研究目的
To develop a label-free Ag nanocluster (AgNC)-based fluorescent probe for the detection of prostate-specific antigen (PSA), a tumor marker, using DNA-Ag nanoclusters (DNA-AgNC) and aptamer hybridization.
研究成果
A label-free, simple DNA-AgNC/aptamer fluorescent sensor for PSA detection was successfully developed, with a detection limit of 1.14 ng mL?1. The sensor was applicable for PSA detection in spiked human serum, offering advantages of economy and simplicity. This work provides a reference for constructing AgNC-based probes for detecting other proteins.
研究不足
The mechanism of fluorescence enhancement of DNA-AgNC by aptamer is highly dependent on the template DNA sequence, which may limit the generalizability of the probe for other targets. The sensitivity and specificity of the probe need to be further optimized for clinical applications.
1:Experimental Design and Method Selection:
DNA sequences complementary to PSA aptamer were used to synthesize DNA-AgNC. The fluorescence enhancement effect of PSA aptamer on DNA-AgNC was utilized for PSA detection.
2:Sample Selection and Data Sources:
PSA and other proteins (AFP, CEA, HCG, HIgG) were used to investigate the specificity of the sensor. Human serum samples were used for applicability evaluation.
3:List of Experimental Equipment and Materials:
LS-55 fluorescence spectrophotometer, UV-2550 UV–vis spectrophotometer, Tecnai G2 20 U-Twin HRTEM, FE20 pH meter, DNA sequences, Ag(NO)3, NaBH4, PSA, AFP, HCG, CEA, HIgG.
4:Experimental Procedures and Operational Workflow:
DNA-AgNC synthesis, optimization of detection conditions (pH, salt concentration, aptamer concentration), fluorescence assay of PSA, selectivity test, and application in serum samples.
5:Data Analysis Methods:
Fluorescence intensity measurements, UV–vis absorption spectra, HRTEM for morphology characterization.
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