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新型免疫原性抗原选择方法用于细颈囊尾蚴感染的血清学诊断。

Novel methods of immunogenic antigen selection for serological diagnosis of Parelaphostrongylus tenuis infection.

机构信息

Biomedical and Diagnostic Sciences, College of Veterinary Medicine, The University of Tennessee, Knoxville, USA.

The University of Tennessee Comparative & Experimental Medicine, Knoxville, USA.

出版信息

Sci Rep. 2023 Jul 7;13(1):10989. doi: 10.1038/s41598-023-37481-7.

Abstract

This paper outlines methods used to identify novel antigens for use in the development of serological assays. Specifically, we applied these methods to a neurogenic parasitic nematode of cervids called Parelaphostrongylus tenuis. This parasite is of particular concern in both wild and domestic ungulates as it causes significant neurological signs and definitive diagnosis is only possible post-mortem, necessitating the development of serologic assays for antemortem diagnosis. Proteins extracted from P. tenuis organisms were affinity isolated using antibodies enriched from seropositive moose (Alces alces). The proteins were analyzed using mass spectrometry and liquid chromatography to obtain amino acid sequences that were then cross-referenced to open reading frames predicted from an assembled transcriptome. An antigen of interest was assessed for immunogenic epitopes and subsequently synthesized into 10-mer synthetic overlapping peptides representing these regions. These synthetic peptides were then assessed for reactivity against positive and negative moose sera and demonstrated potential use as a serological assay in diagnostic laboratories. Known negative moose sera revealed significantly lower optical density when compared to the positive samples (p < 0.05). This method serves as a pipeline for the construction of diagnostic assays of pathogens in both human and veterinary medicine.

摘要

本文概述了用于鉴定新型抗原以开发血清学检测方法的方法。具体来说,我们将这些方法应用于一种叫做 Parelaphostrongylus tenuis 的神经源性寄生线虫。这种寄生虫在野生和家养有蹄类动物中都非常令人担忧,因为它会引起严重的神经症状,只有在死后才能进行明确诊断,因此需要开发血清学检测方法进行生前诊断。从 P. tenuis 生物体中提取的蛋白质使用从血清阳性驼鹿(Alces alces)中富集的抗体进行亲和分离。使用质谱和液相色谱分析蛋白质,以获得氨基酸序列,然后将其与组装的转录组预测的开放阅读框进行交叉引用。对感兴趣的抗原进行免疫原性表位评估,然后将其合成代表这些区域的 10 聚体合成重叠肽。然后评估这些合成肽对阳性和阴性驼鹿血清的反应性,并证明它们有可能在诊断实验室中用作血清学检测方法。与阳性样本相比,已知的阴性驼鹿血清的光密度显著降低(p < 0.05)。该方法为人类和兽医医学中病原体诊断检测方法的构建提供了一个途径。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/59af/10329008/63986111d2c1/41598_2023_37481_Fig1_HTML.jpg

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