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5-氟尿嘧啶治疗后结肠肿瘤组织中胸苷酸合成酶活性的测定。

Determination of thymidylate synthase activity in colon tumor tissues after treatment with 5-fluorouracil.

作者信息

Houghton J A, Radparvar S, Torrance P M, Williams L G, Houghton P J

出版信息

Biochem Pharmacol. 1987 Apr 15;36(8):1285-9. doi: 10.1016/0006-2952(87)90083-9.

Abstract

The formation and isolation of [6-3H]FdUMP-thymidylate synthase-5,10-methylenetetrahydrofolate covalent complex have been examined in tumor cytosols incubated with albumin-dextran coated charcoal used to remove endogenous nucleotide. Charcoal suspension (10% charcoal, 0.5% albumin, 0.05% dextran) absorbed greater than 98% of dUMP added to cytosols, but it reduced by 42-87% covalent complex isolated from subsequent incubation with [6-3H]FdUMP and cofactor using cytosols from different tumors. Initial treatment of ternary complex with charcoal suspension did not cause a decrease in stability of covalent complex during subsequent incubation (37 degrees), but complex separated from free ligand by 10% charcoal suspension was not stable to further treatment with 4% charcoal suspension. Treatment of tumor cytosols with 10% charcoal suspension, to remove nucleotide, did not decrease the rate at which enzyme catalyzed the release of 3H2O from [5-3H]dUMP, or release active enzyme from the ternary complex. Based on these observations, a sensitive procedure for determining thymidylate synthase activity has been developed in which unbound nucleotides (dUMP, FdUMP) are removed prior to assay of enzyme activity. The procedure is suitable for assay of small samples of tissue or of tissues with a low (or inhibited) level of thymidylate synthase activity.

摘要

在与用于去除内源性核苷酸的白蛋白 - 葡聚糖包被活性炭一起孵育的肿瘤胞质溶胶中,研究了[6 - 3H]氟尿嘧啶脱氧核苷酸 - 胸苷酸合成酶 - 5,10 - 亚甲基四氢叶酸共价复合物的形成与分离。活性炭悬浮液(10%活性炭、0.5%白蛋白、0.05%葡聚糖)吸收了添加到胞质溶胶中的超过98%的脱氧尿苷一磷酸(dUMP),但从不同肿瘤的胞质溶胶后续与[6 - 3H]氟尿嘧啶脱氧核苷酸(FdUMP)和辅因子孵育所分离出的共价复合物减少了42% - 87%。用活性炭悬浮液对三元复合物进行初始处理在随后的孵育(37摄氏度)过程中并未导致共价复合物稳定性下降,但通过10%活性炭悬浮液从游离配体中分离出的复合物对4%活性炭悬浮液的进一步处理不稳定。用10%活性炭悬浮液处理肿瘤胞质溶胶以去除核苷酸,并未降低酶催化从[5 - 3H]dUMP释放3H2O的速率,也未降低从三元复合物中释放活性酶的速率。基于这些观察结果,已开发出一种用于测定胸苷酸合成酶活性的灵敏方法,其中在测定酶活性之前先去除未结合的核苷酸(dUMP、FdUMP)。该方法适用于测定少量组织样本或胸苷酸合成酶活性水平低(或受抑制)的组织样本。

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