A new integrated method for tissue extracellular vesicle enrichment and proteome profiling

Extracellular vesicles (EVs) are membranous vesicles released by cells that carry a number of biologically important components such as lipids, proteins, and mRNAs. EVs can mediate cancer cell migration, invasion, angiogenesis, and cell survival, greatly contributing to cell-to-cell communication in...

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Autores principales: Zhang, Miaomiao, Liu, Tong, Du, Zhuokun, Li, Hang, Qin, Weijie
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Royal Society of Chemistry 2022
Materias:
Chemistry
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9679920/
https://www.ncbi.nlm.nih.gov/pubmed/36425162
http://dx.doi.org/10.1039/d2ra06185f
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author Zhang, Miaomiao
Liu, Tong
Du, Zhuokun
Li, Hang
Qin, Weijie
author_facet Zhang, Miaomiao
Liu, Tong
Du, Zhuokun
Li, Hang
Qin, Weijie
author_sort Zhang, Miaomiao
collection PubMed
description Extracellular vesicles (EVs) are membranous vesicles released by cells that carry a number of biologically important components such as lipids, proteins, and mRNAs. EVs can mediate cancer cell migration, invasion, angiogenesis, and cell survival, greatly contributing to cell-to-cell communication in the tumor microenvironment. Additionally, EVs have been found to have diagnostic and prognostic significance in various cancers. However, the direct isolation of pure EVs remains challenging, especially from tissue samples. Currently available EV isolation approaches, e.g., ultracentrifugation, are time-consuming, instrumental dependent, and have a low recovery rate with limited purity. It is urgent to develop rapid and efficient methods for enriching tissue EVs for biological and clinical studies. Here, we developed a novel isolation approach for tissue EVs using an extraction kit combined with TiO(2) microspheres (kit-TiO(2)). The EVs were first precipitated from the tissue fluid using a precipitation agent and then further enriched using microspheres based on the specific interaction between TiO(2) and the phosphate groups on the lipid bilayer of the EVs. Kit-TiO(2) approach led to improved purity and enrichment efficiency of the isolated EVs, as demonstrated by western blot and proteomic analysis, compared with previously reported methods. A total of 1966 protein groups were identified from the tissue EVs. We compared the proteomic profiles of the liver tissue EVs from healthy and hepatocellular carcinoma (HCC) bearing-mice. Twenty-five significantly upregulated and 75 downregulated protein groups were found in the HCC EVs. Among the differentially expressed proteins, Atic, Copa, Cont3, Me1, Anxa3, Fth1, Anxa5, Phb1, Acaa2, ATPD, and Glud1 were reported to be highly relevant to HCC. This novel isolation strategy has provided a powerful tool for enriching EVs directly from tissues, and may be applied in biomarker discovery and drug screening of HCC.
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spelling pubmed-96799202022-11-23 A new integrated method for tissue extracellular vesicle enrichment and proteome profiling Zhang, Miaomiao Liu, Tong Du, Zhuokun Li, Hang Qin, Weijie RSC Adv Chemistry Extracellular vesicles (EVs) are membranous vesicles released by cells that carry a number of biologically important components such as lipids, proteins, and mRNAs. EVs can mediate cancer cell migration, invasion, angiogenesis, and cell survival, greatly contributing to cell-to-cell communication in the tumor microenvironment. Additionally, EVs have been found to have diagnostic and prognostic significance in various cancers. However, the direct isolation of pure EVs remains challenging, especially from tissue samples. Currently available EV isolation approaches, e.g., ultracentrifugation, are time-consuming, instrumental dependent, and have a low recovery rate with limited purity. It is urgent to develop rapid and efficient methods for enriching tissue EVs for biological and clinical studies. Here, we developed a novel isolation approach for tissue EVs using an extraction kit combined with TiO(2) microspheres (kit-TiO(2)). The EVs were first precipitated from the tissue fluid using a precipitation agent and then further enriched using microspheres based on the specific interaction between TiO(2) and the phosphate groups on the lipid bilayer of the EVs. Kit-TiO(2) approach led to improved purity and enrichment efficiency of the isolated EVs, as demonstrated by western blot and proteomic analysis, compared with previously reported methods. A total of 1966 protein groups were identified from the tissue EVs. We compared the proteomic profiles of the liver tissue EVs from healthy and hepatocellular carcinoma (HCC) bearing-mice. Twenty-five significantly upregulated and 75 downregulated protein groups were found in the HCC EVs. Among the differentially expressed proteins, Atic, Copa, Cont3, Me1, Anxa3, Fth1, Anxa5, Phb1, Acaa2, ATPD, and Glud1 were reported to be highly relevant to HCC. This novel isolation strategy has provided a powerful tool for enriching EVs directly from tissues, and may be applied in biomarker discovery and drug screening of HCC. The Royal Society of Chemistry 2022-11-22 /pmc/articles/PMC9679920/ /pubmed/36425162 http://dx.doi.org/10.1039/d2ra06185f Text en This journal is © The Royal Society of Chemistry https://creativecommons.org/licenses/by-nc/3.0/
spellingShingle Chemistry
Zhang, Miaomiao
Liu, Tong
Du, Zhuokun
Li, Hang
Qin, Weijie
A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title_full A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title_fullStr A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title_full_unstemmed A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title_short A new integrated method for tissue extracellular vesicle enrichment and proteome profiling
title_sort new integrated method for tissue extracellular vesicle enrichment and proteome profiling
topic Chemistry
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9679920/
https://www.ncbi.nlm.nih.gov/pubmed/36425162
http://dx.doi.org/10.1039/d2ra06185f
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