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Comparison of the Whole Cell Proteome and Secretome of Epidemic Bordetella pertussis Strains From the 2008–2012 Australian Epidemic Under Sulfate-Modulating Conditions

机译:硫酸盐调节条件下2008-2012年澳大利亚流行性百日咳博德特氏菌菌株全细胞蛋白质组和分泌组的比较

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摘要

Sulfate is an important modulator for virulence factor expression in Bordetella pertussis, the causative organism for whooping cough. During infection, sulfate is released when respiratory epithelial cells are damaged which can affect gene expression. The current predominant strains in Australia are found in single nucleotide polymorphism (SNP) cluster I (ptxP3/prn2). It has been reported that ptxP3 strains have higher mRNA expression of virulence genes than ptxP1 strains under intermediate sulfate-modulating conditions (5 mM MgSO4). Our previous proteomic study compared L1423 (cluster I, ptxP3) and L1191 (cluster II, ptxP1) in Thalen–IJssel (THIJS) media without sulfate modulation and identified an upregulation of transport proteins and a downregulation of immunogenic proteins. To determine whether proteomic differences exist between cluster I and cluster II strains in intermediate modulating conditions, this study compared the whole cell proteome and secretome between L1423 and L1191 grown in THIJS media with 5 mM MgSO4 using iTRAQ and high-resolution multiple reaction monitoring (MRM-hr). Two proteins (BP0200 and BP1175) in the whole cell were upregulated in L1423 [fold change (FC) >1.2, false discovery rate (FDR) <0.05]. In the secretome, four proteins from the type III secretion system (T3SS) effectors were downregulated (FC < 0.8, FDR < 0.05) while six proteins, including two adhesins, pertactin (Prn) and tracheal colonization factor A (TcfA), were upregulated which were consistent with our previous proteomic study. The upregulation of Prn and TcfA in SNP cluster I may result in improved adhesion while the downregulation of the T3SS and other immunogenic proteins may reduce immune recognition, which may contribute to the increased fitness of cluster I B. pertussis strains.
机译:硫酸盐是百日咳博德氏杆菌中致病因子表达的重要调节剂,百日咳是百日咳的病原体。在感染期间,当呼吸道上皮细胞受损时会释放硫酸盐,这会影响基因表达。澳大利亚目前的主要菌株发现于单核苷酸多态性(SNP)群I(ptxP3 / prn2)中。据报道,在中等硫酸盐调节条件下(5 mM MgSO4),ptxP3菌株比ptxP1菌株具有更高的毒力基因mRNA表达。我们之前的蛋白质组学研究在没有硫酸盐调节的Thalen–IJssel(THIJS)培养基中比较了L1423(I类,ptxP3)和L1191(II类,ptxP1),并鉴定了转运蛋白的上调和免疫原性蛋白的下调。为了确定在中间调节条件下群集I和群集II菌株之间是否存在蛋白质组学差异,本研究使用iTRAQ和高分辨率多反应监测(MRM)对在5 mM MgSO4的THIJS培养基中生长的L1423和L1191之间的全细胞蛋白质组和分泌组进行了比较。 -hr)。整个细胞中的两种蛋白质(BP0200和BP1175)在L1423中上调[倍数变化(FC)> 1.2,错误发现率(FDR)<0.05]。在分泌组中,来自III型分泌系统(T3SS)效应子的四种蛋白被下调(FC <0.8,FDR <0.05),而包括两种粘附素,百日咳杆菌粘附素(Prn)和气管定植因子A(TcfA)的六种蛋白被上调。这与我们以前的蛋白质组学研究一致。 SNP簇I中Prn和TcfA的上调可能会改善粘附,而T3SS和其他免疫原性蛋白的下调可能会降低免疫识别,这可能有助于增加百日咳百日咳杆菌B.菌株的适应性。

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