A fluorescent aptasensor for enzyme-free and sensitive detection of kanamycin based on entropy-driven strand displacement reaction

Longjie Xie; Cong Fan; Yang Liu; Qin Chen; Xian Chen

doi:10.1016/j.aca.2024.342659

A fluorescent aptasensor for enzyme-free and sensitive detection of kanamycin based on entropy-driven strand displacement reaction

Anal Chim Acta. 2024 Jun 15:1308:342659. doi: 10.1016/j.aca.2024.342659. Epub 2024 Apr 27.

Authors

Longjie Xie¹, Cong Fan¹, Yang Liu¹, Qin Chen², Xian Chen³

Affiliations

¹ College of Chemistry, Fuzhou University, 2 Xueyuan Road, Fuzhou, 350116, China.
² Fujian Cancer Hospital & Fujian Medical University Cancer Hospital, Fuzhou, 350014, China.
³ College of Chemistry, Fuzhou University, 2 Xueyuan Road, Fuzhou, 350116, China. Electronic address: xchen_fzu@126.com.

PMID: 38740459
DOI: 10.1016/j.aca.2024.342659

Abstract

Background: Kanamycin is an antibiotic that can easily cause adverse side effects if used improperly. Due to the extremely low concentrations of kanamycin in food, quantitative detection of kanamycin becomes a challenge. As one of the DNA self-assembly strategies, entropy-driven strand displacement reaction (EDSDR) does not require enzymes or hairpins to participate in the reaction, which greatly reduces the instability of detection results. Therefore, it is a very beneficial attempt to construct a highly sensitive and specific fluorescence detection method based on EDSDR that can detect kanamycin easily and quickly while ensuring that the results are effective and stable.

Results: We created an enzyme-free fluorescent aptamer sensor with high specificity and sensitivity for detecting kanamycin in milk by taking advantage of EDSDR and the high specific binding between the target and its aptamer. The specific binding can result in the release of the promoter chain, which then sets off the pre-planned EDSDR cycle. Fluorescent label modification on DNA combined with the fluorescence quenching-recovery mechanism gives the sensor impressive fluorescence response capabilities. The research results showed that within the concentration range of 0.1 nM-50 nM, there was a good relationship between the fluorescence intensity of the solution and the concentration of kanamycin. Specificity experiments and actual sample detection experiments confirmed that the biosensor could achieve highly sensitive and specific detection of trace amounts of kanamycin in food, with a detection limit of 0.053 nM (S/N = 3).

Significance: To our knowledge, this is the first strategy to combine EDSDR with fluorescence to detect kanamycin in food. Accurate results can be obtained in as little as 90 min with no enzymes or hairpins involved in the reaction. Furthermore, our enzyme-free biosensing method is straightforward, highly sensitive, and extremely specific. It has many possible applications, including monitoring antibiotic residues and food safety.

Keywords: Aptamer; Entropy-driven strand displacement reaction; Fluorescent biosensing; Kanamycin; Signal amplification.

MeSH terms

Animals
Anti-Bacterial Agents / analysis
Anti-Bacterial Agents / chemistry
Aptamers, Nucleotide* / chemistry
Biosensing Techniques* / methods
Entropy*
Fluorescent Dyes* / chemistry
Food Contamination / analysis
Kanamycin* / analysis
Kanamycin* / chemistry
Limit of Detection
Milk* / chemistry
Spectrometry, Fluorescence

Substances

Kanamycin
Aptamers, Nucleotide
Fluorescent Dyes
Anti-Bacterial Agents