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来自乳酸乳球菌MG1614的两个苏氨酸生物合成基因的克隆及转录分析。

Cloning and transcriptional analysis of two threonine biosynthetic genes from Lactococcus lactis MG1614.

作者信息

Madsen S M, Albrechtsen B, Hansen E B, Israelsen H

机构信息

Department of Research and Development, Biotechnological Institute, Denmark.

出版信息

J Bacteriol. 1996 Jul;178(13):3689-94. doi: 10.1128/jb.178.13.3689-3694.1996.

Abstract

Two genes, hom and thrB, involved in threonine biosynthesis in Lactococcus lactis MG1614, were cloned and sequenced. These genes, which encode homoserine dehydrogenase and homoserine kinase, were initially identified by the homology of their gene products with known homoserine dehydrogenases and homoserine kinases from other organisms. The identification was supported by construction of a mutant containing a deletion in hom and thrB that was unable to grow in a defined medium lacking threonine. Transcriptional analysis showed that the two genes were located in a bicistronic operon with the order 5' hom-thrB 3' and that transcription started 66 bp upstream of the translational start codon of the hom gene. A putative -10 promoter region (TATAAT) was located 6 bp upstream of the transcriptional start point, but no putative -35 region was identified. A DNA fragment covering 155 bp upstream of the hom translational start site was functional in pAK80, an L. lactis promoter probe vector. In addition, transcriptional studies showed no threonine-dependent regulation of hom-thrB transcription.

摘要

克隆并测序了乳酸乳球菌MG1614中参与苏氨酸生物合成的两个基因,即hom和thrB。这两个基因分别编码高丝氨酸脱氢酶和高丝氨酸激酶,最初是通过其基因产物与其他生物体中已知的高丝氨酸脱氢酶和高丝氨酸激酶的同源性来鉴定的。通过构建一个在hom和thrB中存在缺失且无法在缺乏苏氨酸的限定培养基中生长的突变体,进一步证实了这一鉴定结果。转录分析表明,这两个基因位于一个双顺反子操纵子中,顺序为5'-hom-thrB-3',转录起始于hom基因翻译起始密码子上游66 bp处。一个推定的-10启动子区域(TATAAT)位于转录起始点上游6 bp处,但未鉴定到推定的-35区域。覆盖hom翻译起始位点上游155 bp的DNA片段在乳酸乳球菌启动子探针载体pAK80中具有功能。此外,转录研究表明,hom-thrB的转录不存在苏氨酸依赖性调控。

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