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Development of an in Vitro Potency Assay for Anti-anthrax Lethal Toxin Neutralizing Antibodies

机译:抗炭疽致死毒素中和抗体体外效价测定的发展。

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摘要

Lethal toxin (LT) of Bacillus anthracis reduces the production of a number of inflammatory mediators, including transcription factors, chemokines and cytokines in various human cell lines, leading to down-regulation of the host inflammatory response. Previously we showed that the reduction of interleukin-8 (IL-8) is a sensitive marker of LT-mediated intoxication in human neutrophil-like NB-4 cells and that IL-8 levels are restored to normality when therapeutic monoclonal antibodies (mAb) with toxin-neutralising (TN) activity are added. We used this information to develop cell-based assays that examine the effects of TN therapeutic mAbs designed to treat LT intoxication and here we extend these findings. We present an in vitro assay based on human endothelial cell line HUVEC jr2, which measures the TN activity of therapeutic anti-LT mAbs using IL-8 as a marker for intoxication. HUVEC jr2 cells have the advantage over NB-4 cells that they are adherent, do not require a differentiation step and can be used in a microtitre plate format and therefore can facilitate high throughput analysis. This human cell-based assay provides a valid alternative to the mouse macrophage assay as it is a more biologically relevant model of the effects of toxin-neutralising antibodies in human infection.
机译:炭疽芽孢杆菌的致死毒素(LT)减少了各种人类细胞系中多种炎症介质(包括转录因子,趋化因子和细胞因子)的产生,从而导致宿主炎症反应的下调。先前我们显示白介素8(IL-8)的减少是人嗜中性粒细胞样NB-4细胞中LT介导的中毒的敏感标志物,当治疗性单克隆抗体(mAb)时IL-8水平恢复正常具有毒素中和(TN)活性。我们使用这些信息来开发基于细胞的检测方法,以检查旨在治疗LT中毒的TN治疗性mAb的作用,在此我们扩展这些发现。我们提出了基于人内皮细胞系HUVEC jr2的体外测定法,该测定法使用IL-8作为中毒标志物来测定治疗性抗LT mAb的TN活性。 HUVEC jr2细胞相对于NB-4细胞具有以下优势:它们具有粘附性,不需要分化步骤,并且可以微量滴定板形式使用,因此可以促进高通量分析。这种基于人体细胞的测定法是小鼠巨噬细胞测定法的有效替代方法,因为它是毒素中和抗体在人类感染中作用的更生物学相关的模型。

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