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通过碳-13核磁共振光谱法研究血管活性肠肽对人结肠腺癌细胞糖原代谢的影响。

Effect of VIP on the glycogen metabolism of human colon adenocarcinoma cells studied by 13C nuclear magnetic resonance spectroscopy.

作者信息

Galons J P, Fantini J, Vion-Dury J, Cozzone P J, Canioni P

机构信息

Centre de Résonance Magnétique Biologique et Médicale, URA CNRS 1186, Université d'Aix-Marseille, Faculté de Médecine, France.

出版信息

Int J Cancer. 1990 Jan 15;45(1):168-73. doi: 10.1002/ijc.2910450130.

Abstract

Metabolic pathways of glucose utilization have been investigated in a human colon adenocarcinoma cell line (HT29) using carbon-13 Nuclear Magnetic Resonance spectroscopy. HT29 cells were adapted to grow on a polystyrene beaded microcarrier and were perfused when attached to the beads in a specially designed NMR cell. Abnormalities in carbohydrate metabolism already observed in several cancer cells were studied in HT29 cells fed with (1-13C)-enriched glucose. The cells were first perfused with a glucose-free medium for 2 h in order to deplete the intracellular store of glycogen, and they were subsequently perfused with a medium containing enriched glucose at an initial concentration of 5.5 mM. Sequential 13C-NMR spectra, recorded at 100.5 MHz (5 min accumulation), show that HT29 cells were able to utilize glucose through the glycolytic pathway while storing glucose as glycogen (glucose was utilized at a rate of 3.9 mumol/mg protein/hr). The glycolytic activity determined by the amount of lactic acid produced was 4.6 microns/mg protein/hr, corresponding to the formation of 1.2 lactic acid per glucose molecule. Glycogen accumulation corresponded to 16 micrograms/mg of protein. Treatment of HT29 with 10 nM vasoactive intestinal peptide (VIP) induced a transient decrease in the level of labelled glycogen to 50% of the initial value. Control level was recovered 12 min after VIP loading.

摘要

利用碳-13核磁共振光谱法,对人结肠腺癌细胞系(HT29)中葡萄糖利用的代谢途径进行了研究。HT29细胞适应于在聚苯乙烯珠状微载体上生长,并在附着于珠子时在专门设计的核磁共振样品管中进行灌注。在以富含(1-13C)葡萄糖喂养的HT29细胞中,研究了在几种癌细胞中已经观察到的碳水化合物代谢异常情况。首先将细胞用无葡萄糖培养基灌注2小时,以耗尽细胞内糖原储备,随后用初始浓度为5.5 mM的富含葡萄糖的培养基进行灌注。在100.5 MHz下记录的连续13C-核磁共振光谱(5分钟累加)表明,HT29细胞能够通过糖酵解途径利用葡萄糖,同时将葡萄糖储存为糖原(葡萄糖的利用速率为3.9 μmol/mg蛋白质/小时)。由产生的乳酸量确定的糖酵解活性为4.6 μmol/mg蛋白质/小时,相当于每个葡萄糖分子形成1.2个乳酸。糖原积累量相当于16 μg/mg蛋白质。用10 nM血管活性肠肽(VIP)处理HT29细胞,导致标记糖原水平短暂下降至初始值的50%。VIP加载12分钟后恢复到对照水平。

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