Proteometabolomics of initial and recurrent glioblastoma highlights an increased immune cell signature with altered lipid metabolism

蛋白质组 肿瘤微环境 代谢组 免疫系统 脂类学 组学 重编程 肿瘤进展 蛋白质组学 代谢组学 癌症研究 计算生物学 巴西金 细胞 生物 生物信息学 免疫学 癌症 生物化学 基因 遗传学 基质金属蛋白酶
作者
Miguel Cosenza‐Contreras,Agnes Schäfer,Justin Sing,Lena Cook,Maren Nicole Stillger,Chia-Yi Chen,José Villacorta Hidalgo,Niko Pinter,Larissa A. Meyer,Tilman Werner,Darleen Bug,Zeno Haberl,Oliver Kübeck,Kai Zhao,Susanne Stei,Anca Violeta Gafencu,Radu Ioniță,Felix Mircea Brehar,Jaime Ferrer-Lozano,Gloria Ribas
出处
期刊:Neuro-oncology [Oxford University Press]
卷期号:26 (3): 488-502 被引量:11
标识
DOI:10.1093/neuonc/noad208
摘要

Abstract Background There is an urgent need to better understand the mechanisms associated with the development, progression, and onset of recurrence after initial surgery in glioblastoma (GBM). The use of integrative phenotype-focused -omics technologies such as proteomics and lipidomics provides an unbiased approach to explore the molecular evolution of the tumor and its associated environment. Methods We assembled a cohort of patient-matched initial (iGBM) and recurrent (rGBM) specimens of resected GBM. Proteome and metabolome composition were determined by mass spectrometry-based techniques. We performed neutrophil-GBM cell coculture experiments to evaluate the behavior of rGBM-enriched proteins in the tumor microenvironment. ELISA-based quantitation of candidate proteins was performed to test the association of their plasma concentrations in iGBM with the onset of recurrence. Results Proteomic profiles reflect increased immune cell infiltration and extracellular matrix reorganization in rGBM. ASAH1, SYMN, and GPNMB were highly enriched proteins in rGBM. Lipidomics indicates the downregulation of ceramides in rGBM. Cell analyses suggest a role for ASAH1 in neutrophils and its localization in extracellular traps. Plasma concentrations of ASAH1 and SYNM show an association with time to recurrence. Conclusions We describe the potential importance of ASAH1 in tumor progression and development of rGBM via metabolic rearrangement and showcase the feedback from the tumor microenvironment to plasma proteome profiles. We report the potential of ASAH1 and SYNM as plasma markers of rGBM progression. The published datasets can be considered as a resource for further functional and biomarker studies involving additional -omics technologies.
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