Your search keyword '"Cervera MT"' showing total 4 results

1. Identification of a pathogenicity determinant of Plum pox virus in the sequence encoding the C-terminal region of protein P3+6K(1).

Author

Sáenz P, Cervera MT, Dallot S, Quiot L, Quiot JB, Riechmann JL, and García JA

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA Primers genetics, DNA, Complementary genetics, DNA, Complementary isolation & purification, DNA, Viral genetics, DNA, Viral isolation & purification, Genes, Genome, Viral, Molecular Sequence Data, Pisum sativum virology, Phenotype, Plants, Toxic, Sequence Homology, Amino Acid, Nicotiana virology, Viral Proteins genetics, Virulence genetics, Plum Pox Virus genetics, Plum Pox Virus pathogenicity

Abstract

A full-length genomic cDNA clone of a plum pox potyvirus (PPV) isolate belonging to the M strain (PPV-PS) has been cloned downstream from a bacteriophage T7 polymerase promoter and sequenced. Transcripts from the resulting plasmid, pGPPVPS, were infectious and, in herbaceous hosts, produced symptoms that differed from those of virus progeny of pGPPV, a full-length genomic cDNA clone of the D strain PPV-R. Viable PPV-R/-PS chimeric viruses were constructed by recombination of the cDNA clones in vitro. Analysis of plants infected with the different chimeras indicated that sequences encoding the most variable regions of the potyvirus genome, the P1 and capsid protein coding sequences, were not responsible for symptom differences between the two PPV isolates in herbaceous hosts. On the contrary, complex symptomatology determinants seem to be located in the central region of the PPV genome. The results indicate that a genomic fragment that encodes 173 aa from the C-terminal part of the P3+6K(1) coding region is enough to confer, on a PPV-R background, a PS phenotype in Nicotiana clevelandii. This pathogenicity determinant also participates in symptom induction in Pisum sativum, although the region defining the PS phenotype in this host is probably restricted to 74 aa.

Published

2000

2. Processing of the plum pox virus polyprotein at the P3-6K1 junction is not required for virus viability.

Author

Riechmann JL, Cervera MT, and García JA

Subjects

Animals, Binding Sites, Endopeptidases, Plum Pox Virus genetics, Plum Pox Virus physiology, Proteins genetics, RNA, Viral analysis, Rabbits, Viral Proteins genetics, Plum Pox Virus metabolism, Protein Processing, Post-Translational, Proteins metabolism, Viral Proteins metabolism

Abstract

Proteolytic processing of the potyvirus polyprotein is mainly performed by the virus-encoded NIa protease, whose cleavage sites are characterized by conserved heptapeptide sequences. Partial processing at the cleavage site present between the P3 and 6K1 cistrons by the plum pox potyvirus (PPV) NIa protease has been previously shown to occur in vitro. We have now studied the role of polyprotein processing at the P3-6K1 junction in vivo, using a full-length PPV cDNA clone. PPV mutant transcripts containing a histidine for glutamine substitution in the cleavage site sequence (a change that abolishes in vitro processability) are able to infect Nicotiana clevelandii plants, indicating that normal processing at the P3-6K1 junction is not required for virus viability. However, disease symptoms were not detected and virus accumulation occurred after a second site mutation was introduced into the 6K1 cistron during replication. This additional change did not restore the in vitro processability of the mutant heptapeptide. Changes at other positions in the heptapeptide (that only slightly altered the in vitro processability of this NIa site) were also engineered and it was found that these mutations affected the time course and severity of the symptom induction process. A possible regulatory effect on the function of the potyvirus P3 + 6K1 protein by processing at the P3-6K1 junction is discussed in light of our present results with PPV.

Published

1995

3. 3'-terminal sequence of the plum pox virus PS and ŏ6 isolates: evidence for RNA recombination within the potyvirus group.

Author

Cervera MT, Riechmann JL, Martín MT, and García JA

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, Consensus Sequence, Molecular Sequence Data, RNA, Viral genetics, Fruit microbiology, Plant Viruses genetics, RNA Viruses genetics, Recombination, Genetic genetics

Abstract

The sequence of the 3'-terminal 1768 nucleotides of the PS and ŏ6 isolates of plum pox virus (PPV) has been determined and compared with that of the equivalent regions of other PPV isolates sequenced previously. The sequenced region is part of the PPV open reading frame encoding the last 186 amino acids of the NIb protein and the coat protein (CP, 330 amino acids), followed by a non-coding region of 220 nucleotides and a poly(A) tail. PPV-PS and PPV(-)ŏ6, just like PPV-El Amar, show rather high levels of nucleotide diversity in the sequence encoding the C-terminal region of the NIb protein (19.4 to 31%) and the N terminus of CP (22.8 to 41.1%) when compared with PPV-Rankovic, PPV-D and PPV-NAT, whereas the level of diversity in the rest of the CP sequence and the 3' non-coding region is low (8 to 10.8% and 5.5 to 7.7%, respectively). However, the first 429 sequenced nucleotides of PPV(-)ŏ6 are very similar to those of the PPV-Rankovic, PPV-D and PPV-NAT isolates, whereas the rest of the sequence clearly resembles PPV-PS. Thus, PPV(-)ŏ6 seems to be the result of a natural recombination event between two wild strains of PPV. To our knowledge this is the first evidence of homologous RNA recombination (a process which could play an important role in the evolution of RNA viruses) within the potyvirus group.

Published

1993

4. Mutational analysis of plum pox potyvirus polyprotein processing by the NIa protease in Escherichia coli.

Author

García JA, Laín S, Cervera MT, Riechmann JL, and Martín MT

Subjects

DNA Mutational Analysis, Endopeptidases genetics, Escherichia coli enzymology, Kinetics, Molecular Weight, Plasmids, Protein Processing, Post-Translational, Endopeptidases metabolism, Escherichia coli genetics, Plant Viruses genetics, Viral Proteins genetics

Abstract

A binary Escherichia coli expression system has been used to study the pathway for proteolytic processing of the plum pox potyvirus (PPV) polyprotein. Trans cleavage at the carboxyl end of the cylindrical inclusion protein occurred, although with lower efficiency than that at the large nuclear inclusion protein-capsid protein junction. No trans cleavage at the carboxyl end of the small nuclear inclusion protein (NIa) was detected. The proteolytic activities at different cleavage sites of several deletion and point mutations of NIa protein have been analysed. The large delta SX deletion and two different point mutations at His 239 abolished proteolytic activity at all sites. The effect of other mutations, particularly a Glu substitution for Asp 274, depended on the particular cleavage site analysed. The results obtained with the PPV NIa protein mutants were similar to those reported for comparable mutations in the tobacco etch virus 49K protease, despite differences in the sequences recognized for processing. No evident competitive inhibition of the proteolytic activity of PPV NIa protease by the presence of an excess of the different protease mutants could be demonstrated.

Published

1990