A label-free T4 polynucleotide kinase fluorescence sensor based on split dimeric G-quadruplex and ligation-induced dimeric G-quadruplex/thioflavin T conformation

硫黄素 化学 DNA G-四倍体 DNA连接酶 单体 荧光 脱氧核糖核酸 多核苷酸 增色性 生物物理学 生物化学 立体化学 结晶学 寡核苷酸 生物 有机化学 医学 物理 疾病 病理 量子力学 阿尔茨海默病 聚合物
作者
Liuya Wei,Xianglong Kong,Mengran Wang,Yixin Zhang,Ruiyan Pan,Yuanzheng Cheng,Zhibao Lv,Jin Zhou,Jingjing Ming
出处
期刊:Analytical and Bioanalytical Chemistry [Springer Nature]
卷期号:414 (27): 7923-7933
标识
DOI:10.1007/s00216-022-04327-6
摘要

The phosphorylation process of DNA by T4 polynucleotide kinase (T4 PNK) plays a crucial role in DNA recombination, DNA replication, and DNA repair. Traditional monomeric G-quadruplex (G4) systems are always activated by single cation such as K+ or Na+. The conformation transformation caused by the coexistence of multiple cations may interfere with the signal readout and limit their applications in physiological system. In view of the stability of dimeric G4 in multiple cation solution, we reported a label-free T4 PNK fluorescence sensor based on split dimeric G4 and ligation-induced dimeric G4/thioflavin T (ThT) conformation. The dimeric G4 was divided into two independent pieces of one normal monomeric G4 and the other monomeric G4 fragment phosphorylated by T4 PNK in order to decrease the background signal. With the introduction of template DNA, DNA ligase, and invasive DNA, the dimeric G4 could be generated and liberated to combine with ThT to show obvious fluorescence signal. Using our strategy, the linear range from 0.005 to 0.5 U mL-1, and the detection limit of 0.0021 U mL-1 could be achieved without the consideration of interference caused by the coexistence of multiple cations. Additionally, research in real sample determination and inhibition effect investigations indicated its further potential application value in biochemical process research and clinic diagnostics.
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