Novel Amplex Red Oxidases Based on Noncanonical DNA Structures: Property Studies and Applications in MicroRNA Detection

Wang, Shaoru; Fu, Boshi; Wang, Jiaqi; Long, Yuelin; Zhang, Xiaoe; Peng, Shuang; Guo, Pengju; Tian, Tian; Zhou, Xiang

doi:10.1021/ac402535a

Cited by 59 publications

(31 citation statements)

References 33 publications

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“…HPLC is the most widely used method and shows high selectivity and sensitivity; however, this method requires expensive sample preparation and equipment 12 . CE also requires expensive instrumentation and ELISA is limited in practice because of its reliance on the surrounding environment 13,14 . Thus, inexpensive, rapid, accurate, and sensitive methods for detecting residual antibiotics in food must be developed.…”

Section: Introductionmentioning

confidence: 99%

Aptasensor for multiplex detection of antibiotics based on FRET strategy combined with aptamer/graphene oxide complex

Youn

Lee

Her

et al. 2019

Sci Rep

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The development of a multiplexed sensing platform is necessary for highly selective, sensitive, and rapid screening of specific antibiotics. In this study, we designed a novel multiplex aptasensor for antibiotics by fluorescence resonance energy transfer (FRET) strategy using DNase I-assisted cyclic enzymatic signal amplification (CESA) method combined with aptamer/graphene oxide complex. The aptamers specific for sulfadimethoxine, kanamycin, and ampicillin were conjugated with Cyanine 3 (Cy3), 6-Carboxyfluorescein (FAM), and Cyanine 5 (Cy5), respectively, and graphene oxide (GO) was adopted to quench the fluorescence of the three different fluorophores with the efficiencies of 94.36%, 93.94%, and 96.97% for Cy3, FAM, and Cy5, respectively. CESA method was used for sensitive detection, resulting in a 2.1-fold increased signal compared to those of unamplified method. The aptasensor rapidly detected antibiotics in solution with limit of detection of 1.997, 2.664, and 2.337 ng/mL for sulfadimethoxine, kanamycin, and ampicillin, respectively. In addition, antibiotics dissolved in milk were efficiently detected with similar sensitivities. Multiplexed detection test proved that the fluorescently modified aptamers could work separately from each other. The results indicate that the aptasensor offers high specificity for each antibiotic and enables simultaneous and multicolor sensing for rapid screening of multiple antibiotics at the same time.

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Section: Introductionmentioning

confidence: 99%

Aptasensor for multiplex detection of antibiotics based on FRET strategy combined with aptamer/graphene oxide complex

Youn

Lee

Her

et al. 2019

Sci Rep

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“…[20][21][22][23] The peroxidase activity is strongly dependent on the specific G4 structures and has been widely employed as a signal amplification tool for detection of nucleic acids, protein, metal ions, and small molecules. [23][24][25][26][27][28] However, the used oxidant H 2 O 2 is concentration decisive for the peroxidase activity [20] and its intrinsic instability is detrimental for reproducibility of the DNAzyme activity-based devices. Additionally, another additive must be further needed to temporally stop the catalytic reaction at the desired incubation time.…”

Section: Introductionmentioning

confidence: 99%

G‐Quadruplex‐Based Photooxidase Driven by Visible Light

Gao

Tong

et al. 2019

ChemCatChem

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The G‐quadruplex (G4)/hemin entity has been widely used as a peroxidase‐mimic DNAzyme to catalyze the substrate oxidation with exogenous and concentrated H2O2 as oxidant for developing various devices. Herein, a G4‐based oxidase‐mimic DNAzyme that can be driven by visible light was developed. The oxidant is in situ produced by light irradiation. As a natural photosensitizer, Hypericin (Hyp) alone in solution is inactive because of aggregation. However, the binding with G4 triggers the fluorescence emission and activates Hyp to produce singlet oxygen (1O2) by energy transfer to the dissolved oxygen. Therefore, the G4/Hyp entity can serve as a photooxidase via the 1O2 pathway to catalyze the substrate oxidation. Since the G4‐bound Hyp can be excited by almost the whole range of visible light, the photooxidase should cover a wide range of photocatalytic applications. Similar to the peroxidase‐mimic DNAzyme, the G4 sequence can regulate the photooxidase activity and metal ions can serve as efficient cofactors to activate the photooxidase capacity for an inactive G4 structure. This work provides an alternative to build a versatile G4‐based photooxidase with straightforward tunability of its activity.

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“…Very recently a new duplex-specific nuclease signal amplification (DSNSA) strategy has been developed for highly sensitive detection of miRNA by Ye's group (Yin et al, 2012). Subsequently, an increasing interest in the development of DSNSA has been presented for the detection of miRNA by fluorescent detection (Degliangeli et al, 2014;Wang et al, 2014;Li et al, 2014), and electrochemical techniques (Ren et al, 2013). Most of the reported DSNSA protocols used the single enhancement of DSN, few dual-amplified strategies have been reported (Tian et al, 2013).…”

Section: Introductionmentioning

confidence: 99%

A dual-amplified electrochemical detection of mRNA based on duplex-specific nuclease and bio-bar-code conjugates

Wang

Luo

et al. 2015

Biosensors and Bioelectronics

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Novel Amplex Red Oxidases Based on Noncanonical DNA Structures: Property Studies and Applications in MicroRNA Detection

Cited by 59 publications

References 33 publications

Aptasensor for multiplex detection of antibiotics based on FRET strategy combined with aptamer/graphene oxide complex

Aptasensor for multiplex detection of antibiotics based on FRET strategy combined with aptamer/graphene oxide complex

G‐Quadruplex‐Based Photooxidase Driven by Visible Light

A dual-amplified electrochemical detection of mRNA based on duplex-specific nuclease and bio-bar-code conjugates

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