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首页> 外文期刊>Tuberculosis >ICAT-based comparative proteomic analysis of non-replicating persistent Mycobacterium tuberculosis.
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ICAT-based comparative proteomic analysis of non-replicating persistent Mycobacterium tuberculosis.

机译:基于ICAT的非复制型持续性结核分枝杆菌的比较蛋白质组学分析。

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The non-replicating persistence (NRP) phenotype of Mycobacterium tuberculosis (NRP-TB) is assumed to be responsible for the maintenance of latent infection and the requirement of a long treatment duration for active tuberculosis. Isotope coded affinity tag-based proteomic analysis was used for the determination of the relative expression of large numbers of M. tuberculosis proteins during oxygen self-depletion under controlled conditions in a multi-chambered fermentor. Expression of the alpha-crystallin homolog protein, acr, was monitored and quantified to confirm entry into NRP. Relative expression of 586 and 628 proteins was determined in log phase vs. early stage NRP (NRP-1) and log phase vs. later stage NRP (NRP-2), respectively. Relative to expression in log phase and using an abundance ratio of +/-2.0 as a cutoff, 6.5% and 20.4% of proteins were found to be upregulated in NRP-1 and NRP-2, respectively while 20.3% and 13.4% were downregulated, respectively. Functional profiling revealed that 42.1%/39.8% of upregulated proteins and 41.2%/45.2% of downregulated proteins in NRP-1/NRP-2, respectively, were involved in small molecule metabolism. Among those proteins the highest proportions of 37.5% in NRP-1 were involved with degradation and of 45.1% in NRP-2 with energy metabolism. These results suggest distinct protein expression profiles in NRP-1 and NRP-2.
机译:结核分枝杆菌(NRP-TB)的非复制持久性(NRP)表型被认为是维持潜在感染和活动性结核病需要较长治疗时间的原因。基于同位素编码的基于亲和标记的蛋白质组学分析用于确定多室发酵罐中受控条件下氧自耗期间大量结核分枝杆菌蛋白的相对表达。监测和定量α-晶状蛋白同源蛋白acr的表达,以确认其进入NRP。分别在对数期相对于早期NRP(NRP-1)和对数期相对于后期NRP(NRP-2)中确定了586和628蛋白的相对表达。相对于对数表达和以+/- 2.0的丰度比作为截止值,发现NRP-1和NRP-2分别上调了6.5%和20.4%的蛋白质,而下调了20.3%和13.4%的蛋白质, 分别。功能分析表明,NRP-1 / NRP-2中分别有42.1%/ 39.8%的上调蛋白和41.2%/ 45.2%的下调蛋白参与小分子代谢。在这些蛋白质中,NRP-1中37.5%的最高比例与降解有关,而NRP-2中的45.1%与能量代谢有关。这些结果表明在NRP-1和NRP-2中蛋白质表达谱截然不同。

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