Oka Hiroaki, Ikeda Kazumasa, Yoshimura Hiromi, Ohuchida Akinobu, Honma Masamitsu
Drug Safety Research Lab., Taiho Pharmaceutical Co. Ltd., 224-2 Ebisuno, Hiraishi, Kawauchi-cho, Tokushima, Japan.
Mutat Res. 2006 Jul 14;606(1-2):52-60. doi: 10.1016/j.mrgentox.2006.02.001. Epub 2006 Apr 3.
Mouse lymphoma L5178Ytk+/- (MOLY) cells and human lymphoblastoid TK6 and WTK-1 cells are widely used to detect mutagens in vitro. MOLY and WTK-1 cells have a p53 mutation, while TK6 cells, which were derived from the same parental line as WTK-1 cells, do not. In this study, we tested the clastogen 5-fluorouracil (5-FU) in the Tk assay and the in vitro micronucleus (MN) assay in MOLY, TK6, and WTK-1 cells to clarify whether differential responses were related to p53 gene status. We also determined the effect of 5-FU on the frequency of apoptotic cells and on cell cycle distribution in each cell line. Furthermore, we measured the activity of the 5-FU metabolizing enzymes (thymidylate synthetase (TS), dihydrouracil dehydrogenase (DPD), orotate phosphoribosyl transferase (OPRT), and thymidine phosphorylase (TP)) in each cell line. We treated MOLY cells with 1.0-8.0 microg/mL 5-FU for 3 h and TK6 and WTK-1 cells with 1.56-25 and 3.13-50 microg/mL, respectively, for 4 h. In MOLY cells, the mutation frequency (MF) and MN frequency increased. In WTK-1 cells, the MN frequency but not the MF increased. In TK6 cells, neither the MF nor the MN frequency increased. Furthermore, the IC50 of 5-FU was lower in MOLY cells than in the human cells. The response to 5-FU treatment differed in other ways as well. At the same level of cytotoxicity, the frequency of apoptotic cell was highest in TK6 cells. The cell cycle was delayed just after treatment in MOLY cells while the delay appeared 24 h later in TK6 and WTK-1 cells. Nothing in our analysis, however, revealed marked differences between the cell lines that could account for the severe cytotoxic and mutagenic responses that 5-FU elicited only in MOLY cells. 5-FU is phosphorylated by OPRT and TP and detoxified by DPD. MOLY cells have higher OPRT activity and markedly lower DPD and TP activity than TK6 and WTK-1 cells. The content of TS, however, the target enzyme of 5-FU, was similar in all cell lines, suggesting that 5-FU was more readily phosphorylated and less readily detoxified in MOLY cells than in TK6 and WTK-1 cells. MOLY cells were more sensitive to 5-FU than WTK-1 cells even though both have a mutated p53 gene, suggesting that the different responses to 5-FU were due to differences in 5-FU metabolism rather than the p53 status.
小鼠淋巴瘤L5178Ytk+/-(MOLY)细胞以及人淋巴母细胞TK6和WTK-1细胞被广泛用于体外检测诱变剂。MOLY和WTK-1细胞存在p53突变,而与WTK-1细胞源自同一亲代细胞系的TK6细胞则没有。在本研究中,我们在Tk试验以及MOLY、TK6和WTK-1细胞的体外微核(MN)试验中检测了诱变剂5-氟尿嘧啶(5-FU),以阐明不同的反应是否与p53基因状态有关。我们还确定了5-FU对各细胞系中凋亡细胞频率和细胞周期分布的影响。此外,我们测量了各细胞系中5-FU代谢酶(胸苷酸合成酶(TS)、二氢尿嘧啶脱氢酶(DPD)、乳清酸磷酸核糖转移酶(OPRT)和胸苷磷酸化酶(TP))的活性。我们分别用1.0 - 8.0μg/mL的5-FU处理MOLY细胞3小时,用1.56 - 25μg/mL和3.13 - 50μg/mL的5-FU处理TK6和WTK-1细胞4小时。在MOLY细胞中,突变频率(MF)和微核频率增加。在WTK-1细胞中,微核频率增加,但突变频率未增加。在TK6细胞中,突变频率和微核频率均未增加。此外,5-FU在MOLY细胞中的半数抑制浓度(IC50)低于人源细胞。对5-FU处理的反应在其他方面也有所不同。在相同细胞毒性水平下,TK6细胞中凋亡细胞的频率最高。MOLY细胞在处理后细胞周期立即延迟,而TK6和WTK-1细胞的延迟在24小时后出现。然而,我们的分析未发现细胞系之间存在明显差异,这些差异可以解释5-FU仅在MOLY细胞中引发的严重细胞毒性和诱变反应。5-FU由OPRT和TP磷酸化,并由DPD解毒。MOLY细胞的OPRT活性高于TK6和WTK-1细胞,而DPD和TP活性则明显低于它们。然而,5-FU的靶酶TS的含量在所有细胞系中相似,这表明与TK6和WTK-1细胞相比,5-FU在MOLY细胞中更容易被磷酸化且更难被解毒。尽管MOLY细胞和WTK-1细胞都有突变的p53基因,但MOLY细胞对5-FU比WTK-1细胞更敏感,这表明对5-FU的不同反应是由于5-FU代谢的差异而非p53状态。
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