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大肠杆菌rplX基因突变导致核糖体蛋白L24缺失的DNA序列及互补分析

DNA sequence and complementation analysis of a mutation in the rplX gene from Escherichia coli leading to loss of ribosomal protein L24.

作者信息

Nishi K, Dabbs E R, Schnier J

出版信息

J Bacteriol. 1985 Sep;163(3):890-4. doi: 10.1128/jb.163.3.890-894.1985.

Abstract

A mutation in Escherichia coli leads to the loss of ribosomal protein L24, severely impaired growth, and a temperature-sensitive phenotype. The mutation was shown to be in rplX, the gene for protein L24, and was due to the alteration of an AAA codon to a TAA stop codon at position 61 in rplX that resulted in a 20-amino acid peptide instead of the 104 amino acids of wild-type L24 protein. rplX genes from three temperature-resistant and fast growing pseudorevertants of the mutant were cloned and sequenced. They were found to have different base substitutions in the TAA codon, resulting in the reappearance of a full-sized protein L24 moiety. Complementation of the slow growth in trans could be achieved with several plasmids containing at least the spc promoter and intact L14 and L24 genes. Plasmids containing genes distal to rplX could further stimulate growth, and the wild type arose when the entire spc operon and the alpha operon were present. In all cases, protein L24 was expressed by the plasmids. Therefore, slow growth could be explained by polarity extending to the alpha operon. However, temperature sensitivity could not be complemented by any of the plasmids in trans, although we found that this phenotype was caused by the mutation in the rplX gene.

摘要

大肠杆菌中的一种突变导致核糖体蛋白L24缺失、生长严重受损以及温度敏感表型。该突变被证明存在于rplX基因中,即蛋白L24的基因,是由于rplX基因第61位的AAA密码子改变为TAA终止密码子,导致产生了一个20个氨基酸的肽段,而非野生型L24蛋白的104个氨基酸。对该突变体的三个温度抗性且生长快速的假回复突变体的rplX基因进行了克隆和测序。发现它们在TAA密码子处有不同的碱基替换,从而使全长的蛋白L24部分重新出现。用几个至少含有spc启动子以及完整的L14和L24基因的质粒可以实现对反式慢生长的互补。含有rplX远端基因的质粒可进一步刺激生长,当整个spc操纵子和α操纵子都存在时会出现野生型。在所有情况下,质粒都表达蛋白L24。因此,慢生长可以用延伸至α操纵子的极性来解释。然而,尽管我们发现这种表型是由rplX基因突变引起的,但任何质粒都无法在反式中互补温度敏感性。

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