Self-protected circular DNAzyme for integrated enrichment and quantification of small extracellular vesicles.
2/5 보강
TL;DR
This work presents a robust paradigm for sEV analysis and lays a solid foundation for their downstream biomedical applications by leveraging the lipid bilayer structure for sEV enrichment and effectively eliminates interference from free proteins.
OpenAlex 토픽 ·
Advanced biosensing and bioanalysis techniques
Extracellular vesicles in disease
interferon and immune responses
This work presents a robust paradigm for sEV analysis and lays a solid foundation for their downstream biomedical applications by leveraging the lipid bilayer structure for sEV enrichment and effectiv
APA
Qianqian Wu, Yican Li, et al. (2026). Self-protected circular DNAzyme for integrated enrichment and quantification of small extracellular vesicles.. The Analyst, 151(8), 2166-2176. https://doi.org/10.1039/d5an01340b
MLA
Qianqian Wu, et al.. "Self-protected circular DNAzyme for integrated enrichment and quantification of small extracellular vesicles.." The Analyst, vol. 151, no. 8, 2026, pp. 2166-2176.
PMID
41784788
Abstract
Small extracellular vesicles (sEVs) hold immense potential for liquid biopsy given the wealth of biological information they carry. Currently, the clinical application of these methods is limited due to their low abundance and the complexities associated with traditional isolation techniques. To address this, we developed a strategy integrating cholesterol-mediated capture with a Self-Protected DNAzyme Walker for the rapid and simultaneous specific isolation and quantification of small extracellular vesicles (sEVs). Upon specific binding to CD63, the blocker strand is released, which activates the DNAzyme catalytic core, leading to substrate cleavage, which triggers the specific release of sEVs from magnetic beads and the generation of a fluorescent signal. Importantly, the circular DNA Shield design provides remarkable stability to the system by safeguarding the DNAzyme core from nuclease degradation. Furthermore, the cyclic cleavage mechanism allows for highly sensitive detection, achieving a limit of detection (LOD) as low as 361 particles per μL. In addition, by leveraging the lipid bilayer structure for sEV enrichment, this strategy effectively eliminates interference from free proteins. Furthermore, the clinical feasibility of this assay was validated by successfully distinguishing Stage I breast cancer patients from healthy individuals with high statistical significance ( < 0.001), highlighting its promise for early cancer diagnosis. This work presents a robust paradigm for sEV analysis and lays a solid foundation for their downstream biomedical applications.
MeSH Terms
DNA, Catalytic; Extracellular Vesicles; Humans; Limit of Detection; Breast Neoplasms; Tetraspanin 30; Female; Cholesterol
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