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使用基于Luminex xMAP技术的Bio-Plex磁珠悬浮阵列特异性检测猪细小病毒W并对该病毒衣壳蛋白上的表位进行特性分析。

Use of Luminex xMAP-derived Bio-Plex bead-based suspension array for specific detection of PPV W and characterization of epitopes on the coat protein of the virus.

作者信息

Croft Heather, Malinowski Tadeusz, Krizbai Laszlo, Mikec Ivan, Kajic Vesna, Reed Christopher, Varga Aniko, James Delano

机构信息

Sidney Laboratory, Canadian Food Inspection Agency, 8801 East Saanich Road, Sidney, British Columbia, Canada V8L 1H3.

出版信息

J Virol Methods. 2008 Nov;153(2):203-13. doi: 10.1016/j.jviromet.2008.07.016. Epub 2008 Sep 6.

DOI:10.1016/j.jviromet.2008.07.016
PMID:18722476
Abstract

A panel of monoclonal antibodies (MAbs) directed against the N-terminus region of the coat protein (CP) of strain PPV W (isolate 3174) was generated by immunizing mice with recombinant peptides. The best performing MAbs were identified as 2C3 and 10G7. MAb 2C3 was selected for comparison of a standard TAS-ELISA protocol with a Luminex xMAP technology-derived bead-based suspension array system described as a triple antibody sandwich-microsphere immunoassay (TAS-MIA). TAS-MIA was as sensitive as TAS-ELISA for the specific detection of PPV W in herbaceous and woody hosts. It was completed in 4h, and used less reagents. Epitope recognition analysis was carried out using a set of overlapping synthetic pin-bound peptides (Mimotopes). Peptides (2)DEEDD(6) and (46)MFNPV(50) were the epitopes recognized most commonly by the best performing MAbs. Linear epitope prediction of B-cell recognition sites confirmed that both peptides fall within highly antigenic and accessible regions. The second glutamic acid residue of the epitope is crucial for MAb recognition, and the context of the epitope is as important as the sequence of the epitope. The results obtained in ELISA, Western blot, and TAS-MIA correlated with B-cell recognition prediction. This is an effective approach to identify suitable antigenic epitopes that generate antibodies for use in reliable diagnostic procedures. This is the first report of the detection of a plant virus using the Luminex xMAP bead-based suspension array system.

摘要

通过用重组肽免疫小鼠,制备了一组针对猪细小病毒W株(分离株3174)衣壳蛋白(CP)N端区域的单克隆抗体(MAb)。性能最佳的单克隆抗体被鉴定为2C3和10G7。选择单克隆抗体2C3,将标准TAS-ELISA方案与一种基于Luminex xMAP技术的磁珠悬浮阵列系统进行比较,该系统被称为三抗体夹心微球免疫测定法(TAS-MIA)。TAS-MIA在草本和木本宿主中对猪细小病毒W的特异性检测与TAS-ELISA一样灵敏。它在4小时内完成,且使用的试剂较少。使用一组重叠的合成针结合肽(模拟表位)进行表位识别分析。肽(2)DEEDD(6)和(46)MFNPV(50)是性能最佳的单克隆抗体最常识别的表位。B细胞识别位点的线性表位预测证实,这两种肽都位于高度抗原性和易接近的区域内。表位的第二个谷氨酸残基对单克隆抗体的识别至关重要,表位的背景与表位序列同样重要。在ELISA、蛋白质印迹和TAS-MIA中获得的结果与B细胞识别预测相关。这是一种识别合适抗原表位的有效方法,这些表位可产生用于可靠诊断程序的抗体。这是首次报道使用基于Luminex xMAP磁珠的悬浮阵列系统检测植物病毒。

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