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Whole-genome methylation profiling of extracellular vesicle DNA in gastric cancer identifies intercellular communication features.

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Nature communications 📖 저널 OA 92.8% 2021: 2/2 OA 2022: 3/3 OA 2023: 3/3 OA 2024: 21/21 OA 2025: 202/202 OA 2026: 178/210 OA 2021~2026 2025 Vol.16(1) p. 8084
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Lin B, Jiao Z, Dong S, Yan W, Jiang J, Du Y, Weng X, Wang H, Hu Z, Liu Y, Zhou X

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Extracellular vesicles (EVs) are promising biomarkers for cancer diagnosis and prognosis due to their ability to carry specific biomolecular cargo, including DNA.

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APA Lin B, Jiao Z, et al. (2025). Whole-genome methylation profiling of extracellular vesicle DNA in gastric cancer identifies intercellular communication features.. Nature communications, 16(1), 8084. https://doi.org/10.1038/s41467-025-63435-w
MLA Lin B, et al.. "Whole-genome methylation profiling of extracellular vesicle DNA in gastric cancer identifies intercellular communication features.." Nature communications, vol. 16, no. 1, 2025, pp. 8084.
PMID 40883299 ↗

Abstract

Extracellular vesicles (EVs) are promising biomarkers for cancer diagnosis and prognosis due to their ability to carry specific biomolecular cargo, including DNA. However, the clinical utility of DNA methylation-based liquid biopsies using EV-DNA remains underexplored. The low quantity and relatively long length of EV-DNA complicate whole-genome methylation profiling. To address this, we develop Tn5-assisted Enzymatic Methyl-sequencing with Post-conversion Tailing (TEMPT), a bisulfite-free whole-genome profiling method for EV-DNA. TEMPT employs single-adapter Tn5 tagmentation, enzymatic conversion of unmodified cytosines, and post-conversion tailing to generate high-depth whole-genome EV-DNA methylomes. We apply TEMPT to EV-DNA from 58 gastric cancer and polyp samples, generating methylomes from sub-nanogram inputs and identifying differentially methylated regions (DMRs) that distinguish cancer from controls. We identify potential cancer biomarkers through DMR-associated genes, highlighting the roles of EVs in cellular communication. Our findings suggest that immune cells may serve as an alternative source of EV-DNA. This approach holds significant promise for advancing EV-DNA research and its applications in early disease diagnosis.

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