Cas12a-based direct visualization of nanoparticle-stabilized fluorescence signal for multiplex detection of DNA methylation biomarkers

多路复用 核酸 计算生物学 DNA DNA甲基化 化学 亚硫酸氢盐测序 分析灵敏度 荧光 亚硫酸氢盐 分子生物学 纳米技术 生物 生物化学 生物信息学 材料科学 基因 医学 基因表达 病理 物理 替代医学 量子力学
作者
Li Yu,Meng Cai,Wenwen Zhang,Ying Liu,Xiaoqing Yuan,Ning Han,J Li,Shengnan Jin,Chunming Ding
出处
期刊:Biosensors and Bioelectronics [Elsevier]
卷期号:244: 115810-115810 被引量:1
标识
DOI:10.1016/j.bios.2023.115810
摘要

The CRISPR-Cas12a RNA-guided complexes hold immense promise for nucleic acid detection. However, limitations arise from their specificity in detecting off-targets and the stability of the signal molecules. Here, we have developed a platform that integrates multiplex amplification and nanomolecular-reporting signals, allowing us to detect various clinically relevant nucleic acid targets with enhanced stability, sensitivity, and visual interpretation. Through the electrostatic co-assembly of the Oligo reporter with oppositely charged nanoparticles, we observed a significant enhancement in its stability in low-pollution environments, reaching up to a threefold increase compared to the original version. Additionally, the fluorescence efficiency was expanded by three orders of magnitude, broadening the detection range considerably. Utilizing a multiplex strategy, this assay can accomplish simultaneous detection of multiple targets and single-point indication detection of nine specific targets. This significant advancement heightened the sensitivity of disease screening and improved the accuracy of diagnosing disease-related changes. We tested this assay in a colorectal cancer model, demonstrating that it can identify DNA methylation features at the aM-level within 40-60 min. Validation using clinical samples yielded consistent results with qPCR and bisulfite sequencing, affirming the assay's reliability and potential for clinical applications.
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