Institute for Molecular Medicine Finland FIMM, University of Helsinki, Finland.
EV group, Division of Biochemistry and Biotechnology, Department of Biosciences and Division of Pharmaceutical Biosciences, Faculty of Pharmacy, University of Helsinki, Finland.
Theranostics. 2017 Aug 23;7(16):3824-3841. doi: 10.7150/thno.19890. eCollection 2017.
Body fluids are a rich source of extracellular vesicles (EVs), which carry cargo derived from the secreting cells. So far, biomarkers for pathological conditions have been mainly searched from their protein, (mi)RNA, DNA and lipid cargo. Here, we explored the small molecule metabolites from urinary and platelet EVs relative to their matched source samples. As a proof-of-concept study of intra-EV metabolites, we compared alternative normalization methods to profile urinary EVs from prostate cancer patients before and after prostatectomy and from healthy controls.
We employed targeted ultra-performance liquid chromatography-tandem mass spectrometry to profile over 100 metabolites in the isolated EVs, original urine samples and platelets. We determined the enrichment of the metabolites in the EVs and analyzed their subcellular origin, pathways and relevant enzymes or transporters through data base searches. EV- and urine-derived factors and ratios between metabolites were tested for normalization of the metabolomics data.
Approximately 1 x 10 EVs were sufficient for detection of metabolite profiles from EVs. The profiles of the urinary and platelet EVs overlapped with each other and with those of the source materials, but they also contained unique metabolites. The EVs enriched a selection of cytosolic metabolites including members from the nucleotide and spermidine pathways, which linked to a number of EV-resident enzymes or transporters. Analysis of the urinary EVs from the patients indicated that the levels of glucuronate, D-ribose 5-phosphate and isobutyryl-L-carnitine were 2-26-fold lower in all pre-prostatectomy samples compared to the healthy control and post-prostatectomy samples (p < 0.05). These changes were only detected from EVs by normalization to EV-derived factors or with metabolite ratios, and not from the original urine samples.
Our results suggest that metabolite analysis of EVs from different samples is feasible using a high-throughput platform and relatively small amount of sample material. With the knowledge about the specific enrichment of metabolites and normalization methods, EV metabolomics could be used to gain novel biomarker data not revealed by the analysis of the original EV source materials.
体液是细胞外囊泡(EVs)的丰富来源,EVs 携带源自分泌细胞的货物。到目前为止,病理条件的生物标志物主要是从其蛋白质、(mi)RNA、DNA 和脂质货物中搜索得到的。在这里,我们探索了与匹配源样本相比,尿液和血小板 EVs 中的小分子代谢物。作为 EV 内代谢物的概念验证研究,我们比较了替代的归一化方法,以分析前列腺癌患者前列腺切除术前和术后以及健康对照组的尿液 EVs。
我们采用靶向超高效液相色谱-串联质谱法对分离的 EVs、原始尿液样本和血小板中的 100 多种代谢物进行了分析。我们确定了代谢物在 EVs 中的富集,并通过数据库搜索分析了它们的亚细胞起源、途径以及相关的酶或转运蛋白。对 EV 和尿液衍生的因子以及代谢物之间的比值进行了测试,以确定代谢组学数据的归一化。
大约 1 x 10 EVs 就足以从 EVs 中检测到代谢物谱。尿液和血小板 EVs 的图谱与各自的来源材料重叠,但它们也含有独特的代谢物。EVs 富集了包括核苷酸和精胺途径成员在内的一系列细胞质代谢物,这些代谢物与许多 EV 驻留酶或转运蛋白有关。对患者尿液 EVs 的分析表明,与健康对照组和前列腺切除术后样本相比,所有前列腺切除术前样本中葡萄糖醛酸、D-核糖 5-磷酸和异丁酰基-L-肉碱的水平低 2-26 倍(p < 0.05)。这些变化仅通过 EV 衍生因子的归一化或代谢物比值从 EVs 中检测到,而不能从原始尿液样本中检测到。
我们的结果表明,使用高通量平台和相对少量的样本材料,对来自不同样本的 EVs 进行代谢物分析是可行的。通过了解代谢物的特定富集和归一化方法,EV 代谢组学可以用于获得原始 EV 源材料分析未揭示的新生物标志物数据。
Zotero 插件
