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氯离子和谷氨酸离子对中度嗜盐菌科氏弧菌体外蛋白质合成的影响。

Effect of chloride and glutamate ions on in vitro protein synthesis by the moderate halophile Vibrio costicola.

作者信息

Kamekura M, Kushner D J

出版信息

J Bacteriol. 1984 Oct;160(1):385-90. doi: 10.1128/jb.160.1.385-390.1984.

Abstract

Vibrio costicola grown in the presence of different NaCl concentrations contains cell-associated Na+ and K+ ions whose sum is equal to or greater than the external Na+ concentration. In the presence of 0.5 M NaCl, virtually no in vitro protein is synthesized in extracts of cells grown in 1.0 M NaCl. However, we report here that active in vitro protein synthesis occurred in 0.6 M or higher concentrations of Na2SO4, sodium formate, sodium acetate, sodium aspartate, or sodium glutamate, whereas 0.6 M NaF, NaCl, or NaBr completely inhibited protein synthesis as measured by polyuridylic acid-directed incorporation of [14C]phenylalanine. Sodium glutamate, sodium aspartate, and betaine (0.3 M) counteracted the inhibitory action of 0.6 M NaCl. The cell-associated Cl- concentration was 0.22 mol/kg in cells grown in 1.0 M NaCl. Of this, the free intracellular Cl- concentration was only 0.02 mol/kg. Cells contained 0.11 mol of glutamate per kg and small concentrations of other amino acids. All of the negative counterions for cell-associated Na+ and K+ have not yet been determined. In vitro protein synthesis by Escherichia coli was inhibited by sodium glutamate. Hybridization experiments with ribosomes and the soluble (S-100) fractions from extracts of E. coli and V. costicola showed that the glutamate-sensitive fraction was found in the soluble, not the ribosomal, part of the system. The phenylalanyl-tRNA synthetase of V. costicola was not inhibited by 0.5 M or higher concentrations of NaCl; it was slightly more sensitive to high concentrations of sodium glutamate. Therefore, this enzyme was not responsible for the salt response of the V. costicola in vitro protein-synthesizing system.

摘要

在不同氯化钠浓度条件下生长的栖稻弧菌含有与细胞相关的钠离子和钾离子,其总和等于或大于外部钠离子浓度。在0.5M氯化钠存在的情况下,在1.0M氯化钠中生长的细胞提取物中几乎没有体外蛋白质合成。然而,我们在此报告,在0.6M或更高浓度的硫酸钠、甲酸钠、乙酸钠、天冬氨酸钠或谷氨酸钠中发生了活跃的体外蛋白质合成,而0.6M氟化钠、氯化钠或溴化钠通过聚尿苷酸指导的[14C]苯丙氨酸掺入完全抑制蛋白质合成。谷氨酸钠、天冬氨酸钠和甜菜碱(0.3M)抵消了0.6M氯化钠的抑制作用。在1.0M氯化钠中生长的细胞中,与细胞相关的氯离子浓度为0.22mol/kg。其中,细胞内游离氯离子浓度仅为0.02mol/kg。细胞每千克含有0.11mol谷氨酸和少量其他氨基酸。与细胞相关的钠离子和钾离子的所有负抗衡离子尚未确定。谷氨酸钠抑制大肠杆菌的体外蛋白质合成。用核糖体以及大肠杆菌和栖稻弧菌提取物的可溶性(S-100)组分进行的杂交实验表明,谷氨酸敏感组分存在于该系统的可溶性部分而非核糖体部分。栖稻弧菌的苯丙氨酰-tRNA合成酶不受0.5M或更高浓度氯化钠的抑制;它对高浓度谷氨酸钠稍敏感。因此,这种酶与栖稻弧菌体外蛋白质合成系统的盐反应无关。

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