9([2-羟基-1-(羟甲基)乙氧基]甲基)鸟嘌呤在感染爱泼斯坦-巴尔病毒的人淋巴母细胞系中的代谢活化。
Metabolic activation of 9([2-hydroxy-1-(hydroxymethyl)ethoxy]methyl)guanine in human lymphoblastoid cell lines infected with Epstein-Barr virus.
作者信息
Lin J C, Nelson D J, Lambe C U, Choi E I
出版信息
J Virol. 1986 Nov;60(2):569-73. doi: 10.1128/JVI.60.2.569-573.1986.
9-([2-Hydroxy-1-(hydroxymethyl)ethoxy]methyl)guanine (BW B759U) is more potent and has a more prolonged inhibitory effect against Epstein-Barr virus (EBV) in vitro than does acyclovir (ACV). To assess the mechanism of this difference, we first compared the extent of phosphorylation of the two drugs in superinfected Raji cells. BW B759U is phosphorylated to levels 100-fold higher than is ACV. In addition, lower levels of phosphorylation of BW B759U and ACV were observed in uninfected Raji cells. Studies on the kinetics of formation of BW B759U triphosphate in superinfected Raji cells indicated that drug-phosphorylating activity was detected as early as 3 h after superinfection; this activity was steadily maintained for the first 7 h, followed by a burst of activity between 7 and 10 h and a doubling of phosphorylation between 10 and 25 h. During the superinfection cycle, the pool sizes of deoxyribonucleoside and ribonucleoside triphosphates were increased and reached their maxima at 10 h after infection. The maximal amount of triphosphorylated drug in a virus producer cell, P3HR-1 (LS), was obtained at 21 h after drug treatment. During long-term drug treatment, approximately 44 and 77% reduction in EBV genome copies per cell was observed on days 3 and 7, respectively. In a separate experiment, after treatment of P3HR-1 (LS) cells with BW B759U for 36 h, 4.2 pmol of BW B759U triphosphate per 10(6) cells was achieved. After the cells were released into drug-free medium, drug triphosphate was rapidly decreased to 11% of the original level in 1 day. Thereafter, the decrease was slow but steady, down to 0.22 pmol/10(6) P3HR-1 cells by 5 days. We calculated that 0.22 pmol of BW B759U triphosphate per 10(6) cells represents a cellular concentration of 0.22 microM, which is theoretically enough to inhibit EBV replication. This is based upon a comparison with the 50% effective dose of BW B759U (0.05 microM) for inhibition of genome replication and a Ki of 0.08 microM for BW B759U triphosphate inhibition of EBV DNA polymerase.
9 -([2 - 羟基 - 1 -(羟甲基)乙氧基]甲基)鸟嘌呤(BW B759U)在体外对爱泼斯坦 - 巴尔病毒(EBV)的抑制作用比阿昔洛韦(ACV)更强且持续时间更长。为评估这种差异的机制,我们首先比较了两种药物在超感染的拉吉细胞中的磷酸化程度。BW B759U的磷酸化水平比ACV高100倍。此外,在未感染的拉吉细胞中观察到BW B759U和ACV的磷酸化水平较低。对超感染的拉吉细胞中BW B759U三磷酸酯形成动力学的研究表明,在超感染后3小时就检测到了药物磷酸化活性;这种活性在前7小时稳定维持,随后在7至10小时之间出现活性爆发,在10至25小时之间磷酸化增加一倍。在超感染周期中,脱氧核糖核苷和核糖核苷三磷酸的池大小增加,并在感染后10小时达到最大值。在病毒产生细胞P3HR - 1(LS)中,药物处理后21小时获得了三磷酸化药物的最大量。在长期药物治疗期间,分别在第3天和第7天观察到每个细胞中EBV基因组拷贝数减少约44%和77%。在另一个实验中,用BW B759U处理P3HR - 1(LS)细胞36小时后,每10⁶个细胞达到4.2皮摩尔的BW B759U三磷酸酯。在将细胞释放到无药物培养基中后,药物三磷酸酯在1天内迅速降至原始水平的11%。此后,下降缓慢但稳定,到第5天时降至0.22皮摩尔/10⁶个P3HR - 1细胞。我们计算得出,每10⁶个细胞0.22皮摩尔的BW B759U三磷酸酯代表细胞浓度为0.22微摩尔,理论上足以抑制EBV复制。这是基于与抑制基因组复制的BW B759U的50%有效剂量(0.05微摩尔)以及BW B759U三磷酸酯抑制EBV DNA聚合酶的Ki值0.08微摩尔进行比较得出的。
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