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J. Virol., Nov 1997, 8362-8367, Vol 71, No. 11
BM Meehan, D Todd, JL Creelan, TJ Connor and MS McNulty
Molecular cloning of the Cux-1 isolate of chicken anemia virus (CAV), which
had been passaged 173 times in cell culture, resulted in the isolation of
an attenuated strain, designated cloned isolate 10, which reverted to
virulence following 10 passages in young chicks (D. Todd, T. J. Connor, V.
M. Calvert, J. L. Creelan, B. M. Meehan, and M. S. McNulty, Avian Pathol.
24:171-187, 1995). The attenuated cloned isolate 10 differs from the
molecularly cloned pathogenic Cux-1 isolate in that it possesses a
21-nucleotide insertion within the nontranscribed region of the CAV genome
and 17 individual nucleotide substitutions dispersed throughout the genome.
Comparative analyses with other published CAV sequences indicated that
cloned isolate 10 was unique at nine nucleotide positions and at five amino
acid positions. The molecular basis of the attenuation exhibited by cloned
isolate 10 was investigated by evaluating the pathogenicities of two sets
of complementary chimeric viruses. These sets were produced by transfection
with chimeric double-stranded replicative-form (RF) DNA equivalents that
contained DNA sequences derived from cloned isolate 10 and the pathogenic
cloned Cux-1 isolate. The construction of the chimeric RFs exploited the
occurrence of unique EcoRI, PstI, and BamHI restriction sites, which
allowed their respective circular CAV RFs to be manipulated as three
restriction fragments of 0.58, 0.93, and 0.71 kbp. Examination of the
levels of anemia and gross pathology in the thymuses and bone marrows of 14
day-old specific-pathogen-free chicks following infection of 1-day-old
chicks with the chimeric and cloned parental isolates indicated that
nucleotide changes in each of the three genomic regions contributed towards
attenuation. The significance of this result to the development and use of
live attenuated CAV vaccines is discussed.
Copyright © 1997, American Society for Microbiology
Investigation of the attenuation exhibited by a molecularly cloned chicken anemia virus isolate by utilizing a chimeric virus approach
Department of Veterinary Science, The Queen's University of Belfast, United Kingdom.
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