PRODUCTION OF MINK ENTERITIS PARVOVIRUS EMPTY CAPSIDS BY EXPRESSION IN A BACULOVIRUS VECTOR SYSTEM - A RECOMBINANT VACCINE FOR MINK ENTERITIS PARVOVIRUS IN MINK

被引:33
作者
CHRISTENSEN, J
ALEXANDERSEN, S
BLOCH, B
AASTED, B
UTTENTHAL, A
机构
[1] ROYAL VET & AGR UNIV,DEPT VET MICROBIOL,VIROL & IMMUNOL LAB,DK-1870 FREDERIKSBERG C,DENMARK
[2] ROYAL VET & AGR UNIV,DEPT PHARMACOL & PATHOBIOL,MOLEC PATHOBIOL LAB,DK-1870 FREDERIKSBERG C,DENMARK
[3] DANISH FUR BREEDERS LAB,DK-2600 GLOSTRUP,DENMARK
关键词
D O I
10.1099/0022-1317-75-1-149
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
The VP-2 gene of mink enteritis parvovirus (MEV) was amplified by the polymerase chain reaction using MEV DNA isolated from the faeces of a naturally infected mink. Subsequently the VP-2 gene was cloned into a baculovirus expression vector. Recombinant baculoviruses were isolated and the MEV VP-2 gene product was characterized after expression in Sf9 insect cells. The MEV VP-2 product had the same size as that reported for the wild-type MEV VP-2 protein and was recognized by convalescent sera from MEV-infected mink and a panel of monoclonal antibodies reactive to MEV. Furthermore, the VP-2 protein was able to form parvovirus-like particles, which had haemagglutinating properties comparable with the wild-type MEV. The cloned VP-2 gene was sequenced and only five nucleotide differences were found after alignment with the known sequences of the MEV type 1 and type 2 isolates. Surprisingly, the VP-2 gene encoded a valine and a tyrosine at amino acid positions 232 and 234, identical to the situation found in MEV type 1, but at position 300 there was a valine which is a determinant of MEV type 2. Immunization of mink with approximately 40000 haemagglutinating units of recombinant MEV VP-2 induced a measurable antibody response as tested by haemagglutination inhibition. Furthermore, the immunized mink did not excrete virus and did not develop clinical disease upon challenge with a virulent isolate of MEV.
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页码:149 / 155
页数:7
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