Department of Physiology and Pharmacology, City University of New York Medical School, 138th Street and Convent Avenue, New York, NY 10031, United States.
Biochem Pharmacol. 2010 Dec 1;80(11):1641-9. doi: 10.1016/j.bcp.2010.08.011. Epub 2010 Aug 24.
β-Catenin is a central player of the Wnt signaling pathway that regulates cell-cell adhesion and may promote leukemia cell proliferation. We examined whether JS-K, an NO-donating prodrug, modulates the Wnt/β-catenin/TCF-4 signaling pathway in Jurkat T-Acute Lymphoblastic Leukemia cells. JS-K inhibited Jurkat T cell growth in a concentration and time-dependent manner. The IC(50)s for cell growth inhibition were 14±0.7 and 9±1.2μM at 24 and 48h, respectively. Treatment of the cells with JS-K for 24h, caused a dose-dependent increase in apoptosis from 16±3.3% at 10μM to 74.8±2% at 100μM and a decrease in proliferation. This growth inhibition was also due, in part, to alterations in the different phases of the cell cycle. JS-K exhibited a dose-dependent cytotoxicity as measured by LDH release at 24h. However, between 2 and 8h, LDH release was less than 20% for any indicated JS-K concentration. The β-catenin/TCF-4 transcriptional inhibitory activity was reduced by 32±8, 63±5, and 93±2% at 2, 10, and 25μM JS-K, respectively, based on luciferase reporter assays. JS-K reduced nuclear β-catenin and cyclin D1 protein levels, but cytosolic β-catenin expression did not change. Based on a time-course assay of S-nitrosylation of proteins by a biotin switch assay, S-nitrsolyation of nuclear β-catenin was determined to precede its degradation. A comparison of the S-nitrosylated nuclear β-catenin to the total nuclear β-catenin showed that β-catenin protein levels were degraded at 24h, while S-nitrosylation of β-catenin occurred earlier at 0-6h. The NO scavenger PTIO abrogated the JS-K mediated degradation of β-catenin demonstrating the need for NO.
β-连环蛋白是 Wnt 信号通路的核心成员,可调节细胞间黏附,并可能促进白血病细胞增殖。我们研究了 NO 供体型前药 JS-K 是否可调节 Jurkat T 急性淋巴细胞白血病细胞中的 Wnt/β-连环蛋白/TCF-4 信号通路。JS-K 呈浓度和时间依赖性地抑制 Jurkat T 细胞生长。细胞生长抑制的 IC50 值分别为 24 和 48 h 时的 14±0.7 和 9±1.2μM。用 JS-K 处理细胞 24 h 后,凋亡呈剂量依赖性增加,从 10μM 时的 16±3.3%增加至 100μM 时的 74.8±2%,同时增殖减少。这种生长抑制部分也是由于细胞周期不同阶段的改变。JS-K 表现出浓度依赖性细胞毒性,用 LDH 释放检测 24 h 时更明显。然而,在 2 至 8 h 之间,任何指示浓度的 JS-K 引起的 LDH 释放都小于 20%。基于荧光素酶报告基因检测,JS-K 分别使 β-连环蛋白/TCF-4 转录抑制活性降低 32±8%、63±5%和 93±2%,浓度为 2、10 和 25μM。JS-K 降低了核 β-连环蛋白和细胞周期蛋白 D1 蛋白水平,但胞浆 β-连环蛋白表达不变。通过生物素转换测定法测定蛋白质的 S-亚硝基化的时间进程实验,确定核 β-连环蛋白的 S-亚硝基化先于其降解。比较 S-亚硝基化核 β-连环蛋白与总核 β-连环蛋白表明,β-连环蛋白蛋白水平在 24 h 降解,而 S-亚硝基化的 β-连环蛋白在 0-6 h 更早发生。NO 清除剂 PTIO 阻断了 JS-K 介导的 β-连环蛋白降解,表明需要 NO。