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丁香假单胞菌丁香致病变种B301D中负责丁香霉素和丁香肽素合成的基因启动子区域中syr - syp框的鉴定。

Identification of the syr-syp box in the promoter regions of genes dedicated to syringomycin and syringopeptin production by Pseudomonas syringae pv. syringae B301D.

作者信息

Wang Nian, Lu Shi-En, Yang Qingwu, Sze Sing-Hoi, Gross Dennis C

机构信息

Department of Plant Pathology and Microbiology, Texas A&M University, College Station, TX 77843, USA.

出版信息

J Bacteriol. 2006 Jan;188(1):160-8. doi: 10.1128/JB.188.1.160-168.2006.

Abstract

The phytotoxins syringopeptin and syringomycin are synthesized by nonribosomal peptide synthetases which are encoded by the syringomycin (syr) and syringopeptin (syp) genomic island of Pseudomonas syringae pv. syringae. Previous studies demonstrated that expression of the syr-syp genes was controlled by the salA-syrF regulatory pathway, which in turn was induced by plant signal molecules. In this study, the 132-kb syr-syp genomic island was found to be organized into five polycistronic operons along with eight individual genes based on reverse transcriptional PCR and bioinformatic analysis. The transcriptional start sites of the salA gene and operons III and IV were located 63, 75, and 104 bp upstream of the start codons of salA, syrP, and syrB1, respectively, using primer extension analysis. The predicted -10/-35 promoter region of operon IV was confirmed based on deletion and site-directed mutagenesis analyses of the syrB1::uidA reporter with beta-glucuronidase assays. A 20-bp conserved sequence (TGtCccgN(6)cggGaCA, termed the syr-syp box) with dyad symmetry around the -35 region was identified via computer analysis for the syr-syp genes/operons responsible for biosynthesis and secretion of syringomycin and syringopeptin. Expression of the syrB1::uidA fusion was decreased 59% when 6 bp was deleted from the 5' end of the syr-syp box in the promoter region of operon IV. These results demonstrate that the conserved promoter sequences of the syr-syp genes contribute to the coregulation of syringomycin and syringopeptin production.

摘要

植物毒素丁香霉素和丁香肽素由非核糖体肽合成酶合成,这些酶由丁香假单胞菌丁香致病变种的丁香霉素(syr)和丁香肽素(syp)基因岛编码。先前的研究表明,syr-syp基因的表达受salA-syrF调控途径控制,而该途径又由植物信号分子诱导。在本研究中,基于逆转录PCR和生物信息学分析,发现132 kb的syr-syp基因岛与8个单个基因一起被组织成5个多顺反子操纵子。使用引物延伸分析,salA基因以及操纵子III和IV的转录起始位点分别位于salA、syrP和syrB1起始密码子上游63、75和104 bp处。基于对带有β-葡萄糖醛酸酶测定的syrB1::uidA报告基因的缺失和定点诱变分析,证实了操纵子IV的预测-10/-35启动子区域。通过计算机分析,针对负责丁香霉素和丁香肽素生物合成和分泌的syr-syp基因/操纵子,在-35区域周围鉴定出一个具有二元对称性的20 bp保守序列(TGtCccgN(6)cggGaCA,称为syr-syp框)。当从操纵子IV启动子区域的syr-syp框5'端缺失6 bp时,syrB1::uidA融合体的表达降低了59%。这些结果表明,syr-syp基因的保守启动子序列有助于丁香霉素和丁香肽素产生的共调控。

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