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培养环境中的氢化可的松可保护急性髓细胞白血病中的原始细胞免受阿糖胞苷的致死作用。

Hydrocortisone in culture protects the blast cells in acute myeloblastic leukemia from the lethal effects of cytosine arabinoside.

作者信息

Yang G S, Wang C, Minkin S, Minden M D, McCulloch E A

机构信息

Ontario Cancer Institute, University of Toronto, Canada.

出版信息

J Cell Physiol. 1991 Jul;148(1):60-7. doi: 10.1002/jcp.1041480108.

Abstract

The blast cells in acute myeloblastic leukemia (AML) respond to many of the same regulatory mechanisms that control normal hemopoiesis. These include the growth factors that bind to membrane receptors and steroid hormones or vitamins that have intracellular receptors. We report the effects in culture of the steroid glucocorticoid hydrocortisone on freshly explanted AML blasts from patients and on two continuous AML cell lines. Only small changes in clonogenic cell numbers in suspension cultures were seen in the presence of hydrocortisone. The most striking effect of the hormone was on the sensitivity of blasts cells to cytosine arabinoside (ara-C). In contrast to the response of AML blast cells to retinoic acid, a ligand for intracellular steroid receptors that sensitizes some blast populations to ara-C, hydrocortisone reduced the toxic effects of the drug. The protective action of hydrocortisone was not mediated through the cell cycle since exposure of blasts to hydrocortisone did not affect the percentage of cells in DNA synthesis as measured with the tritiated thymidine (3HTdR) "suicide" technique. The hydrocortisone effect could be demonstrated using a pulse (20 min) exposure protocol. Blasts pulsed with increasing specific activities of 3HTdR showed the usual response pattern with an initial loss in plating efficiency to about 50% of control, followed by a plateau, regardless of whether the cells had been exposed to hydrocortisone. Control blasts exposed to increasing ara-C concentrations gave very similar dose-response curves; in striking contrast, blast cells cultured in hydrocortisone, then pulsed with ara-C did not lose colony-forming ability even though the same population was sensitive to 3HTdR. The hydrocortisone effect was dose and time related; protection from ara-C increased from 10(-8) to 10(-5) M and was seen after 4 hr exposure but required 8 hr to reach a maximum. We conclude that hydrocortisone can protect blasts from the lethal effects of ara-C even while the cells are in active DNA synthesis.

摘要

急性髓细胞白血病(AML)中的原始细胞对许多控制正常造血的调节机制有反应。这些机制包括与膜受体结合的生长因子以及具有细胞内受体的类固醇激素或维生素。我们报告了类固醇糖皮质激素氢化可的松对来自患者的新鲜分离的AML原始细胞以及两种连续AML细胞系在培养中的作用。在氢化可的松存在下,悬浮培养中的克隆形成细胞数量仅有微小变化。该激素最显著的作用是对原始细胞对阿糖胞苷(ara-C)的敏感性。与AML原始细胞对维甲酸(一种细胞内类固醇受体的配体,可使一些原始细胞群体对ara-C敏感)的反应不同,氢化可的松降低了该药物的毒性作用。氢化可的松的保护作用不是通过细胞周期介导的,因为用氚标记胸腺嘧啶核苷(3HTdR)“自杀”技术测量,原始细胞暴露于氢化可的松并不影响DNA合成中的细胞百分比。氢化可的松的作用可以通过脉冲(20分钟)暴露方案来证明。用增加比活性的3HTdR脉冲处理的原始细胞显示出通常的反应模式,即接种效率最初下降至对照的约50%,随后趋于平稳,无论细胞是否暴露于氢化可的松。暴露于增加浓度ara-C的对照原始细胞给出非常相似的剂量反应曲线;形成鲜明对比的是,在氢化可的松中培养然后用ara-C脉冲处理的原始细胞即使同一群体对3HTdR敏感也不会丧失集落形成能力。氢化可的松的作用与剂量和时间相关;对ara-C的保护作用从10^(-8) M增加到10^(-5) M,在暴露4小时后可见,但需要8小时达到最大值。我们得出结论,即使细胞处于活跃的DNA合成状态,氢化可的松也能保护原始细胞免受ara-C的致死作用。

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