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泼尼松龙、喜树碱或替尼泊苷引发的大鼠胸腺细胞凋亡对G0期细胞具有选择性,且可被蛋白酶抑制剂所抑制。

Apoptosis of rat thymocytes triggered by prednisolone, camptothecin, or teniposide is selective to G0 cells and is prevented by inhibitors of proteases.

作者信息

Bruno S, Lassota P, Giaretti W, Darzynkiewicz Z

机构信息

Cancer Research Institute, New York Medical College, Valhalla 10523.

出版信息

Oncol Res. 1992;4(1):29-35.

PMID:1374671
Abstract

Rat thymocytes were treated in culture with prednisolone or the DNA topoisomerase I or II inhibitors, camptothecin (CAM) or teniposide (TN), and proportions of cells in different phases of the cell cycle were estimated by flow cytometry using a staining methodology which makes it possible to discriminate between G0 and G1 cells, as well as to recognize the cells which undergo apoptosis. The appearance of apoptotic cells in cultures treated with pharmacological concentrations of these drugs, observed as early as 3-6 hr after treatment, coincided with the selective loss of G0 cells in these cultures, while no significant changes in the proportion of S or G2+M cells were apparent. Agarose gel electrophoresis of DNA isolated from the treated cells indicated degradation of the internucleosomal spacer sections, typical of the endonucleolytic activity which accompanies apoptotic cell death. The data indicate that G0 thymocytes were particularly sensitive to agents that induce apoptosis while cells progressing through the cell cycle were resistant. This suggests that under in vivo conditions (immunological response), the selective death of G0 cells may promote the clonal expansion of stimulated thymocytes which enter the cell cycle. Together with our earlier studies on the effects of CAM and TN on MOLT-4 and HL-60 leukemic cell lines, these data indicate that both, phenotypic- and and cell cycle phase specific- factors modify the ability of cells to respond to toxic agents, including chemotherapeutics by apoptosis.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

将大鼠胸腺细胞置于含有泼尼松龙、DNA拓扑异构酶I或II抑制剂喜树碱(CAM)或替尼泊苷(TN)的培养基中培养,使用一种染色方法通过流式细胞术估算细胞周期不同阶段的细胞比例,该方法能够区分G0期和G1期细胞,并识别正在经历凋亡的细胞。在用这些药物的药理浓度处理的培养物中,早在处理后3 - 6小时就观察到凋亡细胞的出现,这与这些培养物中G0期细胞的选择性丢失相吻合,而S期或G2 + M期细胞的比例没有明显变化。从处理过的细胞中分离的DNA进行琼脂糖凝胶电泳显示核小体间间隔区降解,这是伴随凋亡细胞死亡的核酸内切酶活性的典型特征。数据表明,G0期胸腺细胞对诱导凋亡的药物特别敏感,而处于细胞周期进程中的细胞具有抗性。这表明在体内条件下(免疫反应),G0期细胞的选择性死亡可能促进进入细胞周期的受刺激胸腺细胞的克隆扩增。连同我们早期关于CAM和TN对MOLT - 4和HL - 60白血病细胞系影响的研究,这些数据表明,表型和细胞周期阶段特异性因素都会改变细胞对包括化疗药物在内的有毒物质通过凋亡作出反应的能力。(摘要截短于250字)

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Apoptosis of rat thymocytes triggered by prednisolone, camptothecin, or teniposide is selective to G0 cells and is prevented by inhibitors of proteases.泼尼松龙、喜树碱或替尼泊苷引发的大鼠胸腺细胞凋亡对G0期细胞具有选择性,且可被蛋白酶抑制剂所抑制。
Oncol Res. 1992;4(1):29-35.
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Cytostatic and cytotoxic effects of fostriecin on human promyelocytic HL-60 and lymphocytic MOLT-4 leukemic cells.福司曲星对人早幼粒细胞HL-60和淋巴细胞MOLT-4白血病细胞的细胞生长抑制和细胞毒性作用。
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Cytometric assessment of DNA damage in relation to cell cycle phase and apoptosis.与细胞周期阶段和细胞凋亡相关的DNA损伤的细胞计数评估。
Cell Prolif. 2005 Aug;38(4):223-43. doi: 10.1111/j.1365-2184.2005.00344.x.
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Actin is cleaved during constitutive apoptosis.
肌动蛋白在程序性细胞死亡过程中被裂解。
Biochem J. 1997 Apr 1;323 ( Pt 1)(Pt 1):233-7. doi: 10.1042/bj3230233.
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Selective induction of apoptosis in Hep 3B cells by topoisomerase I inhibitors: evidence for a protease-dependent pathway that does not activate cysteine protease P32.拓扑异构酶I抑制剂对Hep 3B细胞凋亡的选择性诱导:一条不激活半胱氨酸蛋白酶P32的蛋白酶依赖性途径的证据。
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Cell proliferation, DNA repair, and p53 function are not required for programmed death of prostatic glandular cells induced by androgen ablation.雄激素去除诱导的前列腺腺细胞程序性死亡不需要细胞增殖、DNA修复和p53功能。
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