Jeney A, Hujber Z, Szoboszlai N, Fullár A, Oláh J, Pap É, Márk Á, Kriston Cs, Kralovánszky J, Kovalszky I, Vékey K, Sebestyén A
1st Department of Pathology and Experimental Cancer Research, Semmelweis University, Üllői út 26, Budapest, 1085 Hungary.
Laboratory of Environmental Chemistry and Bioanalytics, Department of Analytical Chemistry, Institute of Chemistry, Eötvös Loránd University, P.O. Box 32, Budapest, 1518 Hungary.
Cancer Cell Int. 2016 Feb 11;16:4. doi: 10.1186/s12935-016-0281-x. eCollection 2016.
Alterations in cellular metabolism are considered as hallmarks of cancers, however, to recognize these alterations and understand their mechanisms appropriate techniques are required. Our hypothesis was to determine whether dominant bioenergetic mechanism may be estimated by comparing the substrate utilisation with different methods to detect the labelled carbon incorporation and their application in tumour cells.
To define the bioenergetic pathways different metabolic tests were applied: (a) measuring CO2 production from [1-(14)C]-glucose and [1-(14)C]-acetate; (b) studying the effect of glucose and acetate on adenylate energy charge; (c) analysing glycolytic and TCA cycle metabolites and the number of incorporated (13)C atoms after [U-(13)C]-glucose/[2-(13)C]-acetate labelling. Based on [1-(14)C]-substrate oxidation two selected cell lines out of seven were analysed in details, in which the highest difference was detected at their substrate utilization. To elucidate the relevance of metabolic characterisation the expression of certain regulatory factors, bioenergetic enzymes, mammalian target of rapamycin (mTOR) complexes (C1/C2) and related targets as important elements at the crossroad of cellular signalling network were also investigated.
Both [U-(13)C]-glucose and [1-(14)C]-substrate labelling indicated high glycolytic capacity of tumour cells. However, the ratio of certain (13)C-labelled metabolites showed detailed metabolic differences in the two selected cell lines in further characterisation. The detected differences of GAPDH, β-F1-ATP-ase expression and adenylate energy charge in HT-1080 and ZR-75.1 tumour cells also confirmed the altered metabolism. Moreover, the highly limited labelling of citrate by [2-(13)C]-acetate-representing a novel functional test in malignant cells-confirmed the defect of TCA cycle of HT-1080 in contrast to ZR-75.1 cells. Noteworthy, the impaired TCA cycle in HT-1080 cells were associated with high mTORC1 activity, negligible protein level and activity of mTORC2, high expression of interleukin-1β, interleukin-6 and heme oxygenase-1 which may contribute to the compensatory mechanism of TCA deficiency.
The applied methods of energy substrate utilisation and other measurements represent simple assay system using (13)C-acetate and glucose to recognize dominant bioenergetic pathways in tumour cells. These may offer a possibility to characterise metabolic subtypes of human tumours and provide guidelines to find biomarkers for prediction and development of new metabolism related targets in personalized therapy.
细胞代谢改变被认为是癌症的标志,然而,要识别这些改变并理解其机制,需要合适的技术。我们的假设是,通过比较不同方法检测标记碳掺入的底物利用情况及其在肿瘤细胞中的应用,来确定主要的生物能量机制是否可以被估计。
为了定义生物能量途径,应用了不同的代谢测试:(a)测量[1-(14)C]-葡萄糖和[1-(14)C]-乙酸盐产生的二氧化碳;(b)研究葡萄糖和乙酸盐对腺苷酸能量电荷的影响;(c)分析糖酵解和三羧酸循环代谢物以及[U-(13)C]-葡萄糖/[2-(13)C]-乙酸盐标记后掺入的(13)C原子数量。基于[1-(14)C]-底物氧化,对七个细胞系中的两个选定细胞系进行了详细分析,在它们的底物利用方面检测到了最大差异。为了阐明代谢特征的相关性,还研究了某些调节因子、生物能量酶、雷帕霉素哺乳动物靶点(mTOR)复合物(C1/C2)以及作为细胞信号网络交叉点重要元素的相关靶点的表达。
[U-(13)C]-葡萄糖和[1-(14)C]-底物标记均表明肿瘤细胞具有高糖酵解能力。然而,某些(13)C标记代谢物的比例在进一步表征中显示出两个选定细胞系存在详细的代谢差异。在HT-1080和ZR-75.1肿瘤细胞中检测到的甘油醛-3-磷酸脱氢酶(GAPDH)、β-F1-ATP酶表达和腺苷酸能量电荷的差异也证实了代谢改变。此外,[2-(13)C]-乙酸盐对柠檬酸的标记高度有限——这是恶性细胞中的一种新型功能测试——与ZR-75.1细胞相比,证实了HT-1080的三羧酸循环存在缺陷。值得注意的是,HT-1080细胞中受损的三羧酸循环与高mTORC1活性、可忽略不计的mTORC2蛋白水平和活性、白细胞介素-1β、白细胞介素-6和血红素加氧酶-1的高表达相关,这可能有助于三羧酸缺乏的补偿机制。
所应用的能量底物利用方法和其他测量方法代表了一种简单的检测系统,使用(13)C-乙酸盐和葡萄糖来识别肿瘤细胞中的主要生物能量途径。这些方法可能提供一种表征人类肿瘤代谢亚型的可能性,并为在个性化治疗中寻找预测生物标志物和开发新的代谢相关靶点提供指导。
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