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基于拉曼光谱的亚细胞药物代谢组学用于转移性黑素瘤细胞。

Raman-guided subcellular pharmaco-metabolomics for metastatic melanoma cells.

机构信息

Division of Chemistry and Chemical Engineering, California Institute of Technology, Pasadena, CA, USA.

Institute for Systems Biology, Seattle, WA, USA.

出版信息

Nat Commun. 2020 Sep 24;11(1):4830. doi: 10.1038/s41467-020-18376-x.

Abstract

Non-invasively probing metabolites within single live cells is highly desired but challenging. Here we utilize Raman spectro-microscopy for spatial mapping of metabolites within single cells, with the specific goal of identifying druggable metabolic susceptibilities from a series of patient-derived melanoma cell lines. Each cell line represents a different characteristic level of cancer cell de-differentiation. First, with Raman spectroscopy, followed by stimulated Raman scattering (SRS) microscopy and transcriptomics analysis, we identify the fatty acid synthesis pathway as a druggable susceptibility for differentiated melanocytic cells. We then utilize hyperspectral-SRS imaging of intracellular lipid droplets to identify a previously unknown susceptibility of lipid mono-unsaturation within de-differentiated mesenchymal cells with innate resistance to BRAF inhibition. Drugging this target leads to cellular apoptosis accompanied by the formation of phase-separated intracellular membrane domains. The integration of subcellular Raman spectro-microscopy with lipidomics and transcriptomics suggests possible lipid regulatory mechanisms underlying this pharmacological treatment. Our method should provide a general approach in spatially-resolved single cell metabolomics studies.

摘要

在单个活细胞内无创探测代谢物是人们非常期望的,但具有挑战性。在这里,我们利用拉曼光谱显微镜对单个细胞内的代谢物进行空间映射,具体目标是从一系列患者来源的黑素瘤细胞系中确定可药物治疗的代谢易感性。每个细胞系代表不同程度的癌细胞去分化特征。首先,我们通过拉曼光谱、受激拉曼散射(SRS)显微镜和转录组学分析,确定脂肪酸合成途径是分化黑素细胞的可药物治疗易感性。然后,我们利用细胞内脂滴的高光谱 SRS 成像来识别内在抵抗 BRAF 抑制的去分化间充质细胞中脂质单不饱和性的先前未知易感性。针对该靶点进行药物治疗会导致细胞凋亡,并伴有相分离的细胞内膜域的形成。亚细胞拉曼光谱显微镜与脂质组学和转录组学的整合表明,这种药物治疗可能存在潜在的脂质调节机制。我们的方法应该为基于空间分辨的单细胞代谢组学研究提供一种通用方法。

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