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SILAC–based quantitative MS approach for real-time recording protein-mediated cell-cell interactions

机译:基于氧化硅酸的定量MS方法,用于实时记录蛋白介导的细胞 - 细胞相互作用

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In tumor microenvironment, interactions among multiple cell types are critical for cancer progression. To understand the molecular mechanisms of these complex interplays, the secreted protein analysis between malignant cancer cells and the surrounding nonmalignant stroma is a good viewpoint to investigate cell-cell interactions. Here, we developed two stable isotope labeling of amino acids in cell culture (SILAC)-based mass spectrometry (MS)/MS approaches termed spike-in SILAC and triple-SILAC to quantify changes of protein secretion level in a cell co-cultured system. Within the co-culture system of CT26 and Ana-1 cells, the spike-in SILAC and triple-SILAC MS approaches are sensitive to quantitatively measure protein secretion changes. Three representative quantified proteins (Galectin-1, Cathepsin L1 and Thrombospondin-1) by two SILAC-based MS methods were further validated by Western blotting, and the coming result matched well with SILACs’. We further applied these two SILACs to human cell lines, NCM460 and HT29 co-culture system, for evaluating the feasibility, which confirmed the spike-in and triple SILAC were capable of monitoring the changed secreted proteins of human cell lines. Considering these two strategies in time consuming, sample complexity and proteome coverage, the triple-SILAC way shows more efficiency and economy for real-time recording secreted protein levels in tumor microenvironment.
机译:在肿瘤微环境中,多种细胞类型之间的相互作用对于癌症进展至关重要。为了了解这些复杂相互作用的分子机制,恶性癌细胞与周围的非正起基质之间的分泌蛋白质分析是研究细胞细胞相互作用的良好观点。在这里,我们开发了两种稳定的同位素标记的细胞培养物(Silac)的质谱(MS)/ MS接近纯硅酸和Triple-Silac的方法,以定量细胞共培养系统中蛋白质分泌水平的变化。在CT26和ANA-1细胞的共培养系统内,穗状花序硅酸和三硅酸三硅酸盐方法对定量测量蛋白质分泌变化敏感。通过Western印迹进一步验证了三种基于硅酸基的MS方法的三种代表性的量化蛋白(Galectin-1,组织蛋白酶L1和血压回合素-1),并且随着Silacs的即将到来的结果良好匹配。我们进一步将这两种硅酸盐施用于人体细胞系,NCM460和HT29共培养系统,用于评估证实穗状体和三氧化件能够监测人细胞系的改变的分泌蛋白质的可行性。考虑到这两种策略,采样复杂性和蛋白质组覆盖率,三氧化铝方式表明了肿瘤微环境中实时记录分泌蛋白水平的更高效率和经济。

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