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Effects of starvation for potassium and other inorganic ions on protein degradation and ribonucleic acid synthesis in Escherichia coli.

机译:饥饿的钾离子和其他无机离子对大肠杆菌中蛋白质降解和核糖核酸合成的影响。

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摘要

Starvation of Escherichia coli for potassium, phosphate, or magnesium ions leads to a reversible increase in the rate of protein degradation and an inhibition of ribonucleic acid (RNA) synthesis. In cells deprived of potassium, the breakdown of the more stable cell proteins increased two- to threefold, whereas the hydrolysis of short-lived proteins, both normal ones and analog-containing polypeptides, did not change. The mechanisms initiating the enhancement of proteolysis during starvation for these ions were examined. Upon starvation for amino acids or amino acyl-transfer RNA (tRNA), protein breakdown increases in relA+ (but not relA) cells as a result of the rapid synthesis of guanosine-5'-diphosphate-3'-diphosphate (ppGpp). However, a lack of amino acyl-tRNA does not appear to be responsible for the increased protein breakdown in cells starved for inorganic ions, since protein breakdown increased in the absence of these ions in both relA+ and relA cultures, and since a large excess of amino acids did not affect this response. In bacteria in which energy production is restricted, ppGpp levels also rise, and protein breakdown increases. The ion-deprived cultures did show a 40 to 75% reduction in adenosine-5'-triphosphate levels,l similar to that seen upon glucose starvation. However, this decrease in ATP content does not appear to cause the increase in protein breakdown or lead to an accumulation of ppGpp. No consistent change in intracellular ppGpp levels was found in relA+ or relA cells starved for these ions. In addition, in relX mutants, removal of these ions led to accelerated protein degradation even though relX cells are unable to increase ppGpp levels or proteolysis when deprived of a carbon source. In the potassium-, phosphate-, and magnesium-deprived cultures, the addition of choramphenicol or tetracycline caused a reduction in protein breakdown toward basal levels. Such findings, however, do not indicate that protein synthesis is essential for the enhancement of protein degradation, since blockage of protein synthesis by inactivation of a temperature-sensitive valyl-tRNA synthetase did not restore protein catabolism to basal levels. These various results and related studies suggest that the mechanism for increased protein catabolism on starvation for inorganic ions differs from that occurring upon amino acid or arbon deprivation and probably involves an enhanced susceptibility of various cell proteins (especially ribosomal proteins) to proteolysis.
机译:大肠杆菌对钾离子,磷酸根离子或镁离子的饥饿导致蛋白质降解速率的可逆增加和对核糖核酸(RNA)合成的抑制。在缺乏钾的细胞中,更稳定的细胞蛋白质的分解增加了两倍至三倍,而正常蛋白质和含类似物的多肽的短期蛋白质的水解均未改变。检查了饥饿期间这些离子引发蛋白水解增强的机制。氨基酸或氨基酰基转移RNA(tRNA)饥饿后,由于鸟苷5'-二磷酸-3'-二磷酸(ppGpp)的快速合成,relA +(而非relA)细胞中的蛋白质分解增加。然而,缺乏氨基酰基-tRNA似乎并不能导致缺乏无机离子的细胞中蛋白质分解的增加,这是因为在relA +和relA培养物中缺乏这些离子时蛋白质分解会增加。氨基酸不影响该反应。在能量产生受到限制的细菌中,ppGpp水平也升高,蛋白质分解增加。缺乏离子的培养物确实显示了5'-三磷酸腺苷水平降低了40%至75%,与葡萄糖饥饿时所见的相似。但是,ATP含量的下降似乎不会引起蛋白质分解的增加或导致ppGpp的积累。在饥饿于这些离子的relA +或relA细胞中,未发现细胞内ppGpp水平出现一致变化。此外,在relX突变体中,这些离子的去除导致蛋白质降解加速,即使relX细胞在缺乏碳源时无法提高ppGpp水平或蛋白水解。在缺钾,缺磷和缺镁的培养物中,添加氯霉素或四环素会导致蛋白质分解减少至基础水平。然而,这些发现并不表明蛋白质合成对于增强蛋白质降解是必不可少的,因为通过失活温度敏感的缬氨酰-tRNA合成酶来阻止蛋白质合成不能将蛋白质分解代谢恢复到基础水平。这些各种结果和相关研究表明,饥饿时无机离子增加蛋白质分解代谢的机理与氨基酸或碳氢化合物剥夺时发生的机理不同,并且可能涉及各种细胞蛋白质(尤其是核糖体蛋白质)对蛋白水解的敏感性增加。

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