
AbstractCirculating cell‐free nucleic acids are considered a promising source of biomarkers for diseases and cancer. Liquid biopsy biomarkers for brain tumours represent a major, still unmet, clinical need. In plasma, nucleic acids can be free or be associated with extracellular vesicles (EVs). Here we report an easy and reproducible method to analyse cell‐free nucleic acids in plasma and EVs by conventional flow cytometry easy to translate into the clinics. Nucleic acids associated with the EVs or present in plasma samples are stained by Pyronin Y, which is a fluorescent dye that is preferably binding double‐stranded nucleic acids. Fluorescent staining of EVs isolated from cell‐conditioned media is suitable for DNA and RNA detection by flow cytometry. The nucleic acids are partially protected from degradation by the EVs’ membrane. Additionally, DNA and RNA can be stained in plasma samples and plasma‐derived EVs. Remarkably, analysis of plasma from patients and healthy individuals reveals a difference in their nucleic acid profiles. Taken together, our results indicate that the proposed methodology, which is based on conventional direct flow cytometry, is a promising easy tool for plasma nucleic acid analysis.
QH573-671, flow cytometry, circulating tumour DNA, glioblastoma, Pyronin Y; cell‐free nucleic acids; circulating tumour DNA; extracellular RNA; extracellular vesicles; flow cytometry; glioblastoma, extracellular RNA, cell‐free nucleic acids, extracellular vesicles, Cytology, Research Article
QH573-671, flow cytometry, circulating tumour DNA, glioblastoma, Pyronin Y; cell‐free nucleic acids; circulating tumour DNA; extracellular RNA; extracellular vesicles; flow cytometry; glioblastoma, extracellular RNA, cell‐free nucleic acids, extracellular vesicles, Cytology, Research Article
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