首页> 美国卫生研究院文献>Biochemical Journal >Effects of chronic 5-((Z)-4-amino-2-butenylmethylamino)-5-deoxy- adenosine (AbeAdo) treatment on polyamine and eIF-5A metabolism in AbeAdo-sensitive and -resistant L1210 murine leukaemia cells.
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Effects of chronic 5-((Z)-4-amino-2-butenylmethylamino)-5-deoxy- adenosine (AbeAdo) treatment on polyamine and eIF-5A metabolism in AbeAdo-sensitive and -resistant L1210 murine leukaemia cells.

机译:慢性5-(((Z)-4-氨基-2-丁烯基甲基氨基)-5-脱氧腺苷(AbeAdo)处理对AbeAdo敏感和耐药L1210小鼠白血病中多胺和eIF-5A代谢的影响细胞。

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摘要

We have previously reported that prolonged chronic exposure to the S-adenosyl-L-methionine decarboxylase (AdoMetDC) inhibitor, 5'-([(Z)-4-amino-2-butenyl]methylamino)-5'-deoxy-adenosine (MDL 73811, AbeAdo), leads to cytostasis of L1210 cells [Byers, Ganem and Pegg (1992) Biochem. J. 287, 717-724]. Further studies to investigate the mechanism by which these effects are brought about were carried out by comparing an L1210-derived cell line (R20) that is resistant to AbeAdo with the parent cells. The R20 cells were derived by two rounds of AbeAdo-induced cytostasis followed by rescue with exogenous polyamines. Cytostasis was induced in L1210 cells treated for 12 days with 10 microM AbeAdo; however, exposure to up to 40 microM AbeAdo did not induce cytostasis in R20 cells. Putrescine levels were elevated and spermine levels were depleted in both treated L1210 and treated R20 cells. Spermidine was depleted in treated L1210 cells but was only partly reduced in treated R20 cells. AdoMetDC activity was below the limit of detection in treated L1210 cells but, although greatly reduced, could be measured in the treated R20 cells. The resistance of the R20 cells to the effects of AbeAdo on cell growth and spermidine depletion correlated with reduced AbeAdo accumulation by R20 cells. In the absence of spermidine synthesis, unhypusinated eukaryotic translation initiation factor 5A (eIF-5A) accumulated in AbeAdo-treated L1210 cells. There was no detectable accumulation of unhypusinated eIF-5A in R20 cells. Unhypusinated eIF-5A accumulated during AbeAdo treatment was depleted in L1210 cells rescued by exogenous spermidine. These findings are consistent with the hypothesis that AbeAdo-induced cytostasis is due to the loss of hypusinated eIF-5A. However, spermine was able to rescue AbeAdo-treated L1210 cells without significantly reducing the unhypusinated eIF-5A accumulated during AbeAdo treatment, suggesting that only a small amount of the unmodified protein must be hypusinated to restore cell growth.
机译:我们以前曾报道过长期长期暴露于S-腺苷-L-蛋氨酸脱羧酶(AdoMetDC)抑制剂5'-([((Z)-4-氨基-2-丁烯基]甲基氨基)-5'-脱氧腺苷( MDL 73811(AbeAdo)导致L1210细胞的细胞停滞[Byers,Ganem和Pegg(1992)Biochem。 J. 287,717-724]。通过比较对AbeAdo有抗性的L1210衍生细胞系(R20)与亲本细胞,进行了进一步研究以探讨产生这些效应的机制。 R20细胞是通过两轮AbeAdo诱导的细胞停泊,然后用外源多胺进行拯救而获得的。在用10 microM AbeAdo处理12天的L1210细胞中诱导了细胞静止。但是,暴露于40 microM AbeAdo并不会在R20细胞中诱导细胞停滞。在处理过的L1210和处理过的R20细胞中,腐胺的水平都升高了,精胺的水平也降低了。亚精胺在处理过的L1210细胞中耗竭,但在处理过的R20细胞中仅部分减少。在处理过的L1210细胞中,AdoMetDC活性低于检测极限,但是,尽管处理后的R20细胞中AdoMetDC活性大大降低,但仍可以检测到。 R20细胞对AbeAdo对细胞生长和亚精胺消耗的影响的抗性与R20细胞减少的AbeAdo积累有关。在没有亚精胺合成的情况下,未经亚磺酰化的真核翻译起始因子5A(eIF-5A)积累在经AbeAdo处理的L1210细胞中。在R20细胞中未检测到未融合的eIF-5A积累。在AbeAdo处理过程中积累的未羟化的eIF-5A在通过外源亚精胺拯救的L1210细胞中被耗尽。这些发现与假说AbeAdo诱导的细胞停滞是由于丢失了经过血处理的eIF-5A所致。然而,精胺能够挽救经AbeAdo处理的L1210细胞,而不会显着降低在AbeAdo处理过程中积累的未经过水处理的eIF-5A,这表明只有少量未修饰的蛋白质需要经过水处理才能恢复细胞生长。

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