Rustum Y M, Raymakers R A
Department of Experimental Therapeutics, Roswell Park Cancer Institute, Buffalo, NY 14263.
Pharmacol Ther. 1992 Dec;56(3):307-21. doi: 10.1016/0163-7258(92)90022-r.
Although the mechanisms of therapeutic efficacy of cytosine arabinoside (Ara-C) are multifactorial, the pharmacodynamic basis for its cytotoxicity and therapeutic efficacy lies in its intracellular metabolism and the retention of the active metabolite, Ara-C triphosphate (Ara-CTP), which is a competitive inhibitor of DNA polymerase. Additional determinants of tumor cell sensitivity include Ara-CMP incorporation into cellular DNA, the size of the competing normal metabolite, deoxycytidine/5'-triphosphate pool, and the heterogeneity in growth kinetics of tumor cells, S-phase vs cells in other phases of the cell cycle. With high-dose Ara-C, substantial amounts of Ara-CTP are formed in phases of the cell cycle. The presence of high intracellular concentration with prolonged retention of Ara-CTP could lead to the inhibition of cell growth of the cells entering S-phase as a consequence of inhibition of DNA-polymerase and/or incorporation into cellular DNA, resulting in a chain termination. Pharmacokinetically, Ara-C is rapidly eliminated from plasma. In mice, pharmacokinetic parameters of Ara-C are not sufficient predictors for the observed differences in their in vivo antitumor activity. Although these mice were bearing different tumor types (L1210 Ara-C sensitive or P-388 relatively more resistant), the observed differences in tumor response were achieved under identical plasma Ara-C concentrations and area under the concentration time curve. The observed antitumor activity in L1210 cells is primarily associated with higher Ara-CTP pools and retention (T1/2 > 4 hr) in tumor cells as compared with normal bone marrow cells. In the least responsive tumor (P-388), although Ara-CTP pools were sufficiently high, retention of the drug in tumor cells and in normal cells is poor with a T1/2 < 2 hr. Thus, unlike mice bearing leukemia L1210 cells, alteration of the mode and dose of administration of Ara-C in mice bearing P-388 could only result in increased host toxicity with no therapeutic gain. Similarly in patients with acute nonlymphocyte leukemia (ANLL), there is no significant correlation between plasma Ara-C concentration and the intracellular concentrations or retentions of Ara-CTP. In some patients the highest Ara-CTP pools in leukemic myeloblast cells are achieved at a lower level of plasma Ara-C and decrease further with the increase of plasma Ara-C. Thus, in the in vivo model system and in ANLL patients with no prior chemotherapy, Ara-CTP retention is a critical factor associated with response to this agent, in particular its direct association with duration of complete response.(ABSTRACT TRUNCATED AT 400 WORDS)
尽管阿糖胞苷(Ara-C)的治疗作用机制是多因素的,但其细胞毒性和治疗效果的药效学基础在于其细胞内代谢以及活性代谢产物三磷酸阿糖胞苷(Ara-CTP)的潴留,Ara-CTP是DNA聚合酶的竞争性抑制剂。肿瘤细胞敏感性的其他决定因素包括Ara-CMP掺入细胞DNA、竞争性正常代谢物脱氧胞苷/5'-三磷酸池的大小以及肿瘤细胞生长动力学的异质性,即S期与细胞周期其他阶段的细胞。使用高剂量Ara-C时,在细胞周期各阶段会形成大量Ara-CTP。细胞内高浓度且Ara-CTP长时间潴留,可能会因抑制DNA聚合酶和/或掺入细胞DNA而导致进入S期的细胞生长受到抑制,从而导致链终止。在药代动力学方面,Ara-C可迅速从血浆中清除。在小鼠中,Ara-C的药代动力学参数并不能充分预测其体内抗肿瘤活性的差异。尽管这些小鼠携带不同类型的肿瘤(对Ara-C敏感的L1210或相对更耐药的P-388),但在相同的血浆Ara-C浓度和浓度-时间曲线下面积时观察到了肿瘤反应的差异。与正常骨髓细胞相比,在L1210细胞中观察到的抗肿瘤活性主要与肿瘤细胞中更高的Ara-CTP池和潴留(T1/2>4小时)有关。在反应最差的肿瘤(P-388)中,尽管Ara-CTP池足够高,但药物在肿瘤细胞和正常细胞中的潴留较差,T1/2<2小时。因此,与携带白血病L1210细胞的小鼠不同,改变携带P-388的小鼠中Ara-C的给药方式和剂量只会导致宿主毒性增加而无治疗益处。同样,在急性非淋巴细胞白血病(ANLL)患者中,血浆Ara-C浓度与Ara-CTP的细胞内浓度或潴留之间没有显著相关性。在一些患者中,白血病成髓细胞中最高的Ara-CTP池是在较低的血浆Ara-C水平时达到的,并且随着血浆Ara-C的增加而进一步降低。因此,在体内模型系统和未接受过化疗的ANLL患者中,Ara-CTP潴留是与该药物反应相关的关键因素,特别是其与完全缓解持续时间的直接关联。(摘要截断于400字)
