Planchon S M, Wuerzberger S, Frydman B, Witiak D T, Hutson P, Church D R, Wilding G, Boothman D A
Department of Human Oncology, School of Medicine, University of Wisconsin-Madison, Madison 53792, USA.
Cancer Res. 1995 Sep 1;55(17):3706-11.
beta-Lapachone and certain of its derivatives directly bind and inhibit topoisomerase I (Topo I) DNA unwinding activity and form DNA-Topo I complexes, which are not resolvable by SDS-K+ assays. We show that beta-lapachone can induce apoptosis in certain cells, such as in human promyelocytic leukemia (HL-60) and human prostate cancer (DU-145, PC-3, and LNCaP) cells, as also described by Li et al. (Cancer Res., 55: 0000-0000, 1995). Characteristic 180-200-bp oligonucleosome DNA laddering and fragmented DNA-containing apoptotic cells via flow cytometry and morphological examinations were observed in 4 h in HL-60 cells after a 4-h, > or = 0.5 microM beta-lapachone exposure. HL-60 cells treated with camptothecin or topotecan resulted in greater apoptotic DNA laddering and apoptotic cell populations than comparable equitoxic concentrations of beta-lapachone, although beta-lapachone was a more effective Topo I inhibitor. beta-Lapachone treatment (4 h, 1-5 microM) resulted in a block at G0/G1, with decreases in S and G2/M phases and increases in apoptotic cell populations over time in HL-60 and three separate human prostate cancer (DU-145, PC-3, and LNCaP) cells. Similar treatments with topotecan or camptothecin (4 h, 1-5 microM) resulted in blockage of cells in S and apoptosis. Thus, beta-lapachone causes a block in G0/G1 of the cell cycle and induces apoptosis in cells before, or at early times during, DNA synthesis. These events are p53 independent, since PC-3 and HL-60 cells are null cells, LNCaP are wild-type, and DU-145 contain mutant p53, yet all undergo apoptosis after beta-lapachone treatment. Interestingly, beta-lapachone treatment of p53 wild type-containing prostate cancer cells (i.e., LNCaP) did not result in the induction of nuclear levels of p53 protein, as did camptothecin-treated cells. Like other Topo I inhibitors, beta-lapachone may induce apoptosis by locking Topo I onto DNA, blocking replication fork movement, and inducing apoptosis in a p53-independent fashion. beta-Lapachone and its derivatives, as well as other Topo I inhibitors, have potential clinical utility alone against human leukemia and prostate cancers.
β-拉帕醌及其某些衍生物可直接结合并抑制拓扑异构酶I(Topo I)的DNA解旋活性,形成DNA-Topo I复合物,而该复合物无法通过SDS-K⁺分析来解析。我们发现,β-拉帕醌可诱导某些细胞发生凋亡,如人早幼粒细胞白血病(HL-60)细胞和人前列腺癌细胞(DU-145、PC-3和LNCaP),Li等人(《癌症研究》,55: 0000 - 0000, 1995)也有相关描述。在HL-60细胞中,经4小时、≥0.5微摩尔β-拉帕醌处理4小时后,通过流式细胞术和形态学检查观察到了特征性的180 - 200碱基对寡核小体DNA梯状条带以及含碎片化DNA的凋亡细胞。与同等毒性浓度的β-拉帕醌相比,用喜树碱或拓扑替康处理HL-60细胞导致的凋亡DNA梯状条带和凋亡细胞群体更多,尽管β-拉帕醌是一种更有效的Topo I抑制剂。β-拉帕醌处理(4小时,1 - 5微摩尔)导致HL-60细胞和三种不同的人前列腺癌细胞(DU-145、PC-3和LNCaP)在G0/G1期阻滞,随着时间推移,S期和G2/M期细胞减少,凋亡细胞群体增加。用拓扑替康或喜树碱进行类似处理(4小时,1 - 5微摩尔)导致细胞在S期阻滞并发生凋亡。因此,β-拉帕醌导致细胞周期在G0/G1期阻滞,并在DNA合成之前或早期诱导细胞凋亡。这些事件与p53无关,因为PC-3和HL-60细胞为p53缺失细胞,LNCaP为野生型,DU-145含有突变型p53,但所有细胞在β-拉帕醌处理后均发生凋亡。有趣的是,与喜树碱处理的细胞不同,用β-拉帕醌处理含p53野生型的前列腺癌细胞(即LNCaP)并未导致p53蛋白核水平的诱导。与其他Topo I抑制剂一样,β-拉帕醌可能通过将Topo I锁定在DNA上、阻断复制叉移动以及以p53非依赖的方式诱导凋亡。β-拉帕醌及其衍生物以及其他Topo I抑制剂单独对人类白血病和前列腺癌具有潜在的临床应用价值。