| Literature DB >> 25832890 |
Meng-Die Ding1, Hong-Ning Wang, Hai-Peng Cao, Wen-Qiao Fan, Bing-Cun Ma, Peng-Wei Xu, An-Yun Zhang, Xin Yang.
Abstract
An indirect enzyme-linked immunosorbent assay (ELISA) method based on a novel multi-epitope antigen of S protein (SE) was developed for antibodies detection against infectious bronchitis virus (IBV). The multi-epitope antigen SE protein was designed by arranging three S gene fragments (166-247 aa, S1 gene; 501-515 aa, S1 gene; 8-30 aa, S2 gene) in tandem. It was identified to be approximately 32 kDa as a His-tagged fusion protein and can bind IBV positive serum by western blot analysis. The conditions of the SE-ELISA method were optimized. The optimal concentration of the coating antigen SE was 3.689 μg/mL and the dilution of the primary antibodies was identified as 1:1000 using a checkerboard titration. The cut-off OD450 value was established at 0.332. The relative sensitivity and specificity between the SE-ELISA and IDEXX ELISA kit were 92.38 and 89.83%, respectively, with an accuracy of 91.46%. This assay is sensitive and specific for detection of antibodies against IBV.Entities:
Keywords: ELISA; antibodies; infectious bronchitis virus (IBV); multi-epitope antigen
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Year: 2015 PMID: 25832890 DOI: 10.1080/09168451.2015.1025692
Source DB: PubMed Journal: Biosci Biotechnol Biochem ISSN: 0916-8451 Impact factor: 2.043