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了解脂阿拉伯甘露聚糖与膜模拟结构的相互作用。

Understanding the interaction of Lipoarabinomannan with membrane mimetic architectures.

机构信息

Chemistry Division, Los Alamos National Laboratory, Los Alamos, NM 87545, USA.

出版信息

Tuberculosis (Edinb). 2012 Jan;92(1):38-47. doi: 10.1016/j.tube.2011.09.006. Epub 2011 Oct 26.

DOI:10.1016/j.tube.2011.09.006
PMID:22033469
Abstract

Lipoarabinomannan (LAM) is a critical virulence factor in the pathogenesis of Mycobacterium tuberculosis, the causative agent of tuberculosis. LAM is secreted in urine and serum from infected patients and is being studied as a potential diagnostic indicator for the disease. Herein, we present a novel ultra-sensitive and specific detection strategy for monomeric LAM based on its amphiphilic nature and consequent interaction with supported lipid bilayers. Our strategy involves the capture of LAM on waveguides functionalized with membrane mimetic architectures, followed by detection with a fluorescently labeled polyclonal antibody. This approach offers ultra-sensitive detection of lipoarabinomannan (10 fM, within 15 min) and may be extended to other amphiphilic markers. We also show that chemical deacylation of LAM completely abrogates its association with the supported lipid bilayers. The loss of signal using the waveguide assay for deacylated LAM, as well as atomic force microscopy (AFM) images that show no change in height upon addition of deacylated LAM support this hypothesis. Mass spectrometry of chemically deacylated LAM indicates the presence of LAM-specific carbohydrate chains, which maintain antigenicity in immunoassays. Further, we have developed the first three-dimensional structural model of mannose-capped LAM that provides insights into the orientation of LAM on supported lipid bilayers.

摘要

阿拉伯半乳聚糖甘露聚糖 (LAM) 是分枝杆菌(结核分枝杆菌)发病机制中的关键毒力因子,分枝杆菌是结核病的病原体。LAM 从感染患者的尿液和血清中分泌出来,目前正在作为该疾病的潜在诊断指标进行研究。在此,我们基于其两亲性及其与支撑脂质双层的相互作用,提出了一种用于检测单体 LAM 的新型超灵敏和特异性检测策略。我们的策略涉及将 LAM 捕获在具有膜模拟结构的波导上,然后用荧光标记的多克隆抗体进行检测。该方法可以超灵敏地检测阿拉伯半乳聚糖甘露聚糖(10 fM,在 15 分钟内),并且可以扩展到其他两亲性标记物。我们还表明,LAM 的化学脱酰基作用完全阻止了其与支撑脂质双层的结合。在去酰化 LAM 的波导分析中信号的丧失,以及原子力显微镜 (AFM) 图像显示加入去酰化 LAM 后高度没有变化,这支持了这一假设。化学去酰化 LAM 的质谱分析表明存在 LAM 特异性碳水化合物链,这些碳水化合物链在免疫测定中保持抗原性。此外,我们还开发了甘露糖封端的 LAM 的第一个三维结构模型,该模型提供了关于 LAM 在支撑脂质双层上取向的见解。

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