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  2. College of Bioresources and Agriculture / 生物資源暨農學院
  3. School of Veterinary Medicine / 獸醫專業學院
  4. Molecular and Comparative Pathobiology / 分子暨比較病理生物學研究所
  5. Expression of Sendai virus nucleocapsid protein in a baculovirus expression system and application to diagnostic assays for Sendai virus infection
 
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Expression of Sendai virus nucleocapsid protein in a baculovirus expression system and application to diagnostic assays for Sendai virus infection

Journal
Journal of Clinical Microbiology
Journal Volume
33
Journal Issue
8
Pages
2007-2011
Date Issued
1995
Author(s)
CHO-HUA WAN  
Riley, M.I.
Hook Jr. R.R.
Franklin, C.L.
Besch-Williford, C.L.
Riley, L.K.
DOI
10.1128/jcm.33.8.2007-2011.1995
URI
http://www.scopus.com/inward/record.url?eid=2-s2.0-0029020944&partnerID=MN8TOARS
http://scholars.lib.ntu.edu.tw/handle/123456789/313696
Abstract
The most common diagnostic technique for the detection of Sendai virus infection in rodents is serological evaluation by enzyme-linked immunosorbent assay (ELISA) with semipurified preparations of whole virions as antigens. This assay often suffers from a lack of specificity. The goal of the present project was to develop more specific antigens for use in diagnostic testing by producing recombinant antigens in insect cells. To identify viral proteins immunoreactive in multiple laboratory rodent species, Western blots (immunoblots) of viral polypeptides were probed with immune sera from mice, rats, and hamsters. The nucleocapsid protein (NP) reacted with immune sera from all species tested. Therefore, the NP gene was selected for cloning and expression in a baculovirus. To construct the recombinant, complementary DNA was synthesized by reverse transcription PCR from Sendai virus RNA with primers from the 5' and 3' termini of the NP-coding region. Amplified DNA was cloned into a baculovirus transfer vector (pBlueBacHis A) and was cotransfected with wild-type baculovirus into insect cells. Baculovirus recombinants containing the NP gene were identified by PCR. Evaluation of the recombinant proteins expressed in insect cells by Western blot analysis revealed specific reactivity with immune sera. In comparison with conventional ELISAs that use whole virions as the antigen, ELISAs that use recombinant NP were more specific.
Other Subjects
antiserum; capsid protein; complementary DNA; recombinant DNA; virus antigen; virus RNA; animal cell; animal experiment; article; Baculovirus; DNA transfection; gene expression; immunoblotting; insect; molecular cloning; nonhuman; priority journal; reverse transcription polymerase chain reaction; rodent; Sendai virus; virus infection; virus nucleocapsid; Animalia; Cricetinae; Insecta; Miridae; Rodentia; Sendai virus; unidentified baculovirus
Type
journal article

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