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嗜盐中度菌栖稻弧菌的体外蛋白质合成:氯离子的作用位点

In vitro protein synthesis by the moderate halophile Vibrio costicola: site of action of Cl- ions.

作者信息

Choquet C G, Kamekura M, Kushner D J

机构信息

Department of Biology, University of Ottawa, Ontario, Canada.

出版信息

J Bacteriol. 1989 Feb;171(2):880-6. doi: 10.1128/jb.171.2.880-886.1989.

Abstract

In vitro protein synthesis in Vibrio costicola [poly(U)-directed incorporation of phenylalanine] was studied. The extent of protein synthesis was limited by the number of ribosomes present. Density gradient centrifugation experiments suggested that, after runoff of ribosomes from the artificial messenger, the 50S subunit was unable to attach to the 30S-messenger complex. As shown previously (M. Kamekura and D. J. Kushner, J. Bacteriol. 160:385-390, 1984), Cl- ions inhibited protein synthesis; indeed, the highest rate of synthesis took place in the lowest attainable Cl- concentration (37 mM). The inhibitory effects were partly reversed by glutamate and betaine, both of which are concentrated within cells of V. costicola. The strongest reversal was seen when both glutamate and betaine were present. Cl- ions can prevent binding of ribosomes to poly(U) and displace ribosomes already bound to this artificial messenger. The effects of Cl- ions on binding were also reversed by glutamate and betaine. Cl- ions did not affect accuracy of translation; they were shown previously (Kamekura and Kushner, J. Bacteriol. 160:385-390, 1984) not to affect phenylalanyl-tRNA synthetase. It was also found that washing ribosomes with inhibitory NaCl concentrations did not interfere with their ability to carry out protein synthesis later in optimal (low) salt concentrations. On the contrary, these ribosomes were more active than before they were washed. We conclude that the main site of action of Cl- in the system studied is on the binding of ribosomes to the mRNA.

摘要

对栖热栖热放线菌中的体外蛋白质合成(聚尿苷酸指导的苯丙氨酸掺入)进行了研究。蛋白质合成的程度受核糖体数量的限制。密度梯度离心实验表明,核糖体从人工信使上脱离后,50S亚基无法附着到30S-信使复合物上。如先前所示(M. Kamekura和D. J. Kushner,《细菌学杂志》160:385 - 390,1984年),氯离子抑制蛋白质合成;实际上,最高合成速率发生在可达到的最低氯离子浓度(37 mM)下。谷氨酸和甜菜碱可部分逆转这种抑制作用,这两种物质在栖热栖热放线菌细胞内均有浓缩。当谷氨酸和甜菜碱同时存在时,逆转作用最强。氯离子可阻止核糖体与聚尿苷酸结合,并使已与这种人工信使结合的核糖体脱离。谷氨酸和甜菜碱也可逆转氯离子对结合的影响。氯离子不影响翻译的准确性;先前已表明(Kamekura和Kushner,《细菌学杂志》160:385 - 390,1984年)它不影响苯丙氨酰 - tRNA合成酶。还发现用抑制性氯化钠浓度洗涤核糖体并不干扰其随后在最佳(低)盐浓度下进行蛋白质合成的能力。相反,这些核糖体比洗涤前更活跃。我们得出结论,在所研究的系统中,氯离子的主要作用位点是核糖体与mRNA的结合。

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本文引用的文献

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Salt-sensitive in vitro protein synthesis by a moderately halophilic bacterium.
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