The ilvIH operon of Escherichia coli (located near min 2) encodes acetohydroxyacid synthase III, an isozyme involved in branched-chain amino acid biosynthesis. A strain with lacZ fused to the ilvIH promoter was constructed. Transposon Tn10 was introduced into this strain, and tetracycline-resistant derivatives were screened for those in which ilvIH promoter expression was markedly reduced. In one such derivative, strain CV1008, beta-galactosidase expression was reduced more than 30-fold. The transposon giving rise to this phenotype inserted near min 20 on the E. coli chromosome. Extract from a wild-type strain contains a protein, the IHB protein, that binds to two sites upstream of the ilvIH promoter (E. Ricca, D. A. Aker, and J. M. Calvo, J. Bacteriol. 171:1658-1664, 1989). Extract from strain CV1008 lacks IHB-binding activity. These results indicate that the IHB protein is a positive regulator of ilvIH operon expression. The gene that encodes the IHB protein, ihb, was cloned by complementing the transposon-induced mutation. Definitive evidence that the cloned DNA encodes the IHB protein was provided by determining the sequence of more than 17 amino acids at the N terminus of the IHB protein and comparing it with the nucleotide sequence. A mutation that prevents repression of the ilvIH operon by leucine in vivo and that alters the DNA-binding characteristics of the IHB protein in vitro was shown to be an allele of the ihb gene. The ihb gene is identical to oppI, a gene that regulates the oppABCDF operon (E. A. Austin, J. C. Andrews, and S. A. Short, Abstr. Mol. Genet. Bacteria Phages, p. 153, 1989). Thus, oppI/ihb encodes a protein that regulates both ilvIH, an operon that is repressed by leucine, and oppABCDF, an operon involved in peptide transport that is induced by leucine. We propose that the designation lrp be used in the future instead of oppI or ihb and that Lrp (leucine-responsive regulatory protein) be used in place of IHB.
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机译:大肠杆菌的ilvIH操纵子(位于第2分钟附近)编码乙酰羟酸合酶III,这是一种参与支链氨基酸生物合成的同工酶。构建了具有融合至ilvIH启动子的lacZ的菌株。将转座子Tn10引入该菌株中,并针对四环素抗性衍生物筛选出其中ilvIH启动子表达显着降低的衍生物。在一种这样的衍生物菌株CV1008中,β-半乳糖苷酶的表达降低了30倍以上。产生此表型的转座子插入大肠杆菌染色体的第20分钟附近。来自野生型菌株的提取物包含结合至ilvIH启动子上游两个位点的蛋白质IHB蛋白质(E.Ricca,D.A.Aker和J.M.Calvo,J.Bacteriol.171:1658-1664,1989)。菌株CV1008的提取物缺乏IHB结合活性。这些结果表明,IHB蛋白是ilvIH操纵子表达的正调节剂。通过补充转座子诱导的突变,克隆了编码IHB蛋白的基因ihb。通过确定IHB蛋白N端超过17个氨基酸的序列并将其与核苷酸序列进行比较,可以提供克隆的DNA编码IHB蛋白的权威证据。突变阻止了体内亮氨酸抑制ilvIH操纵子,并在体外改变了IHB蛋白的DNA结合特性,这是ihb基因的等位基因。 ihb基因与调节oppABCDF操纵子的基因oppI相同(E. A. Austin,J。C. Andrews和S. A. Short,抽象分子细菌噬菌体,第153页,1989)。因此,oppI / ihb编码一种蛋白质,它调节被亮氨酸抑制的操纵子ilvIH和被亮氨酸诱导的肽转运的操纵子oppABCDF。我们建议将来使用lrp代替oppI或ihb,并使用Lrp(亮氨酸反应性调节蛋白)代替IHB。
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