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首页> 外文期刊>The biochemical journal >The control of ribonucleic acid synthesis in bacteria. Steady-state content of messenger ribonucleic acid in Escherichia coli M.R.E. 600
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The control of ribonucleic acid synthesis in bacteria. Steady-state content of messenger ribonucleic acid in Escherichia coli M.R.E. 600

机译:细菌中核糖核酸合成的控制。大肠杆菌M.R.E.中信使核糖核酸的稳态含量600

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p1. The technique of DNA–RNA hybridization was used to follow changes in the amount and average lifetime of unstable messenger RNA in iEscherichia coli/i M.R.E. 600 over a wide range of different growth conditions. The method of analysis was based on the kinetics of incorporation of exogenous labelled nucleic acid bases into the RNA of steadily growing cultures, as described by Bolton & McCarthy (1962). 2. The ratio of the average lifetime of messenger RNA to the mean generation time of iE. coli/i cultures was constant over the temperature range 25–45°C in a given medium, but the constant varied with the nature of the growth medium. For cultures growing in sodium lactate–salts or glucose–salts media the ratio was 0.046±0.005 and in enriched broth it was 0.087±0.009. Measurements of the amounts of transfer RNA, ribosomal RNA and messenger RNA were also made. The results confirmed earlier reports that the ratio of the amount of messenger RNA to the amount of ribosomes in the cells is virtually constant. On the other hand, the ratio of the amount of transfer RNA to the amount of ribosomal RNA decreased with increasing growth rate at a given temperature. 3. In cultures at temperatures higher than necessary for optimum rates of growth the average lifetime of messenger RNA lengthened in harmony with the increased time required for cell division. It seems that suboptimum growth rates at higher temperatures cannot be explained simply as a combination of increased rates of synthesis and breakdown of messenger RNA with a grossly decreased efficiency of translation. The absolute rate of messenger RNA synthesis was lowered, and its amount in the cells was typical of all other cultures grown at lower temperatures in the same medium. 4. The rate of entry of exogenous labelled uracil into unstable messenger RNA and stable ribosomal RNA was constant in all media at all temperatures in the approximate ratio 1:2. In media supporting a lower rate of growth, e.g. lactate–salts or glucose–salts media, the messenger RNA fraction constituted 2.2±0.3% of the total cellular RNA. In enriched broth 3.6±0.3% of the total RNA was messenger./p
机译:> 1。 DNA-RNA杂交技术用于追踪大肠杆菌中不稳定信使RNA的数量和平均寿命的变化。 600种不同的生长条件。分析方法是基于将外源标记的核酸碱基掺入稳定生长的培养物的RNA中的动力学,如Bolton& A.A.S.等人所述。麦卡锡(1962)。 2.信使RNA的平均寿命与E的平均产生时间之比。在给定培养基中,大肠杆菌培养物在25–45°C的温度范围内保持恒定,但该常数随生长培养基的性质而变化。对于在乳酸钠盐或葡萄糖盐培养基中生长的培养物,该比例为0.046±0.005,在高汤中为0.087±0.009。还测量了转移RNA,核糖体RNA和信使RNA的量。该结果证实了较早的报道,即细胞中信使RNA的量与核糖体的量之比实际上是恒定的。另一方面,在给定温度下,随着生长速率的增加,转移RNA的量与核糖体RNA的量之比降低。 3.在高于最佳生长速率所需温度的培养物中,信使RNA的平均寿命与细胞分裂所需的时间增加一致地延长。似乎不能将较高温度下的最佳生长速率简单地解释为合成速率的提高和信使RNA的分解以及翻译效率的大幅降低。信使RNA合成的绝对速率降低,并且其在细胞中的量是在相同培养基中在较低温度下生长的所有其他培养物的典型值。 4.外源标记的尿嘧啶进入不稳定的信使RNA和稳定的核糖体RNA的速率在所有温度下在所有培养基中都是恒定的,比率约为1:2。支持较低增长率的媒体,例如在乳酸盐或葡萄糖盐介质中,信使RNA组分占细胞总RNA的2.2±0.3%。在浓缩肉汤中,总RNA的3.6±0.3%是信使。

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