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新生霉素和佛波醇-12-肉豆蔻酸酯-13-乙酸酯诱导人白血病细胞分化,同时拓扑异构酶II活性降低。

Novobiocin- and phorbol-12-myristate-13-acetate-induced differentiation of human leukemia cells associated with a reduction in topoisomerase II activity.

作者信息

Constantinou A, Henning-Chubb C, Huberman E

机构信息

Medical Research Division, Argonne National Laboratory, Illinois 60439.

出版信息

Cancer Res. 1989 Mar 1;49(5):1110-7.

PMID:2537141
Abstract

Studies were conducted to determine the possible involvement of DNA topoisomerase II (Topo II) in the induction of differentiation in two human promyelocytic HL-60 leukemia cell variants that are either susceptible or resistant to differentiation induced by phorbol-12-myristate-13-acetate (PMA), a protein kinase C activator. The acquisition of maturation markers and changes in the activity, level, and phosphorylation of Topo II were determined after treatment with either novobiocin, a Topo II inhibitor, or PMA. Novobiocin at 50-150 microM induced differentiation in the HL-205 cells but not in the HL-525 cells, although both cell types were equally susceptible to novobiocin-evoked cytotoxicity. In both cell types, novobiocin induced similar reductions in topoisomerase I activity but different reductions in Topo II activity. Treatment with novobiocin at 150 microM for 6 h or at 2 mM for 30 min resulted in a 4-fold or higher reduction in Topo II activity in the differentiation-susceptible HL-205 cells but not in the differentiation-resistant HL-525 cells. A differential response in Topo II activity was also observed after treatment with PMA. The novobiocin-evoked decrease in Topo II activity seems to be due to an enhanced enzyme proteolysis, whereas the PMA-elicited decrease in Topo II activity is associated with an increase in Topo II phosphorylation. 1-(5-Isoquinolinesulfonyl)-2-methylpiperazine, which is an inhibitor of protein kinases, including protein kinase C, diminished the novobiocin-elicited proteolysis of Topo II and the PMA-induced Topo II phosphorylation, as well as the decrease in Topo II activity and the acquisition of differentiation markers induced by either novobiocin or PMA. These results suggest that induction of differentiation in HL-60 cells by novobiocin or PMA is associated with a reduction in Topo II activity, mediated directly or indirectly by a protein kinase(s), perhaps protein kinase C.

摘要

开展了多项研究,以确定DNA拓扑异构酶II(Topo II)是否可能参与两种人早幼粒细胞HL - 60白血病细胞变体的分化诱导过程。这两种变体对佛波醇-12-肉豆蔻酸酯-13-乙酸酯(PMA,一种蛋白激酶C激活剂)诱导的分化,一种敏感,另一种耐药。在用拓扑异构酶II抑制剂新生霉素或PMA处理后,测定了成熟标志物的获得情况以及Topo II的活性、水平和磷酸化的变化。50 - 150微摩尔的新生霉素可诱导HL - 205细胞分化,但不能诱导HL - 525细胞分化,尽管两种细胞类型对新生霉素引起的细胞毒性同样敏感。在两种细胞类型中,新生霉素诱导拓扑异构酶I活性出现类似程度的降低,但Topo II活性降低程度不同。用150微摩尔新生霉素处理6小时或2毫摩尔处理30分钟,可使易分化的HL - 205细胞中的Topo II活性降低4倍或更多,但耐药的HL - 525细胞中则不会。在用PMA处理后,也观察到Topo II活性的差异反应。新生霉素引起的Topo II活性降低似乎是由于酶蛋白水解增强,而PMA引起的Topo II活性降低与Topo II磷酸化增加有关。1 -(5 - 异喹啉磺酰基)- 2 - 甲基哌嗪是包括蛋白激酶C在内的蛋白激酶抑制剂,它减少了新生霉素引起的Topo II蛋白水解、PMA诱导的Topo II磷酸化,以及Topo II活性降低和新生霉素或PMA诱导的分化标志物的获得。这些结果表明,新生霉素或PMA诱导HL - 60细胞分化与Topo II活性降低有关,这是由一种蛋白激酶(可能是蛋白激酶C)直接或间接介导的。

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