work reports an efficient [(C-6)(2)Ir(dppz)]+PF6- (C6 = coumarin 6 and dppz = dipyridophenazine)-sensitized NiO photocathode and its application in photoelectrochemical (PEC) bioanalysis field for the first time. This dye-sensitized NiO photocathode was found to exhibit a markedly enhanced cathodic photocurrent. A sensitive cathodic PEC platform was proposed integrating the as-prepared photocathode with enzyme-free cascaded amplification strategies of the catalytic hairpin assembly (CHA) and the hybridization chain reaction (HCR) for DNA methyltransferase (MTase) assay. A hairpin DNA(HDam) with specific recognition site of Dam MTase in its stem was designed. The site of HDam was methylated in the presence of Dam MTase and then cut by endonuclease DpnI. The released loop fragment, as an initiator, triggered the CHA circuit and the follow-up HCR circuit, resulting in long dsDNA concatemers on the ITO electrode. Numerous [(C-6)(2)Ir(dppz)]+PF6- were intercalated into dsDNA, and highly efficient signal amplification was realized. Benefiting from the superior iridium(III) complex-sensitized NiO photocathode and effective amplification strategy, a detection limit of 0.0028 U/mL for the determination of Dam MTase was achieved. Moreover, this work further demonstrated that these proposed tactics could be applied to screen Dam MTase activity inhibitors.
引用
收藏
页码:6103 / 6111
页数:9
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