Esteve-Gassent Maria D, Smith Trever C, Small Christina M, Thomas Derek P, Seshu J
South Texas Center for Emerging Infectious Diseases, The University of Texas at San Antonio, San Antonio, TX-78249, United States of America; Department of Biology, The University of Texas at San Antonio, San Antonio, TX-78249, United States of America.
South Texas Center for Emerging Infectious Diseases, The University of Texas at San Antonio, San Antonio, TX-78249, United States of America; Center of Excellence in Infection Genomics, The University of Texas at San Antonio, San Antonio, TX-78249, United States of America.
PLoS One. 2015 Aug 31;10(8):e0136707. doi: 10.1371/journal.pone.0136707. eCollection 2015.
Borrelia burgdorferi, the causative agent of Lyme disease, alters its gene expression in response to environmental signals unique to its tick vector or vertebrate hosts. B. burgdorferi carries one superoxide dismutase gene (sodA) capable of controlling intracellular superoxide levels. Previously, sodA was shown to be essential for infection of B. burgdorferi in the C3H/HeN model of Lyme disease. We employed two-dimensional electrophoresis (2-DE) and immunoblot analysis with antibodies specific to carbonylated proteins to identify targets that were differentially oxidized in the soluble fractions of the sodA mutant compared to its isogenic parental control strain following treatment with an endogenous superoxide generator, methyl viologen (MV, paraquat). HPLC-ESI-MS/MS analysis of oxidized proteins revealed that several proteins of the glycolytic pathway (BB0057, BB0020, BB0348) exhibited increased carbonylation in the sodA mutant treated with MV. Levels of ATP and NAD/NADH were reduced in the sodA mutant compared with the parental strain following treatment with MV and could be attributed to increased levels of oxidation of proteins of the glycolytic pathway. In addition, a chaperone, HtpG (BB0560), and outer surface protein A (OspA, BBA15) were also observed to be oxidized in the sodA mutant. Immunoblot analysis revealed reduced levels of Outer surface protein C (OspC), Decorin binding protein A (DbpA), fibronectin binding protein (BBK32), RpoS and BosR in the sodA mutant compared to the control strains. Viable sodA mutant spirochetes could not be recovered from both gp91/phox-⁄- and iNOS deficient mice while borrelial DNA was detected in multiple tissues samples from infected mice at significantly lower levels compared to the parental strain. Taken together, these observations indicate that the increased oxidation of select borrelial determinants and reduced levels of critical pathogenesis-associated lipoproteins contribute to the in vivo deficit of the sodA mutant in the mouse model of Lyme disease. This study, utilizing the sodA mutant, has provided insights into adaptive capabilities critical for survival of B. burgdorferi in its hosts.
莱姆病的病原体伯氏疏螺旋体(Borrelia burgdorferi)会根据其蜱虫载体或脊椎动物宿主特有的环境信号改变基因表达。伯氏疏螺旋体携带一个能够控制细胞内超氧化物水平的超氧化物歧化酶基因(sodA)。此前,在莱姆病的C3H/HeN模型中,sodA被证明对伯氏疏螺旋体的感染至关重要。我们采用二维电泳(2-DE)和针对羰基化蛋白的特异性抗体进行免疫印迹分析,以鉴定在用内源性超氧化物生成剂甲基紫精(MV,百草枯)处理后,与同基因亲本对照菌株相比,sodA突变体可溶性组分中差异氧化的靶点。对氧化蛋白的HPLC-ESI-MS/MS分析表明,糖酵解途径的几种蛋白(BB0057、BB0020、BB0348)在用MV处理的sodA突变体中羰基化增加。与亲本菌株相比,用MV处理后的sodA突变体中ATP和NAD/NADH水平降低,这可能归因于糖酵解途径蛋白氧化水平的增加。此外,还观察到伴侣蛋白HtpG(BB0560)和外表面蛋白A(OspA,BBA15)在sodA突变体中被氧化。免疫印迹分析显示,与对照菌株相比,sodA突变体中外表面蛋白C(OspC)、饰胶蛋白聚糖结合蛋白A(DbpA)、纤连蛋白结合蛋白(BBK32)、RpoS和BosR的水平降低。在gp91/phox-/-和iNOS缺陷小鼠中均无法回收存活的sodA突变体螺旋体,而与亲本菌株相比,在感染小鼠的多个组织样本中检测到的伯氏疏螺旋体DNA水平显著降低。综上所述,这些观察结果表明,特定伯氏疏螺旋体决定簇的氧化增加以及关键致病相关脂蛋白水平的降低,导致了莱姆病小鼠模型中sodA突变体的体内缺陷。这项利用sodA突变体的研究,为伯氏疏螺旋体在其宿主中生存所必需的适应能力提供了见解。
Zotero 插件