HIGH-LEVEL EXPRESSION OF THE TICK-BORNE ENCEPHALITIS-VIRUS NS1 PROTEIN BY USING AN ADENOVIRUS-BASED VECTOR - PROTECTION ELICITED IN A MURINE MODEL

被引：93

作者：

JACOBS, SC ^{[1
]}

STEPHENSON, JR ^{[1
]}

WILKINSON, GWG ^{[1
]}

机构：

[1] CTR APPL MICROBIOL & RES,DIV BIOL,PUBL HLTH LAB,MOLEC VIROL GRP,SALISBURY SP4 0JG,ENGLAND

来源：

JOURNAL OF VIROLOGY | 1992年 / 66卷 / 04期

关键词：

D O I：

10.1128/JVI.66.4.2086-2095.1992

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

Tick-borne encephalitis virus (TBEV) encodes an abundant, highly immunogenic nonstructural glycoprotein, NS1. The function of this protein has yet to be determined. We have cloned the NS1 gene from the Neudorfl strain of TBEV under the control of the powerful constitutive cytomegalovirus major immediate-early promoter into an adenovirus E1 deletion mutant. The novel combination of the cytomegalovirus immediate-early promoter and the adenovirus vector produced extremely high levels of NS1 expression in cells which do not support replication of the adenovirus deletion mutant. The recombinant protein was shown to be indistinguishable from authentic TBEV NS1 in its (i) apparent molecular weight by polyacrylamide gel electrophoresis, (ii) glycosylation pattern, (iii) ability to form high-molecular-weight complexes, and (iv) ability to be secreted from cells. Appropriate processing of NS1 expressed by the adenovirus recombinant occurred independently of any additional TBEV-encoded gene function. When directly inoculated into mice, the recombinant adenovirus RAd51 was shown to elicit an antibody response to the TBEV NS1 protein. Immunization with RAd51 conferred protection against challenge with TBEV.

引用

页码：2086 / 2095

页数：10

共 42 条

[1] CHARACTERIZATION OF PROTEASE CLEAVAGE SITES INVOLVED IN THE FORMATION OF THE ENVELOPE GLYCOPROTEIN AND 3 NONSTRUCTURAL PROTEINS OF DENGUE VIRUS TYPE-2, NEW-GUINEA C-STRAIN [J].

BIEDRZYCKA, A ;

CAUCHI, MR ;

BARTHOLOMEUSZ, A ;

GORMAN, JJ ;

WRIGHT, PJ .

JOURNAL OF GENERAL VIROLOGY, 1987, 68 :1317-1326

[2] THE PMTL NIC-CLONING VECTORS .1. IMPROVED PUC POLYLINKER REGIONS TO FACILITATE THE USE OF SONICATED DNA FOR NUCLEOTIDE SEQUENCING [J].

CHAMBERS, SP ;

PRIOR, SE ;

BARSTOW, DA ;

MINTON, NP .

GENE, 1988, 68 (01) :139-149

[3] FLAVIVIRUS GENOME ORGANIZATION, EXPRESSION, AND REPLICATION [J].

CHAMBERS, TJ ;

HAHN, CS ;

GALLER, R ;

RICE, CM .

ANNUAL REVIEW OF MICROBIOLOGY, 1990, 44 :649-688

[4] PRODUCTION OF YELLOW-FEVER VIRUS PROTEINS IN INFECTED-CELLS - IDENTIFICATION OF DISCRETE POLYPROTEIN SPECIES AND ANALYSIS OF CLEAVAGE KINETICS USING REGION-SPECIFIC POLYCLONAL ANTISERA [J].

CHAMBERS, TJ ;

MCCOURT, DW ;

RICE, CM .

VIROLOGY, 1990, 177 (01) :159-174

[5]

FALGOUT B, 1990, NEW ASPECTS OF POSITIVE-STRAND RNA VIRUSES, P192

[6] PROPER PROCESSING OF DENGUE VIRUS NONSTRUCTURAL GLYCOPROTEIN-NS1 REQUIRES THE N-TERMINAL HYDROPHOBIC SIGNAL SEQUENCE AND THE DOWNSTREAM NONSTRUCTURAL PROTEIN-NS2A [J].

FALGOUT, B ;

CHANOCK, R ;

LAI, CJ .

JOURNAL OF VIROLOGY, 1989, 63 (05) :1852-1860

[7] IMMUNIZATION OF MICE WITH RECOMBINANT VACCINIA VIRUS EXPRESSING AUTHENTIC DENGUE VIRUS NONSTRUCTURAL PROTEIN NS1 PROTECTS AGAINST LETHAL DENGUE VIRUS ENCEPHALITIS [J].

FALGOUT, B ;

BRAY, M ;

SCHLESINGER, JJ ;

LAI, CJ .

JOURNAL OF VIROLOGY, 1990, 64 (09) :4356-4363

[8] MEMBRANE ASSOCIATION AND SECRETION OF THE JAPANESE ENCEPHALITIS-VIRUS NS1 PROTEIN FROM CELLS EXPRESSING NS1 CDNA [J].

FAN, W ;

MASON, PW .

VIROLOGY, 1990, 177 (02) :470-476

[9] NEUTRALIZING (54K) AND NONNEUTRALIZING (54K AND K-48) MONOCLONAL-ANTIBODIES AGAINST STRUCTURAL AND NONSTRUCTURAL YELLOW-FEVER VIRUS PROTEINS CONFER IMMUNITY IN MICE [J].

GOULD, EA ;

BUCKLEY, A ;

BARRETT, ADT ;

CAMMACK, N .

JOURNAL OF GENERAL VIROLOGY, 1986, 67 :591-595

[10]

Graham F L, 1991, Methods Mol Biol, V7, P109, DOI 10.1385/0-89603-178-0:109

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