ASSEMBLY AND TRANSCRIPTION OF SYNTHETIC VESICULAR STOMATITIS-VIRUS NUCLEOCAPSIDS

被引：56

作者：

MOYER, SA ^{[1
]}

SMALLWOODKENTRO, S ^{[1
]}

HADDAD, A ^{[1
]}

PREVEC, L ^{[1
]}

机构：

[1] MCMASTER UNIV, DEPT BIOL, HAMILTON L8S 4K1, ONTARIO, CANADA

来源：

JOURNAL OF VIROLOGY | 1991年 / 65卷 / 05期

关键词：

D O I：

10.1128/JVI.65.5.2170-2178.1991

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The functional template for transcription of vesicular stomatitis virus (VSV) RNA is a ribonucleoprotein particle (nucleocapsid) consisting of the negative-strand sense genomic RNA completely encapsidated by the viral nucleocapsid (N) protein. As an approach to create nucleocapsids in vitro, we demonstrate here the specific encapsidation by purified of in vitro-synthesized RNA sequences representing the 5' end of both the negative- and positive-strand VSV genome-length RNAs. As few as 19 nucleotides would allow partial (50%) encapsidation. Sequences downstream of the binding site can be of any origin. Specific encapsidation of VSV sequences was dependent on the presence of uninfected cell cytoplasmic extracts or poly(A). The synthetic nucleocapsids have the properties of RNase resistance and a buoyant density typical of wild-type VSV nucleocapsids. We have encapsidated a synthetic virionlike RNA species which contained just the terminal sequences of the virion RNA: the N encapsidation signal from the 5' end and the leader gene from the 3' end. This assembled nucleocapsid could function in vitro as a transcription template for the VSV RNA polymerase.

引用

页码：2170 / 2178

页数：9

共 36 条

[1] INTERACTION OF MESSENGER-RNA WITH PROTEINS IN VESICULAR STOMATITIS VIRUS-INFECTED CELLS [J].

ADAM, SA ;

CHOI, YD ;

DREYFUSS, G .

JOURNAL OF VIROLOGY, 1986, 57 (02) :614-622

[2] ROLE OF THE NUCLEOCAPSID PROTEIN IN REGULATING VESICULAR STOMATITIS-VIRUS RNA-SYNTHESIS [J].

ARNHEITER, H ;

DAVIS, NL ;

WERTZ, G ;

SCHUBERT, M ;

LAZZARINI, RA .

CELL, 1985, 41 (01) :259-267

[3] ENCAPSIDATION OF SENDAI VIRUS GENOME RNAS BY PURIFIED NP PROTEIN DURING INVITRO REPLICATION [J].

BAKER, SC ;

MOYER, SA .

JOURNAL OF VIROLOGY, 1988, 62 (03) :834-838

[4] INFECTIOUS MEASLES-VIRUS FROM CLONED CDNA [J].

BALLART, I ;

ESCHLE, D ;

CATTANEO, R ;

SCHMID, A ;

METZLER, M ;

CHAN, J ;

PIFKOHIRST, S ;

UDEM, SA ;

BILLETER, MA .

EMBO JOURNAL, 1990, 9 (02) :379-384

[5] TRANSCRIPTION AND REPLICATION OF RHABDOVIRUSES [J].

BANERJEE, AK .

MICROBIOLOGICAL REVIEWS, 1987, 51 (01) :66-87

[6] N-PROTEIN OF VESICULAR STOMATITIS-VIRUS SELECTIVELY ENCAPSIDATES LEADER RNA INVITRO [J].

BLUMBERG, BM ;

GIORGI, C ;

KOLAKOFSKY, D .

CELL, 1983, 32 (02) :559-567

[7] INTERACTION OF VSV LEADER RNA AND NUCLEOCAPSID PROTEIN MAY CONTROL VSV GENOME REPLICATION [J].

BLUMBERG, BM ;

LEPPERT, M ;

KOLAKOFSKY, D .

CELL, 1981, 23 (03) :837-845

[8] INTRACELLULAR VESICULAR STOMATITIS-VIRUS LEADER RNAS ARE FOUND IN NUCLEOCAPSID STRUCTURES [J].

BLUMBERG, BM ;

KOLAKOFSKY, D .

JOURNAL OF VIROLOGY, 1981, 40 (02) :568-576

[9] PREPARATION AND ANALYSIS OF THE NUCLEOCAPSID PROTEINS OF VESICULAR STOMATITIS-VIRUS AND SENDAI VIRUS, AND ANALYSIS OF THE SENDAI VIRUS LEADER-NP GENE REGION [J].

BLUMBERG, BM ;

GIORGI, C ;

ROSE, K ;

KOLAKOFSKY, D .

JOURNAL OF GENERAL VIROLOGY, 1984, 65 (APR) :769-779

[10] INVITRO REPLICATION OF SENDAI VIRUS WILD-TYPE AND DEFECTIVE INTERFERING PARTICLE GENOME RNAS [J].

CARLSEN, SR ;

PELUSO, RW ;

MOYER, SA .

JOURNAL OF VIROLOGY, 1985, 54 (02) :493-500

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