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乙醇会导致分化中的HL-60细胞加速进入G1期停滞。

Ethanol causes accelerated G1 arrest in differentiating HL-60 cells.

作者信息

Cook R T, Keiner J A, Yen A

机构信息

Department of Pathology, Department of Veterans Affairs Medical Center, Iowa City, Iowa.

出版信息

Alcohol Clin Exp Res. 1990 Oct;14(5):695-703. doi: 10.1111/j.1530-0277.1990.tb01229.x.

DOI:10.1111/j.1530-0277.1990.tb01229.x
PMID:1702269
Abstract

The effects of clinically relevant ethanol concentrations on myeloid differentiation in the HL-60 cell promyelocytic leukemia line have been studied. The exposure of noninduced stem cells to 60 mM ethanol results in an increase in G1 cells, but there is no increase in superoxide production or expression of the Mo1 antigen. When HL-60 cells are induced to differentiate along the myeloid line with dimethylsulfoxide (DMSO) or retinoic acid (RA), there is a shift to smaller cell size, an increase in G1 cells and acquisition of the ability to produce superoxide as reported previously by several authors. When ethanol is present during differentiation, there are further increases in G1 cells, and increases in the percentage of cells which produce superoxide and express Mo1, and decreases in mean cell size and total growth during the incubation period. Regrowth experiments after periods of differentiation indicate that the increased G1 arrest seen in the presence of ethanol represents terminal commitment if inducer is present, but in the absence of inducer the increased G1 percentage is readily reversible. Examination of RNA content by flow cytometry reveals a decrease in both the peak and mean G1 RNA content during DMSO or RA induced differentiation. These decreases are accentuated by the presence of ethanol, resulting in a higher G1A/G1B ratio than in nonexposed cells. These findings indicate that ethanol enhances G1 growth arrest in HL-60 cells exposed to myeloid inducers. Partial differentiation occurs during this process, resulting in terminally arrested cells, some of which have undergone fewer postinduction cell divisions than normal and may not be fully competent.

摘要

已经研究了临床相关乙醇浓度对HL - 60早幼粒细胞白血病细胞系髓系分化的影响。未诱导的干细胞暴露于60 mM乙醇会导致G1期细胞增加,但超氧化物产生或Mo1抗原表达没有增加。当HL - 60细胞用二甲基亚砜(DMSO)或视黄酸(RA)诱导沿髓系分化时,如先前几位作者报道的那样,会出现细胞尺寸变小、G1期细胞增加以及获得产生超氧化物的能力。当在分化过程中存在乙醇时,G1期细胞进一步增加,产生超氧化物并表达Mo1的细胞百分比增加,孵育期内平均细胞尺寸和总生长减少。分化期后的再生长实验表明,如果存在诱导剂,在乙醇存在下观察到的G1期阻滞增加代表终末分化,但在没有诱导剂的情况下,增加的G1期百分比很容易逆转。通过流式细胞术检测RNA含量发现,在DMSO或RA诱导分化期间,G1期RNA含量的峰值和平均值均降低。乙醇的存在加剧了这些降低,导致G1A/G1B比值高于未暴露细胞。这些发现表明,乙醇增强了暴露于髓系诱导剂的HL - 60细胞中的G1期生长阻滞。在此过程中发生部分分化,导致终末阻滞细胞,其中一些细胞诱导后经历的细胞分裂比正常细胞少,可能不完全成熟。

相似文献

1
Ethanol causes accelerated G1 arrest in differentiating HL-60 cells.乙醇会导致分化中的HL-60细胞加速进入G1期停滞。
Alcohol Clin Exp Res. 1990 Oct;14(5):695-703. doi: 10.1111/j.1530-0277.1990.tb01229.x.
2
Reversible G1 arrest induced by dimethyl sulfoxide in human lymphoid cell lines: dimethyl sulfoxide inhibits IL-6-induced differentiation of SKW6-CL4 into IgM-secreting plasma cells.二甲基亚砜诱导人淋巴细胞系发生可逆性G1期阻滞:二甲基亚砜抑制IL-6诱导SKW6-CL4分化为分泌IgM的浆细胞。
Exp Cell Res. 1996 Jan 10;222(1):218-24. doi: 10.1006/excr.1996.0027.
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Precommitment states induced during HL-60 myeloid differentiation: possible similarities of retinoic acid- and DMSO-induced early events.HL-60髓系分化过程中诱导的预承诺状态:维甲酸和二甲基亚砜诱导的早期事件可能存在的相似性。
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Characterization of differentiation-inducer-resistant HL-60 cells.分化诱导剂抗性HL-60细胞的特性分析。
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Retinoic acid-induced blr1 expression promotes ERK2 activation and cell differentiation in HL-60 cells.维甲酸诱导的blr1表达促进HL-60细胞中的ERK2激活和细胞分化。
Exp Cell Res. 2000 Feb 1;254(2):287-98. doi: 10.1006/excr.1999.4766.
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Magnesium deprivation inhibits the expression of differentiation-related phenotypes in human promyelocytic leukemia HL-60 cells.镁缺乏会抑制人早幼粒细胞白血病HL-60细胞中分化相关表型的表达。
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Effects of lithium on dimethyl sulfoxide induced differentiation of HL-60 promyelocytic leukemia cells.锂对二甲基亚砜诱导的HL-60早幼粒细胞白血病细胞分化的影响。
Leuk Res. 1992 Aug;16(8):823-8. doi: 10.1016/0145-2126(92)90162-z.

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