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乙醇诱导细胞分裂短暂停滞(G2 + M期阻滞),随后是G0/G1期阻滞:短期和长期乙醇暴露对细胞周期和细胞功能的剂量效应。

Ethanol induces transient arrest of cell division (G2 + M block) followed by G0/G1 block: dose effects of short- and longer-term ethanol exposure on cell cycle and cell functions.

作者信息

Mikami K, Haseba T, Ohno Y

机构信息

Department of Legal Medicine, Nippon Medical School, Tokyo, Japan.

出版信息

Alcohol Alcohol. 1997 Mar-Apr;32(2):145-52. doi: 10.1093/oxfordjournals.alcalc.a008248.

Abstract

To study the cytophysiological effects of ethanol systematically, L929 cells, a fibroblastic cell line derived from mouse connective tissue, were exposed to various concentrations of ethanol (12.5, 50, 100 and 200 mM) for short (3 and 6 h) and longer (24 or 26 h) durations. Ethanol-induced cellular responses were analysed by a combination of the following assays: number of cells, amounts of DNA and protein, MTT (3-[4,5-dimethylthiazol-2-yl]-2,5-diphenyltetrazolium bromide) assay and cell cycle. Ethanol dose-dependently suppressed these cellular functions, except that 12.5 mM exposures for both 6 and 26 h increased the amount of protein in spite of almost no change in other cellular functions, compared to the control. The most marked dose-dependency was observed in a reduction of formazan product in an MTT assay after both 6 and 26 h exposures to ethanol, being independent of the number of cells and probably reflecting dose-dependent depression of mitochondrial respiration. A G2 + M block in the cell cycle, an inhibition of cell division, was induced after short-term exposures (3 and 6 h) to 100 and 200 mM ethanol, but the block was released before 24 h had passed. Alternatively, prolonged exposures (24 h) to 50-200 mM ethanol induced a G0/G1 block, resulting in a decrease in the amount of DNA below the control value. Moreover, the percentage of the S phase was decreased gradually and dose-dependently throughout the 24 h exposure. Thus, high concentrations of ethanol (50, 100 and 200 mM) perturbed the cell cycle progression by causing both a transient G2 + M block (an inhibition of mitosis) and a continuous G0/G1 block, though the latter was masked by the G2 + M block during short-term exposure. The cells seem finally to acquire some tolerance to ethanol so as to pass through mitosis, but much less tolerance to pass through the checkpoint from the G1 to the S phase, which results in a decline in proliferation.

摘要

为了系统地研究乙醇的细胞生理效应,将源自小鼠结缔组织的成纤维细胞系L929细胞暴露于不同浓度的乙醇(12.5、50、100和200 mM)中,暴露时间分为短时间(3和6小时)和较长时间(24或26小时)。通过以下检测方法组合分析乙醇诱导的细胞反应:细胞数量、DNA和蛋白质含量、MTT(3-[4,5-二甲基噻唑-2-基]-2,5-二苯基四氮唑溴盐)检测和细胞周期。乙醇剂量依赖性地抑制这些细胞功能,但与对照组相比,6小时和26小时暴露于12.5 mM乙醇时,尽管其他细胞功能几乎没有变化,但蛋白质含量增加。在6小时和26小时暴露于乙醇后,MTT检测中azan产物的减少表现出最明显的剂量依赖性,这与细胞数量无关,可能反映了线粒体呼吸的剂量依赖性抑制。短期暴露(3和6小时)于100和200 mM乙醇后,细胞周期中出现G2+M期阻滞,即细胞分裂受到抑制,但在24小时之前阻滞解除。或者,长时间暴露(24小时)于50-200 mM乙醇会诱导G0/G1期阻滞,导致DNA含量低于对照值。此外,在整个24小时暴露过程中,S期的百分比逐渐降低且呈剂量依赖性。因此,高浓度乙醇(50、100和200 mM)通过引起短暂的G2+M期阻滞(有丝分裂抑制)和持续的G0/G1期阻滞来干扰细胞周期进程,尽管在短期暴露期间后者被G2+M期阻滞所掩盖。细胞似乎最终对乙醇获得了一定的耐受性以便通过有丝分裂,但对从G1期到S期的检查点的耐受性要低得多,这导致细胞增殖下降。

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