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中国仓鼠V79细胞系中代谢协同作用抑制剂体外测定法的进一步特性研究。

Further characterization of the in vitro assay for inhibitors of metabolic cooperation in the Chinese hamster V79 cell line.

作者信息

Jone C, Trosko J E, Aylsworth C F, Parker L, Chang C C

出版信息

Carcinogenesis. 1985 Mar;6(3):361-6. doi: 10.1093/carcin/6.3.361.

Abstract

12-O-Tetradecanoylphorbol-13-acetate (TPA) has been previously shown to inhibit metabolic cooperation in Chinese hamster V79 cells. An in vitro assay, based on this phenomenon, has been developed to study tumor promoters. Several parameters concerning the metabolic cooperation assay using V79 Chinese hamster cells were further investigated in this report. Pretreatment of the cells with TPA in situ for different periods of time did not result in any detectable change in the inhibition of metabolic cooperation. If cells were replated after TPA treatment, a different result was obtained. There was an apparent decrease in the ability of TPA to inhibit metabolic cooperation when TPA was added back to the TPA-pretreated cultures. However, when TPA was omitted from the TPA pretreated cultures after replating, the inhibition of metabolic cooperation remained high. It was also found that pretreatment of the cells with another chemical, aldrin, exhibited the same pattern as the in situ TPA pretreatment effect on inhibition of metabolic cooperation. In order to obtain a high level of inhibition of metabolic cooperation when using aldrin in this assay, it was determined that the chemical needed to be present for more than one day. Our studies also showed that a 24 h treatment with 6-thioguanine did not kill 6-thioguanine-sensitive cells quickly, nor did it prevent them from performing metabolic cooperation. The relationship of cell density and TPA concentration was also studied. It was observed that a higher cell density required higher TPA concentration to inhibit, maximally, metabolic cooperation. A 'down regulation' type effect was noted when culture was challenged with different concentrations of TPA. These results were interpreted to be consistent with the hypothesis that inhibited gap-junctional intercellular communication is one of the components of tumor promotion.

摘要

12 - O - 十四烷酰佛波醇 - 13 - 乙酸酯(TPA)先前已被证明可抑制中国仓鼠V79细胞中的代谢协同作用。基于这一现象,已开发出一种体外测定法来研究肿瘤促进剂。本报告进一步研究了使用V79中国仓鼠细胞进行代谢协同测定的几个参数。在原位用TPA对细胞进行不同时间段的预处理,并未导致代谢协同抑制出现任何可检测到的变化。如果在TPA处理后重新接种细胞,则会得到不同的结果。当将TPA重新添加到经TPA预处理的培养物中时,TPA抑制代谢协同的能力明显下降。然而,在重新接种后从经TPA预处理的培养物中省略TPA时,代谢协同的抑制作用仍然很高。还发现用另一种化学物质艾氏剂对细胞进行预处理,表现出与原位TPA预处理对代谢协同抑制作用相同的模式。为了在该测定中使用艾氏剂时获得高水平的代谢协同抑制,确定该化学物质需要存在超过一天。我们的研究还表明,用6 - 硫鸟嘌呤处理24小时不会迅速杀死对6 - 硫鸟嘌呤敏感的细胞,也不会阻止它们进行代谢协同。还研究了细胞密度与TPA浓度的关系。观察到更高的细胞密度需要更高的TPA浓度才能最大程度地抑制代谢协同。当用不同浓度的TPA刺激培养物时,注意到一种“下调”类型的效应。这些结果被解释为与以下假设一致,即间隙连接细胞间通讯的抑制是肿瘤促进的组成部分之一。

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