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能量源下调后大肠杆菌中70S单核糖体的积累。

Accumulation of 70S monoribosomes in Escherichia coli after energy source shift-down.

作者信息

Ruscetti F W, Jacobson L A

出版信息

J Bacteriol. 1972 Jul;111(1):142-51. doi: 10.1128/jb.111.1.142-151.1972.

Abstract

When Escherichia coli is shifted from glucose-minimal to succinate-minimal medium, a transient inhibition of protein synthesis and a time-dependent redistribution of ribosomes from polysomes to 70S monosomes occurs. These processes are reversed by a shift-up with glucose. In a lysate made from a mixture of log-phase and down-shifted cells, the 70S monosomes are derived solely from the down-shifted cells and are therefore not produced by polysome breakage during preparation. This conclusion is supported by the absence of nascent proteins from the 70S peak. The monosomes are not dissociated by NaCl or by a crude ribosome dissociation factor, so they behave as "complexed" rather than "free" particles. When down-shifted cells are incubated with rifampin to block ribonucleic acid (RNA) synthesis, the 70S monosomes disappear with a half-life of 15 min. When glucose is also added this half-life decreases to 3 min. The 70S particles are stable in the presence of rifampin when chloramphenicol is added to block protein synthesis. We interpret these data to mean that the existence of the 70S monosomes depends on the continued synthesis of messenger RNA and their conversion to free ribosomes (which dissociate under our conditions) is a result of their participation in protein synthesis. Finally, a significant fraction of the RNA labeled during a brief pulse of (3)H-uracil is found associated with the 70S peak. These results are consistent with the hypothesis that the 70S monosomes are initiation complexes of single ribosomes and messenger RNA, which do not initiate polypeptide synthesis during a shift-down.

摘要

当大肠杆菌从葡萄糖基本培养基转移至琥珀酸基本培养基时,会出现蛋白质合成的短暂抑制以及核糖体从多核糖体向70S单体的时间依赖性重新分布。这些过程可通过添加葡萄糖进行上调而逆转。在由对数期细胞和下调细胞混合物制成的裂解物中,70S单体仅源自下调细胞,因此并非在制备过程中由多核糖体断裂产生。70S峰中不存在新生蛋白质支持了这一结论。单体不会被氯化钠或粗核糖体解离因子解离,因此它们表现为“复合”而非“游离”颗粒。当下调细胞与利福平一起孵育以阻断核糖核酸(RNA)合成时,70S单体以15分钟的半衰期消失。当同时添加葡萄糖时,该半衰期降至3分钟。当添加氯霉素以阻断蛋白质合成时,70S颗粒在利福平存在下是稳定的。我们将这些数据解释为意味着70S单体的存在取决于信使RNA的持续合成,并且它们向游离核糖体的转化(在我们的条件下会解离)是它们参与蛋白质合成的结果。最后,在短暂的(3)H-尿嘧啶脉冲期间标记的很大一部分RNA与70S峰相关。这些结果与70S单体是单个核糖体和信使RNA的起始复合物的假设一致,它们在下调过程中不会起始多肽合成。

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本文引用的文献

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