Proteomics analysis of serum small extracellular vesicles for the longitudinal study of a glioblastoma multiforme mouse model

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作者
Federica Anastasi
Francesco Greco
Marialaura Dilillo
Eleonora Vannini
Valentina Cappello
Laura Baroncelli
Mario Costa
Mauro Gemmi
Matteo Caleo
Liam A. McDonnell
机构
[1] NEST Laboratories,Department of Biomedical Sciences
[2] Scuola Normale Superiore,undefined
[3] Fondazione Pisana per la Scienza ONLUS,undefined
[4] Institute of Life Sciences,undefined
[5] Sant’Anna School of Advanced Studies,undefined
[6] CNR,undefined
[7] Neuroscience Institute,undefined
[8] Fondazione Umberto Veronesi,undefined
[9] Istituto Italiano di Tecnologia,undefined
[10] Center for Nanotechnology Innovation @NEST,undefined
[11] IRCCS Fondazione Stella Maris,undefined
[12] University of Padua,undefined
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Scientific Reports | / 10卷
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摘要
Longitudinal analysis of disease models enables the molecular changes due to disease progression or therapeutic intervention to be better resolved. Approximately 75 µl of serum can be drawn from a mouse every 14 days. To date no methods have been reported that are able to analyze the proteome of small extracellular vesicles (sEV’s) from such low serum volumes. Here we report a method for the proteomics analysis of sEV's from 50 µl of serum. Two sEV isolation procedures were first compared; precipitation based purification (PPT) and size exclusion chromatography (SEC). The methodological comparison confirmed that SEC led to purer sEV’s both in terms of size and identified proteins. The procedure was then scaled down and the proteolytic digestion further optimized. The method was then applied to a longitudinal study of serum-sEV proteome changes in a glioblastoma multiforme (GBM) mouse model. Serum was collected at multiple time points, sEV’s isolated and their proteins analyzed. The protocol enabled 274 protein groups to be identified and quantified. The longitudinal analysis revealed 25 deregulated proteins in GBM serum sEV's including proteins previously shown to be associated with GBM progression and metastasis (Myh9, Tln-1, Angpt1, Thbs1).
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