4.7 Article

Hairpin DNAs conformational changes inducing opposite-polarity photoelectric signals recovery for simultaneous monitoring of dual microRNAs

Journal

SENSORS AND ACTUATORS B-CHEMICAL
Volume 382, Issue -, Pages -

Publisher

ELSEVIER SCIENCE SA
DOI: 10.1016/j.snb.2023.133565

Keywords

Opposite polarity semiconductors; Photoelectrochemical; Biosensors; Two -component assay; MicroRNAs

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A unique multiplexed photoelectrochemical (PEC) biosensor for simultaneous detection of miRNA-141 and miRNA-155 was developed using Fe3O4 @SiO2 @CdS-HP1-Ag2S NPs and CdTe QDs-HP2-Au NPs nanobioprobes polarity switching mode. The biosensor exhibited a linear range of 50 fM to 10 nM and detection limits of 40.8 fM and 37.5 fM, respectively, without the need for bioamplification technology. It also demonstrated significant advantages in terms of compactness, short signal acquisition time, cost-effectiveness, stability, and replicability, offering a new perspective for simultaneous monitoring of multiple miRNAs.
Building flexible and reliable photoelectrochemical (PEC) sensors capable of measuring multiple miRNAs simultaneously still suffers from a challenge. In this protocol, a unique multiplexed PEC biosensor for miRNA-141 and miRNA-155 was developed by Fe3O4 @SiO2 @CdS-HP1-Ag2S NPs and CdTe QDs-HP2-Au NPs nanobioprobes polarity switching mode. HP1 and HP2 can be simultaneously unfolded by the two targets. The corresponding rigid DNA double-strand structure makes the distance between CdS shells and Ag2S NPs even greater, exposing more photoactive sites of CdS shells and thus the enhanced photoanode current. Similarly, the exciton-plasmon interaction (EPI) between the CdTe QDs and the Au NPs is disrupted, resulting in the photocurrent recovery of the CdTe QDs. Through external magnetic force, the one-step electrode modification of each above nanobioprobe was realized and the photocurrent polarity switching was also achieved. The linearity range of the designed multiplexed PEC biosensor was from 50 fM to 10 nM, and the detection limits reached 40.8 fM and 37.5 fM, respectively, without using any bioamplification technology. In addition, the manufactured PEC biosensor has significant advantages in compactness, short signal acquisition time, cost-effectiveness, as well as stability and replicability. The unique design provides a new perspective for monitoring multiple miRNAs simultaneously.

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