Pathogen-derived resistance to dengue type virus 2 in mosquito cells by expression of the premembrane coding region of the viral genome

被引：54

作者：

Gaines, PJ ^{[1
]}

Olson, KE ^{[1
]}

Higgs, S ^{[1
]}

Powers, AM ^{[1
]}

Beaty, BJ ^{[1
]}

Blair, CD ^{[1
]}

机构：

[1] COLORADO STATE UNIV, DEPT MICROBIOL, ARTHROPOD BORNE & INFECT DIS LAB, FT COLLINS, CO 80523 USA

来源：

JOURNAL OF VIROLOGY | 1996年 / 70卷 / 04期

关键词：

D O I：

10.1128/JVI.70.4.2132-2137.1996

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The full-length premembrane (prM) coding region of the dengue virus type 2 (DEN-2; Jamaica) genome was expressed in C6/36 (Adedes albopictus) cells in either the sense or the antisense orientation from a double subgenomic Sindbis (dsSIN) virus. Northern (RNA) blot analysis confirmed the expression of sense or antisense DEN-2 prM RNA in infected C6/36 cells. PrM protein was demonstrated in cells infected with dsSIN viruses expressing DEN-2 sense RNAs by an immunofluorescence assay. C6/36 cells were infected with each dsSIN virus at a multiplicity of infection (MOI) of 50 and challenged 48 h later with DEN-2 virus at an MOI of 0.1. Whereas C6/36 cells infected with a control dsSIN virus supported high levels of DEN-2 replication, C6/36 cells infected with the dsSIN virus expressing prM antisense RNA were completely resistant to DEN-2 challenge. Cells expressing prM protein or untranslatable prM sense RNA also were resistant to DEN-2 challenge. Cells expressing prM protein demonstrated some breakthrough of DEN-2 virus when challenged at an MOI of 10. However, expressed untranslatable sense prM RNA conferred complete protection to challenge at the high MOI.

引用

页码：2132 / 2137

页数：6

共 30 条

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

CHAMBERS, TJ ;

HAHN, CS ;

GALLER, R ;

RICE, CM .

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

[2] MONOCLONAL-ANTIBODIES TO SINDBIS VIRUS GLYCOPROTEIN-E1 CAN NEUTRALIZE, ENHANCE INFECTIVITY, AND INDEPENDENTLY INHIBIT HEMAGGLUTINATION OR HEMOLYSIS [J].

CHANAS, AC ;

GOULD, EA ;

CLEGG, JCS ;

VARMA, MGR .

JOURNAL OF GENERAL VIROLOGY, 1982, 58 (JAN) :37-46

[3] SINGLE-STEP METHOD OF RNA ISOLATION BY ACID GUANIDINIUM THIOCYANATE PHENOL CHLOROFORM EXTRACTION [J].

CHOMCZYNSKI, P ;

SACCHI, N .

ANALYTICAL BIOCHEMISTRY, 1987, 162 (01) :156-159

[4] TRANSGENIC MOSQUITOS - A FUTURE VECTOR CONTROL STRATEGY [J].

CRAMPTON, J ;

MORRIS, A ;

LYCETT, G ;

WARREN, A ;

EGGLESTON, P .

PARASITOLOGY TODAY, 1990, 6 (02) :31-36

[5] CHARACTERIZATION OF RNA-MEDIATED RESISTANCE TO TOMATO SPOTTED WILT VIRUS IN TRANSGENIC TOBACCO PLANTS [J].

DEHAAN, P ;

GIELEN, JJL ;

PRINS, M ;

WIJKAMP, IG ;

VANSCHEPEN, A ;

PETERS, D ;

VANGRINSVEN, MQJM ;

GOLDBACH, R .

BIO-TECHNOLOGY, 1992, 10 (10) :1133-1137

[6] MECHANISM OF ACTION OF ANTISENSE RNA - SOMETIME INHIBITION OF TRANSCRIPTION, PROCESSING, TRANSPORT, OR TRANSLATION [J].

DENHARDT, DT .

ANNALS OF THE NEW YORK ACADEMY OF SCIENCES-SERIES, 1992, 660 :70-76

[7] NUCLEOTIDE-SEQUENCE AND DEDUCED AMINO-ACID-SEQUENCE OF THE STRUCTURAL PROTEINS OF DENGUE TYPE-2 VIRUS, JAMAICA GENOTYPE [J].

DEUBEL, V ;

KINNEY, RM ;

TRENT, DW .

VIROLOGY, 1986, 155 (02) :365-377

[8] EXAMINATION OF THE IMMUNOLOGICAL RELATIONSHIPS BETWEEN FLAVIVIRUSES USING YELLOW-FEVER VIRUS MONOCLONAL-ANTIBODIES [J].

GOULD, EA ;

BUCKLEY, A ;

CAMMACK, N ;

BARRETT, ADT ;

CLEGG, JCS ;

ISHAK, R ;

VARMA, MGR .

JOURNAL OF GENERAL VIROLOGY, 1985, 66 (JUL) :1369-1382

[9]

GUBLER DJ, 1995, EMERG INFECT DIS, V1, P55

[10] INFECTIOUS SINDBIS VIRUS TRANSIENT EXPRESSION VECTORS FOR STUDYING ANTIGEN PROCESSING AND PRESENTATION [J].

HAHN, CS ;

HAHN, YS ;

BRACIALE, TJ ;

RICE, CM .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1992, 89 (07) :2679-2683

← 1 2 3 →