Van Meter Timothy E, Broaddus William C, Cash Dana, Fillmore Helen
Department of Neurosurgery, Virginia Commonwealth University, Medical College of Virginia Campus, Richmond, Virginia 23230, USA.
Cancer. 2006 Nov 15;107(10):2446-54. doi: 10.1002/cncr.22248.
Heightened activity of the AKT signaling pathway is prominent in malignant gliomas and has been suggested to play a role in treatment resistance. Selective targeting of AKT, therefore, may increase chemosensitivity. Recently, a novel class of AKT-selective inhibitors has been described, including SH-6, a phosphatidylinositol analogue.
The effects of SH-6 on AKT signaling were tested in glioma cells, and the putative role of AKT signaling in chemoresistance was tested by attenuating AKT signaling pharmacologically and genetically. The initial characterization of SH-6 included treatment of glioma cells with increasing doses of SH-6 (0.30-30 microM) and examining the effects on AKT signaling proteins by Western blot analyses and in kinase assays with immunoprecipitated AKT1. Dose-response studies with SH-6 administered to glioma cell lines were performed using a luminescent cell-viability assay (0.1-30 microM). Studies examining the effect of carmustine, either alone or in combination with either the phosphatidylinositol 3-kinase inhibitor LY294002 or SH-6, were performed by cell viability assays and clonogenic survival assays. The effect of carmustine on AKT activity as a response to treatment also was examined. Caspase assays were used to examine the potential role of apoptosis in SH-6/ carmustine -elicited cell death. Finally, the induction of a dominant-negative AKT1 transgene was used in combination with carmustine to demonstrate the role of AKT1 in carmustine chemoresistance.
Serum-stimulated phosphorylation of AKT1 was inhibited by SH-6 at doses > or =10 microM (>70% decrease in Threonine 308 and Serine 473 phosphorylation of AKT1). In adenosine triphosphate assays, 72 hours of treatment with SH-6 led to 50% lethal doses near 10 microM for 2 cell lines tested. SH-6 enhancement of carmustine-mediated cell death led to synergistic increases in Caspase 3/Capsase 7 activity, implicating apoptosis as the cell death mechanism. In clonogenic assays, SH-6 cotreatment with carmustine significantly decreased the number of colonies at 10 microM (P < .05) compared with carmustine alone. No decrease was observed in cells that were treated with SH-6 alone (10 microM). LY294002 (10 microM) was also able to enhance the effects of carmustine significantly in both cell lines.
In the current study, the authors characterized the efficacy of a new class of adjuvant chemotherapeutics that show promise in enhancing the efficacy of standard chemotherapy regimens in gliomas.
AKT信号通路活性增强在恶性胶质瘤中很突出,且被认为在治疗耐药中起作用。因此,选择性靶向AKT可能会增加化疗敏感性。最近,已描述了一类新型的AKT选择性抑制剂,包括磷脂酰肌醇类似物SH-6。
在胶质瘤细胞中测试SH-6对AKT信号的影响,并通过药理学和遗传学方法减弱AKT信号来测试AKT信号在化疗耐药中的假定作用。SH-6的初步特性包括用递增剂量的SH-6(0.30 - 30 microM)处理胶质瘤细胞,并通过蛋白质印迹分析和免疫沉淀的AKT1激酶测定来检测对AKT信号蛋白的影响。使用发光细胞活力测定法(0.1 - 30 microM)对胶质瘤细胞系进行SH-6的剂量反应研究。通过细胞活力测定和克隆形成存活测定来研究卡莫司汀单独或与磷脂酰肌醇3激酶抑制剂LY294002或SH-6联合使用的效果。还检测了卡莫司汀对AKT活性作为治疗反应的影响。使用半胱天冬酶测定来检测凋亡在SH-6/卡莫司汀诱导的细胞死亡中的潜在作用。最后,将显性负性AKT1转基因的诱导与卡莫司汀联合使用,以证明AKT1在卡莫司汀化疗耐药中的作用。
SH-6在剂量≥10 microM时可抑制血清刺激的AKT1磷酸化(AKT1苏氨酸308和丝氨酸473磷酸化降低>70%)。在三磷酸腺苷测定中,用SH-6处理72小时导致所测试的2种细胞系在接近10 microM时出现50%致死剂量。SH-6增强卡莫司汀介导的细胞死亡导致半胱天冬酶3/半胱天冬酶7活性协同增加,提示凋亡是细胞死亡机制。在克隆形成测定中,与单独使用卡莫司汀相比,SH-6与卡莫司汀联合处理在10 microM时显著减少了集落数量(P <.05)。单独用SH-6(10 microM)处理的细胞未观察到集落数量减少。LY294002(10 microM)在两种细胞系中也能够显著增强卡莫司汀的作用。
在当前研究中,作者描述了一类新型辅助化疗药物的疗效,这类药物在增强胶质瘤标准化疗方案的疗效方面显示出前景。