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多胺在大鼠肝癌细胞中对蛋白质合成起始因子eIF-4D的翻译后修饰

Post-translational modification of the protein-synthesis initiation factor eIF-4D by spermidine in rat hepatoma cells.

作者信息

Gerner E W, Mamont P S, Bernhardt A, Siat M

出版信息

Biochem J. 1986 Oct 15;239(2):379-86. doi: 10.1042/bj2390379.

Abstract

The rates of synthesis and turnover of the rare amino acid hypusine [N6-(4-amino-2-hydroxybutyl)-2,6-diaminohexanoic acid] in protein were studied in relationship to polyamine metabolism and growth rates in rat hepatoma tissue-culture (HTC) cells. Hypusine is selectively formed in the eukaryotic translation initiation factor eIF-4D, by a post-translational mechanism involving spermidine [Cooper, Park, Folk, Safer & Braverman (1983) Proc. Natl. Acad. Sci. U.S.A. 80, 1854-1857]. The half-life of the hypusine-containing protein was longer than 24 h. In cells whose intracellular spermidine pools had been initially depleted, by using DL-alpha-difluoromethylornithine (DFMO), maximum synthesis rates of hypusine in protein were 5-10 times higher, on restoration of endogenous spermidine contents by exogenous addition, than those observed in untreated exponential-phase cultures. In cells pretreated with DFMO, the rate of hypusine synthesis was constant for up to 1 h after the addition of 5 microM-spermidine, whereas endogenous spermidine contents varied from less than 1 to more than 10 nmol/mg of protein. However, the overall amount of hypusine formed, during the first 1 h after the addition of various concentrations of spermidine (0.05-10 microM) to the culture medium, was markedly dependent on the final endogenous spermidine content achieved at the end of the 1 h measurement interval. Early in exponential-phase growth, protein-bound hypusine was synthesized at a rate of 1-2 pmol/h per mg of protein. This rate decreased to less than 0.5 pmol/h per mg of protein when cell growth rates decreased as cultures reached high cell densities. Analysis of the polyamine substrate specificity for hypusine formation showed that N1-acetylspermidine did not compete with spermidine in the reaction, nor did N1-(buta-2,3-dienyl)-N2-methylbutane-1,4-diamine, and irreversible inhibitor of polyamine oxidase, block the reaction. On the basis of comparative radiolabelling experiments, spermine was either a poor substrate, or not a substrate, for hypusine formation. These results confirm that spermidine is the likely precursor of the aminohydroxybutyl moiety of hypusine, and show that overall hypusine formation, but not necessarily the synthesis rate, is dependent on the endogenous spermidine concentration, especially under conditions where spermidine concentrations are initially low, as is the case after DFMO treatment, and then increase.

摘要

在大鼠肝癌组织培养(HTC)细胞中,研究了稀有氨基酸hypusine[N6-(4-氨基-2-羟基丁基)-2,6-二氨基己酸]在蛋白质中的合成和周转速率与多胺代谢及生长速率的关系。Hypusine是在真核生物翻译起始因子eIF-4D中通过一种涉及亚精胺的翻译后机制选择性形成的[库珀、帕克、福克、萨弗尔和布拉弗曼(1983年)《美国国家科学院院刊》80, 1854 - 1857]。含hypusine的蛋白质半衰期超过24小时。在细胞内亚精胺池最初已被耗尽的细胞中,通过使用DL-α-二氟甲基鸟氨酸(DFMO),当通过外源添加恢复内源性亚精胺含量时,蛋白质中hypusine的最大合成速率比未处理的指数生长期培养物中观察到的高5 - 10倍。在用DFMO预处理的细胞中,添加5μM亚精胺后长达1小时内hypusine的合成速率保持恒定,而内源性亚精胺含量从每毫克蛋白质少于1纳摩尔变化到超过10纳摩尔。然而,在向培养基中添加各种浓度的亚精胺(0.05 - 10μM)后的最初1小时内形成的hypusine总量明显取决于在1小时测量间隔结束时达到的最终内源性亚精胺含量。在指数生长期早期,蛋白质结合的hypusine以每毫克蛋白质1 - 2皮摩尔/小时的速率合成。当培养物达到高细胞密度时细胞生长速率下降,该速率降至每毫克蛋白质少于0.5皮摩尔/小时。对hypusine形成的多胺底物特异性分析表明,N1-乙酰亚精胺在反应中不与亚精胺竞争,多胺氧化酶的不可逆抑制剂N1-(丁-2,3-二烯基)-N2-甲基丁烷-1,4-二胺也不阻断该反应。基于比较放射性标记实验,精胺要么是hypusine形成的不良底物,要么不是底物。这些结果证实亚精胺可能是hypusine氨基羟基丁基部分 的前体,并表明总体hypusine形成,但不一定是合成速率,取决于内源性亚精胺浓度,特别是在亚精胺浓度最初较低的情况下,如DFMO处理后,然后增加的情况。

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