Publication
Nucleotide sequence of the capsid protein cistron from six potato virus Y (PVY) strains infecting tobacco
Details
Author(s):
SL Sudarsono; SA Woloshuk; Z Lommel; Z Xiong; GM Hellman; EA Wernsman; AK Weissinger
Type of Document:
Scholarly Article
Publisher/Journal:
Archives of Virology
Date of Publication:
n.d.
Place of Publication:
Not Available
Description
Abstract: Complementary DNA libraries representing the capsid protein cistron of the potato virus Y (PVY) isolate Chilean, Hungarian, MsNr, NsNr, O, and Potato US were synthesized and used as template for polymerase chain reaction (PCR) amplification. An AUG codon for initiating a discrete capsid protein (CP) open reading frame was embedded upstream of the first codon of the CP cistrons. PCR-amplified products of the expected size of 0.8 kilo bases were cloned into the transcription vector pBS(+). The fidelity of each PCR-amplified PVY CP cistron was tested by transcribing recombinant plasmids in vitro and translating the transcripts in two cell free translation systems. Translation analysis of in vitro transcribed PVY CP cistrons consistently yielded a polypeptide co-migrating with authentic CP that was immunoprecipitated by anti PVY Chilean antibodies. The nucleotide sequence of each capsid protein gene was determined by dideoxy sequence analysis. Each capsid protein gene was determined to be 801 nucleotides in length, encoding a deduced protein of 267 amino acids with calculated Mr ranging from 29 799 to 29 980. The nucleic acid sequence similarity between the six isolates ranged between 89 to 97% and the amino acid similarity between 91 to 99%. The high level of amino acid sequence similarity confirms the classification of these viruses as isolates of PVY.