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Nano-Mechanical DNA Devices Coupled With CRISPR-Cas12a for CA15-3 Detection.

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Small (Weinheim an der Bergstrasse, Germany) 📖 저널 OA 15.6% 2024: 1/2 OA 2025: 4/33 OA 2026: 5/29 OA 2024~2026 2026 Vol.22(10) p. e11023
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Zhao J, Long Y, Zhang Y, Hou C, Huo D

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Accurate monitoring of cancer markers is crucial for clinical treatment and prognosis.

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APA Zhao J, Long Y, et al. (2026). Nano-Mechanical DNA Devices Coupled With CRISPR-Cas12a for CA15-3 Detection.. Small (Weinheim an der Bergstrasse, Germany), 22(10), e11023. https://doi.org/10.1002/smll.202511023
MLA Zhao J, et al.. "Nano-Mechanical DNA Devices Coupled With CRISPR-Cas12a for CA15-3 Detection.." Small (Weinheim an der Bergstrasse, Germany), vol. 22, no. 10, 2026, pp. e11023.
PMID 41457810 ↗

Abstract

Accurate monitoring of cancer markers is crucial for clinical treatment and prognosis. CA15-3 activity levels are strongly associated with clinical progression of breast cancer, but their monitoring often relies on large instruments and professionals, and the process is time-consuming and costly. To address these concerns, we proposed an electrochemical biosensing strategy that integrated nano-mechanical DNA devices coupled with the CRISPR-Cas12a to drive molecularly gated functionalized substrates for the ultrasensitive detection of CA15-3. Specifically, Triple helical molecular switch (THMS) as a signal input switch to ensure target recognition specificity and the diffusion-limited 3D DNA walking machine coupled with CRISPR-Cas12a technology as signal amplification means. Based on the bimolecular dynamics model, the rate constants k (1.40 × 10 Msec) and k (2.5 × 10 Msec) of the GNP-PEG(+)/T 3D orbitals modified with positively charged SH-PEG-NH are larger than those of unmodified orbitals, proving that nanointerface diffusion restriction effect can accelerate the toehold-mediated chain displacement reaction (TMDR). With the assistance of Co-N/C modified screen-printed electrode (SPE-Co-N/C) sensing interface, the calculated detection limit of CA15-3 is as low as 7.14 × 10 U mL. The proposed assay, which demonstrated satisfactory selectivity and reproducibility, and correlated highly with ELISA kit results, offered a promising tool for breast cancer early detection and therapeutic monitoring.

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