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温度对顺铂和卡铂与细胞DNA相互作用的影响。

Effects of temperature on the interaction of cisplatin and carboplatin with cellular DNA.

作者信息

Los G, van Vugt M J, den Engelse L, Pinedo H M

机构信息

Division of Experimental Chemotherapy, The Netherlands Cancer Institute, Amsterdam.

出版信息

Biochem Pharmacol. 1993 Oct 5;46(7):1229-37. doi: 10.1016/0006-2952(93)90472-9.

Abstract

Increased levels of cisplatin (cDDP)- and carboplatin (CBDCA)-DNA adducts were detected in cDDP (10 microM)- and CBDCA (6 mM)-treated CC531 cells when the temperature was raised from 37 degrees to 43 degrees. In the case of cDDP, increased DNA adduct formation was already detectable at 38.5 degrees; additional temperature steps led to further increases in DNA modification. Increased CBDCA-DNA adduct formation was observed only at temperatures higher than 40 degrees. In vitro studies on the interaction of CDDP and CBDCA with isolated salmon sperm DNA, however, demonstrated no significant differences in the DNA binding rate between 37 degrees and 43 degrees for cDDP and a minor effect for CBDCA only at 43 degrees, almost totally excluding a direct temperature effect on DNA platination in this temperature range. Furthermore, neither the stability of the formed platinum-DNA adducts nor the rate of adduct loss in CC531 cells was changed at higher temperatures. The observed difference in cellular adduct formation, however, could be related to increased uptake of cDDP and CBDCA into CC531 cells at higher temperatures. In the case of cDDP, a temperature shift from 37 degrees to 38.5 degrees resulted in a significantly higher intracellular platinum concentration (0.03 +/- 0.01 vs 0.071 +/- 0.021 micrograms platinum/10(6) cells, respectively); for CBDCA, temperatures > or = 41.5 degrees were needed to increase the platinum concentration significantly above 37 degree values (0.3 +/- 0.1 vs 0.6 +/- 0.1 micrograms platinum/10(6) cells, respectively). In addition, the increase in DNA adduct formation of cDDP and CBDCA at elevated temperatures was comparable with the increase in cDDP-DNA adducts after a cDDP concentration escalation at 37 degrees, indicating a concentration-dependent increase in cDDP-DNA adducts. It seems that heat affects primarily the cellular uptake of cDDP and CBDCA and not their covalent binding to DNA.

摘要

当温度从37摄氏度升至43摄氏度时,在经顺铂(cDDP,10微摩尔)和卡铂(CBDCA,6毫摩尔)处理的CC531细胞中,检测到顺铂和卡铂与DNA加合物的水平升高。就顺铂而言,在38.5摄氏度时就已可检测到DNA加合物形成增加;进一步升高温度会导致DNA修饰进一步增加。仅在高于40摄氏度的温度下观察到卡铂与DNA加合物形成增加。然而,对顺铂和卡铂与分离的鲑鱼精子DNA相互作用的体外研究表明,顺铂在37摄氏度至43摄氏度之间的DNA结合率无显著差异,而卡铂仅在43摄氏度时有轻微影响,几乎完全排除了在此温度范围内温度对DNA铂化的直接影响。此外,在较高温度下,CC531细胞中形成的铂 - DNA加合物的稳定性和加合物损失率均未改变。然而,观察到的细胞加合物形成差异可能与较高温度下顺铂和卡铂进入CC531细胞的摄取增加有关。就顺铂而言,温度从37摄氏度转变为38.5摄氏度会导致细胞内铂浓度显著升高(分别为0.03±0.01与0.071±0.021微克铂/10⁶个细胞);对于卡铂,需要温度≥41.5摄氏度才能使铂浓度显著高于37摄氏度时的值(分别为0.3±0.1与0.6±0.1微克铂/10⁶个细胞)。此外,高温下顺铂和卡铂的DNA加合物形成增加与37摄氏度时顺铂浓度升高后顺铂 - DNA加合物的增加相当,表明顺铂 - DNA加合物呈浓度依赖性增加。似乎热主要影响顺铂和卡铂的细胞摄取,而不是它们与DNA的共价结合。

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