Department of Biology, Georgia State University, Atlanta, GA 30303, USA.
Cell Death Differ. 2011 Apr;18(4):632-44. doi: 10.1038/cdd.2010.133. Epub 2010 Nov 5.
We have previously shown that a non-toxic noscapinoid, EM011 binds tubulin without altering its monomer/polymer ratio. EM011 is more active than the parent molecule, noscapine, in inducing G2/M arrest, inhibiting cellular proliferation and tumor growth in various human xenograft models. However, the mechanisms of mitotic-block and subsequent cell death have remained elusive. Here, we show that EM011-induced attenuation of microtubule dynamics was associated with impaired association of microtubule plus-end tracking proteins, such as EB1 and CLIP-170. EM011 treatment then led to the formation of multipolar spindles containing 'real' centrioles indicating drug-induced centrosome amplification and persistent centrosome declustering. Centrosome amplification was accompanied by an upregulation of Aurora A and Plk4 protein levels, as well as a surge in the kinase activity of Aurora A, suggesting a deregulation of the centrosome duplication cycle. Cell-cycle phase-specific experiments showed that the 'cytotoxicity-window' of the drug encompasses the late S-G2 period. Drug-treatment, excluding S-phase, not only resulted in lower sub-G1 population but also attenuated centrosome amplification and spindle multipolarity, suggesting that drug-induced centrosome amplification is essential for maximal cell death. Subsequent to a robust mitotic arrest, EM011-treated cells displayed diverse cellular fates suggesting a high degree of intraline variation. Some 'apoptosis-evasive' cells underwent aberrant cytokinesis to generate rampant aneuploidy that perhaps contributed to drug-induced cell death. These data indicate that spindle multipolarity induction by means of centrosome amplification has an exciting chemotherapeutic potential that merits further investigation.
我们之前已经表明,一种非毒性的石蒜碱类似物 EM011 能够结合微管蛋白而不改变其单体/聚合物的比例。EM011 在诱导 G2/M 期阻滞、抑制各种人异种移植模型中的细胞增殖和肿瘤生长方面比母体分子石蒜碱更有效。然而,有丝分裂阻滞和随后的细胞死亡的机制仍然难以捉摸。在这里,我们表明,EM011 诱导的微管动力学衰减与微管末端追踪蛋白(如 EB1 和 CLIP-170)的结合受损有关。EM011 处理随后导致含有“真正”中心体的多极纺锤体的形成,表明药物诱导的中心体扩增和持续的中心体去聚类。中心体扩增伴随着 Aurora A 和 Plk4 蛋白水平的上调,以及 Aurora A 的激酶活性的激增,表明中心体复制周期的失调。细胞周期阶段特异性实验表明,药物的“细胞毒性窗口”涵盖晚期 S-G2 期。药物治疗(不包括 S 期)不仅导致较低的亚 G1 群体,而且还减弱了中心体扩增和纺锤体多极性,表明药物诱导的中心体扩增对于最大细胞死亡是必要的。在强大的有丝分裂阻滞之后,EM011 处理的细胞显示出多种细胞命运,表明高度的内在变异。一些“逃避凋亡”的细胞经历了异常的胞质分裂,产生了猖獗的非整倍体,这也许有助于药物诱导的细胞死亡。这些数据表明,通过中心体扩增诱导的纺锤体多极性具有令人兴奋的化疗潜力,值得进一步研究。