A novel open reading frame in tobacco mosaic virus genome coding for a putative small, positively charged protein

From sequence comparisons between the tobamovirus genomes an open reading frame (ORF-X) potentially encoding a small, positively charged protein (33- to 45-amino-acids long) was found to overlap the immediate 3′ and 5′ sides of the transport protein gene and coat protein gene, respectively. In vitro...

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Bibliographic Details
Published inBiochimie Vol. 75; no. 8; pp. 659 - 665
Main Authors Morozov, S.Yu, Denisenko, O.N., Zelenina, D.A., Fedorkin, O.N., Solovyev, A.G., Maiss, E., Casper, R., Atabekov, J.G.
Format Journal Article
LanguageEnglish
Published France Elsevier Masson SAS 1993
Subjects
ADN RECOMBINADO
ADN RECOMBINE
Amino Acid Sequence
Base Sequence
Cell-Free System
DNA, Viral
DNA-Directed RNA Polymerases
Electrochemistry
GENETICA MOLECULAR
GENETIQUE MOLECULAIRE
GENOMAS
GENOME
GENOMES
in vitro translation
MOLECULAR GENETICS
Molecular Sequence Data
Mutagenesis, Site-Directed
NUCLEOTIDE SEQUENCE
Open Reading Frames
plant virus
PLANT VIRUSES
Protein Biosynthesis
PROTEINAS
PROTEINE
PROTEINS
RECOMBINANT DNA
RNA, Messenger - genetics
RNA, Messenger - metabolism
RNA, Viral - genetics
RNA, Viral - metabolism
SECUENCIA NUCLEICA
SEQUENCE NUCLEIQUE
TOBACCO MOSAIC TOBAMOVIRUS
tobacco mosaic virus
Tobacco Mosaic Virus - genetics
TOBAMOVIRUS DEL MOSAICO DEL TABACO
TOBAMOVIRUS MOSAIQUE DU TABAC
Viral Proteins - genetics
VIRUS DE LAS PLANTAS
VIRUS DES VEGETAUX
recombinant DNA
tobacco mosaic virus
in vitro translation
plant virus
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Summary:From sequence comparisons between the tobamovirus genomes an open reading frame (ORF-X) potentially encoding a small, positively charged protein (33- to 45-amino-acids long) was found to overlap the immediate 3′ and 5′ sides of the transport protein gene and coat protein gene, respectively. In vitro translation of the monocistronic artificial transcripts generated with T7 RNA polymerase yielded a protein of M r 4000 (p4) and an unexpected trypsin-sensitive complex of M r 54000 that was resistant to reduction with 2-mercaptoethanol but could be dissociated by 8 M urea. Assembly of this complex was inhibited completely by site-directed mutagenesis within a conserved, positively charged 5-amino-acid long segment of the ORF-X protein. After centrifugation in low salt buffer the 54-kDa complex remained mostly associated with ribosomes. Apparently this complex represents a specific aggregate of the p4 product of ORF-X with a protein of approximate M r 50000 that is a component of the translation apparatus.
Bibliography:9504484
H20
ISSN:0300-9084
1638-6183
DOI:10.1016/0300-9084(93)90096-B