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大肠杆菌苏氨酸操纵子衰减反应的特异性由前导转录本中的苏氨酸和异亮氨酸密码子决定。

Specificity of the attenuation response of the threonine operon of Escherichia coli is determined by the threonine and isoleucine codons in the leader transcript.

作者信息

Lynn S P, Burton W S, Donohue T J, Gould R M, Gumport R I, Gardner J F

出版信息

J Mol Biol. 1987 Mar 5;194(1):59-69. doi: 10.1016/0022-2836(87)90715-7.

Abstract

Expression of the threonine (thr) operon enzymes of Escherichia coli is regulated by an attenuation mechanism. The regulatory portion of the operon contains a region coding for a leader peptide that contains consecutive threonine and isoleucine codons. It is thought that translation of the leader peptide controls the frequency of transcription termination at the attenuator site. Using oligonucleotide-directed site-specific mutagenesis we have altered the putative control codons of the leader peptide coding region. In two of the mutants the threonine and isoleucine codons were changed to produce peptides containing histidine and tyrosine codons. Both mutants showed loss of regulation by threonine and isoleucine. A hisT mutation, which leads to an undermodification of tRNA(His), increased thr operon expression in the mutants threefold but did not affect expression of the wild-type thr operon. Two other mutants were constructed that contained two histidine codons early in the leader peptide. Expression in both of these mutants was unaltered by the presence of the hisT allele or by the addition of threonine and isoleucine to the growth medium. In addition, a wild-type strain containing a temperature-sensitive threonyl-tRNA synthetase mutation showed increased thr operon expression at the non-permissive temperature, whereas none of the mutants showed any change. Taken together these data indicate that the specificity of the attenuation response is effected by specific control codons within the thr leader peptide coding region. We have also directly demonstrated thr leader peptide synthesis in vitro using a plasmid encoding the wild-type thr leader region to direct the synthesis of a peptide of the appropriate molecular weight when labeled with [3H]threonine but not with [3H]histidine or [3H]tyrosine. Conversely, when extracts were incubated with templates containing the mutated DNAs, peptides were labeled that showed patterns consistent with the expected amino acid compositions. These data indicate that the thr leader RNA is translated into the predicted leader peptide.

摘要

大肠杆菌苏氨酸(thr)操纵子酶的表达受衰减机制调控。该操纵子的调控部分包含一个编码前导肽的区域,此前导肽含有连续的苏氨酸和异亮氨酸密码子。据认为,前导肽的翻译控制着衰减子位点转录终止的频率。我们利用寡核苷酸定向位点特异性诱变技术改变了前导肽编码区的假定控制密码子。在两个突变体中,苏氨酸和异亮氨酸密码子被改变,以产生含有组氨酸和酪氨酸密码子的肽段。这两个突变体均表现出对苏氨酸和异亮氨酸调控的丧失。hisT突变导致tRNA(His)修饰不足,使突变体中的thr操纵子表达增加了三倍,但不影响野生型thr操纵子的表达。构建了另外两个突变体,它们在前导肽的早期含有两个组氨酸密码子。这两个突变体的表达不受hisT等位基因的存在或生长培养基中添加苏氨酸和异亮氨酸的影响。此外,一个含有温度敏感型苏氨酰-tRNA合成酶突变的野生型菌株在非允许温度下显示thr操纵子表达增加,而所有突变体均未表现出任何变化。综合这些数据表明,衰减反应的特异性受thr前导肽编码区内特定控制密码子的影响。我们还利用编码野生型thr前导区的质粒在体外直接证明了thr前导肽的合成,当用[3H]苏氨酸而非[3H]组氨酸或[3H]酪氨酸标记时,该质粒可指导合成具有适当分子量的肽段。相反,当提取物与含有突变DNA的模板一起孵育时,标记的肽段显示出与预期氨基酸组成一致的模式。这些数据表明thr前导RNA被翻译成了预测中的前导肽。

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