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Analysis of mammalian cell proliferation and macromolecule synthesis using deuterated water and gas chromatography-mass spectrometry.

机译:用氘水和气相色谱-质谱法分析哺乳动物细胞的增殖和大分子合成。

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摘要

Deuterated water (²H₂O), a stable isotopic tracer, provides a convenient and reliable way to label multiple cellular biomass components (macromolecules), thus permitting the calculation of their synthesis rates. Here, we have combined ²H₂O labelling, GC-MS analysis and a novel cell fractionation method to extract multiple biomass components (DNA, protein and lipids) from the one biological sample, thus permitting the simultaneous measurement of DNA (cell proliferation), protein and lipid synthesis rates. We have used this approach to characterize the turnover rates and metabolism of a panel of mammalian cells in vitro (muscle C2C12 and colon cancer cell lines). Our data show that in actively-proliferating cells, biomass synthesis rates are strongly linked to the rate of cell division. Furthermore, in both proliferating and non-proliferating cells, it is the lipid pool that undergoes the most rapid turnover when compared to DNA and protein. Finally, our data in human colon cancer cell lines reveal a marked heterogeneity in the reliance on the de novo lipogenic pathway, with the cells being dependent on both \u27self-made\u27 and exogenously-derived fatty acid.
机译:氘水(2 H 2 O)是一种稳定的同位素示踪剂,为标记多种细胞生物质组分(大分子)提供了一种方便可靠的方法,从而可以计算其合成速率。在这里,我们结合了²H2 O标记,GC-MS分析和一种新颖的细胞分级分离方法,以从一个生物样品中提取多种生物质成分(DNA,蛋白质和脂质),从而可以同时测量DNA(细胞增殖),蛋白质和脂质合成率。我们已经使用这种方法来表征一组哺乳动物细胞(肌肉C2C12和结肠癌细胞系)的周转率和代谢。我们的数据表明,在活跃增殖的细胞中,生物质合成速率与细胞分裂速率密切相关。此外,在增殖细胞和非增殖细胞中,与DNA和蛋白质相比,脂质池的周转速度最快。最后,我们在人类结肠癌细胞系中的数据揭示了依赖于从头脂肪形成途径的显着异质性,这些细胞既依赖于自身脂肪酸,也依赖于外源性脂肪酸。

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