Keywords (Extracted from title, table of contents and
abstract of thesis)
Subsequent, Biological,
Differential, Pathogenic, Molecular, Virus, Characterization,
Sensitivity, Primers, Influenza, Avian, Vaccines, Antigenic,
Poultry, Population |
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Abstract
During the Avian
Influenza (AI) outbreaks in different areas of Pakistan (2003 - 06),
a number of Avian Influenza Virus (AIV) isolates were recovered from
the clinical samples. The samples were subjected to comparative
diagnostic evaluation using in-ovo propagation, Virus Neutralization
Test (VNT), rapid detection kits and Reverse Transcriptase-
Polymerase Chain Reaction (RT-PCR). The data revealed that RT-PCR
technique was most sensitive and specific for the detection of Avian
Influenza Virus subtypes and for differentially diagnosing it from
other avian respiratory pathogenic viruses. These isolates were
further utilized for the development of multiplex RT-PCR. A
multiplex reverse transcriptase polymerase chain reaction (mRT-PCR)
was developed and standardized for the detection of type A influenza
viruses, Avian Influenza Virus (AIV) subtype H7, H9 and H5
haemagglutinin gene with simultaneous detection of 3 other poultry
respiratory pathogens Newcastle disease virus (NDV), infectious
bronchitis virus (IBV) and infectious laryngotracheitis virus (ILTV).
Seven sets of specific oligonucleotide primers were used in this
study for the M-Gene of AIV and haemagglutinin gene of subtypes of
H7, H9 and H5 of AIV. Three sets of other specific oligonucleotide
primers were used for the detection of avian respiratory pathogens
other than AIV. The mRT-PCR DNA products were visualized by Agarose
Gel Electrophoresis and consisted of DNA fragments of 1023bp for
M-Gene of AIV, 149bp for IBV, 320bp for NDV and 647bp for ILTV. The
second set of primers used for m-RT-PCR of H7N3, H9N2 and H5N1
provided DNA products of 300bp for H7, 456bp for H5 and 808bp for
H9. The mRT-PCR products for the third format consisted of DNA
fragments of 149bp for IBV, 320bp for NDV, 647bp for ILTV, 300bp for
H7, 456bp for H5, 808bp for H9. The sensitivity and specificity of
mRT-PCR was determined and the test was found to be sensitive and
specific for the detection of AIV and other poultry respiratory
pathogens. In the present study, multiplex PCR technique has been
developed to simultaneously detect and differentiate three most
important subtypes of AIV’s alongwith 3 most common avian
respiratory pathogens prevalent in poultry in Pakistan.
The non-structural 1 (NS1) protein of avian influenza viruses has
been earlier described as a remarkably conserved protein amongst
type A influenza viruses, however with subsequent findings of is
truncation during extensive circulation in poultry has led to
further investigate its mutation in association with point mutations
simultaneously occurring in more variable genes such as HA and NA.
Apart from affecting any of the biological functions of these
viruses, these mutations may affect the immunogenic component(s) of
these viruses, affecting the efficacy of prevalent vaccines.To
establish if Pakistani H7N3 Avian influenza viruses undergo any
truncation in non-structural genes,
the non-structural gene 1 (NS1) of 22 H7N3 Avian influenza A viruses
isolated from commercial and domestic poultry was sequenced and
compared phylogenetically. The isolates included in the present
study were both of low pathogenecity (LPAI) and highly pathogenic
strains (HPAI) of H7N3 avian influenza viruses as observed in the
field with regards to their mortality rates. These isolates
circulated in N.W.F.P, Punjab, and Sindh areas of Pakistan from 1995
to 2005. Size variation in the predicted amino acid sequence of each
NS1 was revealed with two different levels of carboxy-terminal
truncation in those isolates. Of the 22 isolates analyzed, 02
isolates A/Chicken/Pakistan/NARC-100/04 and
A/Chicken/Pakistan/NARC-1282/04 encoded a full length NS1 protein of
230 amino acids, whereas 20 encoded a truncated protein of 217 amino
acids.The isolates exhibiting the truncated carboxy terminal NS1
protein, clustered together and appeared to be closest to A/Duck/Jiang
Xi/6146/03 (H5N3), A/Duck/Hong Kong/610/79 (H9N2) and A/Aquatic
Bird/Korea/CN-1/04 (H3N6) at the nucleotide level and amino acid
level. In contrast, the nucleotide sequence of one of the isolates
with the full length NS1 protein (A/Chicken/Pakistan/NARC-1282/04)
showed 99.9% nucleotide homology and 99.6% homology to a set of
Italian H7N3 isolates of Turkey from 2002 at the NS1 gene e.g
A/turkey/Italy/8912/2002(H7N3) and A/turkey/Italy/214845/02(H7N3).
The other isolate (A/Chicken/Pakistan/NARC-100/04) with the full
length NS1 protein showed the highest homology (96%) with the NS1
gene of an H5N7 subtype virus A/mallard/Denmark/64650/03.
Out of these 22 H7N3 isolates sequenced for the NS1 gene, 6 isolates
from the Northern Parts of Pakistan were further sequenced for the
HA and NA genes. One of the isolates had an untruncated NS1 whereas
5 were truncated. The 5 H7N3 isolates with truncated NS1 sequenced
were HPAI, for the HA gene and showed the presence of typical highly
pathogenic pattern of deduced amino acid sequence at the HA cleavage
site.The phylogenetic analysis of these H7N3 isolates indicated a
close resemblance to other Pakistani isolate sequences in the
GenBank, with the next closest resemblance to the H7N3 isolate from
a Peregrine Falcon in U.A.E in the GenBank besides the other
Pakistani isolates. The untruncated isolate for the NS1 gene,
A/Chicken/Pakistan/NARC- 1282/04, showed a typical low pathogenicity
cleavage site sequence at the HA cleavage site. Phylogenetic
Analysis of this isolate indicated a close resemblance to Italian
H7N3 isolates especially A/Chicken/Italy/682/2003 (H7N3) and
A/turkey/Italy/8535/2002 (H7N3). The NA gene was analyzed for the
presence or absence of a stalk region in the isolates sequenced. The
5 truncated H7N3 isolates for the NS1 Gene and HP for HA gene had a
stalked NA protein as in H7N3 isolates reported in wild birds
showing a close resemblance to other previously sequenced H7N3
Pakistani isolate sequences in the GenBank, whereas the untruncated
NS1 H7N3 isolate also showing a LPAI cleavage site sequence
A/Chicken/Pakistan/NARC-1282/04 had a deleted NA stalk region,
deduced amino acid sequence showing a deletion of 24 amino acids in
concordance with other italian H7N3 isolates reflecting a probable
introduction of a highly circulating virus in domestic poultry. It
was concluded from the present study that the H7N3 isolates from
Pakistan show slow antigenic drift and continue to evolve in a slow
manner during a ten year period in the poultry population. With
information obtained from the data on NS1, HA1 and NA, continuous
monitoring of circulating viruses is possible and subsequent
production of homologous vaccines from field strains is key to the
control of HPAI in poultry.
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