Biological time and the effects of hydroxyurea on DNA synthetic activity of bone marrow and tumor cells in mice bearing the Ehrlich ascites carcinoma.

E R Burns
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Abstract

The objective of this experiment was to attempt to induce, with hydroxyurea (HU), significant quantitative differences in the level of DNA-synthetic activity (DNA-SA) between a neoplastic cell population (the Ehrlich ascites carcinoma or EAC) and bone marrow in the same animal. Mice bearing a 5-day-old EAC were standardized to and kept on an LD 12:12 cycle (light 0600-1800 hr). They were treated with 500 mg/kg HU at 0500 hr (23 hr after lights on, or HALO) or at 1700 hr (11 HALO). DNA-SA was determined by liquid scintillation counting of 3H-thymidine incorporation into chemically isolated DNA. DNA-SA in bone marrow and EAC cells was monitored over the next 60 hr with subgroups of ten mice each killed every 3 hr beginning 3 hr after treatment with HU. The circadian system of the host influenced the response of the bone marrow to HU; i.e., the response to HU administered at 0500 hr was different both qualitatively and quantitatively from that for HU given at 1700 hr. Comparisons of DNA-SA in bone marrow and EAC from the same animal revealed time points after treatment with HU when DNA-SA in the EAC was high, but DNA-SA in bone marrow was low. These differences in the level of DNA-SA between a tumor cell population and bone marrow should be of therapeutic value; i.e., executor doses of anti-DNA-SA drugs such as cytosine arabinoside could be given at that point in time after treatment with HU when DNA-SA in the tumor was high, but DNA-SA in the bone marrow was low.

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生物时间及羟基脲对埃利希腹水癌小鼠骨髓及肿瘤细胞DNA合成活性的影响。
本实验的目的是试图用羟基脲(HU)诱导同一动物的肿瘤细胞群(Ehrlich腹水癌或EAC)和骨髓中dna合成活性(DNA-SA)水平的显著定量差异。将5日龄EAC小鼠标准化并保持在LD 12:12循环(光照0600-1800小时)。在0500小时(开灯后23小时,或光晕)或1700小时(光晕后11小时)给予500 mg/kg HU治疗。DNA- sa是通过液体闪烁计数的3h -胸腺嘧啶并入化学分离的DNA。在接下来的60小时内监测骨髓和EAC细胞中的DNA-SA,从HU治疗后3小时开始,每3小时杀死10只小鼠的亚组。宿主的昼夜节律系统影响骨髓对HU的反应;也就是说,0500小时给药后的反应在质量和数量上都不同于1700小时给药后的反应。比较同一动物骨髓和EAC的DNA-SA,发现HU治疗后EAC中DNA-SA较高,而骨髓中DNA-SA较低。肿瘤细胞群和骨髓之间DNA-SA水平的差异应该具有治疗价值;即在HU治疗后肿瘤DNA-SA高而骨髓DNA-SA低的时间点,给予胞嘧啶阿拉伯糖苷等抗DNA-SA药物执行剂量。
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