Castillo A, Nasser W, Condemine G, Reverchon S
Laboratoire de Génétique Moléculaire des Microorganismes, CNRS UMR 5577 INSA, Bat 406, 20 Avenue Albert Einstein, 69621 Villeurbanne, France.
Biochim Biophys Acta. 1998 Nov 8;1442(2-3):148-60. doi: 10.1016/s0167-4781(98)00158-4.
Erwinia chrysanthemi is a broad host range phytopathogenic enterobacterium responsible for soft-rot disease of many plant species. The pecT gene encodes a repressor that negatively regulates the expression of virulence factors, such as pectinases, motility or exopolysaccharide synthesis. The cloned pecT gene was overexpressed using a phage T7 system. The purification of PecT involved the use of a TSK-heparin column and delivered the PecT protein that was purified to near homogeneity. The purified repressor displayed a 34 kDa apparent molecular mass. Gel-filtration experiments revealed that the PecT protein is a dimer. Band-shift assays demonstrated that the tetramer of the PecT protein could specifically bind in vitro to the regulatory regions of the pectate lyase genes with variable affinities. In addition, we demonstrated that PecT represses its own synthesis by interacting independently with two 200 bp regions, R1 and R2, located from -382 to -632 and -17 to -234, respectively, from the distal P1 promoter and from -465 to -715 and -100 to -317 from the P2 proximal promoter. We propose a model that explains the regulation exerted by PecT on its target genes and that integrates the phenotype obtained with a PecT overproducing pec-1 mutant or a pecT mutant.
菊欧文氏菌是一种寄主范围广泛的植物病原性肠杆菌,可引发多种植物物种的软腐病。pecT基因编码一种阻遏蛋白,该蛋白对诸如果胶酶、运动性或胞外多糖合成等毒力因子的表达起负调控作用。利用噬菌体T7系统使克隆的pecT基因过量表达。PecT的纯化过程使用了TSK-肝素柱,并得到了近乎纯一的PecT蛋白。纯化后的阻遏蛋白表观分子量为34 kDa。凝胶过滤实验表明PecT蛋白是一种二聚体。凝胶迁移实验证明,PecT蛋白的四聚体能够在体外以不同亲和力特异性结合果胶酸裂解酶基因的调控区域。此外,我们还证明,PecT通过分别与位于远端P1启动子-382至-632以及-17至-234位置的两个200 bp区域R1和R2,以及近端P2启动子-465至-715以及-100至-317位置的区域独立相互作用,从而抑制自身的合成。我们提出了一个模型,该模型解释了PecT对其靶基因的调控作用,并整合了用PecT过量表达的pec-1突变体或pecT突变体所获得的表型。
