三苯基锡香豆素3-羧酸酯及其单齿供氧配体配合物对eb病毒(EBV)-DNA阳性Raji和P-388小鼠白血病细胞系的体外高抗肿瘤活性,以及有机锡抑制EBV裂解周期早期抗原复合物的证据

J Koshy, V G Das, S Balabaskaran, S W Ng, N Wahab
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引用次数: 0

摘要

与标准药物5-氟尿嘧啶的LC(50)值分别为11和>50马克/毫升相比,三苯基锡香豆素-3-羧酸盐及其与乙醇、氧化三苯基膦、氧化三苯基larsine、二苯基环丙烯和喹啉n-氧化物的配合物对EBV-DNA阳性Raji细胞和P-388白血病细胞的体外细胞毒性较高(LC(50)值在0.25-3.4马克/毫升之间)。在肿瘤启动子、TPA和丁酸钠存在的情况下,用喹啉n -氧化物复合物孵育的Raji细胞进行的其他测试显示,相对于只含有启动子的对照组,早期抗原复合物的扩散和限制性蛋白质成分受到抑制,这表明在EBV早期裂解周期中作为反激活因子参与的基因功能受损。与对照相比,限制性内切酶Eco R1和Hind III无法切割从这些处理过的细胞中提取的DNA,再加上PCR技术扩增了BMLF-1基因(仅在对照的DNA上实现,而不是在处理过的样本上实现),这表明有机素与Raji细胞的核DNA存在惩罚性相互作用。
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High In-Vitro Antitumour Activity of Triphenyltin Coumarin 3-Carboxylate and its Coordination Complexes With Monodentate Oxygen Donor Ligands Against the Epstein Barr Virus (EBV)-DNA Positive Raji and the P-388 Murine Leukaemia Cell Lines, and Evidence for the Suppression by Organotin of the Early Antigen Complex in the EBV Lytic Cycle.

Triphenyltin coumarin-3-carboxylate and its coordination complexes with ethanol, triphenylphosphine oxide, triphenylarsine oxide, diphenylcyclopropenone and quinoline N-oxide exhibited high in vitro cytotoxicity (LC(50) values in the range 0.25-3.4 mug/mL) when tested against EBV-DNA positive Raji cells and P-388 leukaemia cells, compared to the standard drug 5-Fluorouracil, which showed LC(50) values of 11 and >50 mug/mL, respectively, against these cells. Additional tests performed on the Raji cells incubated with the quinoline N-oxide complex in the presence of the tumour promoters, TPA and sodium butyrate, revealed that the diffused and restricted protein components of the early antigen complex were suppressed relative to the control containing only the promoters, indicating impaired function of the genes involved as transactivators in the early lytic cycle of the EBV. The failure of the restriction enzymes Eco R1 and Hind III to cleave the extracted DNA from such treated cells in contrast to the control, coupled with the amplification of the BMLF-1 gene by the PCR technique which was realised only with the DNA of the control and not of the treated sample, point to a punitive interaction of the organotin with the nuclear DNA of the Raji cells.

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