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通过流式细胞术检测亚砜钌化合物和顺铂对体外TLX5淋巴瘤细胞周期和活力的影响。

Modification of cell cycle and viability of TLX5 lymphoma in vitro by sulfoxide-ruthenium compounds and cisplatin detected by flow cytometry.

作者信息

Capozzi I, Clerici K, Cocchietto M, Salerno G, Bergamo A, Sava G

机构信息

Institutes of Biological Research, Trieste, Italy.

出版信息

Chem Biol Interact. 1998 May 1;113(1):51-64. doi: 10.1016/s0009-2797(98)00022-2.

Abstract

The effects of Na[trans-RuCl4(DMSO)Im] (NAMI), Na[trans-RuCl4(TMSO) Ind] (TIND) and Na[trans-RuCl4(TMSO)Iq] TEQU) were tested in vitro on TLX5 lymphoma cells in comparison to cisplatin by means of the sulforhodamine-B test SRB) for protein content determination, by acridine orange and propidium iodide staining and by means of the bromodeoxyuridine test, for cell cycle modifications. After 1 h drug exposure with metal-based drugs, TLX5 lymphoma cells require a further 72 h in vitro cultivation to show alteration of cell cycle. Ruthenium compounds show a different pattern of effects: TEQU causes the same dose-dependent cytotoxicity and DNA fragmentation shown by cisplatin, TIND reduces absorbance with the SRB test and slightly increases S and G2M populations with a time-dependent drug exposure of tumour cells, and NAMI is virtually devoid of any detectable effect. By in vivo bioassay of in vitro treated tumour cells, TIND and TEQU are effective independently of the time of drug exposure of tumour cells, this effect being confirmed by the same cell uptake of ruthenium after 1 or 4 h treatment, determined by atomic absorption spectroscopy. These data stress the lack of the involvement of direct cytotoxic effects in the potent anti-metastatic action of NAMI.

摘要

通过磺酰罗丹明 - B试验(SRB)测定蛋白质含量、吖啶橙和碘化丙啶染色以及溴脱氧尿苷试验检测细胞周期变化,在体外对TLX5淋巴瘤细胞测试了反式 - 四氯钌(二甲基亚砜)亚胺钠(NAMI)、反式 - 四氯钌(三甲基亚砜)吲哚钠(TIND)和反式 - 四氯钌(三甲基亚砜)异喹啉钠(TEQU)的效果,并与顺铂进行比较。在用金属基药物处理1小时后,TLX5淋巴瘤细胞需要在体外进一步培养72小时才能显示细胞周期的改变。钌化合物表现出不同的效应模式:TEQU引起与顺铂相同的剂量依赖性细胞毒性和DNA片段化,TIND通过SRB试验降低吸光度,并随着肿瘤细胞药物暴露时间的延长,S期和G2M期细胞群略有增加,而NAMI几乎没有任何可检测到的效应。通过对体外处理的肿瘤细胞进行体内生物测定,TIND和TEQU的有效性与肿瘤细胞的药物暴露时间无关,通过原子吸收光谱法测定,在1或4小时处理后钌的细胞摄取相同证实了这一效应。这些数据强调了直接细胞毒性作用在NAMI强大的抗转移作用中并未发挥作用。

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