Adaptation of a velogenic Newcastle disease virus to Vero cells: Assessing the molecular changes before and after adaptation

A velogenic Newcastle disease virus isolate was passaged 50 times in Vero cell culture and the virus was assessed for the molecular changes associated with the passaging. At every 10th passage, the virus was characterized conventionally by mean death time (MDT) analysis, intracerebral pathogenicity...

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Bibliographic Details
Published in:Veterinary research communications 2007-04, Vol.31 (3), p.371-383
Main Authors: Madhan Mohan, C, Dey, Sohini, Kumanan, K, Murali Manohar, B, Mahalinga Nainar, A
Format: Article
Language:English
Subjects:
Amino Acid Sequence
amino acid sequences
Animals
Base Sequence
bursa of Fabricius
Cell Culture Techniques - methods
cell lines
Cercopithecus aethiops
Chickens
Cloning, Molecular
cultured cells
Cytopathogenic Effect, Viral
genes
genetic variation
hemorrhage
histopathology
lymphocytes
Male
microbial genetics
Molecular Sequence Data
monkeys
Newcastle Disease - virology
Newcastle disease virus
Newcastle disease virus - genetics
Newcastle disease virus - pathogenicity
Newcastle disease virus - physiology
nucleotide sequences
protein structure
reverse transcriptase polymerase chain reaction
Reverse Transcriptase Polymerase Chain Reaction - veterinary
RNA, Viral - chemistry
RNA, Viral - genetics
Sequence Alignment
spleen
strain differences
thymus gland
tonsils
Vero cells
Vero Cells - virology
viral fusion proteins
Viral Fusion Proteins - genetics
Virulence
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Summary:A velogenic Newcastle disease virus isolate was passaged 50 times in Vero cell culture and the virus was assessed for the molecular changes associated with the passaging. At every 10th passage, the virus was characterized conventionally by mean death time (MDT) analysis, intracerebral pathogenicity index (ICPI) and virus titration. At increasing passage levels, a gradual reduction in the virulence of the virus was observed. Molecular characterization of the virus included cloning and sequencing of a portion of the fusion gene (1349 bp) encompassing the fusion protein cleavage site (FPCS), which was previously amplified by reverse transcription-polymerase chain reaction. Sequence analysis revealed a total of 135 nucleotide substitutions which resulted in the change of 42 amino acids between the velogenic virus and the 50th passage virus. The predicted amino acid motif present at the cleavage site of the virulent virus was (109)SRRRRQRRFVG(119) and the corresponding region of the adapted adapted virus was (109)SGGRRQKRFIG(119). Pathogenicity studies conducted in 20-week-old seronegative birds revealed gross lesions such as petechial haemorrhages in the trachea, proventricular junction and intestines, and histopathological changes such as depletion and necrosis of the lymphocytes in thymus, spleen, bursa and caecal tonsils in the birds injected with the velogenic virus and absence of the lesions in birds injected with the adapted virus. The 50th-passage cell culture virus was back-passaged five times in susceptible chickens and subjected to virulence attribute analysis and sequence analysis of the FPCS region, with minor difference found between them.
ISSN:0165-7380
1573-7446
DOI:10.1007/s11259-006-3502-2