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PFKFB3基因沉默可降低糖酵解、诱导细胞周期延迟并抑制HeLa细胞的非锚定依赖性生长。

PFKFB3 gene silencing decreases glycolysis, induces cell-cycle delay and inhibits anchorage-independent growth in HeLa cells.

作者信息

Calvo M N, Bartrons R, Castaño E, Perales J C, Navarro-Sabaté A, Manzano A

机构信息

Unitat de Bioquímica, Departament de Ciències Fisiològiques II, Campus de Ciències de la Salut, IDIBELL-Universitat de Barcelona, Feixa Llarga s/n E-08907 L'Hospitalet, Barcelona, Spain.

出版信息

FEBS Lett. 2006 May 29;580(13):3308-14. doi: 10.1016/j.febslet.2006.04.093. Epub 2006 May 8.

DOI:10.1016/j.febslet.2006.04.093
PMID:16698023
Abstract

The high rate of glycolysis despite the presence of oxygen in tumor cells (Warburg effect) suggests an important role for this process in cell division. The glycolytic rate is dependent on the cellular concentration of fructose 2,6-bisphosphate (Fru-2,6-P2), which, in turn, is controlled by the bifunctional enzyme 6-phosphofructo-2-kinase/fructose-2,6-bisphosphatase (PFK-2). The ubiquitous PFK-2 isoenzyme (uPFK-2, alternatively named UBI2K5 or ACG) coded by the pfkfb3 gene is induced by different stimuli (serum, progesterone, insulin, hypoxia, etc.) and has the highest kinase/phosphatase activity ratio amongst all PFK-2 isoenzymes discovered to date, which is consistent with its role as a powerful activator of glycolysis. uPFK-2 is expressed in brain, placenta, transformed cells and proliferating cells. In the present work, we analyze the impact of small interfering RNA (siRNA)-induced silencing of uPFK-2 on the inhibition of cell proliferation. HeLa cells treated with uPFK-2 siRNA showed a decrease in uPFK-2 RNA levels measured at 24h. uPFK-2 protein levels were severely depleted at 48-72h when compared with cells treated with an unrelated siRNA, correlating with decreased glycolytic activity, Fru-2,6-P2, lactate and ATP concentrations. These metabolic changes led to reduced viability, cell-cycle delay and an increase in the population of apoptotic cells. Moreover, uPFK-2 suppression inhibited anchorage-independent growth. The results obtained highlight the importance of uPFK-2 on the regulation of glycolysis, on cell viability and proliferation and also on anchorage-independent growth. These data underscore the potential for uPFK-2 as an effective tumor therapeutic target.

摘要

尽管肿瘤细胞中存在氧气,但糖酵解速率仍很高(瓦伯格效应),这表明该过程在细胞分裂中起着重要作用。糖酵解速率取决于果糖2,6-二磷酸(Fru-2,6-P2)的细胞浓度,而Fru-2,6-P2又由双功能酶6-磷酸果糖-2-激酶/果糖-2,6-二磷酸酶(PFK-2)控制。由pfkfb3基因编码的普遍存在的PFK-2同工酶(uPFK-2,也称为UBI2K5或ACG)受到不同刺激(血清、孕酮、胰岛素、缺氧等)的诱导,并且在迄今为止发现的所有PFK-2同工酶中具有最高的激酶/磷酸酶活性比,这与其作为糖酵解强大激活剂的作用一致。uPFK-2在脑、胎盘、转化细胞和增殖细胞中表达。在本研究中,我们分析了小干扰RNA(siRNA)诱导的uPFK-2沉默对细胞增殖抑制的影响。用uPFK-2 siRNA处理的HeLa细胞在24小时时测量的uPFK-2 RNA水平降低。与用无关siRNA处理的细胞相比,uPFK-2蛋白水平在48 - 72小时时严重降低,这与糖酵解活性、Fru-2,6-P2、乳酸和ATP浓度的降低相关。这些代谢变化导致活力降低、细胞周期延迟和凋亡细胞数量增加。此外,uPFK-2的抑制抑制了非锚定依赖性生长。获得的结果突出了uPFK-2在糖酵解调节、细胞活力和增殖以及非锚定依赖性生长方面的重要性。这些数据强调了uPFK-2作为有效肿瘤治疗靶点的潜力。

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