GENE-MAPPING AND EXPRESSION OF 2 IMMUNODOMINANT EPSTEIN-BARR-VIRUS CAPSID PROTEINS

被引：50

作者：

VANGRUNSVEN, WMJ ^{[1
]}

VANHEERDE, EC ^{[1
]}

DEHAARD, HJW ^{[1
]}

SPAAN, WJM ^{[1
]}

MIDDELDORP, JM ^{[1
]}

机构：

[1] LEIDEN UNIV, DEPT VIROL, 2300 AH LEIDEN, NETHERLANDS

来源：

JOURNAL OF VIROLOGY | 1993年 / 67卷 / 07期

关键词：

D O I：

10.1128/JVI.67.7.3908-3916.1993

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The genomic localization of two immunodominant genes encoding two proteins of the Epstein-Barr virus capsid antigen (VCA) complex, VCA-p18 and VCA-p40, has been identified. For that purpose, lambda gt11-based cDNA libraries were constructed from HH514.c16 cells induced for virus production. The libraries were screened with a monoclonal antibody, EBV.OT41A, directed against VCA-p40 or with affinity-purified human antibodies against VCA-p18. Sequencing of the inserts of positive plaques showed that VCA-p18 and VCA-p40 are encoded within open reading frames (ORFs) BFRF3 and BdRF1, respectively. Peptide scanning analysis of the predicted protein of ORF BdRF1 resulted in defining the epitope of monoclonal antibody EBV.OT41A at the C-terminal region. The dominant VCA-p18 reactivity of human sera can be completely inhibited by preadsorption with Escherichia coli-expressed BFRF3-beta-galactosidase. Serum of a rabbit immunized with BFRF3-betagalactosidase reacts with a VCA-specific protein of 18 kDa. In addition, BFRF3-beta-galactosidase affinity-purified antibodies react with VCA-p18 of virus-producing cells (HH514.c16). Complete inhibition of viral DNA polymerase activity by phosphonoacetic acid is associated with the absence of RNAs and protein products of both ORFs, indicating that VCA-p18 and VCA-p40 are true late antigens.

引用

页码：3908 / 3916

页数：9

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