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使用外泌体代谢通量分析(Exo-MFA)量化细胞外囊泡介导的代谢转移:一个综合的实验和计算平台。

Quantifying Metabolic Transfer Mediated by Extracellular Vesicles Using Exo-MFA: An Integrated Empirical and Computational Platform.

作者信息

Achreja Abhinav, Meurs Noah, Nagrath Deepak

机构信息

Department of Biomedical Engineering, University of Michigan, Ann Arbor, MI, USA.

Biointerfaces Institute, University of Michigan, Ann Arbor, MI, USA.

出版信息

Methods Mol Biol. 2020;2088:205-221. doi: 10.1007/978-1-0716-0159-4_10.

Abstract

Extracellular vesicles (EVs) are ubiquitous nanoscale particles released from many different types of cells. They have been shown to contain proteins, DNA, RNA, miRNA, and, most recently, metabolites. These particles can travel through the intercellular space and bloodstream to have regulatory effects on distant recipients. When an EV reaches a target cell, it is taken up and degraded to release its contents for utilization within the cell. In addition to regulatory effects, EVs have been shown to supplement the high metabolic demands of recipient cells in a nutrient-deprived tumor microenvironment. We developed an integrated empirical and computational platform to quantify metabolic contribution of source cell-derived EVs to recipient cells. The versatile Exo-MFA software tool utilizes C stable-isotope tracing data to quantify the metabolic contributions of EVs from a source cell type on a recipient cell type. This is accomplished by creating EV-depleted culture medium, producing isotope-labeled EVs from the source cells, isolating the labeled EVs from the culture supernatant, culturing the recipient cells in the presence of the labeled EVs, and measuring the resulting metabolite levels across several time points.

摘要

细胞外囊泡(EVs)是从许多不同类型细胞中释放出来的普遍存在的纳米级颗粒。已证明它们含有蛋白质、DNA、RNA、微小RNA(miRNA),以及最近发现的代谢物。这些颗粒可以穿过细胞间空间和血液循环,对远处的受体产生调节作用。当一个细胞外囊泡到达靶细胞时,它会被摄取并降解,以释放其内容物供细胞内利用。除了调节作用外,细胞外囊泡还被证明在营养缺乏的肿瘤微环境中补充受体细胞的高代谢需求。我们开发了一个综合的实证和计算平台,以量化源细胞衍生的细胞外囊泡对受体细胞的代谢贡献。通用的Exo-MFA软件工具利用碳稳定同位素示踪数据来量化一种源细胞类型的细胞外囊泡对一种受体细胞类型的代谢贡献。这是通过创建无细胞外囊泡的培养基、从源细胞产生同位素标记的细胞外囊泡、从培养上清液中分离标记的细胞外囊泡、在标记的细胞外囊泡存在下培养受体细胞,以及在几个时间点测量产生的代谢物水平来实现的。

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