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首页> 外文期刊>Journal of Microbiological Methods >A luciferase-based assay for rapid assessment of drug activity against Mycobacterium tuberculosis including monitoring of macrophage viability
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A luciferase-based assay for rapid assessment of drug activity against Mycobacterium tuberculosis including monitoring of macrophage viability

机译:一种基于荧光素酶的测定法,用于快速评估抗结核分枝杆菌的药物活性,包括监测巨噬细胞的生存能力

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摘要

The intracellular (IC) effect of drugs against Mycobacterium tuberculosis (Mtb) is not well established but increasingly important to consider when combining current and future multidrug regimens into the best possible treatment strategies. For this purpose, we developed an IC model based on a genetically modified Mtb H37Rv strain, expressing the Vibrio harvei luciferase (H37Rv-lux) infecting the human macrophage like cell line THP-1. Cells were infected at a low multiplicity of infection (1:1) and subsequently exposed to isoniazid (INH), ethambutol (EMB), amikacin (AMI) or levofloxacin (LEV) for 5 days in a 96-well format. Cell viability was evaluated by Calcein AM and was maintained throughout the experiment. The number of viable H37Rv-lux was determined by luminescence and verified by a colony forming unit analysis. The results were compared to the effects of the same drugs in broth cultures. AMI, EMB and LEV were significantly less effective intracellularly (MIC90: >4 mg/L, 8 mg/L and 2 mg/L, respectively) compared to extracellularly (MIC90: 0.5 mg/L for AMI and EMB; 0.25 mg/L for LEV). The reverse was the case for INH (IC: 0.064 mg/L vs EC: 0.25 mg/L). In conclusion, this luciferase based method, in which monitoring of cell viability is included, has the potential to become a useful tool while evaluating the intracellular effects of anti-mycobacterial drugs. (C) 2014 Elsevier B.V. All rights reserved.
机译:药物对结核分枝杆菌(Mtb)的细胞内(IC)效果尚不充分,但在将当前和未来的多药方案结合到最佳治疗策略中时,考虑的重要性越来越重要。为此,我们开发了一种基于基因改造的Mtb H37Rv菌株的IC模型,该模型表达了感染人类巨噬细胞样细胞系THP-1的哈维弧菌荧光素酶(H37Rv-lux)。以低感染复数(1:1)感染细胞,然后以96孔形式暴露于异烟肼(INH),乙胺丁醇(EMB),丁胺卡那霉素(AMI)或左氧氟沙星(LEV)5天。通过钙黄绿素AM评估细胞活力,并在整个实验过程中保持细胞活力。通过发光确定存活的H37Rv-lux的数目,并通过菌落形成单位分析进行验证。将结果与相同药物在肉汤培养中的效果进行比较。与细胞外(AMI90和EMB的MIC90:0.5 mg / L; 0.25 mg / L的细胞外)相比,AMI,EMB和LEV在细胞内的有效性(分别为MIC90:> 4 mg / L,8 mg / L和2 mg / L)明显较低。对于LEV)。 INH的情况则相反(IC:0.064 mg / L,EC:0.25 mg / L)。总之,这种基于荧光素酶的方法(包括监测细胞的生存能力)在评估抗分枝杆菌药物的细胞内作用时,有可能成为有用的工具。 (C)2014 Elsevier B.V.保留所有权利。

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