Rapid exosome isolation and in situ multiplexed detection of exosomal surface proteins and microRNAs on microfluidic platform

外体 适体 CD63 微流控 原位 微泡 癌症生物标志物 小RNA 化学 蛋白质微阵列 癌症 计算生物学 纳米技术 癌症研究 分子生物学 生物 生物化学 微阵列 材料科学 基因 基因表达 遗传学 有机化学
作者
Yulin Chen,Dan Gao,Qingyun Zhu,Bizhu Chu,Jie Peng,Jian Wang,Liping Liu,Yuyang Jiang
出处
期刊:Analyst [Royal Society of Chemistry]
卷期号:148 (10): 2387-2394 被引量:9
标识
DOI:10.1039/d3an00335c
摘要

Exosomes are considered as promising biomarkers for early cancer diagnosis and prognosis. However, the majority of the research studies focused on a single type of exosomal biomarkers, which cannot comprehensively reflect the state of cancer for accurate diagnosis. To address this problem, we presented a ship-shaped microfluidic device containing a microcolumn array for simultaneous in situ detection of exosomal surface proteins and miRNAs. Exosomes were first captured in the microchannels modified with CD63 protein aptamer. Exosomal surface proteins and miRNAs were simultaneously detected in four parallel channels to avoid the interference of fluorescent signals using specific aptamers labeled by Cy5 and catalytic hairpin assembly (CHA) based signal amplification strategy. The limit of detection for multiplexed markers in exosomes was 83 exosomes per μL, which is comparable to previously reported methods. Through quantitative analysis of two disease-specific surface proteins and miRNAs derived from different cancer cells and clinical serum samples, different cancer subtypes as well as cancer patients and healthy people could be significantly distinguished. These results suggest that this simple, highly sensitive, and more accurate analytical strategy by simultaneous in situ profiling of different types of exosomal biomarkers has potential applications in cancer diagnosis and stage monitoring.
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