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Common and Unique Gene Expression Signatures of Human Macrophages in Response to Four Strains of Mycobacterium avium That Differ in Their Growth and Persistence Characteristics

机译:人类巨噬细胞对四种菌株的生长和持久性特性不同的反应中人类巨噬细胞的共同和独特的基因表达签名。

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摘要

Classification of pathogenic species according to the distinct host transcriptional responses that they elicit may become a relevant tool for microarray-based diagnosis of infection. Individual strains of Mycobacterium avium, an opportunistic pathogen in humans, have previously been shown to differ in terms of growth and persistence. In order to cover a wide spectrum of virulence, we selected four M. avium isolates (2151SmO, 2151SmT, SE01, TMC724) that have distinct intramacrophage replication characteristics and cause differential activation in human macrophages. Following infection with each of these strains, the expression of 12,558 genes in human macrophages was systematically analyzed by microarray technology. Fifty genes (including genes encoding proinflammatory cytokines, chemokines, signaling, and adhesion molecules) were differentially expressed more than twofold in response to all of the M. avium isolates investigated and therefore constitute a common macrophage signature in response to M. avium. The magnitude of regulation of most of these genes was directly correlated with the host cell-activating capacity of the particular M. avium strain. The regulation of a number of genes not previously associated with mycobacterial infections was apparent; these genes included genes encoding lymphocyte antigen 64 and myosin X. In addition, individual response patterns typical for some M. avium isolates could be defined by the pronounced upregulation of interleukin-12p40 (IL-12p40) (in the case of 2151SmO) or the specific upregulation of SOCS-1 and IL-10 (in the case of SE01) in macrophages. TMC724, a strain of avian origin, could not be classified by any one of these schemes, possibly indicating the limits of pathogen categorization solely by immune response signatures.
机译:根据病原菌引起的不同宿主转录反应对其进行分类可能会成为基于微阵列的感染诊断的相关工具。禽分枝杆菌是人类的一种机会病原体,其个别菌株先前已显示出其生长和持久性有所不同。为了涵盖广谱的毒力,我们选择了四种具有独特的巨噬细胞内复制特性并在人类巨噬细胞中引起差异激活的鸟毛支原体分离株(2151SmO,2151SmT,SE01,TMC724)。这些菌株中的每一个感染后,通过微阵列技术系统地分析了人类巨噬细胞中的12,558个基因的表达。五十个基因(包括编码促炎细胞因子,趋化因子,信号传导和粘附分子的基因)响应于所研究的所有鸟分枝杆菌而差异表达了两倍以上,因此构成了对鸟分枝杆菌的共同巨噬细胞标记。这些基因中大多数的调节强度与特定鸟分枝杆菌菌株的宿主细胞激活能力直接相关。以前与分枝杆菌感染无关的许多基因的调控是显而易见的。这些基因包括编码淋巴细胞抗原64和肌球蛋白X的基因。此外,某些禽鸟分枝杆菌典型的个体应答模式可以通过白介素12p40(IL-12p40)(在2151SmO的情况下)或巨噬细胞中SOCS-1和IL-10的特异性上调(对于SE01)。 TMC724是一种禽源毒株,无法通过任何一种方案进行分类,这可能表明仅通过免疫应答签名即可确定病原体分类的局限性。

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