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环境信号和保守残基对伯氏疏螺旋体碳储存调节剂 A 功能的贡献。

Contributions of environmental signals and conserved residues to the functions of carbon storage regulator A of Borrelia burgdorferi.

机构信息

South Texas Center for Emerging Infectious Diseases, Center of Excellence in Infection Genomics and Department of Biology, The University of Texas at San Antonio, San Antonio, Texas, USA.

出版信息

Infect Immun. 2013 Aug;81(8):2972-85. doi: 10.1128/IAI.00494-13. Epub 2013 Jun 10.

Abstract

Carbon storage regulator A of Borrelia burgdorferi (CsrABb) contributes to vertebrate host-specific adaptation by modulating activation of the Rrp2-RpoN-RpoS pathway and is critical for infectivity. We hypothesized that the functions of CsrABb are dependent on environmental signals and on select residues. We analyzed the phenotype of csrABb deletion and site-specific mutants to determine the conserved and pathogen-specific attributes of CsrABb. Levels of phosphate acetyltransferase (Pta) involved in conversion of acetyl phosphate to acetyl-coenzyme A (acetyl-CoA) and posttranscriptionally regulated by CsrABb in the csrABb mutant were reduced from or similar to those in the control strains under unfed- or fed-tick conditions, respectively. Increased levels of supplemental acetate restored vertebrate host-responsive determinants in the csrABb mutant to parental levels, indicating that both the levels of CsrABb and the acetyl phosphate and acetyl-CoA balance contribute to the activation of the Rrp2-RpoN-RpoS pathway. Site-specific replacement of 8 key residues of CsrABb (8S) with alanines resulted in increased levels of CsrABb and reduced levels of Pta and acetyl-CoA, while levels of RpoS, BosR, and other members of rpoS regulon were elevated. Truncation of 7 amino acids at the C terminus of CsrABb (7D) resulted in reduced csrABb transcripts and posttranscriptionally reduced levels of FliW located upstream of CsrABb. Electrophoretic mobility shift assays revealed increased binding of 8S mutant protein to the CsrA binding box upstream of pta compared to the parental and 7D truncated protein. Two CsrABb binding sites were also identified upstream of fliW within the flgK coding sequence. These observations reveal conserved and unique functions of CsrABb that regulate adaptive gene expression in B. burgdorferi.

摘要

伯氏疏螺旋体的碳储存调节因子 A(CsrABb)通过调节 Rrp2-RpoN-RpoS 途径的激活来促进脊椎动物宿主的特异性适应,并且对于感染性至关重要。我们假设 CsrABb 的功能依赖于环境信号和特定的残基。我们分析了 csrABb 缺失和定点突变体的表型,以确定 CsrABb 的保守和病原体特异性属性。在未喂食或喂食蜱的条件下,与对照菌株相比,csrABb 突变体中涉及将乙酰磷酸转化为乙酰辅酶 A(乙酰-CoA)的磷酸乙酰转移酶(Pta)水平降低或相似,csrABb 突变体中 Pta 水平受 CsrABb 转录后调控。补充乙酸水平的增加恢复了 csrABb 突变体中脊椎动物宿主反应决定因素的水平,表明 CsrABb 的水平以及乙酰磷酸和乙酰-CoA 的平衡都有助于 Rrp2-RpoN-RpoS 途径的激活。用丙氨酸替代 CsrABb 的 8 个关键残基(8S)的定点替换导致 CsrABb 水平升高,Pta 和乙酰-CoA 水平降低,而 RpoS、BosR 和 rpoS 调控子的其他成员水平升高。CsrABb 的 C 末端截断 7 个氨基酸(7D)导致 csrABb 转录物减少,并且上游的 CsrABb 的 FliW 转录后水平降低。电泳迁移率变动分析显示,与亲本和 7D 截断蛋白相比,8S 突变蛋白与 CsrA 结合盒的结合增加,该结合盒位于 pta 的上游。还在 flgK 编码序列内鉴定了 fliW 上游的两个 CsrABb 结合位点。这些观察结果揭示了 CsrABb 的保守和独特功能,这些功能调节伯氏疏螺旋体中的适应性基因表达。

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