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ADP-核糖基转移酶抑制剂对DNA干扰剂损伤的中国仓鼠卵巢细胞G2期进程和致死率的不同影响。

Diverse effects of ADP-ribosyl transferase inhibitors on G2 progression and lethality in Chinese hamster ovary cells damaged by DNA-interfering agents.

作者信息

Ujiie T, Goshima T

机构信息

Department of Experimental Therapeutics, Kanazawa University, Japan.

出版信息

Jpn J Exp Med. 1988 Apr;58(2):99-107.

PMID:3137384
Abstract

DNA-damaging agents used in this study could be divided into two groups, according to their ability to retard G2 traverse. One group included monofunctional alkylating agents, such as N-methyl-N-nitrosourea, dimethyl sulfate, and Streptozotocin. Cells treated with them, which at the tested doses only slightly affected cell cycle progression from the G2 phase to mitosis, were retarded in going through mitosis by subsequent treatment with adenosine diphosphate-ribosyl transferase (ADPRT) inhibitors, such as benzamide, 3-aminobenzamide, nicotinamide, and theophylline, but not by caffeine. Effects of caffeine on G2 progression could be distinguished from those of the other ADPRT inhibitors, and even from the effects of another methylxanthine, theophylline. In addition, the lethality of the monofunctional alkylating agents was markedly enhanced by all of the ADPRT inhibitors, including caffeine. The other group consisted of a variety of agents, including intercalators (Adriamycin and Actinomycin D), a radiomimetic agent, Bleomycin, and a bifunctional alkylating antibiotic, Mitomycin C. They prevented cells from going through mitosis to different degrees. The G2-prolonged cells were variously responsive to ability of the ADPRT inhibitors to release G2-arrest and to enhance cell death.

摘要

根据其延迟G2期进程的能力,本研究中使用的DNA损伤剂可分为两组。一组包括单功能烷基化剂,如N-甲基-N-亚硝基脲、硫酸二甲酯和链脲佐菌素。用这些试剂处理的细胞,在测试剂量下仅轻微影响从G2期到有丝分裂的细胞周期进程,在用二磷酸腺苷核糖基转移酶(ADPRT)抑制剂(如苯甲酰胺、3-氨基苯甲酰胺、烟酰胺和茶碱)后续处理时,其有丝分裂进程受到阻碍,但咖啡因处理则无此效果。咖啡因对G2期进程的影响可与其他ADPRT抑制剂的影响区分开来,甚至与另一种甲基黄嘌呤茶碱的影响区分开来。此外,所有ADPRT抑制剂(包括咖啡因)均显著增强了单功能烷基化剂的致死性。另一组由多种试剂组成,包括嵌入剂(阿霉素和放线菌素D)、一种拟放射剂博来霉素和一种双功能烷基化抗生素丝裂霉素C。它们不同程度地阻止细胞进行有丝分裂。G2期延长的细胞对ADPRT抑制剂释放G2期阻滞和增强细胞死亡的能力有不同的反应。

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