Generation of full-length cDNA of the two genomic dsRNA segments of Infectious Bursal Disease virus

Generation of full-length cDNA of the two genomic dsRNA segments of Infectious Bursal Disease virus

To determine the complete nucleotide sequence of Infectious Bursal Disease virus (IBDV) isolates, an efficient method was developed to generate full-length cDNA of both the genomic A- and B-segments. Reverse transcription was carried out at the highest possible temperature (50°C) for the reverse tra...

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Veröffentlicht in:Journal of virological methods 2000, Vol.84 (1), p.49-58
Hauptverfasser: Boot, Hein J., ter Huurne, Agnes H.M., Peeters, Ben P.H.
Format: Artikel
Sprache:eng
Schlagworte:
Animals
ARN
Base Sequence
Biological and medical sciences
Birnaviridae Infections - veterinary
Birnaviridae Infections - virology
Chickens
CLONACION MOLECULAR
CLONAGE MOLECULAIRE
CLONE
CLONES
Cloning, Molecular
COMPLEMENTARY DNA
DNA Primers - genetics
DNA, Complementary - genetics
DNA, Viral - genetics
Full length cDNA
Fundamental and applied biological sciences. Psychology
Genome, Viral
ID Lelystad, Institute for Animal Science and Health
ID-Lelystad, Instituut voor Dierhouderij en Diergezondheid
INFECTIOUS BURSAL DISEASE VIRUS
Infectious bursal disease virus - genetics
Infectious bursal disease virus - isolation & purification
Infectious bursal disease virus - pathogenicity
Microbiology
MOLECULAR CLONING
Poultry Diseases - virology
Protein Biosynthesis
Reverse Transcriptase Polymerase Chain Reaction - methods
REVERSE TRANSCRIPTION
RNA
RNA, Double-Stranded - genetics
RNA, Double-Stranded - isolation & purification
RNA, Viral - genetics
RNA, Viral - isolation & purification
Techniques used in virology
TRANSCRIPCION INVERSA
TRANSCRIPTION INVERSE
Transcription, Genetic
Virology
Virology - methods
VIRUS BURSITE INFECTIEUSE
VIRUS BURSITIS INFECCIOSA
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Zusammenfassung:To determine the complete nucleotide sequence of Infectious Bursal Disease virus (IBDV) isolates, an efficient method was developed to generate full-length cDNA of both the genomic A- and B-segments. Reverse transcription was carried out at the highest possible temperature (50°C) for the reverse transcriptase enzyme, and the single stranded cDNA was subsequently amplified by using an optimized PCR. The double stranded, full-length cDNA was efficiently cloned into a high copy number plasmid. Our results show that the entire cDNA of both the A- and B-segment of a classical attenuated isolate (CEF94), and a very virulent field isolate (D6948), can be cloned. The method will simplify greatly the procedure to generate full-length cDNA and determine the nucleotide sequence of the entire genome of IBDV isolates.
ISSN:0166-0934
1879-0984
DOI:10.1016/S0166-0934(99)00132-9