首页> 外文期刊>Journal of bacteriology >Identification and Characterization of Sporulation-Dependent Promoters Upstream of the Enterotoxin Gene (cpe) of Clostridium perfringens
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Identification and Characterization of Sporulation-Dependent Promoters Upstream of the Enterotoxin Gene (cpe) of Clostridium perfringens

机译:产气荚膜梭菌肠毒素基因(cpe)上游依赖于孢子的启动子的鉴定和表征

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Three promoter sites (P1, P2, and P3) responsible for the sporulation-associated synthesis of Clostridium perfringensenterotoxin, a common cause of food poisoning in humans and animals, were identified. Nested and internal deletions of the cpepromoter region were made to narrow down the location of promoter elements. To measure the effects of the deletions on the expression ofcpe, translational fusions containing the promoter deletions were made with the gusA gene of Escherichia coli, which codes for β-glucuronidase; E. coli-C. perfringens shuttle vectors carrying the fusions were introduced into C. perfringens by electroporation. In addition, in vitro transcription assays were performed with the cpepromoter region as the DNA template for extracts made from sporulating cells. DNA sequences upstream of P1 were similar to consensus SigK-dependent promoters, while P2 and P3 were similar to consensus SigE-dependent promoters. SigE and SigK are sporulation-associated sigma factors known to be active in the mother cell compartment of sporulating cells of Bacillus subtilis, the same compartment in which enterotoxin is synthesized in C. perfringens.
机译:确定了三个启动子位点(P1,P2和P3),它们与产气荚膜梭菌肠毒素(人和动物食物中毒的常见原因)的孢子形成有关。嵌套和内部删除了 cpe 启动子区域,以缩小启动子元件的位置。为了测量缺失对 cpe 表达的影响,将含有启动子缺失的翻译融合体与大肠杆菌 gusA 基因进行了融合,其中编码β-葡萄糖醛酸苷酶; E。绞痛。将带有融合蛋白的perfringens 穿梭载体导入 C。电穿孔产生的产气荚膜炎。另外,以 cpe 启动子区域作为从孢子形成细胞制成的提取物的DNA模板进行体外转录测定。 P1上游的DNA序列类似于共有SigK依赖性启动子,而P2和P3类似于共有SigE依赖性启动子。 SigE和SigK是与孢子形成相关的sigma因子,已知在枯草芽孢杆菌(Bemillus subtilis)的孢子形成细胞的母细胞区室中活跃,而在 C中合成肠毒素。产气菌。

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