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Clp和RpfF上调野油菜黄单胞菌野油菜致病变种中编码主要果胶酸裂解酶的pelA1基因的转录。

Clp and RpfF up-regulate transcription of pelA1 gene encoding the major pectate lyase in Xanthomonas campestris pv. campestris.

作者信息

Hsiao Yi-Min, Fang Mei-Chiung, Sun Pei-Fang, Tseng Yi-Hsiung

机构信息

Department of Medical Laboratory Science and Biotechnology, Central Taiwan University of Science and Technology, Taichung 406, Taiwan, Republic of China.

出版信息

J Agric Food Chem. 2009 Jul 22;57(14):6207-15. doi: 10.1021/jf900701n.

DOI:10.1021/jf900701n
PMID:19601664
Abstract

Exopolysaccharide and several extracellular enzymes of Xanthomonas campestris pv. campestris (Xcc), the causative agent of black rot in crucifers, are virulence determinants. In this study, two Xcc annotated extracellular pectate lyase genes, pelA1 and pelA2, belonging to family 1 of the polysaccharide lyase, were characterized. Sequence and mutational analyses have demonstrated that pelA1 encodes the major pectate lyase, whereas pelA2 is not transcribed. Using the 5' RACE method, the pelA1 transcription initiation site was mapped at nucleotide G, 103 nt upstream of the pelA1 start codon. Promoter analysis demonstrated that polygalacturonic acid and CaCl(2) induce the expression of pelA1. Transcriptional fusion assays also indicated that Clp (cAMP receptor protein-like protein) and RpfF (an enoyl-CoA hydratase homologue that is required for the synthesis of cis-11-methyl-2-dodecenoic acid, a low molecular weight diffusible signal factor, DSF) positively regulate pelA1 transcription. Gel retardation assays showed that Clp exerts a positive control over expression of pelA1 by direct binding to the upstream Clp-binding site. In conclusion, the present research demonstrated that pelA1 codes for the major pectate lyase in Xcc strain Xc17 and that its expression is up-regulated by Clp and RpfF. This is the first study to characterize pectate lyase gene expression in Xcc.

摘要

野油菜黄单胞菌野油菜致病变种(Xcc)是十字花科植物黑腐病的病原体,其胞外多糖和几种胞外酶是毒力决定因素。在本研究中,对Xcc中两个注释的胞外果胶酸裂解酶基因pelA1和pelA2进行了表征,它们属于多糖裂解酶家族1。序列和突变分析表明,pelA1编码主要的果胶酸裂解酶,而pelA2不转录。使用5'RACE方法,pelA1转录起始位点定位在pelA1起始密码子上游103 nt的核苷酸G处。启动子分析表明,聚半乳糖醛酸和CaCl₂可诱导pelA1的表达。转录融合试验还表明,Clp(类cAMP受体蛋白)和RpfF(一种烯酰辅酶A水合酶同系物,是顺式-11-甲基-2-十二碳烯酸合成所必需的,顺式-11-甲基-2-十二碳烯酸是一种低分子量可扩散信号因子,DSF)正向调节pelA1转录。凝胶阻滞试验表明,Clp通过直接结合上游Clp结合位点对pelA1的表达发挥正调控作用。总之,本研究表明,pelA1编码Xcc菌株Xc17中的主要果胶酸裂解酶,其表达受Clp和RpfF上调。这是首次对Xcc中果胶酸裂解酶基因表达进行表征的研究。

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