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Engineering Synthetic Lipopeptide Antigen for Specific Detection of Mycobacterium avium subsp. paratuberculosis Infection

机译:工程合成脂肽抗原特异性检测分枝杆菌亚空间。 paratuberculosis感染

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摘要

Unlike other MAC members, Mycobacterium avium subsp. paratuberculosis (MAP) does not produce glycopeptidolipids (GPL) on the surface of the cell wall but a lipopentapeptide called L5P (also termed Lipopeptide-I or Para-LP-01) characterized in C-type (bovine) strains. This lipopeptide antigen contains a pentapeptide core, D-Phenylalanine-N-methyl-L-Valine-L-Isoleucine-L-Phenylalanine-L-Alanine, in which the N-terminal D-Phenylalanine is amido-linked with a fatty acid (C18–C20). The molecular and genetic characterization of this antigen demonstrated that L5P is unique to MAP. Knowledge of the structure of L5P enabled synthetic production of this lipopeptide in large quantities for immunological evaluation. Various studies described the immune response directed against L5P and confirmed its capability for detection of MAP infection. However, the hydrophobic nature of lipopeptide antigens make their handling and use in organic solvents unsuitable for industrial processes. The objectives of this study were to produce, by chemical synthesis, a water-soluble variant of L5P and to evaluate these compounds for the serological diagnosis of MAP using well-defined serum banks. The native L5P antigen and its hydrosoluble analog were synthesized on solid phase. The pure compounds were evaluated on collections of extensively characterized sera from infected and non-infected cattle. ROC analysis showed that L5P and also its water-soluble derivative are suitable for the development of a serological test for Johne's disease at a population level. However, these compounds used alone in ELISA have lower sensitivity (Se 82% for L5P and Se 62% for the water-soluble variant of L5P) compared to the Se 98% of a commercial test. Advantageously, these pure synthetic MAP specific antigens can be easily produced in non-limiting quantities at low cost and in standardized batches for robust studies. The fact that L5P has not been validated in the context of ovine paratuberculosis highlights the need to better characterize the antigens expressed from the different genetic lineages of MAP to discover new diagnostic antigens. In the context of infections due to other mycobacteria such as M. bovis or the more closely related species M. avium subsp. hominissuis, the L5P did not cross react and therefore may be a valuable antigen to solve ambiguous results in other tests.
机译:与其他MAC成员不同,分枝杆菌亚空间。副伯曲线(MAP)不会在细胞壁的表面上产生糖肽脂脂(GPL),而是一种称为L5P(也称为Lipopepidide-I或第LP-01)的脂肪肽,其特征在于C型(牛)菌株。这种脂肽抗原含有五肽芯,D-苯丙氨酸-N-甲基-1-缬氨酸-L-脱氨酸-1-苯丙氨酸-1-丙氨酸,其中N-末端D-苯丙氨酸与脂肪酸相连( C18-C20)。该抗原的分子和遗传表征证明L5P是映射的独特。了解L5P的结构,使得这种脂肪肽的综合生产大量用于免疫学评价。各种研究描述了针对L5P的免疫应答,并确认了其检测地图感染的能力。然而,脂肽抗原的疏水性质使其处理并在不适合工业过程的有机溶剂中使用。本研究的目的是通过化学合成,通过明确定义的血清堤,评估这些化合物的水溶性变体并评估这些化合物用于地图的血清学诊断。在固相上合成天然L5P抗原及其加氢溶解模拟。在来自感染和未感染的牛的广泛表征血清的收集中评价纯化合物。 ROC分析表明,L5P和其水溶性衍生物适合于在人口水平下对约翰病的血清学检测进行血清学试验。然而,与商业测试的SE 98%相比,单独使用的这些化合物具有较低的灵敏度(对于L5P的L5P和L5P的L5P和SE 62%的SE 62%)。有利地,这些纯合成映射特异性抗原可以在低成本和标准化批量中以低成本和稳健性研究的标准化批量来容易地生产这些纯合成映射特异性抗原。 L5P在卵巢对伞菌的背景下尚未验证的事实突出了更好地表征从地图的不同遗传谱系表达的抗原的需要,以发现新的诊断抗原。在感染的背景下,由于其他分枝杆菌如M. Bovis或更紧密相关的物种M. Avium subsp。 Hominissuis,L5P没有交叉反应,因此可以是求解其他测试中的模糊结果的有价值的抗原。

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