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Characterization of the Promoter, MxiE Box and 5′ UTR of Genes Controlled by the Activity of the Type III Secretion Apparatus in Shigella flexneri

机译:弗氏志贺氏菌III型分泌物活性控制基因的启动子,MxiE框和5'UTR的表征

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摘要

Activation of the type III secretion apparatus (T3SA) of Shigella flexneri, upon contact of the bacteria with host cells, and its deregulation, as in ipaB mutants, specifically increases transcription of a set of effector-encoding genes controlled by MxiE, an activator of the AraC family, and IpgC, the chaperone of the IpaB and IpaC translocators. Thirteen genes carried by the virulence plasmid (ospB, ospC1, ospD2, ospD3, ospE1, ospE2, ospF, ospG, virA, ipaH1.4, ipaH4.5, ipaH7.8 and ipaH9.8) and five genes carried by the chromosome (ipaHa-e) are regulated by the T3SA activity. A conserved 17-bp MxiE box is present 5′ of most of these genes. To characterize the promoter activity of these MxiE box-containing regions, similar ∼67-bp DNA fragments encompassing the MxiE box of 14 MxiE-regulated genes were cloned 5′ of lacZ in a promoter probe plasmid; β-galactosidase activity detected in wild-type and ipaB strains harboring these plasmids indicated that most MxiE box-carrying regions contain a promoter regulated by the T3SA activity and that the relative strengths of these promoters cover an eight-fold range. The various MxiE boxes exhibiting up to three differences as compared to the MxiE box consensus sequence were introduced into the ipaH9.8 promoter without affecting its activity, suggesting that they are equally efficient in promoter activation. In contrast, all nucleotides conserved among MxiE boxes were found to be involved in MxiE-dependent promoter activity. In addition, we present evidence that the 5′ UTRs of four MxiE-regulated genes enhance expression of the downstream gene, presumably by preventing degradation of the mRNA, and the 5′ UTRs of two other genes carry an ancillary promoter.
机译:细菌与宿主细胞接触后,弗氏志贺氏菌III型分泌装置(T3SA)的激活以及其失活(如ipaB突变体一样)会特别增加一组受MxiE(一种激活蛋白)控制的效应子编码基因的转录。 AraC家族和IpgC,即IpaB和​​IpaC易位分子的伴侣。毒力质粒携带的13个基因(ospB,ospC1,ospD2,ospD3,ospE1,ospE2,ospF,ospG,virA,ipaH1.4,ipaH4.5,ipaH7.8和ipaH9.8)和染色体携带的5个基因( ipaHa-e)受T3SA活性调节。这些基因中大多数的5'存在一个保守的17 bp MxiE盒。为了表征这些含有MxiE盒的区域的启动子活性,将包含14个MxiE调控基因的MxiE盒的约67bp的DNA片段克隆到lacZ的5'启动子探针质粒中。在带有这些质粒的野生型和ipaB菌株中检测到的β-半乳糖苷酶活性表明,大多数MxiE框携带区都含有受T3SA活性调节的启动子,这些启动子的相对强度覆盖八倍范围。与MxiE框共有序列相比,展示出最多三个差异的各种MxiE框被引入ipaH9.8启动子而不影响其活性,表明它们在启动子激活方面同样有效。相反,发现在MxiE盒之间保守的所有核苷酸都参与了MxiE依赖性启动子活性。此外,我们提供证据表明,四个MxiE调控基因的5'UTR可能通过防止mRNA的降解来增强下游基因的表达,另外两个基因的5'UTR则带有辅助启动子。

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