Expression of recombinant VP2 gene in insect sf9 cells and screening of clinical specimens.
- Author:
Ling-fang TENG
1
;
Feng LIN
;
Me-yun ZHENG
;
Chang-hua ZHENG
;
Feng WU
;
Ai-ping ZENG
;
En-pei HUANG
;
Yi-han MO
;
Min-qiao ZHENG
;
Xu-yang LI
;
Jian-yi HOU
Author Information
- Publication Type:Journal Article
- MeSH: Animals; Antibodies, Viral; blood; Bocavirus; genetics; immunology; Capsid Proteins; genetics; immunology; Child, Preschool; Female; Gene Expression; Humans; Infant; Male; Parvoviridae Infections; blood; diagnosis; immunology; virology; Recombinant Proteins; genetics; immunology; Spodoptera
- From: Chinese Journal of Experimental and Clinical Virology 2009;23(6):427-429
- CountryChina
- Language:Chinese
-
Abstract:
OBJECTIVETo clone and express VP, gene from HBoV, and the expressed VP, protein was as the antigen in order to detect serum from children in Wenling area with lower respiratory tract infections.
METHODSThe VP, gene was recombined with the genome of Baculovirus, which infected the insect cell. The fusion protein with HA tag was applied to confirm the specificity of expressed protein. Furthermore, the recombinant protein was observed using electron microscopy. The 176 serum from children in Wenling area with lower respiratory tract infections was screened using Western blot.
RESULTSThe expressed VP2 protein was more than 60% in total proteins from insect cell, and MWt about 60 x 10(3). The virus-like particle (VLP) was observed using electron microscopy, and size about 20 nm. The 176 serum from children in wenling area with lower respiratory tract infections was screened using Western blot. The HBoV positive rate was 2.28% (4/176).
CONCLUSIONThe VP2 protein from human bocavirus was expressed in insect cell successfully. Through HA tag the VP2 protein was specific, and then the assay using SDS-PAGE with Western blot could detect and screen the antibody in serum from children with lower respiratory tract infections rapidly and accurately.
