Pereira E, Tarasiuk J, Garnier-Suillerot A
Laboratoire de Physicochimie Biomoléculaire et Cellulaire (UPRES-A 7033), Université Paris-Nord, Bobigny, France.
Chem Biol Interact. 1998 Jul 3;114(1-2):61-76. doi: 10.1016/s0009-2797(98)00036-2.
Cells that overexpress the mdr 1 gene have decreased steady-state accumulation and increased efflux of many anticancer drugs including anthracyclines and vinca alkaloids. The mechanism(s) of P-glycoprotein-mediated efflux of drugs is (are) still poorly understood. In an attempt to identify mechanism(s) by which multidrug resistance can be circumvented, the cellular accumulation has been examined of pirarubicin, doxorubicin and idarubicin alone and in conjunction with four vinca alkaloid derivatives--vinblastine, navelbine, vindesine and vincristine. The present study was performed using a spectrofluorometric method with which it is possible to follow continuously the uptake and release of fluorescent molecules by living cells, as the incubation of the cells with the drug proceeds. Erythroleukemia K562 cell lines were used. It has been shown that the P-glycoprotein-mediated efflux of these three anthracyclines can be inhibited by vinca alkaloids derivatives. At pH 7.2, 50% of the P-glycoprotein-mediated efflux of daunorubicin and idarubicin was inhibited by about 40 +/- 10 microM vinblastine and that of pirarubicin by 10 +/- 2 microM vinblastine. The vinblastine concentration required to inhibit 50% of the active efflux of these anthracyclines did not depend on the anthracycline concentrations used, indicating that the inhibition was non competitive. The ability of navelbine, vincristine and vindesine to inhibit the active efflux of pirarubicin was also checked; 15 +/- 3 microM navelbine are required to inhibit 50% of the active efflux but at concentrations lower than 100 microM, neither vincristine nor vindesine were able to inhibit this efflux, indicating that the vinca alkaloids compounds which are the most efficient are the most lipophilic. For the four vinca alkaloids, the concentration required to inhibit 50% of the efflux was lower as the pH was higher. A detailed kinetics analysis of the P-glycoprotein-mediated efflux of pirarubicin in the presence of vinblastine indicates a non competitive inhibition with K(I) = 12 +/- 2 microM.
过表达mdr 1基因的细胞对包括蒽环类药物和长春花生物碱在内的多种抗癌药物的稳态蓄积减少,外排增加。P-糖蛋白介导的药物外排机制仍知之甚少。为了确定能够规避多药耐药性的机制,研究了单独及与四种长春花生物碱衍生物(长春碱、诺维本、长春地辛和长春新碱)联合使用时吡柔比星、多柔比星和伊达比星的细胞蓄积情况。本研究采用荧光分光光度法进行,随着细胞与药物的孵育过程,可以持续跟踪活细胞对荧光分子的摄取和释放。使用了红白血病K562细胞系。结果表明,长春花生物碱衍生物可抑制这三种蒽环类药物的P-糖蛋白介导的外排。在pH 7.2时,约40±10 μM长春碱可抑制50%柔红霉素和伊达比星的P-糖蛋白介导的外排,10±2 μM长春碱可抑制50%吡柔比星的外排。抑制50%这些蒽环类药物主动外排所需的长春碱浓度不依赖于所用蒽环类药物的浓度,表明该抑制作用是非竞争性的。还检测了诺维本、长春新碱和长春地辛抑制吡柔比星主动外排的能力;抑制50%主动外排需要15±3 μM诺维本,但在浓度低于100 μM时,长春新碱和长春地辛均无法抑制这种外排,表明最有效的长春花生物碱化合物是亲脂性最强的。对于这四种长春花生物碱,随着pH升高,抑制50%外排所需的浓度降低。在长春碱存在的情况下,对吡柔比星的P-糖蛋白介导的外排进行详细的动力学分析表明,这是一种非竞争性抑制,K(I)=12±2 μM。
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