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细胞培养中氨基酸的空间稳定同位素标记:用于全球蛋白质组分析的三维多细胞球体的脉冲追踪标记

Spatial Stable Isotopic Labeling by Amino Acids in Cell Culture: Pulse-Chase Labeling of Three-Dimensional Multicellular Spheroids for Global Proteome Analysis.

作者信息

Beller Nicole C, Lukowski Jessica K, Ludwig Katelyn R, Hummon Amanda B

机构信息

Department of Chemistry and Biochemistry, The Ohio State University, Columbus, Ohio 43210, United States.

Department of Chemistry and Biochemistry, University of Notre Dame, Notre Dame, Indiana 46556, United States.

出版信息

Anal Chem. 2021 Dec 7;93(48):15990-15999. doi: 10.1021/acs.analchem.1c03461. Epub 2021 Nov 23.

DOI:10.1021/acs.analchem.1c03461
PMID:34813286
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9248019/
Abstract

Three-dimensional cell cultures, or spheroids, are important model systems for cancer research because they recapitulate chemical and phenotypic aspects of in vivo tumors. Spheroids develop radially symmetric chemical gradients, resulting in distinct cellular populations. Stable isotopic labeling by amino acids in cell culture (SILAC) is a well-established approach to quantify protein expression and has previously been used in a pulse-chase format to evaluate temporal changes. In this article, we demonstrate that distinct isotopic signatures can be introduced into discrete spatial cellular populations, effectively tracking proteins to original locations in the spheroid, using a platform that we refer to as spatial SILAC. Spheroid populations were grown with light, medium, and heavy isotopic media, and the concentric shells of cells were harvested by serial trypsinization. Proteins were quantitatively analyzed by ultraperformance liquid chromatography-tandem mass spectrometry. The isotopic signatures correlated with the spatial location and the isotope position do not significantly impact the proteome of each individual layer. Spatial SILAC can be used to examine the proteomic changes in the different layers of the spheroid and to identify protein biomarkers throughout the structure. We show that SILAC labels can be discretely pulsed to discrete positions, without altering the spheroid's proteome, promising future combined pharmacodynamic and pharmacokinetic studies.

摘要

三维细胞培养物,即球体,是癌症研究的重要模型系统,因为它们概括了体内肿瘤的化学和表型特征。球体形成径向对称的化学梯度,从而产生不同的细胞群体。细胞培养中氨基酸的稳定同位素标记(SILAC)是一种成熟的定量蛋白质表达的方法,此前已用于脉冲追踪形式以评估时间变化。在本文中,我们证明可以使用我们称为空间SILAC的平台将不同的同位素标记引入离散的空间细胞群体中,从而有效地将蛋白质追踪到球体中的原始位置。用轻、中、重同位素培养基培养球体群体,并通过连续胰蛋白酶消化收获细胞的同心壳层。通过超高效液相色谱-串联质谱对蛋白质进行定量分析。同位素标记与空间位置相关,且同位素位置不会显著影响各层的蛋白质组。空间SILAC可用于检查球体不同层的蛋白质组变化,并在整个结构中鉴定蛋白质生物标志物。我们表明,可以将SILAC标记离散地脉冲到离散位置,而不会改变球体的蛋白质组,这为未来联合药效学和药代动力学研究带来了希望。

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