Aherne G W, Hardcastle A, Raynaud F, Jackman A L
CRC Centre for Cancer Therapeutics, Institute of Cancer Research, Surey, U.K.
Biochem Pharmacol. 1996 May 17;51(10):1293-301. doi: 10.1016/0006-2952(96)00035-4.
The inhibition of thymidylate synthase (TS) as a drug development target has received much attention in recent years, and several compounds have reached clinical evaluation. During drug development, the effectiveness of target inhibition can be assessed by determination of the perturbations of deoxythymidine 5-triphosphate (TTP) and deoxyuridine 5'-monophosphate (dUMP) pools in drug-treated cells. Rapid, sensitive, and reproducible radioimmunoassays for TTP pools and immunoreactive dUMP pools have been developed to meet our requirement for the rapid assessment of TS inhibition by quinazoline antifolates. The assays can be carried out on 1-2 million cells, and require minimal sample preparation. The limit of detection for TTP is 1 pmole/10(6) cells and for immunoreactive dUMP ("dUMP"), 3.0 pmole/10(6) cells, both assays being performed on the same cell extract. TTP and "dUMP" pools have been measured in mouse L1210 leukaemia cells treated with the quinazoline antifolates ZD1694 (N-(5-[N-(3,4-dihydro-2-methyl-4-oxoquinazolin-6-ylmethyl )-N-methylamine]-2-thenoyl)-L-glutamic acid) and CB30900 (N-[N-[4-[N-[(3,4-dihydro-2,7-dimethyl-4-oxo-6-quinazolinyl)methyl ]-N-prop-2- ynylamino]-2-fluorobenzoyl]-L-gamma-glutamyl]-D-glutamic acid). Unlike ZD1694, CB30900 is a TS inhibitor that does not rely on polyglutamation for activity. In L1210 cells, both compounds caused a rapid inhibition of TTP pools in a dose- and time-related manner. Greater than 90% TS inhibition was achieved following a 4-hr exposure to each compound at equitoxic doses (up to 100 times the IC50 determine by a 48-hr growth inhibition assay). For both compounds, this was accompanied by a 5-10-fold increase in "dUMP" pools. For ZD1694, neither the TTP pool or "dUMP" levels were normalised when cells were resuspended in a drug-free medium for 4 hr and, at the higher doses studied, TS was still inhibited after a 16-hr period in the absence of drug. This is consistent with the formation and intracellular retention of potent polyglutamated forms of ZD1694. In contrast, TS activity as determined by repletion of the TTP pools and normalisation of "dUMP" levels were demonstrated for CB30900. However, at a high dose (50 microM, equivalent to 250 times the IC50), retention of TS inhibition was observed following 4 hr, but not 16 hr in the absence of drug. The radioimmunoassays described will prove useful to further define the extent and time-course of TS inhibition by novel antifolate compounds, and will also provide valuable in vitro and in vivo pharmacodynamic information on established antimetabolites when used alone or in combination with other drugs and modulators.
近年来,将胸苷酸合成酶(TS)作为药物开发靶点的抑制作用备受关注,已有多种化合物进入临床评估阶段。在药物开发过程中,可通过测定药物处理细胞中脱氧胸苷5'-三磷酸(TTP)和脱氧尿苷5'-单磷酸(dUMP)库的扰动情况来评估靶点抑制的有效性。为满足我们对喹唑啉类抗叶酸药物快速评估TS抑制作用的需求,已开发出针对TTP库和免疫反应性dUMP库的快速、灵敏且可重复的放射免疫测定法。这些测定法可在100 - 200万个细胞上进行,且样品制备要求极低。TTP的检测限为1皮摩尔/10⁶个细胞,免疫反应性dUMP(“dUMP”)的检测限为3.0皮摩尔/10⁶个细胞,两种测定均在同一细胞提取物上进行。已对用喹唑啉类抗叶酸药物ZD1694(N-(5-[N-(3,4 - 二氢 - 2 - 甲基 - 4 - 氧代喹唑啉 - 6 - 基甲基)-N - 甲胺]-2 - 噻吩甲酰基)-L - 谷氨酸)和CB30900(N-[N-[4-[N-[(3,4 - 二氢 - 2,7 - 二甲基 - 4 - 氧代 - 6 - 喹唑啉基)甲基]-N - 丙 - 2 - 炔基氨基]-2 - 氟苯甲酰基]-L - γ - 谷氨酰基]-D - 谷氨酸)处理的小鼠L1210白血病细胞中的TTP和“dUMP”库进行了测定。与ZD1694不同,CB30900是一种不依赖多聚谷氨酸化发挥活性的TS抑制剂。在L1210细胞中,两种化合物均以剂量和时间相关的方式迅速抑制TTP库。在等毒性剂量(高达通过48小时生长抑制试验确定的IC50的100倍)下,每种化合物处理4小时后,TS抑制率均超过90%。对于这两种化合物,这都伴随着“dUMP”库增加5 - 10倍。对于ZD1694,当细胞在无药物培养基中重悬4小时后,TTP库或“dUMP”水平均未恢复正常,并且在较高剂量研究中,在无药物的情况下16小时后TS仍被抑制。这与ZD1694的强效多聚谷氨酸化形式的形成和细胞内保留一致。相比之下,通过补充TTP库和使“dUMP”水平恢复正常来测定的CB30900的TS活性得到了证实。然而,在高剂量(50微摩尔,相当于IC50的250倍)下,在无药物的情况下4小时后观察到TS抑制作用持续存在,但16小时后则未观察到。所描述的放射免疫测定法将有助于进一步确定新型抗叶酸化合物对TS抑制的程度和时间进程,并且在单独使用或与其他药物和调节剂联合使用时,还将为已有的抗代谢物提供有价值的体外和体内药效学信息。
